Time to Change: A Systems Pharmacology Approach to Disentangle Mechanisms of Drug-Induced Mitochondrial Toxicity

Charlotte A. Hoogstraten; Jonathan J. Lyon; Jan A.M. Smeitink; Frans G.M. Russel; Tom J.J. Schirris

doi:10.1124/pharmrev.122.000568

Visual Overview

Abstract

An increasing number of commonly prescribed drugs are known to interfere with mitochondrial function, which is associated with almost half of all Food and Drug Administration black box warnings, a variety of drug withdrawals, and attrition of drug candidates. This can mainly be attributed to a historic lack of sensitive and specific assays to identify the mechanisms underlying mitochondrial toxicity during drug development. In the last decade, a better understanding of drug-induced mitochondrial dysfunction has been achieved by network-based and structure-based systems pharmacological approaches. Here, we propose the implementation of a tiered systems pharmacology approach to detect adverse mitochondrial drug effects during preclinical drug development, which is based on a toolset developed to study inherited mitochondrial disease. This includes phenotypic characterization, profiling of key metabolic alterations, mechanistic studies, and functional in vitro and in vivo studies. Combined with binding pocket similarity comparisons and bottom-up as well as top-down metabolic network modeling, this tiered approach enables identification of mechanisms underlying drug-induced mitochondrial dysfunction. After validation of these off-target mechanisms, drug candidates can be adjusted to minimize mitochondrial activity. Implementing such a tiered systems pharmacology approach could lead to a more efficient drug development trajectory due to lower drug attrition rates and ultimately contribute to the development of safer drugs.

Significance Statement Many commonly prescribed drugs adversely affect mitochondrial function, which can be detected using phenotypic assays. However, these methods provide only limited insight into the underlying mechanisms. In recent years, a better understanding of drug-induced mitochondrial dysfunction has been achieved by network-based and structure-based system pharmacological approaches. Their implementation in preclinical drug development could reduce the number of drug failures, contributing to safer drug design.

I. Mitochondrial Dysfunction as a Major Determinant in Adverse Drug Reactions

Mitochondria are well known for their classic role in cellular energy production, as they harbor many central metabolic pathways, including the tricarboxylic acid (TCA) cycle and the oxidative phosphorylation (OXPHOS; Fig. 1). Consequently, they generate the majority of cellular ATP (Galluzzi et al., 2012a, 2012b). When cellular energy demand is high, such as in renal proximal tubule and heart muscle cells, fatty acids (FA) are used as preferred substrate for ATP production via β-oxidation. In the cytosol, FAs are converted into acyl-CoA and transferred into the mitochondrial matrix by the carnitine/acylcarnitine carrier, driving β-oxidation and leading to the production of acetyl-CoA that fuels the TCA (Fig. 1). Although fatty acid β-oxidation is the most efficient ATP-producing mechanism, this pathway implies a high oxygen request and will therefore be limited to such conditions, whereas other substrates might be used when high oxygen requirement cannot be fulfilled.

Fig. 1

The mitochondrion and its main characteristics. Mitochondrial ATP production from glucose starts with the import of glycolytic pyruvate and conversion into acetyl-coenzyme A (acetyl-CoA) by the pyruvate dehydrogenase complex. Subsequently, acetyl-CoA enters the TCA cycle producing reduced NADH and reduced flavin adenine dinucleotide (FADH₂), which function as substrates for the first and second multisubunit enzyme complexes of the mitochondrial respiratory chain, respectively. This enables the transfer of protons from the mitochondrial matrix into the intermembrane space by the respiratory chain complexes I, III, and IV, while oxygen is consumed at complex IV. The resulting electrochemical membrane potential is used by the F₁F₀-ATP synthase, also known as complex V, to generate the majority of cellular ATP from ADP. In addition, the matrix harbors various other metabolic pathways, placing mitochondria in the center of cellular catabolic and anabolic pathways. β-Oxidation accounts, for example, for the production of acetyl-CoA and NADH from fatty acids, imported through the carnitine transport system (Hoppel, 1982) and is used by the TCA cycle and OXPHOS system, respectively. Other metabolic pathways located in the mitochondrial matrix include heme biosynthesis, steroidogenesis (and the first steps of cholesterol synthesis), part of amino acid metabolism, iron-sulfur cluster assembly, part of gluconeogenesis, and calcium storage. Inside the mitochondrial matrix, mtDNA resides and may be subjected to damage from reactive oxygen species (ROS).

The compartmentalized structure of mitochondria provides the required microenvironment for these and many other metabolic pathways located within the mitochondrial matrix, such as heme biosynthesis, iron-sulfur cluster assembly, part of gluconeogenesis, ketogenesis, part of amino acid metabolism, and calcium storage (Galluzzi et al., 2012b). Additionally, mitochondria play a pivotal role in cellular life, stress, and death and are more recently implicated in the initiation and propagation of inflammatory responses (Galluzzi et al., 2012b; Weinberg et al., 2015; Riley and Tait, 2020; Tiku et al., 2020). Combined with their metabolic roles, this led to the inevitable association with many common diseases, for instance neurodegenerative disorders (i.e., Alzheimer’s and Parkinson’s disease), type II diabetes, several cancers, and cardiovascular disease (Sivitz and Yorek, 2010; Walters et al., 2012; Galluzzi et al., 2013; Alam and Rahman, 2014; Rao et al., 2014; Weinberg and Chandel, 2015; Murphy and Hartley, 2018). Hence, mitochondria have gained much interest as therapeutic targets (Lanzillotta et al., 2019; Patel et al., 2019; Seo et al., 2019; Roth et al., 2020).

In addition, an increasing number of commonly prescribed drugs are known to interfere with mitochondrial function (e.g., cholesterol-lowering and antidiabetic drugs, antibiotics, chemotherapeutics, and immunosuppressants). Accordingly, these drugs often affect tissues with a high energy demand, including the central nervous system, skeletal muscle, heart, liver, and kidneys (Rolo et al., 2004; Amacher, 2005; Begriche et al., 2011; Montaigne et al., 2012; Pessayre et al., 2012; Schirris et al., 2015a; Wallace et al., 2020). The relevance of mitochondrial toxicity as targets for adverse drug effects is exemplified by the observation that approximately 50% of all U.S. Food and Drug Administration black box warnings are associated with drug-induced mitochondrial dysfunction (a representative overview for cardiovascular, renal, and hepatic toxicity of drugs is shown in Table 1) (Dykens and Will, 2007; Nadanaciva and Will, 2009; Pereira et al., 2009). A screen of 676 unique compounds demonstrated that 73% negatively affected mitochondrial function (e.g., inhibition of the mitochondrial electron transport chain and mitochondrial uncoupling) in an in vitro assay using primary renal proximal tubule cells (Wills et al., 2015). Although drugs could interfere with the protein binding pocket and thereby the function of all approximately 1200 mitochondrial proteins (Calvo et al., 2016), off-target mechanisms are generally categorized as (1) inhibition of multisubunit OXPHOS complexes (Fosslien, 2001; Schirris et al., 2015a); (2) respiratory uncoupling (Madiraju et al., 2014); (3) permeability transition pore opening; (4) suppression of fatty acid β-oxidation and carnitine shuttling pathways for several drugs, including diclofenac, ibuprofen, and zidovudine (Massart et al., 2013; El-Gharbawy and Vockley, 2018; Console et al., 2020); (5) mitochondrial transporter inhibition (Dolce et al., 2001; Divakaruni et al., 2013; Kalghatgi et al., 2013); and (6) affected mitochondrial DNA replication, transcription, or translation (Brinkman et al., 1998; Chan et al., 2005; Dykens, 2008; Payne et al., 2011; McGill et al., 2012). Functionally, these mechanisms are often associated with a reduction of oxygen consumption, increased levels of reactive oxygen species (ROS) or changes in mitochondrial substrates [e.g., reduced nicotinamide adenine dinucleotide (NADH)], decreased ATP levels, or increased oxygen consumption with uncouplers, as well as disturbed calcium homeostasis. Although many compounds are “mito-active” in vitro (and thus have an intrinsic mitochondrial hazard), it is important to emphasize that not all result in mitochondrial toxicity in vivo (i.e., pose a mitochondrial toxicity risk), and in some cases the activity is central to a drug’s pharmacology. Translation of in vitro hazard to in vivo risk is determined by multiple factors but predominant are potency, exposure (including to specific sensitive tissues), and the target tissue’s ability to adapt to the metabolic challenge.

View this table:

TABLE 1

Overview of example drugs with FDA black box warnings for cardiovascular, renal and hepatic toxicity^a

As alluded to, for some drugs the potential to perturb mitochondrial function contributes to their therapeutic efficacy (Lin et al., 2015). The antidiabetic effect of the commonly used drug metformin has, for example, been reported to act through inhibition of mitochondrial glycerol-3-phosphate dehydrogenase and mitochondrial complex I activity at micro- and millimolar concentrations, respectively. The consequent reduced pyruvate and increased adenosine monophosphate levels result in a decreased hepatic gluconeogenesis, via respective positive feedback signaling and adenosine monophosphate-activated protein kinase activation, explaining its use as first-line therapy in type II diabetes mellitus (Owen et al., 2000; Madiraju et al., 2014). The ability of metformin to inhibit mitochondrial function also led to the exploration of its potential use in several cancer types (Viollet et al., 2012; Kheirandish et al., 2018; Thakur et al., 2018). In addition, drug-induced mitochondrial dysfunction has been associated with the therapeutic efficacy of many other anticancer drugs, including etoposide (cell death induction via the mitochondrial-dependent p53 pathway), doxorubicin [inhibition of OXPHOS complexes, respiratory uncoupling, suppression of FA- and TCA- associated protein expression, inhibition of topoisomerase II, and reduction in mitochondrial DNA (mtDNA) content], taxol [opening of the mitochondrial permeability transition pore (mPTP)], thapsigargin (opening of the mPTP), and apicidin (apoptosis via mitochondrial-dependent caspase cascade) (Kwon et al., 2002; Swain et al., 2003; Dykens, 2008; Lebrecht et al., 2010; Quintanilla et al., 2013; Canta et al., 2015; Jamil et al., 2015; Yadav et al., 2015; Babaei et al., 2020).

The impact of drug-induced mitochondrial toxicity can be very significant as emphasized by the market withdrawal of a number of commonly prescribed drugs due to serious mitochondrial adverse effects, such as troglitazone-induced severe liver injury (respiratory uncoupling and opening of the mPTP), cerivastatin-induced rhabdomyolysis (respiratory uncoupling, inhibition of glutamate-driven respiration, and induction of ultrastructural changes), and fatal lactic acidosis by phenformin and buformin (Furberg and Pitt, 2001; Tirmenstein et al., 2002; Bova et al., 2005; Seachrist et al., 2005; Westwood et al., 2005; Kaufmann et al., 2006; Masubuchi et al., 2006; Dykens and Will, 2008; Bridges et al., 2014; Segawa et al., 2018; Totten et al., 2021). Although the withdrawals of phenformin and buformin date from the 1970s, it was only over the last two decades that mitochondrial activity of drugs gained more attention (Dykens and Will, 2008; Amoedo et al., 2017; Meyer et al., 2018; Rana et al., 2019; Bellance et al., 2020). A comprehensive overview of novel cases of mitochondrial toxicity, including enhanced insights into the underlying pathomechanisms, has been reviewed by others (Will et al., 2019; Wu et al., 2020; Leuthner and Meyer, 2021). To understand the physiologic effects of a drug or compound on mitochondrial function and correlate this mechanistic, biologic, and chemical information with clinically relevant toxicity, an extensive mitochondrial toxicity database (MitoTox) has recently been established (Lin et al., 2021). It combines pharmaceutical information with experimental data of over 1,400 small molecules and drugs and aims to integrate knowledge on mitochondria-related toxicants and their targets. Molecules related to mitochondrial toxicity are classified according to their action on the target, including membrane potential (e.g., depolarization, hyperpolarization, uncoupling, and redox cycling), function of mitochondria (e.g., oxidative phosphorylation and glucose/lipid/amino acid metabolism), organization of mitochondria (e.g., morphology, mass, biogenesis, mitophagy, fission, and fusion), movement of mitochondria (e.g., mitochondrial transport and motility), oxidative stress (e.g., ROS generation, antioxidants, and scavenger of mitochondrial superoxide), mtDNA (e.g., mtDNA replication, maintenance, and mutation), cell death (e.g., apoptosis, necroptosis, and autophagy), and signaling (e.g., mTOR, adenosine monophosphate-activated protein kinase, and mitogen-activated protein kinase), as summarized in Fig. 2A (Lin et al., 2021). In this review, we focus on specific mitochondrial characteristics that explain why mitochondria are particularly prone to adverse drug effects (Fig. 2). These include the lipid abundance of both mitochondrial membranes that facilitates accumulation of lipophilic drugs. Second, the inner mitochondrial membrane contains high levels of the phospholipid cardiolipin, required for proper functioning of many proteins embedded in this membrane (e.g., OXPHOS complexes). Cardiolipin’s negative charge, however, enhances interactions with cationic drugs (de Wolf et al., 1993; Parker et al., 2001). Such interactions exacerbate membrane fluidity, which together with drug accumulation can eventually result in mitochondrial dysfunction (Unsay et al., 2013). Third, mitochondrial transport proteins and channels, such as the mitochondrial calcium uniporter, allow accumulation of drugs in the mitochondrial matrix and specifically metal ions (e.g., lithium) that interact with essential proteins or disturb the redox cycle (Salimi et al., 2017; Pathak and Trebak, 2018). Fourth, the highly negative electrochemical membrane potential (approximately 120–180 mV) (Griffiths, 2000) over the mitochondrial inner membrane facilitates a strong accumulation (approximately 300- to 500-fold) of lipophilic and amphiphilic cationic drugs (Boelsterli and Lim, 2007; Meyer et al., 2013). Fifth, mitochondrial DNA repair mechanisms are limited (Meyer et al., 2013), and mtDNA is more vulnerable to drug-induced damage compared with nuclear DNA, which is explained by the difference in DNA packing by protective histones, although recent studies have suggested that mtDNA is less “naked” than previously anticipated and packed in histone-like nucleoids (Bogenhagen, 2012; Campbell et al., 2012; Gilkerson et al., 2013; Meyer et al., 2013). Increased mtDNA vulnerability to drug exposure compared with nuclear DNA is especially relevant in the elderly. Both mitochondrial function and mtDNA content decline with age, while simultaneously an increase in age-related diseases and a consequent higher use of medication in the elderly is observed, which is expected to lead to an increase in drug-induced mitochondrial dysfunction (Will et al., 2019). Sixth, mtDNA is closely located to major cellular ROS generation sites, and the scarcity of noncoding sequences that are particularly involved in regulation of gene expression prevents this control, thereby increasing vulnerability to potentially harmful substances, including drugs (Boelsterli and Lim, 2007; Meyer et al., 2013). The functioning of mtDNA is also influenced by other factors, as shown by recent developments in environmental exposure assessment linking environmental toxicants, including airborne pollutants, heavy metals, and therapeutic drugs, to impaired mitochondrial epigenetics (e.g., reduced mtDNA methylation), leading to altered expression patterns of mtDNA-coding proteins. Since the interaction between these and nuclear proteins is required for maintenance of cellular health and homeostasis, as well as mitochondrial metabolic pathways, epigenetic perturbations have been linked to a variety of conditions such as cancer, neurodegenerative disorders, disturbed cellular metabolism, and alterations in circadian rhythm (Meyer et al., 2017, 2018; Ramachandran et al., 2018; Zhou and Huang, 2018; Sharma et al., 2019; Zhou et al., 2020). Seventh, mitochondria harbor several cytochrome P450 enzymes that can convert certain drugs into toxic metabolites that could damage mitochondrial proteins, DNA, and lipids (Hartman et al., 2017; Orhan et al., 2021). Finally, the interplay of biogenesis, fission, fusion, and mitophagy makes mitochondrial morphology highly dynamic (Bereiter-Hahn and Voth, 1994), which may further increase mitochondrial vulnerability to adverse drug effects. The dynamic character arises from sequentially switching between fusion of two separate mitochondria or budding off smaller structures from a single mitochondrion (fission). This enables the adequate coordination of mitochondrial metabolism in response to cellular demands (Tilokani et al., 2018; Ramachandran et al., 2021). Elongated mitochondria are generally associated with conditions in which ATP production is increased; therefore, mitochondrial fusion presumably stimulates the distribution of these high-energy molecules throughout the cell (Mitra et al., 2009; Mishra and Chan, 2016; Ramachandran et al., 2021). Stability and replication of mtDNA and tolerance to mtDNA mutations are also thought to be fusion-dependent, as it was found in skeletal muscle that these events appear to be linked to proteins that regulate the inner and outer mitochondrial membrane fusion [e.g., mitofusin (MFN) 1 and 2] (Chen et al., 2010; Silva Ramos et al., 2019; Sidarala et al., 2022). In cells undergoing stress, mitochondrial fission seems to be the predominant dynamic event, and it is suggested to occur as an adaptive mechanism and a necessary step for the induction of mitophagy, in which dysfunctional or severely damaged mitochondria are directed to Parkin-mediated lysosomal degradation, as has been reviewed in detail (Ni et al., 2015; Tilokani et al., 2018; Ramachandran et al., 2021).

Fig. 2

Unique functional and structural characteristics render mitochondria particularly vulnerable to adverse drug effects. (A) Drug-induced mitochondrial liabilities are categorized in eight main groups according to their action on the different targets, as specified in Section I. (B) Mitochondria harbor various structural and functional characteristics that enhance their vulnerability for adverse drug effects. (I) Lipophilic drugs easily accumulate in the phospholipid-rich inner and outer mitochondrial membrane (Comte et al., 1976) and can interact with cardiolipin (CL). Especially, cationic drugs are as such trapped in the mitochondrial matrix due to cardiolipin’s negative charge. (II) Mitochondrial transport proteins and channels, such as the mitochondrial calcium uniporter, allow accumulation of drugs and metal ions in the mitochondrial matrix; the latter can interact with essential proteins or disturb the redox cycle. The additional highly negative electrochemical membrane potential over the mitochondrial inner membrane causes strong accumulation (approximately 300- to 500-fold) of lipophilic and amphiphilic cationic drugs. (III) Only a limited number of mechanisms exist that repair damaged mtDNA, of which base excision repair is the main and best understood DNA repair pathway in human mitochondria (Alexeyev et al., 2013; Zinovkina, 2018). (IV) mtDNA is packed in histone-like nucleoids, consisting of proteins including Twinkle, Tfam, and mitochondrial single-strand DNA-binding protein (SSB). The noncoding displacement or D-Loop region acts as promotor in replication of mitochondrial DNA (Sharma et al., 2005). (V) OXPHOS complexes are main generation sites of radicals, such as reactive oxygen species (ROS). mtDNA is in close proximity to these sites. Moreover, mitochondria harbor several cytochrome P450 enzymes that facilitate the conversion of xenobiotics into toxic and reactive metabolites, which could accumulate in the matrix but also directly damage mitochondrial proteins and DNA and lipids.

It has been shown that after challenging cells to various toxic conditions, mitochondrial dynamics induce changes in organelle number and morphology to maintain cell viability (Karbowski and Youle, 2003). These changes are linked to the regulation of mitochondrial metabolism and have been shown to influence each other (e.g., for cardiac and muscle cell contraction) (Mishra and Chan, 2016; Wai and Langer, 2016; Abdelwahid, 2017). Consequently, mitochondrial biogenesis, typically occurring in response to loss of functional mitochondria, is fundamental to maintaining cellular homeostasis and regeneration. Especially after exposure to toxic compounds, controlled mitochondrial biogenesis, mediated by the upregulation of the transcription factor PGC1α, enables recovery of cellular function by maintaining respiration and other vital processes. This coordinated action is regulated between mitochondria on the one hand and nuclear transcription and translation on the other, to ensure proper functioning of newly synthesized mitochondria (Ramachandran et al., 2021).

An example involving drug interference with mitochondrial dynamics is cardiotoxicity induced by doxorubicin (Kuznetsov et al., 2011; Tang et al., 2017). In vitro exposure to doxorubicin has been shown to decrease the mitochondrial fusion proteins optic atrophy (OPA) 1 and MFN1/2 and to increase phosphorylation of dynamin-1-like protein 1, which is a fundamental component of mitochondrial fission, resulting in inhibition of fusion and promotion of fission (Li et al., 2014; Tang et al., 2017; Osataphan et al., 2020). In addition, etoposide (OXPHOS inhibition, dissipation of the mitochondrial membrane potential, and ROS elevation), zidovudine (nucleoside reverse transcriptase inhibitor—OXPHOS inhibition, opening of mPTP, dissipation of the mitochondrial membrane potential, inhibition of ATP/ADP carrier, antioxidant enzyme, and DNA polymerase, and remdesivir (antiviral—OXPHOS inhibition) have also been identified as disruptors of mitochondrial dynamics, thereby promoting their fragmentation (Nomura et al., 2017; Nemade et al., 2018; Kwok et al., 2022; Tang et al., 2022). Moreover, in liver injury it has been demonstrated that exposure to acetaminophen (analgesic—inhibition of OXPHOS complexes by toxic metabolite, opening of the mPTP, and respiratory uncoupling) to primary mouse hepatocytes resulted in spheroid-shaped mitochondria before progressing to pathologic irreversibly fragmented mitochondria (Kon et al., 2004; Hanawa et al., 2008; Hu et al., 2016; Umbaugh et al., 2021). On the other hand, liver regeneration after acetaminophen-associated toxicity could be induced by facilitating mitochondrial biogenesis, which is in line with the observation that impaired biogenesis contributes to age-dependent liver damage in experimental sepsis (Du et al., 2017). Since mitochondrial biogenesis restores oxidative metabolism in bacterial sepsis, it is considered an important and early prosurvival factor (Haden et al., 2007). Sustained cellular stress could also lead to mitochondrial remodeling, as alterations in morphology and biogenesis are thought to shift mitochondrial homeostasis to support cell survival. This is a phenomenon observed in various processes associated with hepatic, cardiovascular, and metabolic diseases, for instance insulin resistance in nonalcoholic fatty liver disease (Gottlieb and Bernstein, 2016; Shannon et al., 2021). It is well established that mitochondrial dynamics underlie cellular homeostasis and that its dysregulation is inseparable from pathophysiological conditions.

Previous drug withdrawals highlight the historic lack of sensitive and specific assays to detect mitochondrial toxicity during drug development. The standard battery of in vivo toxicology studies mandated during drug development relies on healthy animals, which have a high metabolic reserve capacity and can easily adapt to moderate metabolic challenges without showing adverse signs or pathology. This contrasts with many patient groups who are subject to comorbidities, comedications, lifestyle choices, age, and genetic factors, which can all erode their metabolic reserve capacity. As part of an alternative approach, systems pharmacology has proven to be effective to pinpoint mitochondrial off-target effects (Bisson et al., 2007; Wagner et al., 2008; Fannin et al., 2010; Lee et al., 2013; Schirris et al., 2015b). This review aims to provide an overview of these strategies. We propose the implementation of a tiered systems pharmacology approach to aid the identification of mechanisms underlying mitochondrial dysfunction of existing and new drugs under development.

II. Current Methods to Identify Drug-Induced Mitochondrial Dysfunction

Regularly applied assays to evaluate drug-induced mitochondrial dysfunction include measurements of OXPHOS complex enzyme activities, mitochondrial membrane potential, lactate and cellular ATP generation, mtDNA, and calcium levels (Dykens and Will, 2018). Most of these parameters are determined as an endpoint observation. Screening of cellular oxygen consumption rates (i.e., using Seahorse extracellular flux analysis or a fluorescent oxygen sensor) has been introduced and is widely applied to detect mitochondrial activity (Hynes et al., 2006; Hynes et al., 2009; Beeson et al., 2010). The importance of measuring respiratory capacity of the mitochondrial energy generating system is based on the notion that virtually all mitochondrial bioenergetic pathways converge in the OXPHOS system. Moreover, OXPHOS complexes are often observed as important off-targets involved in adverse effects of drugs (Nadanaciva et al., 2007; Hargreaves et al., 2016), and their adequate function depends on the presence of an electrochemical membrane potential. Consequently, measuring respiratory rates instantly provides information about a variety of mitochondrial functional parameters. A reduced oxygen consumption rate and decreased OXPHOS function are associated with increased reductive stress. The resulting surplus of electrons may react with cellular oxygen to produce excessive ROS. A gamut of intracellular molecular probes to sense ROS (Forkink et al., 2010) or detect ROS-induced damage (i.e., lipid and protein peroxidation) are increasingly applied in the investigation of drug-induced mitochondrial damage (Belousov et al., 2006; Forkink et al., 2010; Kalyanaraman, 2011). These fluorescent compounds include small molecules such as hydroethidine, CM-H₂DCFDA, dihydrorhodamine 123, and C11-BODIPY that require incubation to get into the cell. On the other hand, protein-based reporter molecules, which can be introduced into the cell by stable or transient transfection, can be used to detect cellular ROS levels, including circularly permuted yellow fluorescent protein, HyPer, and reduction-oxidation sensitive green fluorescent protein. It is important to note that each of these probes can be used to gain insight into the formation of ROS molecules, which are known to have different origins. For example, the primary mitochondrial ROS molecule O₂^– results from electron reduction of O₂ and is generally detected by HEt. The importance of these experimental approaches to distinguish between ROS types is emphasized by the notion that ROS molecules can also serve as cellular signaling molecules. Low levels of ROS and downstream products are key to cellular health and have beneficial effects, for example, in the defense against microbial agents (Valko et al., 2007). Consequently, distinguishing different ROS molecules is useful in separating oxidative stress-related toxic mechanisms from beneficial signaling events (Forkink et al., 2010).

Although phenotypic assays have proven to be very powerful in the detection of drug-induced mitochondrial dysfunction (Wills et al., 2015), these do not provide information about the exact mitochondrial off-target. Furthermore, whether a drug directly affects mitochondria or whether mitochondrial function is influenced secondary to other cellular mechanisms is difficult to distinguish.

The introduction of high-content imaging with mitochondria-selective fluorescent and phosphorescent dyes has facilitated the evaluation of mitochondrial function, morphology, and mitochondrial biogenesis using live-cell imaging (Ferrick et al., 2008; Wagner et al., 2008; Iannetti et al., 2016; Düssmann et al., 2017; Zhang et al., 2017), which enables monitoring of drug effects over prolonged time courses. Besides overcoming the limitation of phenotypic endpoint assays, it also allowed the simultaneous determination of multiple parameters using multiple probes. Recently, spectral unmixing (e.g., linear unmixing) methods have further advanced high-content imaging, as it allows scientists to analyze fluorescent probes with overlapping excitation and emission spectra (Valm et al., 2016; Megjhani et al., 2017). This application has increased the number of fluorescent labels up to 120 for live-cell imaging. Moreover, combining imaging techniques with machine learning made it particularly amenable to disentangle the effects of drugs on mitochondrial function and morphology (Blanchet et al., 2015; Iannetti et al., 2016; Iannetti et al., 2019). These methods have enabled the successful, unbiased identification of beneficial drug effects on primary cells with a genetically encoded mitochondrial defect and of drug-induced mitochondrial dysfunction (Leonard et al., 2015; Zahedi et al., 2018). They have also significantly aided in the screening of large drug libraries for mitochondrial activity. Importantly, the sensitivity to detect drug-induced mitochondrial dysfunction has been shown to increase in such assays with multiple parameters (Wagner et al., 2008; Wills et al., 2015). The high costs of fluorescent live-cell imaging and rather low capacity, however, limit their use to late-phase compound characterization (Haney et al., 2006; Smith et al., 2012). Clearly, the identification of therapeutic targets and pharmaceutical drug development finally requires in situ complementation studies and even in vivo validation of lead compounds to exclude any potential compound-associated (mitochondrial) toxic hazard and verify safety in a physiologic system, as described in more detail in the section “A Tiered Approach to Implement Mitochondrial Systems Pharmacology in Drug Development.”

Even though these advanced methodologies have increased the capability to detect drug-induced mitochondrial dysfunction, they still predominantly measure the phenotypic consequences, rather than identifying the primary target being affected. In addition, the large number of possible pathways regulating mitochondrial function limits the use of traditional research techniques that are based on an a priori hypothesis about the mechanisms involved. Only a subset is represented, which is expected to hamper the detection of relevant off-target mechanisms. Consequently, there is a great need for an unbiased systems analysis in which the complete network of cellular metabolic processes and pathways is considered. This, however, will depend on the availability of large data sets collected without an a priori hypothesis, to avoid inherent selection bias of known pathways (Go et al., 2018).

III. Application of Systems Pharmacology to Investigate Drug-Induced Mitochondrial Dysfunction

In contrast to hypothesis-driven strategies as described previously, systems biology integrates data on multiple levels, including experimental (e.g., mechanistic studies), omics, and predictive bioinformatics data sets. This enables an overall understanding of mechanisms underlying mitochondrial dysfunction on a systems level, which opens up opportunities for targeted investigations of adverse events.

Integrative and unbiased observations from big databases allow the examination of global fluctuations in cellular metabolism, instead of studying the effects on a smaller scale (e.g., single genes, proteins) (Fasano et al., 2016). However, to understand these metabolic effects, gene expression and metabolite concentrations need to be mapped on cellular metabolic networks to connect all individual reactions. The feedback inhibition of amino acid biosynthetic pathways was one of the first metabolic networks constructed more than 60 years ago. Despite this, a clear definition of systems biology is lacking, but it is generally considered to be an integrative approach at the level of full organism, tissue, or cell. It is aimed to understand the physiology and pathology using complex molecular response networks (Klipp et al., 2009). Systems biology is based on a holistic methodology combining all possible targets and pathways involved. The classic systems biology cycle is initiated by data acquisition at a patient, animal, or cell model level, as described in Fig. 3. Types of data include clinical phenotypes; cellular responses; omics-derived data (e.g., genomics, transcriptomics, proteomics, and metabolomics); biochemical reactions or pathways; and drug-related data on pharmacodynamics, pharmacokinetics, and toxicity. Clinical samples, for example, use patient-derived body fluids (e.g., blood or plasma) for RNA sequencing and mass spectrometry–based untargeted metabolomics (e.g., next-generation metabolic screening), as increasingly applied in diagnostic screening for inborn errors of metabolism and mitochondrial disease (Miller et al., 2015; Tebani et al., 2016a,b; Bonte Buzkova et al., 2018; Coene et al., 2018; Hoegen et al., 2021; Thistlethwaite et al., 2022). By measuring as many metabolites as possible, a metabolic fingerprint can be generated that is representative of a biochemical phenotype, thereby offering novel opportunities for diagnostic screening (Hoegen et al., 2021). The next step is to integrate data by incorporating the obtained knowledge of biochemical pathways, molecular interactions, and omics-derived data into a computer database coupled to correct ontology terms, used for interpretation of a given pathway or process. A similar systematic approach has previously been applied to build the Kyoto Encyclopedia of Genes and Genomes (KEGG) databases, which collects, combines, and maintains data on genetics (KEGG GENES database), biochemistry (KEGG PATHWAY database), and molecular and cellular biology (KEGG LIGAND database) (Kanehisa, 1997; Ogata et al., 1999). Computational methods are then employed to model various experimental conditions, including gene functions in terms of gene networks and molecules, reconstruction of biochemical pathways, and prediction of biologic systems. The three modeling approaches that are characteristically applied are discussed in detail later and in Fig. 4. Computational models are typically validated with experimental data ranging from in vitro (cells), in vivo (animal) to clinical studies investigating mitochondrial function (e.g., OXPHOS enzyme activities, cellular ATP levels, and mtDNA, as described in the section “Current Methods to Identify Drug-Induced Mitochondrial Dysfunction”). If model refinement is needed, the cycle is reinitiated. Systems biology typically employs top-down, bottom-up, or middle-out models (Fig. 4). The top-down approach applies a coarse-grained model of an entire system, which is often refined using large-scale omics data, including proteomic, interactomic (viz. all interactions between and among proteins and molecules within a cell and their consequences), transcriptomic, genomic, or metabolic data (Rolland et al., 2014; Wan et al., 2015; Bludau and Aebersold, 2020). The use of these “omics” data sets enable the construction of biologic networks that represent interactions between genes, transcripts, proteins, and metabolites and aids in the identification of novel pathophysiological mechanisms, as well as new biomarkers and therapeutic targets, as extensively discussed by Maldonado et al. (Suomalainen et al., 2011; Maldonado et al., 2019). These network models represent interacting molecules by nodes (e.g., genes or proteins) and edges (e.g., chemical transformations such as biochemical reactions or regulatory relationships) (Albert, 2007). Nodes that interact with several others are referred to as hubs that split the network into isolated clusters upon loss, whereas node disruption does not cause major loss of connectivity (Albert, 2007; Maldonado et al., 2019). In the context of mitochondrial disease, these network-based approaches are powerful in studying mitochondrial (dys)function as numerous interactions can be explored, enabling the elucidation of integrative mitochondrial functions that may have been missed using traditional experimental techniques (Maldonado et al., 2019). These top-down network models are generally holistic by their nature as they involve an in-depth investigation of the whole system. As an example, a top-down workflow applied in mitochondrial research involves sample (e.g., patient-derived) collection, processing by high throughput methods (e.g., omics), and analysis by bioinformatics tools to gain a better understanding of function (Maldonado et al., 2019). Bottom-up models rely on mechanistic hypothesis-driven studies of molecular interactions. In contrast to the top-down strategy, they are typically based on (database or literature-driven) experimental data and described by a smaller number of interactions involved. Processes are studied individually and integrated into a model, such as certain metabolic pathways, including glycolysis and catabolism (Teusink et al., 2000; Klipp et al., 2009; Cortassa et al., 2019; Marín-Hernández et al., 2020) mitochondrial malate-aspartate and citrate-pyruvate shuttles (Korla et al., 2015), mitochondrial messenger RNA translation (Korla and Mitra, 2014), ROS generation in the mitochondrial matrix (Korla, 2016), and more comprehensive mitochondrial (Wu et al., 2007) and cellular models (Grass et al., 2022). Interestingly, such bottom-up dynamic metabolic models have recently been further refined with the inclusion of circadian cellular patterns, as time-dependent changes in metabolic activity (Rowland Adams and Stefanovska, 2021). The construction of genome-scale metabolic models using pre-existing databases combined with literature input is also powerful in modeling biologic systems, as they aim to fully encompass all interactions within a system. Especially in the context of mitochondrial disorders, generation of these metabolic models has contributed to the assessment of the functional consequences of genetic changes or to the identification of therapeutic targets facilitating the design or repurposing of drugs (O'Brien et al., 2015; Brunk et al., 2018; Maldonado et al., 2019). As described earlier for the use of a top-down strategy in mitochondrial research, the bottom-up workflow can be characterized by identification and collection of molecular data (e.g., database-driven data on glycolysis), formatting this into a model (e.g., genome-scale metabolic models), followed by prediction of solutions to gain a better understanding of the underlying mechanisms (Maldonado et al., 2019).

Fig. 3

Representation of the classic systems biology cycle. Systems biology strategies are typically initiated with biologic data collection, which can originate from a variety of sources as indicated. Subsequently, collected data are integrated in computational models to simulate conditions of interest. Depending on available data and outcomes, different types of models can be applied, including top-down, bottom-up, or middle-out modeling (also see Fig. 4). Next, resulting predictions are experimentally verified in vitro and in vivo. After validation, new knowledge and insights originate and could also reinitiate the cycle to further adjust and refine the model. In this way, the predictive power of simulations can be improved.

Fig. 4

Overview of different types of systems biology approaches. Systems biology approaches can be categorized as either top-down, bottom-up, or middle-out strategies. Top-down methods are initiated by the collection of big data sets often obtained using omics approaches (e.g., proteomics, genomics, transcriptomics, and metabolomics) to construct network models representing the interactions between genes, transcripts, proteins, and metabolites in a biologic system. In this modeling methodology, the nodes represent the molecular targets (viz. interacting molecules in a biologic network). Interactions between nodes are represented by edges. Hubs are defined as nodes that pose interactions with other nodes. In contrast, bottom-up approaches use hypothesis-driven data and is applied to simulate a smaller set of interactions. For the generation of such dynamic models, biochemical data are preferentially used. This type of data is often modeled as ordinary and partial differential equations, which represent the dynamics of the molecular interactions involved. These models are based on experimental data, including Michaelis-Menten kinetics (as shown in the equation). “v” describes the reaction rate, related to the substrate concentrations “s”. At saturating substrate concentration, V_max represents the maximum reaction rate, while K_m is the substrate concentration at which half V_max is reached. The middle-out strategy uses elements from both approaches in a dynamic network model that aims to implement data from different levels of complexity. This modeling strategy connects the network to the dynamic behavior of the system by describing how known interactions among defined elements determine the state of the elements and how the whole system may change over time under different conditions (Albert, 2007).

While bottom-up models are built on the individual kinetic equations describing biochemical reactions, such as the Michaelis-Menten kinetics for enzyme activity, the top-down model is designed to represent a good global fit of the in vivo behavior (Klipp et al., 2009). Nevertheless, it is clear that integration of different data types is key in creating a complete representation of biology, but although the available integrative tools are expanding, they are still scarce and complex to use (Maldonado et al., 2019). As previously reviewed, studying the mechanisms underlying mitochondrial diseases benefits from a multidisciplinary approach that combines clinical, molecular, and computational research to achieve better diagnostics and improve the development of therapeutic agents (Maldonado et al., 2019). Recent developments in multiomics approaches have already been demonstrated to be a valuable tool in improving patient care (Maldonado et al., 2019). However, as the integration of large omics data sets can lead to modeling problems, methods such as similarity network fusion have been developed to aggregate and analyze multiple complex omics data sets on a genomic scale (Wang et al., 2014). xMWAS is an approach that identifies associations and correlations between molecules based on multiomics data and allows integration of more than two data sets (Uppal et al., 2018; Hu et al., 2020). Expansion of these knowledge bases, including xMWAS and MitoCarta, is an essential next step toward more efficient integration of multiomics data for providing deeper insights into specific mitochondrial network responses. (Hu et al., 2020).

In practice, the data types used are the ones that are sufficiently available from various experimental conditions and models, often applying a combination of bottom-up and top-down methodologies, known as the middle-out strategy. This method aims to integrate data from different levels of complexity using a dynamic network modeling approach. Here, the biologic network of interactions connects to the dynamic behavior of a system and has proven powerful in effectively integrating experimental and literature data to gain a holistic understanding of complex biologic systems (Albert, 2007; Sun et al., 2018) (Fig. 3). A similar systems biology approach has been applied successfully to identify Alzheimer’s disease (AD)-related genes and to discriminate molecular regulatory networks and pathways associated with healthy and diseased states in AD (Hu et al., 2017). Moreover, aberrant function of cellular metabolic pathways has been associated with phenotypic disease characteristics in AD using multiple high-throughput technologies, including genomics, transcriptomics, proteomics, and even interactomics (Soler-López et al., 2011; Kristensen et al., 2012; Zhang et al., 2014; Ng et al., 2017; Wang et al., 2019). Such integrative approaches benefit the construction of interpretable and predictive models.

Over the last 20 years, systems biology analyses were also applied in pharmacological and toxicological research (Kongsbak et al., 2014; Turner et al., 2015; Hartung et al., 2017; Yahya et al., 2021). To evaluate the dynamic interaction between drugs and biologic networks, physiochemical-based macromolecular structure modeling has been incorporated in experimental data-driven and mathematical-based pharmacokinetic and pharmacodynamic models (Ward et al., 2013; Xie et al., 2014). Combined with pharmacogenomic data, these models typically represent a systems pharmacology approach that allows deeper insight into mechanisms underlying both beneficial and adverse drug effects (Xie et al., 2014) and predicts personalized drug responses.

Systems pharmacology can methodologically be categorized in either pathway- and network-based approaches or proteome-wide exploration of drug targets using binding pocket similarity comparison. Successful identification of drug-induced metabolic network perturbations has been demonstrated using relatively simple pathway models. However, more extensive genome-scale metabolic networks combined with metabolomic or proteomic data have the potential to detect drug-induced mitochondrial dysfunction. The use of metabolomics as a comprehensive analysis strategy of metabolites and low molecular weight molecules in a biologic specimen goes beyond the scope of standard clinical laboratory techniques and allows precise analyses of hundreds to thousands of compounds. The application of techniques such as liquid/gas chromatography and mass spectrometry provides an objective lens to view the complex link between physiology and external conditions and measure responses to perturbations such as those associated with disease. In addition, as metabolomics allows detailed characterization of metabolic phenotypes, these techniques are valuable for discovering new therapeutic targets and biomarkers used to diagnose disease or monitor effects of therapeutic compounds (Clish, 2015). Unraveling drug-induced alterations in biochemical pathways because of mitochondrial dysfunction has benefitted from using metabolomic approaches, as previously illustrated for acetaminophen and troglitazone (Fannin et al., 2010; Lee et al., 2013). Recently, systematic evaluation of the effects of electron transport chain (ETC) inhibitors on both mitochondrial and cellular signaling identified that the induction of the specific amino acid response is initiated by ETC inhibition (van der Stel et al., 2022). Combining experimental data with in silico methods, including pathway and gene network analysis, proved promising in unraveling mechanisms of mitochondrial toxicity. These studies also emphasize the importance of experimental data to inform mechanistic computational models, enabling the identification of drug-induced mitochondrial toxicity (van der Stel et al., 2020, 2022). In parallel, significant progress has been made in the development of a bottom-up description of mitochondrial metabolism. Comprehensive dynamic models of one or more mitochondrial metabolic pathways, such as the OXPHOS system, the TCA cycle, or metabolite transport, have been constructed (Wu et al., 2007; Heiske et al., 2017; Bolaji O, 2018). Recently, the application of mathematical modeling of time-dependent high-content imaging data has shown great promise in obtaining a quantitative understanding of mitochondrial adaptation upon exposure to a set of known ETC inhibitors (Yang et al., 2021). By modeling the dynamics of the mitochondrial membrane potential and integrating this with the pharmacokinetics of the studied compounds, it was concluded that data-driven computational modeling is a powerful tool to unravel experimental complexities, such as drug-induced mitochondrial toxicity (Yang et al., 2021). These types of dynamic models benefit from the combined application of system-level metabolic responses and flux stimulations, which is not possible with general metabolic pathway databases such as the KEGG and the BioPlanet database (Kanehisa, 1997; Huang et al., 2019). Over the years, more human metabolic network models have become available, such as Edinburgh Human Metabolic Network (Ma et al., 2007), Human Metabolic Reaction (Agren et al., 2012), and Recon1/2, the latter being a comprehensive consensus-based network (Thiele et al., 2013). A reconstruction of the human metabolic network has recently also been applied to predict drug-induced mitochondrial dysfunction of 18 steatogenic drugs (AbdulHameed et al., 2019). Such molecular networks have also been applied to identify gene ontologies, as for example in the development of the Ingenuity Pathway Analysis software, which applies algorithms to infer omics networks based on functional similarity (Calvano et al., 2005). Recently, Recon3D was developed to functionally characterize disease-associated mutations and identify metabolic responses upon exposure to drugs using three-dimensional metabolite and protein structure data (Brunk et al., 2018).

In addition to network-based approaches, the use of structure-based off-target predictions has acquired a central position in the field of systems pharmacology and toxicology. These are based on the notion that virtually all drugs are promiscuous and bind multiple targets (i.e., polypharmacology). Drug-network studies estimated that the average number of drug targets can be as high as 6.3, if therapeutic and predicted drug targets are included (Mestres et al., 2008; Schenone et al., 2013). Hence, various in silico techniques were developed to explore similarity between structural features of primary drug-binding pocket and other binding pockets to reveal drug off-targets (Xie et al., 2011; Ferreira et al., 2015). Although all examine binding pocket similarity, different methods are applied, such as comparison of the protein binding pocket itself (e.g., ProBiS; Konc and Janezic, 2012), SMAP (Ren et al., 2010), comparison of binding pocket pharmacophores (e.g., KRIPO; Ritschel et al., 2014), or ligand comparison (e.g., SEA; Keiser et al., 2007). These algorithms were successfully applied to identify (mitochondrial) targets, including antimicrobial activity of several drugs (i.e., fosfomycin, sulfathiazole, and trimethoprim; Chang et al., 2013), mitochondrial complex III inhibition by statins (Schirris et al., 2015a), mitochondrial ADP/ATP exchange inhibition (Schirris et al., 2015b), inhibition of heat shock protein 27 (Heinrich et al., 2016), and β-secretase (i.e., BACE-1) by gefitinib (Niu et al., 2014). More recently, application of deep learning (i.e., DeepDrug3D and BionoiNet; Pu et al., 2019; Shi et al., 2020) and artificial intelligence has further advanced these techniques, which increased their accuracy by accommodating for specific binding characteristics, such as involvement of hydrogen-bond acceptor and donor sides, as well as aromatic and hydrophobic contacts.

Other strategies adapted from drug design methodology have been used to systematically search for off-targets based on drug promiscuity and target similarity, such as inverse virtual screening (Salentin et al., 2014). In parallel, several experimental techniques to search for protein-small molecule interactions have been described that have developed into proteome-wide target identification. A powerful example is provided by stable isotope labeling of amino acids in cell culture, combined with affinity chromatography and mass spectrometry (Ong et al., 2009; Xie et al., 2011). Although these are robust methods to identify drug off-targets, they can also be used in a more targeted manner to validate in silico structural off-target predictions described above.

Finally, efforts in the field of systems toxicology contributed to the development of a global toxicological network that spans various hierarchical levels of biologic organization and drug-induced perturbations of physiologic mechanisms (Bai and Abernethy, 2013). Using genomic, transcriptomic, and adverse phenotypic data, interrelated network models on drug-protein, protein-pathway, pathway-organ, and organ-phenotype interactions have been constructed. Data sources provided to these models can be experimental, literature-based, or adverse event reporting databases, which most optimally are organized according to ontology terms. In this respect, the recently developed, online-available, fully searchable database MitoTox integrates comprehensive information on mitochondrial toxicity-related molecules and their targets. Over 1,400 small-molecule compounds, 870 mitochondrial targets, and more than 4,000 mitochondrial toxin-target associations described in scientific journals and electronic databases are included (Lin et al., 2021). It correlates chemical, biologic, and mechanistic data on clinically relevant mitochondrial toxicity and provides applications that include toxicity classification, prediction, reference, and even education. Moreover, a recent study combined metabolic networking with pharmacokinetic models to construct whole-body physiologically based pharmacokinetic models, which demonstrated phenotype-specific cases of drug-induced metabolic perturbations (Cordes et al., 2018). Lastly, integration of data from experiments, modeling prediction, and exposure assessment in adverse outcome pathways (AOPs) has aided toxicological risk assessment and has shown to be promising in replacing animal studies for these purposes (Hecker and LaLone, 2019). The use of AOP-based testing strategies in exploring the opportunities to flag chemicals and structurally related substances for potential mitochondrial respiratory chain-mediated neurotoxicity hazards was described by van der Stel et al. (2021). This shows that practical application of AOPs integrated with new approach methods, including in silico docking and in vitro assays, could be a promising strategy for drug safety assessment (Van der Stel et al., 2021).

In summary, various applications of systems pharmacology have demonstrated great potential to identify drug off-targets. Knowledge about off-target actions is potentially providing a rationale for novel interventions to attenuate drug adverse effects, for example by stimulation of metabolic compensatory pathways. Second, a newly identified off-target effect could indicate novel susceptibility factors, such as genetic variation of the off-target drug binding site. Lastly, expanding knowledge on off-target effects can be valuable in the construction of toxicological networks, in which combinations of drugs and targets are integrated with other relevant parameters of different levels of complexity.

IV. A Tiered Approach to Implement Mitochondrial Systems Pharmacology in Drug Development

Efforts in the field of systems pharmacology and toxicology have successfully contributed to elucidating the mechanisms underlying adverse drug effects, including drug-induced pertubation of mitochondrial function (Yang et al., 2015; Watkins, 2020). Consequently, these strategies hold great promise to detect drug-induced mitochondrial dysfunction in early stages of drug discovery. In view of the large number of drugs that have a mitochondrial liability (Wills et al., 2015) and the serious consequences if this translates into mitochondrial toxicity (Nadanaciva and Will, 2009; Pereira et al., 2009), the early understanding of drug actions on mitochondria is expected to help reduce drug attrition during late-stage drug development. Currently, systems pharmacology methods are still labor intensive, making their application most suitable when a smaller number of compounds (i.e., 5–10) is evaluated, like lead development stages. Here, we propose a tiered evaluation of drug-induced mitochondrial dysfunction in preclinical drug development, with a key position for systems pharmacology approaches during lead development. This approach is based on a toolset developed for the clinical investigation of inherited mitochondrial disease, as described in Fig. 5 and Table 2. It is important to note that the proposal here is set out in such a way that the resource required at each stage matches the stage of development of the compound(s). However, once the capability is built for each tier, there are a number of elements of the proposal that could be moved progressively earlier as the case knowledge and validation increase to the point where early chemistry decisions can be influenced to remove or significantly reduce the intrinsic hazard of mitochondrial activity.

Fig. 5

A tiered approach for the implementation of systems pharmacology to detect and ameliorate mitochondrial activity during drug development. We propose a step-by-step strategy to incorporate systems pharmacology in the drug development pipeline, based on a similar approach used to diagnose mitochondrial diseases. The first tier in this diagnostic workflow consists of phenotypic observations, which are comparable with phenotypic screening methods to detect mitochondrial dysfunction in early drug development stages like hit identification. The second tier in patients consists of clinical chemistry and can in drug development be compared with the lead development phase. This tier could consist of more in-depth phenotypic characterization of the previously observed mitochondrial liability. In this tier we suggest incorporating systems pharmacology to aid identification of the mechanisms underlying drug-induced mitochondrial dysfunction. These approaches can consist of network-based or structure-based modeling to identify off-target mechanisms. Subsequent computational techniques of systems biology and corresponding in vitro evaluation (e.g., biochemical and cellular assays) would result in an optimized lead or clinical candidate. If mitochondrial activity is though observed, the systems biology cycle can be reinitiated, with slight chemical adjustments to the potential lead. The third tier of the diagnosis of a mitochondrial disease is genetic screening. In drug development this phase would compare with the lead optimization phase, in which only a small number of compounds is considered as well. Here, more mechanistic insights into the underlying off-target mechanism could be obtained using more advanced techniques including medium- and high-throughput and microscopic imaging and the used of knockout strategies like CRISPR-Cas9. The fourth and last tier compares to functional in situ studies as performed in clinical diagnosis of mitochondrial diseases, which can in drug development be used to assess a drugs effect on mitochondrial function in vivo and most likely be used as an in vivo validation of the previously applied systems pharmacology approaches to attenuate mitochondrial dysfunction.

View this table:

TABLE 2

Overview of example assays that can be applied in our proposed tiered evaluation of drug-induced mitochondrial dysfunction, based on methodologies used in the clinical investigation of inherited mitochondrial disease

A. Tier 1: Phenotypic Screening During Hit Identification

The first diagnostic phase for mitochondrial diseases is mainly focused on clinical chemistry abnormalities, which can be compared with a phenotypic toxicity screening during drug development, as both aim to identify most significant phenotypes. Clinically, a broad range of parameters is assessed to examine which is most relevant for disease state. Similarly, general measures of mitochondrial function could be used to initially flag compounds with a potential intrinsic mitochondrial toxic hazard. Clinical chemistry abnormalities leading to a high suspicion of mitochondrial defects include increased blood lactic acid concentrations. However, only 30% of mitochondrial-diseased children present with elevated venous lactate levels (Munnich et al., 1996). Therefore, the suspicion of a mitochondrial defect depends on multiple signals, and the chance of such a disease increases with the number of phenotypic alterations observed. Low suspicion of mitochondrial disease often results from single-organ system effects (cardiomyopathy, impaired neurodevelopment, exercise intolerance) and reduced ATP production (Koopman et al., 2016). In the case of drug-induced mitochondrial dysfunction, reduced ATP levels are expected to have a lower predictive value, as cellular ATP levels are maintained by compensatory mechanisms (Dykens et al., 2007). For example, phosphagen pools and relevant kinases hold ATP at unity by maintaining adenine nucleotide pools. Phosphagens (e.g., phosphocreatine) are found in tissues that experience quickly changing energy demands, such as muscles and nerves, and function as immediate access reserve of high-energy phosphates needed to rapidly generate ATP from ADP (Dykens et al., 1996). Therefore, a reduction in cellular ATP levels mostly associates with severe and not mild mitochondrial activity (Will and Dykens, 2014). Phenotypic assays for mitochondrial activity assessment are not universally incorporated in drug development pipelines at present, and where they are used, the approach taken can vary considerably. One of the more commonly applied early screening methods is the glucose-galactose assay, which is based on the observation that cells obtain less ATP from glycolysis under galactose conditions (Will and Dykens, 2014). Accordingly, cells rely much more on mitochondrial metabolism, which may render them more susceptible to mitochondrial toxicants. Nonetheless, only 2% to 5% of all mitochondrial toxicants are detected by this assay, underscoring its limited predictive value (Hynes et al., 2013) as a stand-alone approach. To improve the predictive value, additional assays for mitochondrial activity are required (Wagner et al., 2008; Wills et al., 2015). To conclude, a combination of low-cost assays with medium- to high-throughput capacity can be seen as a first tier of our strategy to demonstrate whether mitochondrial function is affected.

B. Tier 2: Key Metabolic Profiling During Lead Development

Upon suspicion of a mitochondrial disease, based on clinical signs and symptoms and clinical chemistry findings, a more detailed biochemical diagnosis is requested. Here, a combination of conventional and complimentary techniques is used to assess several biochemical features associated with mitochondrial diseases. Such histopathological or biochemical analyses are often performed in muscle biopsies in specialized laboratories. Histopathological alterations include morphologic structural changes and altered enzyme-based stainings (e.g., cytochrome C oxidase, NADH reductase, succinic dehydrogenase). Biochemical measures most often include determination of ATP production and substrate oxidation rates, as well as analysis of the individual activities of the OXPHOS complexes (Rodenburg, 2011). Additionally, oxygen consumption and OXPHOS complex assembly can be determined as a follow-up strategy. These contribute to a robust insight into whether mitochondrial function is truly impaired. The aims are very similar to those of mitochondrial assessment during lead development (i.e., to confirm activity and help to identify the most potent compounds) (Hughes et al., 2011) by generating concentration-response curves and subsequent IC₅₀s (inhibitory concentration 50%) or minimal effect concentration. Such a rigorous assessment of mitochondrial function would be relevant for those compounds that have demonstrated a mitochondrial activity flag in Tier 1 but are still interesting drug candidates for further development by virtue of a favorable profile (e.g., high pharmacological potency for the primary target, efficacy in human-derived disease model assays, or good projected pharmacokinetic properties). Several methods to detect mitochondrial activity described earlier (e.g., mitochondrial membrane potential, ROS, oxygen consumption measurements using the Seahorse platform) could also be used to provide an initial understanding of the underlying mechanisms. Subsequently, more comprehensive techniques can be applied to further define mechanisms, including systems pharmacology approaches. Hereinto, we propose to follow the classic systems biology cycle (Fig. 3), starting with data collection. Which type of data to collect depends on the chosen systems pharmacology approach: network-based or structure-based. Data of metabolic networks can consist of transcriptomic, proteomic, or metabolomic data of cells exposed to a concentration of the candidate compound, which resulted in mitochondrial dysfunction in Tier 1 and 2 assays. Structure-based data includes X-ray protein structures, homology models derived from similar structures, or ligand-based pharmacophores. Subsequently, the various systems pharmacology approaches described previously can be applied to explore mitochondrial drug off-targets.

C. Tier 3: Mechanistic Studies During Lead Optimization

Upon biochemical diagnosis of a mitochondrial disorder, further insight into the disease etiology is provided by next-generation sequencing. The introduction of genetic screens, including whole exome sequencing, resulted in the association of more than 1,500 nuclear genes with mitochondrial diseases (Wallace et al., 1988; Goto et al., 1990; Lodi et al., 2000; Van Goethem et al., 2001; Winterthun et al., 2005; McCormick et al., 2013; Wortmann et al., 2015; Theunissen et al., 2018; Panneman et al., 2020). Various gene panels, based on suspected strength of a mitochondrial disease in Tier 1, are used (Wortmann et al., 2015). Panels cover variants known to directly disturb activity of the electron transport chain (van den Heuvel et al., 1998; Koopman et al., 2012; Nouws et al., 2012; Jonckheere et al., 2013; Hallmann et al., 2016), which is most evidently linked to mitochondrial dysfunction (DiMauro et al., 1999; Dimauro et al., 2004). Moreover, these panels include many other genes associated with mitochondrial diseases (Wortmann et al., 2015) encoding for mitochondrial carriers (e.g., SLC25A3, MPC1), proteins involved in mtDNA maintenance (e.g., POLG), mitochondrial fission and fusion (e.g., OPA1, MFN2), and mitochondrial phospholipid metabolism (e.g., SERAC1). In analogy to these steps in the diagnosis of mitochondrial disease, more detailed insights into causal molecular mechanisms underlying drug-induced mitochondrial dysfunction are required next. Applying a systems pharmacology approach at the end of Tier 2 would be a valuable starting point. To validate such etiologic relevance of an off-target for the observed mitochondrial activity, various cell biologic methods could be applied, including the use of a knockout or overexpression model of common mitochondrial off-targets generated preemptively using techniques such as CRISPR-Cas9 or using RNAi-mediated knockdown (i.e., siRNA, shRNA) and selected off-the-shelf as required. Ideally, such approaches are combined with high-content microscopic imaging to simultaneously investigate various mitochondrial and cellular parameters. To integrate these parameters, this can be combined with machine learning techniques, as described before, along with specific bespoke mechanism of action investigations driven by hypotheses derived from the machine learning output. Implications for mitochondrial function can be further validated in vivo in Tier 4, as described next.

D. Tier 4: Functional In Situ Studies Versus In Vivo Efficacy and Safety Studies

Once the genetic cause of a mitochondrial disorder is identified, deeper understanding of molecular and cellular pathogenesis can be obtained through mechanistic studies in patient-derived fibroblasts or even induced pluripotent stem cells. Moreover, these studies are essential to validate the etiologic role of the identified genetic polymorphisms or mutations. Besides the notion that these cells can be obtained less invasively via skin biopsy and have a proliferative capacity, they carry all patient-specific mutations. Although biologic properties at the cellular level are therefore preserved (Saada, 2011; Hu et al., 2019), potential tissue-specific differences in mtDNA heteroplasmy levels should be considered. A relevant addition is complementation studies, in which wild-type DNA of the suspected disease-causing mutated gene is introduced into these patient-derived cells by viral transduction or transient transfection (Kirby et al., 2004; Hoefs et al., 2008; Jonckheere et al., 2011; Koopman et al., 2016), followed by functional confirmation of pathogenicity using protein expression levels or enzymatic activity (Hoefs et al., 2008; Jonckheere et al., 2013; Koopman et al., 2016). A known pathogenesis will help in the identification and development of potential therapeutic targets. Although complementation studies are comparable to the cellular validation steps performed as part of the systems pharmacology design, clearly for compound development an in vivo validation is required. A validation step using a relevant animal model could also closely resemble the use of patient-derived cells as a model for the patient’s cellular response. To investigate whether the proposed approach to lead optimization indeed helped reduce the intrinsic mitochondrial toxicity hazard of the lead and that the mechanistic insights gained in vitro in Tier 3 have allowed the risk posed by any residual mitochondrial activity to be correctly assessed, one needs robust methodologies to measure mitochondrial function in vivo. In this respect some recently developed methods significantly enhance the capabilities to monitor in vivo mitochondrial function at the molecular level. Development of the MITO-Tag Mice, for example, enabled the rapid determination of mitochondrial metabolites in various tissues (Bayraktar et al., 2019). High-resolution Fourier-transform mass spectrometry on isolated mitochondria provides an alternative approach (Go et al., 2014). Application of the same hemagglutinin-tag–based rapid mitochondrial isolation technique has also been previously applied in animal and plant cells (Chen et al., 2016; Kuhnert et al., 2020), which also demonstrated its ability for enzymatic evaluation of OXPHOS complex activity. Even without the isolation of organelles, functional analysis of mitochondrial complexes in permeabilized muscle fibers, tissues, and cells has been demonstrated previously (Kuznetsov et al., 2008). In addition, injection of an exogenous probe, followed by its evaluation ex vivo, enabled the in vivo determination of superoxide, hydrogen sulfide, hydrogen peroxide, and the mitochondrial membrane potential (Cochemé et al., 2011; Logan et al., 2016; Arndt et al., 2017; Shchepinova et al., 2017). Other assays use genetically encoded fluorescent markers and two-photon imaging to measure in vivo ROS and ATP production (van Hameren et al., 2019). The latter could provide real-time imaging of these levels, and if costs are justified by results, the dedicated equipment required may not limit its use in drug development.

V. Concluding Remarks and Future Perspectives

Consciousness of potential mitochondrial off-target effects is key during design and development of new drugs. Implementation of systems pharmacology in the drug developmental process is expected to significantly enhance the detection and prevention of drug-induced mitochondrial dysfunction. The proposed tiered strategy aims to reduce drug-induced mitochondrial dysfunction before entering clinical drug development stages (see also Fig. 5) and follows a workflow similar to that applied in the clinical setting to detect inherited mitochondrial disorders.

The ultimate aim is to deploy systems pharmacology approaches early enough in compound development such that the chemistry of the lead molecules can be adjusted (e.g., compound structure) to remove or substantially diminish the intrinsic mitochondrial activity hazard, thereby negating or reducing the risk of later mitochondrial toxicity. An example of such an adaptive systems pharmacology method has been demonstrated by our group for the potential antiobesity drug ibipinabant (Schirris et al., 2015b). Using a structure-based approach, we demonstrated inhibition of mitochondrial ADP/ATP exchange as off-target mechanism explaining the observed muscle toxicity, which could be reversed upon minor chemical modification of ibipinabant. As the capabilities in each tier mature, supported by systems pharmacology, applied methods could be moved progressively earlier. Then in silico strategies like molecular docking and pharmacophore modeling could offer an appropriate starting point in drug design, with subsequent testing in enzymatic or cellular assays to evaluate the potential off-target effects of early compound leads as part of an iterative chemistry development effort.

We propose the implementation of systems pharmacology in early stages of drug development (e.g., lead development) to reduce drug-related adverse effects and to enable the early detection of molecules with mitochondrial liabilities, thereby minimizing the number of drug attritions in later development phases and improving patient safety.

Acknowledgments

This research was supported by a grant from the Radboud University Medical Center (RIMLS 017-010a).

Authorship Contributions

Participated in research design: Hoogstraten, Schirris.

Performed data analysis: Hoogstraten, Schirris.

Wrote or contributed to the writing of the manuscript: Hoogstraten, Lyon, Smeitink, Russel, Schirris.

Footnotes

Received January 10, 2022.
Accepted November 21, 2022.

This research was supported by a grant from the Radboud University Medical Center (RIMLS 017-010a).
F.G.M.R is coinventor on patent EP2010/066792 “Novel Conditionally Immortalized Human Proximal Tubule Cell Line Expressing Functional Influx and Efflux Transporters” assigned to Radboud University Medical Center, which has been licensed to Cell4Pharma. J.A.M.S. is the founding CEO of Khondrion BV, a Radboud University Medical Center spin-out company founded by J.A.M.S. J.J.L. is employed by GlaxoSmithKline; however, contents of this paper are reflective of personal opinions.
This work has not (yet) been presented.
dx.doi.org/10.1124/pharmrev.122.000568.

Abbreviations

AD: Alzheimer’s disease
AOP: adverse outcome pathway
ETC: electron transport chain
FA: fatty acid
KEGG: Kyoto Encyclopedia of Genes and Genomes
MFN: mitofusin
mPTP: mitochondrial permeability transition pore
mtDNA: mitochondrial DNA
OPA: optic atrophy
OXPHOS: oxidative phosphorylation
ROS: reactive oxygen species
TCA: tricarboxylic acid

This is an open access article distributed under the CC BY-NC Attribution 4.0 International license.

References

↵
1. Abdelwahid E
(2017) Mitochondrial dynamics regulate myocardial contractility and vice versa. Int J Cardiol 247:35.
OpenUrl
↵
1. AbdulHameed MDM,
2. Pannala VR, and
3. Wallqvist A
(2019) Mining public toxicogenomic data reveals insights and challenges in delineating liver steatosis adverse outcome pathways. Front Genet 10:1007.
OpenUrl
↵
1. Agren R,
2. Bordel S,
3. Mardinoglu A,
4. Pornputtapong N,
5. Nookaew I, and
6. Nielsen J
(2012) Reconstruction of genome-scale active metabolic networks for 69 human cell types and 16 cancer types using INIT. PLOS Comput Biol 8:e1002518.
OpenUrl CrossRef PubMed
1. Ahadpour M,
2. Eskandari MR,
3. Mashayekhi V,
4. Haj Mohammad Ebrahim Tehrani K,
5. Jafarian I,
6. Naserzadeh P, and
7. Hosseini MJ
(2016) Mitochondrial oxidative stress and dysfunction induced by isoniazid: study on isolated rat liver and brain mitochondria. Drug Chem Toxicol 39:224–232.
OpenUrl CrossRef
1. Aires CC,
2. Ijlst L,
3. Stet F,
4. Prip-Buus C,
5. de Almeida IT,
6. Duran M,
7. Wanders RJ, and
8. Silva MF
(2010) Inhibition of hepatic carnitine palmitoyl-transferase I (CPT IA) by valproyl-CoA as a possible mechanism of valproate-induced steatosis. Biochem Pharmacol 79:792–799.
OpenUrl CrossRef PubMed
↵
1. Alam MA and
2. Rahman MM
(2014) Mitochondrial dysfunction in obesity: potential benefit and mechanism of co-enzyme Q10 supplementation in metabolic syndrome. J Diabetes Metab Disord 13:60.
OpenUrl
↵
1. Albert R
(2007) Network inference, analysis, and modeling in systems biology. Plant Cell 19:3327–3338.
OpenUrl FREE Full Text
↵
1. Alexeyev M,
2. Shokolenko I,
3. Wilson G, and
4. LeDoux S
(2013) The maintenance of mitochondrial DNA integrity—critical analysis and update. Cold Spring Harb Perspect Biol 5:a012641.
OpenUrl Abstract/FREE Full Text
↵
1. Amacher DE
(2005) Drug-associated mitochondrial toxicity and its detection. Curr Med Chem 12:1829–1839.
OpenUrl CrossRef PubMed
↵
1. Amoedo ND,
2. Obre E, and
3. Rossignol R
(2017) Drug discovery strategies in the field of tumor energy metabolism: limitations by metabolic flexibility and metabolic resistance to chemotherapy. Biochim Biophys Acta Bioenerg 1858:674–685.
OpenUrl
↵
1. Arndt S,
2. Baeza-Garza CD,
3. Logan A,
4. Rosa T,
5. Wedmann R,
6. Prime TA,
7. Martin JL,
8. Saeb-Parsy K,
9. Krieg T,
10. Filipovic MR et al.
(2017) Assessment of H₂S in vivo using the newly developed mitochondria-targeted mass spectrometry probe MitoA. J Biol Chem 292:7761–7773.
OpenUrl Abstract/FREE Full Text
1. Atashbar S,
2. Jamali Z,
3. Khezri S, and
4. Salimi A
(2022) Celecoxib decreases mitochondrial complex IV activity and induces oxidative stress in isolated rat heart mitochondria: an analysis for its cardiotoxic adverse effect. J Biochem Mol Toxicol 36:e22934.
OpenUrl
↵
1. Babaei H,
2. Razmaraii N,
3. Assadnassab G,
4. Mohajjel Nayebi A,
5. Azarmi Y,
6. Mohammadnejad D, and
7. Azami A
(2020) Ultrastructural and echocardiographic assessment of chronic doxorubicin-induced cardiotoxicity in rats. Arch Razi Inst 75:55–62.
OpenUrl
↵
1. Bai JP and
2. Abernethy DR
(2013) Systems pharmacology to predict drug toxicity: integration across levels of biological organization. Annu Rev Pharmacol Toxicol 53:451–473.
OpenUrl CrossRef PubMed
1. Ball AL,
2. Kamalian L,
3. Alfirevic A,
4. Lyon JJ, and
5. Chadwick, AE
(2016) Identification of the additional mitochondrial liabilities of 2-hydroxyflutamide when compared with its parent compound, flutamide in HepG2 cells. Toxicol Sci 153:341–351.
OpenUrl CrossRef PubMed
↵
1. Bayraktar EC,
2. Baudrier L,
3. Özerdem C,
4. Lewis CA,
5. Chan SH,
6. Kunchok T,
7. Abu-Remaileh M,
8. Cangelosi AL,
9. Sabatini DM,
10. Birsoy K et al.
(2019) MITO-tag mice enable rapid isolation and multimodal profiling of mitochondria from specific cell types in vivo. Proc Natl Acad Sci USA 116:303–312.
OpenUrl Abstract/FREE Full Text
↵
1. Beeson CC,
2. Beeson GC, and
3. Schnellmann RG
(2010) A high-throughput respirometric assay for mitochondrial biogenesis and toxicity. Anal Biochem 404:75–81.
OpenUrl CrossRef PubMed
↵
1. Begriche K,
2. Massart J,
3. Robin MA,
4. Borgne-Sanchez A, and
5. Fromenty B
(2011) Drug-induced toxicity on mitochondria and lipid metabolism: mechanistic diversity and deleterious consequences for the liver. J Hepatol 54:773–794.
OpenUrl CrossRef PubMed
↵
1. Bellance N,
2. Furt F,
3. Melser S,
4. Lalou C,
5. Thoraval D,
6. Maneta-Peyret L,
7. Lacombe D,
8. Moreau P, and
9. Rossignol R
(2020) Doxorubicin inhibits phosphatidylserine decarboxylase and modifies mitochondrial membrane composition in HeLa cells. Int J Mol Sci 21:1317.
OpenUrl
↵
1. Belousov VV,
2. Fradkov AF,
3. Lukyanov KA,
4. Staroverov DB,
5. Shakhbazov KS,
6. Terskikh AV, and
7. Lukyanov S
(2006) Genetically encoded fluorescent indicator for intracellular hydrogen peroxide. Nat Methods 3:281–286.
OpenUrl CrossRef PubMed
1. Benzer F,
2. Kandemir FM,
3. Kucukler S,
4. Comaklı S, and
5. Caglayan C
(2018) Chemoprotective effects of curcumin on doxorubicin-induced nephrotoxicity in Wistar rats: by modulating inflammatory cytokines, apoptosis, oxidative stress and oxidative DNA damage. Arch Physiol Biochem 124:448–457.
OpenUrl
1. Bereiter-Hahn J and
2. Vöth M
(1994) Dynamics of mitochondria in living cells: shape changes, dislocations, fusion, and fission of mitochondria. Microsc Res Tech 27:198–219.
OpenUrl CrossRef PubMed
↵
1. Bisson WH,
2. Cheltsov AV,
3. Bruey-Sedano N,
4. Lin B,
5. Chen J,
6. Goldberger N,
7. May LT,
8. Christopoulos A,
9. Dalton JT,
10. Sexton PM et al.
(2007) Discovery of antiandrogen activity of nonsteroidal scaffolds of marketed drugs. Proc Natl Acad Sci USA 104:11927–11932.
OpenUrl Abstract/FREE Full Text
↵
1. Blanchet L,
2. Smeitink JA,
3. van Emst-de Vries SE,
4. Vogels C,
5. Pellegrini M,
6. Jonckheere AI,
7. Rodenburg RJ,
8. Buydens LM,
9. Beyrath J,
10. Willems PH et al.
(2015) Quantifying small molecule phenotypic effects using mitochondrial morpho-functional fingerprinting and machine learning. Sci Rep 5:8035.
OpenUrl CrossRef PubMed
1. Bloom MW,
2. Hamo CE,
3. Cardinale D,
4. Ky B,
5. Nohria A,
6. Baer L,
7. Skopicki H,
8. Lenihan DJ,
9. Gheorghiade M,
10. Lyon AR et al.
(2016) Cancer therapy-related cardiac dysfunction and heart failure: part 1: definitions, pathophysiology, risk factors, and imaging. Circ Heart Fail 9:e002661.
OpenUrl Abstract/FREE Full Text
↵
1. Bludau I and
2. Aebersold R
(2020) Proteomic and interactomic insights into the molecular basis of cell functional diversity. Nat Rev Mol Cell Biol 21:327–340.
OpenUrl CrossRef PubMed
↵
1. Boelsterli UA and
2. Lim PL
(2007) Mitochondrial abnormalities—a link to idiosyncratic drug hepatotoxicity? Toxicol Appl Pharmacol 220:92–107.
OpenUrl CrossRef PubMed
↵
1. Bogenhagen DF
(2012) Mitochondrial DNA nucleoid structure. Biochim Biophys Acta 1819:914–920.
OpenUrl CrossRef PubMed
1. Bolaji OKE
(2018) Dynamic modelling of mitochondrial metabolism. IFAC Papers Online 51:126–127.
OpenUrl
1. Bonte R,
2. Bongaerts M,
3. Demirdas S,
4. Langendonk JG,
5. Huidekoper HH,
6. Williams M,
7. Onkenhout W,
8. Jacobs EH,
9. Blom HJ, and
10. Ruijter GJG
(2019) Untargeted metabolomics-based screening method for inborn errors of metabolism using semi-automatic sample preparation with an UHPLC-Orbitrap-MS platform. Metabolites 9:289.
OpenUrl
↵
1. Bova MP,
2. Tam D,
3. McMahon G, and
4. Mattson MN
(2005) Troglitazone induces a rapid drop of mitochondrial membrane potential in liver HepG2 cells. Toxicol Lett 155:41–50.
OpenUrl CrossRef PubMed
1. Brandão SR,
2. Reis-Mendes A,
3. Domingues P,
4. Duarte JA,
5. Bastos ML,
6. Carvalho F,
7. Ferreira R, and
8. Costa VM
(2021) Exploring the aging effect of the anticancer drugs doxorubicin and mitoxantrone on cardiac mitochondrial proteome using a murine model. Toxicology 459:152852.
OpenUrl
1. Brandolini L,
2. Antonosante A,
3. Giorgio C,
4. Bagnasco M,
5. d’Angelo M,
6. Castelli V,
7. Benedetti E,
8. Cimini A, and
9. Allegretti M
(2020) NSAIDs-dependent adaption of the mitochondria-proteasome system in immortalized human cardiomyocytes. Sci Rep 10:18337.
OpenUrl
↵
1. Bridges HR,
2. Jones AJ,
3. Pollak MN, and
4. Hirst J
(2014) Effects of metformin and other biguanides on oxidative phosphorylation in mitochondria. Biochem J 462:475–487.
OpenUrl Abstract/FREE Full Text
1. Brinkman K and
2. Kakuda TN
(2000) Mitochondrial toxicity of nucleoside analogue reverse transcriptase inhibitors: a looming obstacle for long-term antiretroviral therapy? Curr Opin Infect Dis 13:5–11.
OpenUrl CrossRef PubMed
↵
1. Brinkman K,
2. ter Hofstede HJM,
3. Burger DM,
4. Smeitink JA, and
5. Koopmans PP
(1998) Adverse effects of reverse transcriptase inhibitors: mitochondrial toxicity as common pathway. AIDS 12:1735–1744.
OpenUrl CrossRef PubMed
↵
1. Brunk E,
2. Sahoo S,
3. Zielinski DC,
4. Altunkaya A,
5. Dräger A,
6. Mih N,
7. Gatto F,
8. Nilsson A,
9. Preciat Gonzalez GA,
10. Aurich MK et al.
(2018) Recon3D enables a three-dimensional view of gene variation in human metabolism. Nat Biotechnol 36:272–281.
OpenUrl CrossRef PubMed
↵
1. Buzkova J,
2. Nikkanen J,
3. Ahola S,
4. Hakonen AH,
5. Sevastianova K,
6. Hovinen T,
7. Yki-Järvinen H,
8. Pietiläinen KH,
9. Lönnqvist T,
10. Velagapudi V et al.
(2018) Metabolomes of mitochondrial diseases and inclusion body myositis patients: treatment targets and biomarkers. EMBO Mol Med 10:e9091.
OpenUrl Abstract/FREE Full Text
↵
1. Calvano SE,
2. Xiao W,
3. Richards DR,
4. Felciano RM,
5. Baker HV,
6. Cho RJ,
7. Chen RO,
8. Brownstein BH,
9. Cobb JP,
10. Tschoeke SK et al.
(2005) A network-based analysis of systemic inflammation in humans. Nature 437:1032–1037.
OpenUrl CrossRef PubMed
↵
1. Calvo SE,
2. Clauser KR, and
3. Mootha VK
(2016) MitoCarta2.0: an updated inventory of mammalian mitochondrial proteins. Nucleic Acids Res 44(D1):D1251–D1257.
OpenUrl CrossRef PubMed
↵
1. Campbell CT,
2. Kolesar JE, and
3. Kaufman BA
(2012) Mitochondrial transcription factor A regulates mitochondrial transcription initiation, DNA packaging, and genome copy number. Biochim Biophys Acta 1819:921–929.
OpenUrl CrossRef PubMed
↵
1. Canta A,
2. Pozzi E, and
3. Carozzi VA
(2015) Mitochondrial dysfunction in chemotherapy-induced peripheral neuropathy (CIPN). Toxics 3:198–223.
OpenUrl
↵
1. Chan K,
2. Truong D,
3. Shangari N, and
4. O’Brien PJ
(2005) Drug-induced mitochondrial toxicity. Expert Opin Drug Metab Toxicol 1:655–669.
OpenUrl CrossRef PubMed
↵
1. Chang RL,
2. Xie L,
3. Bourne PE, and
4. Palsson BO
(2013) Antibacterial mechanisms identified through structural systems pharmacology. BMC Syst Biol 7:102.
OpenUrl
↵
1. Chen H,
2. Vermulst M,
3. Wang YE,
4. Chomyn A,
5. Prolla TA,
6. McCaffery JM, and
7. Chan DC
(2010) Mitochondrial fusion is required for mtDNA stability in skeletal muscle and tolerance of mtDNA mutations. Cell 141:280–289.
OpenUrl CrossRef PubMed
1. Chen PI,
2. Cao A,
3. Miyagawa K,
4. Tojais NF,
5. Hennigs JK,
6. Li CG,
7. Sweeney NM,
8. Inglis AS,
9. Wang L,
10. Li D et al.
(2017a) Amphetamines promote mitochondrial dysfunction and DNA damage in pulmonary hypertension. JCI Insight 2:e90427.
OpenUrl
1. Chen Q,
2. Cui Y,
3. Ding G,
4. Jia Z,
5. Zhang Y,
6. Zhang A, and
7. Huang S
(2017b) PEA3 protects against gentamicin nephrotoxicity: role of mitochondrial dysfunction. Am J Transl Res 9:2153–2162.
OpenUrl
↵
1. Chen WW,
2. Freinkman E,
3. Wang T,
4. Birsoy K, and
5. Sabatini DM
(2016) Absolute quantification of matrix metabolites reveals the dynamics of mitochondrial metabolism. Cell 166:1324–1337.e11.
OpenUrl CrossRef PubMed
↵
1. Clish CB
(2015) Metabolomics: an emerging but powerful tool for precision medicine. Csh Mol Case Stud 1:a000588.
OpenUrl
↵
1. Cochemé HM,
2. Quin C,
3. McQuaker SJ,
4. Cabreiro F,
5. Logan A,
6. Prime TA,
7. Abakumova I,
8. Patel JV,
9. Fearnley IM,
10. James AM et al.
(2011) Measurement of H2O2 within living Drosophila during aging using a ratiometric mass spectrometry probe targeted to the mitochondrial matrix. Cell Metab 13:340–350.
OpenUrl CrossRef PubMed
1. Coe KJ,
2. Jia Y,
3. Ho HK,
4. Rademacher P,
5. Bammler TK,
6. Beyer RP,
7. Farin FM,
8. Woodke L,
9. Plymate SR,
10. Fausto N et al.
(2007) Comparison of the cytotoxicity of the nitroaromatic drug flutamide to its cyano analogue in the hepatocyte cell line TAMH: evidence for complex I inhibition and mitochondrial dysfunction using toxicogenomic screening. Chem Res Toxicol 20:1277–1290.
OpenUrl CrossRef PubMed
↵
1. Coene KLM,
2. Kluijtmans LAJ,
3. van der Heeft E,
4. Engelke UFH,
5. de Boer S,
6. Hoegen B,
7. Kwast HJT,
8. van de Vorst M,
9. Huigen MCDG,
10. Keularts IMLW et al.
(2018) Next-generation metabolic screening: targeted and untargeted metabolomics for the diagnosis of inborn errors of metabolism in individual patients. J Inherit Metab Dis 41:337–353.
OpenUrl
↵
1. Comte J,
2. Maïsterrena B, and
3. Gautheron DC
(1976) Lipid composition and protein profiles of outer and inner membranes from pig heart mitochondria. Comparison with microsomes. Biochim Biophys Acta 419:271–284.
OpenUrl CrossRef PubMed
↵
1. Console L,
2. Scalise M,
3. Giangregorio N,
4. Tonazzi A,
5. Barile M, and
6. Indiveri C
(2020) The link between the mitochondrial fatty acid oxidation derangement and kidney injury. Front Physiol 11:794.
OpenUrl CrossRef
↵
1. Cordes H,
2. Thiel C,
3. Baier V,
4. Blank LM, and
5. Kuepfer L
(2018) Integration of genome-scale metabolic networks into whole-body PBPK models shows phenotype-specific cases of drug-induced metabolic perturbation. NPJ Syst Biol Appl 4:10.
OpenUrl
↵
1. Cortassa S,
2. Aon MA, and
3. Sollott SJ
(2019) Control and regulation of substrate selection in cytoplasmic and mitochondrial catabolic networks. A systems biology analysis. Front Physiol 10:201.
OpenUrl
1. de Arriba G,
2. Calvino M,
3. Benito S, and
4. Parra T
(2013) Cyclosporine A-induced apoptosis in renal tubular cells is related to oxidative damage and mitochondrial fission. Toxicol Lett 218:30–38.
OpenUrl CrossRef PubMed
↵
1. de Wolf FA,
2. Staffhorst RW,
3. Smits HP,
4. Onwezen MF, and
5. de Kruijff B
(1993) Role of anionic phospholipids in the interaction of doxorubicin and plasma membrane vesicles: drug binding and structural consequences in bacterial systems. Biochemistry 32:6688–6695.
OpenUrl CrossRef PubMed
↵
1. DiMauro S,
2. Bonilla E, and
3. De Vivo DC
(1999) Does the patient have a mitochondrial encephalomyopathy? J Child Neurol 14(Suppl 1):S23–S35.
OpenUrl CrossRef PubMed
↵
1. Dimauro S,
2. Tay S, and
3. Mancuso M
(2004) Mitochondrial encephalomyopathies: diagnostic approach. Ann N Y Acad Sci 1011:217–231.
OpenUrl CrossRef PubMed
↵
1. Divakaruni AS,
2. Wiley SE,
3. Rogers GW,
4. Andreyev AY,
5. Petrosyan S,
6. Loviscach M,
7. Wall EA,
8. Yadava N,
9. Heuck AP,
10. Ferrick DA et al.
(2013) Thiazolidinediones are acute, specific inhibitors of the mitochondrial pyruvate carrier. Proc Natl Acad Sci USA 110:5422–5427.
OpenUrl Abstract/FREE Full Text
↵
1. Dolce V,
2. Fiermonte G,
3. Runswick MJ,
4. Palmieri F, and
5. Walker JE
(2001) The human mitochondrial deoxynucleotide carrier and its role in the toxicity of nucleoside antivirals. Proc Natl Acad Sci USA 98:2284–2288.
OpenUrl Abstract/FREE Full Text
↵
1. Du K,
2. Ramachandran A,
3. McGill MR,
4. Mansouri A,
5. Asselah T,
6. Farhood A,
7. Woolbright BL,
8. Ding WX, and
9. Jaeschke H
(2017) Induction of mitochondrial biogenesis protects against acetaminophen hepatotoxicity. Food Chem Toxicol 108(Pt A):339–350.
OpenUrl
↵
1. Düssmann H,
2. Perez-Alvarez S,
3. Anilkumar U,
4. Papkovsky DB, and
5. Prehn JH
(2017) Single-cell time-lapse imaging of intracellular O₂ in response to metabolic inhibition and mitochondrial cytochrome-c release. Cell Death Dis 8:e2853.
OpenUrl
1. Dykens J and
2. Will Y
(2008) Drug‐Induced Mitochondrial Dysfunction, John Wiley, Hoboken, NJ.
↵
1. Dykens J and
2. Will Y
(2018) Mitochondrial Dysfunction Caused by Drugs and Environmental Toxicants, John Wiley, Hoboken, NJ.
↵
1. Dykens JA,
2. Jamieson JD,
3. Marroquin LD,
4. Nadanaciva S,
5. Xu JJ,
6. Dunn MC,
7. Smith AR, and
8. Will Y
(2008) In vitro assessment of mitochondrial dysfunction and cytotoxicity of nefazodone, trazodone, and buspirone. Toxicol Sci 103:335–345.
OpenUrl CrossRef PubMed
↵
1. Dykens JA,
2. Marroquin LD, and
3. Will Y
(2007) Strategies to reduce late-stage drug attrition due to mitochondrial toxicity. Expert Rev Mol Diagn 7:161–175.
OpenUrl CrossRef PubMed
↵
1. Dykens JA and
2. Will Y
(2007) The significance of mitochondrial toxicity testing in drug development. Drug Discov Today 12:777–785.
OpenUrl CrossRef PubMed
↵
1. Dykens JA,
2. Wiseman RW, and
3. Hardin CD
(1996) Preservation of phosphagen kinase function during transient hypoxia via enzyme abundance or resistance to oxidative inactivation. J Comp Physiol B 166:359–368.
OpenUrl CrossRef PubMed
↵
1. El-Gharbawy A and
2. Vockley J
(2018) Inborn errors of metabolism with myopathy: defects of fatty acid oxidation and the carnitine shuttle system. Pediatr Clin North Am 65:317–335.
OpenUrl
1. Elimadi A,
2. Morin D,
3. Albengres E,
4. Chauvet-Monges AM,
5. Allain V,
6. Crevat A, and
7. Tillement JP
(1997) Differential effects of zidovudine and zidovudine triphosphate on mitochondrial permeability transition and oxidative phosphorylation. Br J Pharmacol 121:1295–1300.
OpenUrl
↵
1. Fannin RD,
2. Russo M,
3. O’Connell TM,
4. Gerrish K,
5. Winnike JH,
6. Macdonald J,
7. Newton J,
8. Malik S,
9. Sieber SO,
10. Parker J et al.
(2010) Acetaminophen dosing of humans results in blood transcriptome and metabolome changes consistent with impaired oxidative phosphorylation. Hepatology 51:227–236.
OpenUrl CrossRef PubMed
↵
1. Fasano M,
2. Monti C, and
3. Alberio T
(2016) A systems biology-led insight into the role of the proteome in neurodegenerative diseases. Expert Rev Proteomics 13:845–855.
OpenUrl
1. Fau D,
2. Eugene D,
3. Berson A,
4. Letteron P,
5. Fromenty B,
6. Fisch C, and
7. Pessayre D
(1994) Toxicity of the antiandrogen flutamide in isolated rat hepatocytes. J Pharmacol Exp Ther 269:954–962.
OpenUrl Abstract/FREE Full Text
↵
1. Ferreira LG,
2. Dos Santos RN,
3. Oliva G, and
4. Andricopulo AD
(2015) Molecular docking and structure-based drug design strategies. Molecules 20:13384–13421.
OpenUrl CrossRef
↵
1. Ferrick DA,
2. Neilson A, and
3. Beeson C
(2008) Advances in measuring cellular bioenergetics using extracellular flux. Drug Discov Today 13:268–274.
OpenUrl CrossRef PubMed
↵
1. Forkink M,
2. Smeitink JA,
3. Brock R,
4. Willems PH, and
5. Koopman WJ
(2010) Detection and manipulation of mitochondrial reactive oxygen species in mammalian cells. Biochim Biophys Acta 1797:1034–1044.
OpenUrl CrossRef PubMed
↵
1. Fosslien E
(2001) Mitochondrial medicine–molecular pathology of defective oxidative phosphorylation. Ann Clin Lab Sci 31:25–67.
OpenUrl Abstract/FREE Full Text
↵
1. Furberg CD and
2. Pitt B
(2001) Withdrawal of cerivastatin from the world market. Curr Control Trials Cardiovasc Med 2:205–207.
OpenUrl CrossRef PubMed
1. Gai Z,
2. Gui T,
3. Kullak-Ublick GA,
4. Li Y, and
5. Visentin M
(2020) The role of mitochondria in drug-induced kidney injury. Front Physiol 11:1079.
OpenUrl
↵
1. Galluzzi L,
2. Kepp O, and
3. Kroemer G
(2012a) Mitochondria: master regulators of danger signalling. Nat Rev Mol Cell Biol 13:780–788.
OpenUrl CrossRef PubMed
↵
1. Galluzzi L,
2. Kepp O,
3. Trojel-Hansen C, and
4. Kroemer G
(2012b) Mitochondrial control of cellular life, stress, and death. Circ Res 111:1198–1207.
OpenUrl Abstract/FREE Full Text
↵
1. Galluzzi L,
2. Kepp O,
3. Vander Heiden MG, and
4. Kroemer G
(2013) Metabolic targets for cancer therapy. Nat Rev Drug Discov 12:829–846.
OpenUrl CrossRef PubMed
1. Ghosh R,
2. Goswami SK,
3. Feitoza LFBB,
4. Hammock B, and
5. Gomes AV
(2016a) Diclofenac induces proteasome and mitochondrial dysfunction in murine cardiomyocytes and hearts. Int J Cardiol 223:923–935.
OpenUrl
1. Ghosh R,
2. Hwang SM,
3. Cui Z,
4. Gilda JE, and
5. Gomes AV
(2016b) Different effects of the nonsteroidal anti-inflammatory drugs meclofenamate sodium and naproxen sodium on proteasome activity in cardiac cells. J Mol Cell Cardiol 94:131–144.
OpenUrl
↵
1. Gilkerson R,
2. Bravo L,
3. Garcia I,
4. Gaytan N,
5. Herrera A,
6. Maldonado A, and
7. Quintanilla B
(2013) The mitochondrial nucleoid: integrating mitochondrial DNA into cellular homeostasis. Cold Spring Harb Perspect Biol 5:a011080.
OpenUrl Abstract/FREE Full Text
1. Gnanapragasam A,
2. Yogeeta S,
3. Subhashini R,
4. Ebenezar KK,
5. Sathish V, and
6. Devaki T
(2007) Adriamycin induced myocardial failure in rats: protective role of Centella asiatica. Mol Cell Biochem 294:55–63.
OpenUrl CrossRef PubMed
↵
1. Go YM,
2. Fernandes J,
3. Hu X,
4. Uppal K, and
5. Jones DP
(2018) Mitochondrial network responses in oxidative physiology and disease. Free Radic Biol Med 116:31–40.
OpenUrl
↵
1. Go YM,
2. Uppal K,
3. Walker DI,
4. Tran V,
5. Dury L,
6. Strobel FH,
7. Baubichon-Cortay H,
8. Pennell KD,
9. Roede JR, and
10. Jones DP
(2014) Mitochondrial metabolomics using high-resolution Fourier-transform mass spectrometry. Methods Mol Biol 1198:43–73.
OpenUrl CrossRef PubMed
↵
1. Goto Y,
2. Nonaka I, and
3. Horai S
(1990) A mutation in the tRNA(Leu)(UUR) gene associated with the MELAS subgroup of mitochondrial encephalomyopathies. Nature 348:651–653.
OpenUrl CrossRef PubMed
↵
1. Gottlieb RA and
2. Bernstein D
(2016) Mitochondrial remodeling: rearranging, recycling, and reprogramming. Cell Calcium 60:88–101.
OpenUrl CrossRef PubMed
↵
1. Grass M,
2. McDougal AD,
3. Blazeski A,
4. Kamm RD,
5. García-Cardeña G, and
6. Dewey Jr CF
(2022) A computational model of cardiomyocyte metabolism predicts unique reperfusion protocols capable of reducing cell damage during ischemia/reperfusion. J Biol Chem 298:101693.
OpenUrl
↵
1. Griffiths EJ
(2000) Mitochondria–potential role in cell life and death. Cardiovasc Res 46:24–27.
OpenUrl CrossRef PubMed
1. Gudbrandsen OA,
2. Rost TH, and
3. Berge RK
(2006) Causes and prevention of tamoxifen-induced accumulation of triacylglycerol in rat liver. J Lipid Res 47:2223–2232.
OpenUrl Abstract/FREE Full Text
1. Guven A,
2. Yavuz O,
3. Cam M,
4. Ercan F,
5. Bukan N, and
6. Comunoglu C
(2007) Melatonin protects against epirubicin-induced cardiotoxicity. Acta Histochem 109:52–60.
OpenUrl PubMed
↵
1. Haden DW,
2. Suliman HB,
3. Carraway MS,
4. Welty-Wolf KE,
5. Ali AS,
6. Shitara H,
7. Yonekawa H, and
8. Piantadosi CA
(2007) Mitochondrial biogenesis restores oxidative metabolism during Staphylococcus aureus sepsis. Am J Respir Crit Care Med 176:768–777.
OpenUrl CrossRef PubMed
1. Haegler, P.,
2. L. Joerin,
3. S. Krähenbühl, and
4. J. Bouitbir
(2017) Hepatocellular toxicity of imidazole and triazole antimycotic agents. Toxicol Sci 157:183–195.
OpenUrl CrossRef
↵
1. Hallmann K,
2. Kudin AP,
3. Zsurka G,
4. Kornblum C,
5. Reimann J,
6. Stüve B,
7. Waltz S,
8. Hattingen E,
9. Thiele H,
10. Nürnberg P et al.
(2016) Loss of the smallest subunit of cytochrome c oxidase, COX8A, causes Leigh-like syndrome and epilepsy. Brain 139:338–345.
OpenUrl CrossRef PubMed
↵
1. Hanawa N,
2. Shinohara M,
3. Saberi B,
4. Gaarde WA,
5. Han D, and
6. Kaplowitz N
(2008) Role of JNK translocation to mitochondria leading to inhibition of mitochondria bioenergetics in acetaminophen-induced liver injury. J Biol Chem 283:13565–13577.
OpenUrl Abstract/FREE Full Text
↵
1. Haney SA,
2. LaPan P,
3. Pan J, and
4. Zhang J
(2006) High-content screening moves to the front of the line. Drug Discov Today 11:889–894.
OpenUrl CrossRef PubMed
↵
1. Hargreaves IP,
2. Al Shahrani M,
3. Wainwright L, and
4. Heales SJ
(2016) Drug-induced mitochondrial toxicity. Drug Saf 39:661–674.
OpenUrl PubMed
↵
1. Hartman JH,
2. Miller GP, and
3. Meyer JN
(2017) Toxicological implications of mitochondrial localization of CYP2E1. Toxicol Res (Camb) 6:273–289.
OpenUrl
↵
1. Hartung T,
2. FitzGerald RE,
3. Jennings P,
4. Mirams GR,
5. Peitsch MC,
6. Rostami-Hodjegan A,
7. Shah I,
8. Wilks MF, and
9. Sturla SJ
(2017) Systems toxicology: real world applications and opportunities. Chem Res Toxicol 30:870–882.
OpenUrl CrossRef
1. He H,
2. Tao H,
3. Xiong H,
4. Duan SZ,
5. McGowan Jr FX,
6. Mortensen RM, and
7. Balschi JA
(2014) Rosiglitazone causes cardiotoxicity via peroxisome proliferator-activated receptor γ-independent mitochondrial oxidative stress in mouse hearts. Toxicol Sci 138:468–481.
OpenUrl CrossRef PubMed
↵
1. Hecker M and
2. LaLone CA
(2019) Adverse outcome pathways: moving from a scientific concept to an internationally accepted framework. Environ Toxicol Chem 38:1152–1163.
OpenUrl
↵
1. Heinrich JC,
2. Donakonda S,
3. Haupt VJ,
4. Lennig P,
5. Zhang Y, and
6. Schroeder M
(2016) New HSP27 inhibitors efficiently suppress drug resistance development in cancer cells. Oncotarget 7:68156–68169.
OpenUrl
↵
1. Heiske M,
2. Letellier T, and
3. Klipp E
(2017) Comprehensive mathematical model of oxidative phosphorylation valid for physiological and pathological conditions. FEBS J 284:2802–2828.
OpenUrl CrossRef
1. Hiller N,
2. Mirtschink P,
3. Merkel C,
4. Knels L,
5. Oertel R,
6. Christ T,
7. Deussen A,
8. Koch T, and
9. Stehr SN
(2013) Myocardial accumulation of bupivacaine and ropivacaine is associated with reversible effects on mitochondria and reduced myocardial function. Anesth Analg 116:83–92.
OpenUrl CrossRef PubMed
↵
1. Hoefs SJG,
2. Dieteren CEJ,
3. Distelmaier F,
4. Janssen RJRJ,
5. Epplen A,
6. Swarts HGP,
7. Forkink M,
8. Rodenburg RJ,
9. Nijtmans LG,
10. Willems PH et al.
(2008) NDUFA2 complex I mutation leads to Leigh disease. Am J Hum Genet 82:1306–1315.
OpenUrl CrossRef PubMed
↵
1. Hoegen B,
2. Zammit A,
3. Gerritsen A,
4. Engelke UFH,
5. Castelein S,
6. van de Vorst M,
7. Kluijtmans LAJ,
8. Huigen MCDG,
9. Wevers RA,
10. van Gool AJ et al.
(2021) Metabolomics-based screening of inborn errors of metabolism: enhancing clinical application with a robust computational pipeline. Metabolites 11:568.
OpenUrl
↵
1. Hoppel CL
(1982) Carnitine and carnitine palmitoyltransferase in fatty acid oxidation and ketosis. Fed Proc 41:2853–2857.
OpenUrl PubMed
↵
1. Hu J,
2. Ramshesh VK,
3. McGill MR,
4. Jaeschke H, and
5. Lemasters JJ
. (2016) Low dose acetaminophen induces reversible mitochondrial dysfunction associated with transient c-Jun N-terminal kinase activation in mouse liver. Toxicol Sci 150:204–215.
OpenUrl CrossRef PubMed
↵
1. Hu SY,
2. Zhuang QQ,
3. Qiu Y,
4. Zhu XF, and
5. Yan QF
(2019) Cell models and drug discovery for mitochondrial diseases. J Zhejiang Univ Sci B 20:449–456.
OpenUrl CrossRef
↵
1. Hu X,
2. Go YM, and
3. Jones DP
(2020) Omics integration for mitochondria systems biology. Antioxid Redox Signal 32:853–872.
OpenUrl
↵
1. Hu YS,
2. Xin J,
3. Hu Y,
4. Zhang L, and
5. Wang J
(2017) Analyzing the genes related to Alzheimer’s disease via a network and pathway-based approach. Alzheimers Res Ther 9:29.
OpenUrl CrossRef PubMed
↵
1. Huang R,
2. Grishagin I,
3. Wang Y,
4. Zhao T,
5. Greene J,
6. Obenauer JC,
7. Ngan D,
8. Nguyen DT,
9. Guha R,
10. Jadhav A et al.
(2019) The NCATS BioPlanet—an integrated platform for exploring the universe of cellular signaling pathways for toxicology, systems biology, and chemical genomics. Front Pharmacol 10:445.
OpenUrl
↵
1. Hughes JP,
2. Rees S,
3. Kalindjian SB, and
4. Philpott KL
(2011) Principles of early drug discovery. Br J Pharmacol 162:1239–1249.
OpenUrl CrossRef PubMed
↵
1. Hynes J,
2. Marroquin LD,
3. Ogurtsov VI,
4. Christiansen KN,
5. Stevens GJ,
6. Papkovsky DB, and
7. Will Y
(2006) Investigation of drug-induced mitochondrial toxicity using fluorescence-based oxygen-sensitive probes. Toxicol Sci 92:186–200.
OpenUrl CrossRef PubMed
↵
1. Hynes J,
2. Nadanaciva S,
3. Swiss R,
4. Carey C,
5. Kirwan S, and
6. Will Y
. (2013) A high-throughput dual parameter assay for assessing drug-induced mitochondrial dysfunction provides additional predictivity over two established mitochondrial toxicity assays. Toxicol In Vitro 27:560–569.
OpenUrl CrossRef PubMed
↵
1. Hynes J,
2. Natoli Jr E, and
3. Will Y
(2009) Fluorescent pH and oxygen probes of the assessment of mitochondrial toxicity in isolated mitochondria and whole cells. Curr Protoc Toxicol Chapter 2:Unit 2.16.
OpenUrl
↵
1. Iannetti EF,
2. Prigione A,
3. Smeitink JAM,
4. Koopman WJH,
5. Beyrath J, and
6. Renkema H
(2019) Live-imaging readouts and cell models for phenotypic profiling of mitochondrial function. Front Genet 10:131.
OpenUrl
↵
1. Iannetti EF,
2. Smeitink JA,
3. Beyrath J,
4. Willems PH, and
5. Koopman WJ
(2016) Multiplexed high-content analysis of mitochondrial morphofunction using live-cell microscopy. Nat Protoc 11:1693–1710.
OpenUrl CrossRef
1. Igoudjil A,
2. Begriche K,
3. Pessayre D, and
4. Fromenty B
(2006) Mitochondrial, metabolic and genotoxic effects of antiretroviral nucleoside reverse-transcriptase inhibitors. Antiinfect Agents Med Chem 5:273–292.
OpenUrl
↵
1. Jamil S,
2. Lam I,
3. Majd M,
4. Tsai SH, and
5. Duronio V
(2015) Etoposide induces cell death via mitochondrial-dependent actions of p53. Cancer Cell Int 15:79.
OpenUrl CrossRef
↵
1. Jonckheere AI,
2. Huigsloot M,
3. Lammens M,
4. Jansen J,
5. van den Heuvel LP,
6. Spiekerkoetter U,
7. von Kleist-Retzow JC,
8. Forkink M,
9. Koopman WJH,
10. Szklarczyk R et al.
(2011) Restoration of complex V deficiency caused by a novel deletion in the human TMEM70 gene normalizes mitochondrial morphology. Mitochondrion 11:954–963.
OpenUrl CrossRef PubMed
↵
1. <
2. >Jonckheere AI,
3. Renkema GH,
4. Bras M,
5. van den Heuvel LP,
6. Hoischen A,
7. Gilissen C,
8. Nabuurs SB,
9. Huynen MA,
10. de Vries MC,
11. Smeitink JAM et al.
(2013) A complex V ATP5A1 defect causes fatal neonatal mitochondrial encephalopathy. Brain 136:1544–1554.
OpenUrl CrossRef PubMed
1. Kalender S,
2. Kalender Y,
3. Ates A,
4. Yel M,
5. Olcay E, and
6. Candan S
(2002) Protective role of antioxidant vitamin E and catechin on idarubicin-induced cardiotoxicity in rats. Braz J Med Biol Res 35:1379–1387.
OpenUrl PubMed
↵
1. Kalghatgi S,
2. Spina CS,
3. Costello JC,
4. Liesa M,
5. Morones-Ramirez JR,
6. Slomovic S,
7. Molina A,
8. Shirihai OS, and
9. Collins JJ
(2013) Bactericidal antibiotics induce mitochondrial dysfunction and oxidative damage in mammalian cells. Sci Transl Med 5:192ra85.
OpenUrl Abstract/FREE Full Text
↵
1. Kalyanaraman B
(2011) Oxidative chemistry of fluorescent dyes: implications in the detection of reactive oxygen and nitrogen species. Biochem Soc Trans 39:1221–1225.
OpenUrl Abstract/FREE Full Text
↵
1. Kanehisa M
(1997) A database for post-genome analysis. Trends Genet 13:375–376.
OpenUrl CrossRef PubMed
↵
1. Karbowski M and
2. Youle RJ
(2003) Dynamics of mitochondrial morphology in healthy cells and during apoptosis. Cell Death Differ 10:870–880.
OpenUrl CrossRef PubMed
1. Karkhanis A,
2. Leow JWH,
3. Hagen T, and
4. Chan ECY
(2018) Dronedarone-induced cardiac mitochondrial dysfunction and its mitigation by epoxyeicosatrienoic acids. Toxicol Sci 163:79–91.
OpenUrl
↵
1. Kaufmann P,
2. Török M,
3. Zahno A,
4. Waldhauser KM,
5. Brecht K, and
6. Krähenbühl S
(2006) Toxicity of statins on rat skeletal muscle mitochondria. Cell Mol Life Sci 63:2415–2425.
OpenUrl CrossRef PubMed
↵
1. Keiser MJ,
2. Roth BL,
3. Armbruster BN,
4. Ernsberger P,
5. Irwin JJ, and
6. Shoichet BK
(2007) Relating protein pharmacology by ligand chemistry. Nat Biotechnol 25:197–206.
OpenUrl CrossRef PubMed
↵
1. Kheirandish M,
2. Mahboobi H,
3. Yazdanparast M,
4. Kamal W, and
5. Kamal MA
(2018) Anti-cancer effects of metformin: recent evidences for its role in prevention and treatment of cancer. Curr Drug Metab 19:793–797.
OpenUrl
1. Khezri S,
2. Atashbar S,
3. Azizian S,
4. Shaikhgermchi Z,
5. Kurdpour P, and
6. Salimi A
(2020) Calcitriol reduces adverse effects of diclofenac on mitochondrial function in isolated rat heart mitochondria. Drug Res (Stuttg) 70:317–324.
OpenUrl
↵
1. Kirby DM,
2. Salemi R,
3. Sugiana C,
4. Ohtake A,
5. Parry L,
6. Bell KM,
7. Kirk EP,
8. Boneh A,
9. Taylor RW,
10. Dahl HHM et al.
(2004) NDUFS6 mutations are a novel cause of lethal neonatal mitochondrial complex I deficiency. J Clin Invest 114:837–845.
OpenUrl CrossRef PubMed
↵
1. Klipp E,
2. Liebermeister W,
3. Wierling C,
4. Kowald A,
5. Lehrach H, and
6. Herwig R
(2009) Systems Biology: A Textbook, Wiley-Blackwell, Weinheim, Germany.
1. Kohler JJ,
2. Hosseini SH,
3. Hoying-Brandt A,
4. Green E,
5. Johnson DM,
6. Russ R,
7. Tran D,
8. Raper CM,
9. Santoianni R, and
10. Lewis W
(2009) Tenofovir renal toxicity targets mitochondria of renal proximal tubules. Lab Invest 89:513–519.
OpenUrl CrossRef PubMed
↵
1. Kon K,
2. Kim JS,
3. Jaeschke H, and
4. Lemasters JJ
(2004) Mitochondrial permeability transition in acetaminophen-induced necrosis and apoptosis of cultured mouse hepatocytes. Hepatology 40:1170–1179.
OpenUrl CrossRef PubMed
↵
1. Konc J and
2. Janezic D
(2012) ProBiS-2012: web server and web services for detection of structurally similar binding sites in proteins. Nucleic Acids Res 40:W214-21.
OpenUrl
↵
1. Kongsbak K,
2. Hadrup N,
3. Audouze K, and
4. Vinggaard AM
(2014) Applicability of computational systems biology in toxicology. Basic Clin Pharmacol Toxicol 115:45–49.
OpenUrl
↵
1. Koopman WJ,
2. Beyrath J,
3. Fung CW,
4. Koene S,
5. Rodenburg RJ,
6. Willems PH, and
7. Smeitink JA
(2016) Mitochondrial disorders in children: toward development of small-molecule treatment strategies. EMBO Mol Med 8:311–327.
OpenUrl Abstract/FREE Full Text
↵
1. Koopman WJH,
2. Willems PHGM, and
3. Smeitink JAM
(2012) Monogenic mitochondrial disorders. N Engl J Med 366:1132–1141.
OpenUrl CrossRef PubMed
↵
1. Korla K
(2016) Reactive oxygen species and energy machinery: an integrated dynamic model. J Biomol Struct Dyn 34:1625–1640.
OpenUrl
↵
1. Korla K and
2. Mitra CK
(2014) Kinetic modelling of mitochondrial translation. J Biomol Struct Dyn 32:1634–1650.
OpenUrl
↵
1. Korla K,
2. Vadlakonda L, and
3. Mitra CK
(2015) Kinetic simulation of malate-aspartate and citrate-pyruvate shuttles in association with Krebs cycle. J Biomol Struct Dyn 33:2390–2403.
OpenUrl
↵
1. Kristensen AR,
2. Gsponer J, and
3. Foster LJ
(2012) A high-throughput approach for measuring temporal changes in the interactome. Nat Methods 9:907–909.
OpenUrl CrossRef PubMed
↵
1. Kuhnert F,
2. Stefanski A,
3. Overbeck N,
4. Drews L,
5. Reichert AS,
6. Stühler K, and
7. Weber APM
(2020) Rapid single-step affinity purification of HA-tagged plant mitochondria. Plant Physiol 182:692–706.
OpenUrl Abstract/FREE Full Text
↵
1. Kuznetsov AV,
2. Margreiter R,
3. Amberger A,
4. Saks V, and
5. Grimm M
(2011) Changes in mitochondrial redox state, membrane potential and calcium precede mitochondrial dysfunction in doxorubicin-induced cell death. Biochim Biophys Acta 1813:1144–1152.
OpenUrl CrossRef PubMed
↵
1. Kuznetsov AV,
2. Veksler V,
3. Gellerich FN,
4. Saks V,
5. Margreiter R, and
6. Kunz WS
(2008) Analysis of mitochondrial function in situ in permeabilized muscle fibers, tissues and cells. Nat Protoc 3:965–976.
OpenUrl CrossRef PubMed
↵
1. Kwok M,
2. Lee C,
3. Li HS,
4. Deng R,
5. Tsoi C,
6. Ding Q,
7. Tsang SY,
8. Leung KT,
9. Yan BP, and
10. Poon EN
(2022) Remdesivir induces persistent mitochondrial and structural damage in human induced pluripotent stem cell-derived cardiomyocytes. Cardiovasc Res 118:2652–2664.
OpenUrl
↵
1. Kwon SH,
2. Ahn SH,
3. Kim YK,
4. Bae GU,
5. Yoon JW,
6. Hong S,
7. Lee HY,
8. Lee YW,
9. Lee HW, and
10. Han JW
(2002) Apicidin, a histone deacetylase inhibitor, induces apoptosis and Fas/Fas ligand expression in human acute promyelocytic leukemia cells. J Biol Chem 277:2073–2080.
OpenUrl Abstract/FREE Full Text
1. Lahoti TS,
2. Patel D,
3. Thekkemadom V,
4. Beckett R, and
5. Ray SD
(2012) Doxorubicin-induced in vivo nephrotoxicity involves oxidative stress-mediated multiple pro- and anti-apoptotic signaling pathways. Curr Neurovasc Res 9:282–295.
OpenUrl
↵
1. Lanzillotta C,
2. Di Domenico F,
3. Perluigi M, and
4. Butterfield DA
(2019) Targeting mitochondria in Alzheimer disease: rationale and perspectives. CNS Drugs 33:957–969.
OpenUrl
1. Larosche I,
2. Lettéron P,
3. Fromenty B,
4. Vadrot N,
5. Abbey-Toby A,
6. Feldmann G,
7. Pessayre D, and
8. Mansouri A
(2007) Tamoxifen inhibits topoisomerases, depletes mitochondrial DNA, and triggers steatosis in mouse liver. J Pharmacol Exp Ther 321:526–535.
OpenUrl Abstract/FREE Full Text
↵
1. Lebrecht D,
2. Kirschner J,
3. Geist A,
4. Haberstroh J, and
5. Walker UA
(2010) Respiratory chain deficiency precedes the disrupted calcium homeostasis in chronic doxorubicin cardiomyopathy. Cardiovasc Pathol 19:e167–e174.
OpenUrl CrossRef PubMed
↵
1. Lee YH,
2. Goh WW,
3. Ng CK,
4. Raida M,
5. Wong L,
6. Lin Q,
7. Boelsterli UA, and
8. Chung MC
(2013) Integrative toxicoproteomics implicates impaired mitochondrial glutathione import as an off-target effect of troglitazone. J Proteome Res 12:2933–2945.
OpenUrl CrossRef PubMed
1. Leite S,
2. Martins NM,
3. Dorta DJ,
4. Curti C,
5. Uyemura SA, and
6. dos Santos AC
(2006) Mitochondrial uncoupling by the sulindac metabolite, sulindac sulfide. Basic Clin Pharmacol Toxicol 99:294–299.
OpenUrl CrossRef PubMed
1. Lelliott CJ,
2. López M,
3. Curtis RK,
4. Parker N,
5. Laudes M,
6. Yeo G,
7. Jimenez-Liñan M,
8. Grosse J,
9. Saha AK,
10. Wiggins D et al.
(2005) Transcript and metabolite analysis of the effects of tamoxifen in rat liver reveals inhibition of fatty acid synthesis in the presence of hepatic steatosis. FASEB J 19:1108–1119.
OpenUrl CrossRef PubMed
↵
1. Leonard AP,
2. Cameron RB,
3. Speiser JL,
4. Wolf BJ,
5. Peterson YK,
6. Schnellmann RG,
7. Beeson CC, and
8. Rohrer B
(2015) Quantitative analysis of mitochondrial morphology and membrane potential in living cells using high-content imaging, machine learning, and morphological binning. Biochim Biophys Acta 1853:348–360.
OpenUrl CrossRef
↵
1. Leuthner TC and
2. Meyer JN
(2021) Mitochondrial DNA mutagenesis: feature of and biomarker for environmental exposures and aging. Curr Environ Health Rep 8:294–308.
OpenUrl
1. Lewis W,
2. Simpson JF, and
3. Meyer RR
(1994) Cardiac mitochondrial DNA polymerase-gamma is inhibited competitively and noncompetitively by phosphorylated zidovudine. Circ Res 74:344–348.
OpenUrl Abstract/FREE Full Text
↵
1. Li J,
2. Li Y,
3. Jiao J,
4. Wang J,
5. Li Y,
6. Qin D, and
7. Li P
(2014) Mitofusin 1 is negatively regulated by microRNA 140 in cardiomyocyte apoptosis. Mol Cell Biol 34:1788–1799.
OpenUrl Abstract/FREE Full Text
1. Li S,
2. Guo J,
3. Ying Z,
4. Chen S,
5. Yang L,
6. Chen K,
7. Long Q,
8. Qin D,
9. Pei D, and
10. Liu X
(2015) Valproic acid-induced hepatotoxicity in Alpers syndrome is associated with mitochondrial permeability transition pore opening-dependent apoptotic sensitivity in an induced pluripotent stem cell model. Hepatology 61:1730–1739.
OpenUrl
↵
1. Lin L,
2. Yee SW,
3. Kim RB, and
4. Giacomini KM
(2015) SLC transporters as therapeutic targets: emerging opportunities. Nat Rev Drug Discov 14:543–560.
OpenUrl
↵
1. Lin YT,
2. Lin KH,
3. Huang CJ, and
4. Wei AC
(2021) MitoTox: a comprehensive mitochondrial toxicity database. BMC Bioinformatics 22(Suppl 10):369.
OpenUrl
↵
1. Lodi R,
2. Montagna P,
3. Cortelli P,
4. Iotti S,
5. Cevoli S,
6. Carelli V, and
7. Barbiroli B
(2000) “Secondary” 4216/ND1 and 13708/ND5 Leber’s hereditary optic neuropathy mitochondrial DNA mutations do not further impair in vivo mitochondrial oxidative metabolism when associated with the 11778/ND4 mitochondrial DNA mutation. Brain 123:1896–1902.
OpenUrl CrossRef PubMed
↵
1. Logan A,
2. Pell VR,
3. Shaffer KJ,
4. Evans C,
5. Stanley NJ,
6. Robb EL,
7. Prime TA,
8. Chouchani ET,
9. Cochemé HM,
10. Fearnley IM et al.
(2016) Assessing the mitochondrial membrane potential in cells and in vivo using targeted click chemistry and mass spectrometry. Cell Metab 23:379–385.
OpenUrl CrossRef PubMed
1. Luo Z,
2. Zhong L,
3. Han X,
4. Wang H,
5. Zhong J, and
6. Xuan Z
(2009) Astragalus membranaceus prevents daunorubicin-induced apoptosis of cultured neonatal cardiomyocytes: role of free radical effect of Astragalus membranaceus on daunorubicin cardiotoxicity. Phytother Res 23:761–767.
OpenUrl CrossRef PubMed
↵
1. Ma H,
2. Sorokin A,
3. Mazein A,
4. Selkov A,
5. Selkov E,
6. Demin O, and
7. Goryanin I
(2007) The Edinburgh human metabolic network reconstruction and its functional analysis. Mol Syst Biol 3:135.
OpenUrl Abstract/FREE Full Text
↵
1. Madiraju AK,
2. Erion DM,
3. Rahimi Y,
4. Zhang XM,
5. Braddock DT,
6. Albright RA,
7. Prigaro BJ,
8. Wood JL,
9. Bhanot S,
10. MacDonald MJ et al.
(2014) Metformin suppresses gluconeogenesis by inhibiting mitochondrial glycerophosphate dehydrogenase. Nature 510:542–546.
OpenUrl CrossRef PubMed
↵
1. Maldonado EM,
2. Taha F,
3. Rahman J, and
4. Rahman S
(2019) Systems biology approaches toward understanding primary mitochondrial diseases. Front Genet 10:19.
OpenUrl
↵
1. Marín-Hernández Á,
2. Gallardo-Pérez JC,
3. Reyes-García MA,
4. Sosa-Garrocho M,
5. Macías-Silva M,
6. Rodríguez-Enríquez S,
7. Moreno-Sánchez R, and
8. Saavedra E
(2020) Kinetic modeling of glucose central metabolism in hepatocytes and hepatoma cells. Biochim Biophys Acta, Gen Subj 1864:129687.
OpenUrl
↵
1. Massart J,
2. Begriche K,
3. Buron N,
4. Porceddu M,
5. Borgne-Sanchez A, and
6. Fromenty B
(2013) Drug-induced inhibition of mitochondrial fatty acid oxidation and steatosis. Curr Pathobiol Rep 1:147–157.
OpenUrl
↵
1. Masubuchi Y,
2. Kano S, and
3. Horie T
(2006) Mitochondrial permeability transition as a potential determinant of hepatotoxicity of antidiabetic thiazolidinediones. Toxicology 222:233–239.
OpenUrl CrossRef PubMed
↵
1. McCormick E,
2. Place E, and
3. Falk MJ
(2013) Molecular genetic testing for mitochondrial disease: from one generation to the next. Neurotherapeutics 10:251–261.
OpenUrl CrossRef PubMed
↵
1. McGill MR,
2. Sharpe MR,
3. Williams CD,
4. Taha M,
5. Curry SC, and
6. Jaeschke H
(2012) The mechanism underlying acetaminophen-induced hepatotoxicity in humans and mice involves mitochondrial damage and nuclear DNA fragmentation. J Clin Invest 122:1574–1583.
OpenUrl CrossRef PubMed
↵
1. Megjhani M,
2. Correa de Sampaio P,
3. Leigh Carstens J,
4. Kalluri R, and
5. Roysam B
(2017) Morphologically constrained spectral unmixing by dictionary learning for multiplex fluorescence microscopy. Bioinformatics 33:2182–2190.
OpenUrl CrossRef
↵
1. Mestres J,
2. Gregori-Puigjané E,
3. Valverde S, and
4. Solé RV
(2008) Data completeness—the Achilles heel of drug-target networks. Nat Biotechnol 26:983–984.
OpenUrl CrossRef PubMed
↵
1. Meyer JN,
2. Hartman JH, and
3. Mello DF.
(2018) Mitochondrial toxicity. Toxicol Sci 162:15–23.
OpenUrl CrossRef
↵
1. Meyer JN,
2. Leung MC,
3. Rooney JP,
4. Sendoel A,
5. Hengartner MO,
6. Kisby GE, and
7. Bess AS
(2013) Mitochondria as a target of environmental toxicants. Toxicol Sci 134:1–17.
OpenUrl CrossRef PubMed
↵
1. Meyer JN,
2. Leuthner TC, and
3. Luz AL
(2017) Mitochondrial fusion, fission, and mitochondrial toxicity. Toxicology 391:42–53.
OpenUrl
1. Mihajlovic M and
2. Vinken M
(2022) Mitochondria as the target of hepatotoxicity and drug-induced liver injury: molecular mechanisms and detection methods. Int J Mol Sci 23:3315.
OpenUrl
↵
1. Miller MJ,
2. Kennedy AD,
3. Eckhart AD,
4. Burrage LC,
5. Wulff JE,
6. Miller LAD,
7. Milburn MV,
8. Ryals JA,
9. Beaudet AL,
10. Sun Q et al.
(2015) Untargeted metabolomic analysis for the clinical screening of inborn errors of metabolism. J Inherit Metab Dis 38:1029–1039.
OpenUrl CrossRef PubMed
1. Miller RP,
2. Tadagavadi RK,
3. Ramesh G, and
4. Reeves WB
(2010) Mechanisms of Cisplatin nephrotoxicity. Toxins (Basel) 2:2490–2518.
OpenUrl
↵
1. Mishra P and
2. Chan DC
(2016) Metabolic regulation of mitochondrial dynamics. J Cell Biol 212:379–387.
OpenUrl Abstract/FREE Full Text
↵
1. Mitra K,
2. Wunder C,
3. Roysam B,
4. Lin G, and
5. Lippincott-Schwartz J
(2009) A hyperfused mitochondrial state achieved at G1-S regulates cyclin E buildup and entry into S phase. Proc Natl Acad Sci USA 106:11960–11965.
OpenUrl Abstract/FREE Full Text
↵
1. Montaigne D,
2. Hurt C, and
3. Neviere R
(2012) Mitochondria death/survival signaling pathways in cardiotoxicity induced by anthracyclines and anticancer-targeted therapies. Biochem Res Int 2012:951539.
OpenUrl PubMed
1. Moreno-Sánchez R,
2. Bravo C,
3. Vásquez C,
4. Ayala G,
5. Silveira LH, and
6. Martínez-Lavín M
(1999) Inhibition and uncoupling of oxidative phosphorylation by nonsteroidal anti-inflammatory drugs: study in mitochondria, submitochondrial particles, cells, and whole heart. Biochem Pharmacol 57:743–752.
OpenUrl CrossRef PubMed
↵
1. Munnich A,
2. Rötig A,
3. Chretien D,
4. Cormier V,
5. Bourgeron T,
6. Bonnefont JP,
7. Saudubray JM, and
8. Rustin P
(1996) Clinical presentation of mitochondrial disorders in childhood. J Inherit Metab Dis 19:521–527.
OpenUrl CrossRef PubMed
↵
1. Murphy MP and
2. Hartley RC
(2018) Mitochondria as a therapeutic target for common pathologies. Nat Rev Drug Discov 17:865–886.
OpenUrl
↵
1. Nadanaciva S,
2. Bernal A,
3. Aggeler R,
4. Capaldi R, and
5. Will Y
(2007) Target identification of drug induced mitochondrial toxicity using immunocapture based OXPHOS activity assays. Toxicol In Vitro 21:902–911.
OpenUrl CrossRef PubMed
↵
1. Nadanaciva S and
2. Will Y
(2009) The role of mitochondrial dysfunction and drug safety. IDrugs 12:706–710.
OpenUrl PubMed
↵
1. Nemade H,
2. Chaudhari U,
3. Acharya A,
4. Hescheler J,
5. Hengstler JG,
6. Papadopoulos S, and
7. Sachinidis A
(2018) Cell death mechanisms of the anti-cancer drug etoposide on human cardiomyocytes isolated from pluripotent stem cells. Arch Toxicol 92:1507–1524.
OpenUrl
↵
1. Ng B,
2. White CC,
3. Klein HU,
4. Sieberts SK,
5. McCabe C,
6. Patrick E,
7. Xu J,
8. Yu L,
9. Gaiteri C,
10. Bennett DA et al.
(2017) An xQTL map integrates the genetic architecture of the human brain’s transcriptome and epigenome. Nat Neurosci 20:1418–1426.
OpenUrl CrossRef PubMed
↵
1. Ni HM,
2. Williams JA, and
3. Ding WX
(2015) Mitochondrial dynamics and mitochondrial quality control. Redox Biol 4:6–13.
OpenUrl
1. Nissim I,
2. Horyn O,
3. Daikhin Y,
4. Nissim I,
5. Luhovyy B,
6. Phillips PC, and
7. Yudkoff M
(2006) Ifosfamide-induced nephrotoxicity: mechanism and prevention. Cancer Res 66:7824–7831.
OpenUrl Abstract/FREE Full Text
↵
1. Niu M,
2. Hu J,
3. Wu S,
4. Xiaoe Z,
5. Xu H,
6. Zhang Y,
7. Zhang J, and
8. Yang Y
(2014) Structural bioinformatics-based identification of EGFR inhibitor gefitinib as a putative lead compound for BACE. Chem Biol Drug Des 83:81–88.
OpenUrl
↵
1. Nomura R,
2. Sato T,
3. Sato Y,
4. Medin JA,
5. Kushimoto S, and
6. Yanagisawa T
(2017) Azidothymidine-triphosphate impairs mitochondrial dynamics by disrupting the quality control system. Redox Biol 13:407–417.
OpenUrl
↵
1. Nouws J,
2. Nijtmans LGJ,
3. Smeitink JA, and
4. Vogel RO
(2012) Assembly factors as a new class of disease genes for mitochondrial complex I deficiency: cause, pathology and treatment options. Brain 135:12–22.
OpenUrl CrossRef PubMed
1. O’Brien EJ,
2. Monk JM, and
3. Palsson BO
(2015) Using genome-scale models to predict biological capabilities. Cell 161:971–987.
OpenUrl CrossRef PubMed
↵
1. Ogata H,
2. Goto S,
3. Sato K,
4. Fujibuchi W,
5. Bono H, and
6. Kanehisa M
(1999) KEGG: Kyoto Encyclopedia of Genes and Genomes. Nucleic Acids Res 27:29–34.
OpenUrl CrossRef PubMed
1. Olszewska A and
2. Szewczyk A
(2013) Mitochondria as a pharmacological target: magnum overview. IUBMB Life 65:273–281.
OpenUrl CrossRef PubMed
↵
1. Ong SE,
2. Schenone M,
3. Margolin AA,
4. Li X,
5. Do K,
6. Doud MK,
7. Mani DR,
8. Kuai L,
9. Wang X,
10. Wood JL et al.
(2009) Identifying the proteins to which small-molecule probes and drugs bind in cells. Proc Natl Acad Sci USA 106:4617–4622.
OpenUrl Abstract/FREE Full Text
↵
1. Orhan H,
2. Karakuş F, and
3. Ergüç A
(2021) Mitochondrial biotransformation of drugs and other xenobiotics. Curr Drug Metab 22:657–669.
OpenUrl
↵
1. Osataphan N,
2. Phrommintikul A,
3. Chattipakorn SC, and
4. Chattipakorn N
(2020) Effects of doxorubicin-induced cardiotoxicity on cardiac mitochondrial dynamics and mitochondrial function: insights for future interventions. J Cell Mol Med 24:6534–6557.
OpenUrl
↵
1. Owen MR,
2. Doran E, and
3. Halestrap AP
(2000) Evidence that metformin exerts its anti-diabetic effects through inhibition of complex 1 of the mitochondrial respiratory chain. Biochem J 348:607–614.
OpenUrl Abstract
1. Oz E,
2. Erbaş D,
3. Sürücü HS, and
4. Düzgün E
(2006) Prevention of doxorubicin-induced cardiotoxicity by melatonin. Mol Cell Biochem 282:31–37.
OpenUrl CrossRef PubMed
1. Paemanee A,
2. Sornjai W,
3. Kittisenachai S,
4. Sirinonthanawech N,
5. Roytrakul S,
6. Wongtrakul J, and
7. Smith DR
(2017) Nevirapine induced mitochondrial dysfunction in HepG2 cells. Sci Rep 7:9194.
OpenUrl CrossRef
↵
1. Panneman DM,
2. Wortmann SB,
3. Haaxma CA,
4. van Hasselt PM,
5. Wolf NI,
6. Hendriks Y,
7. Küsters B,
8. van Emst-de Vries S,
9. van de Westerlo E,
10. Koopman WJH et al.
(2020) Variants in NGLY1 lead to intellectual disability, myoclonus epilepsy, sensorimotor axonal polyneuropathy and mitochondrial dysfunction. Clin Genet 97:556–566.
OpenUrl
↵
1. Parker MA,
2. King V, and
3. Howard KP
(2001) Nuclear magnetic resonance study of doxorubicin binding to cardiolipin containing magnetically oriented phospholipid bilayers. Biochim Biophys Acta 1514:206–216.
OpenUrl CrossRef PubMed
↵
1. Patel CH,
2. Leone RD,
3. Horton MR, and
4. Powell JD
(2019) Targeting metabolism to regulate immune responses in autoimmunity and cancer. Nat Rev Drug Discov 18:669–688.
OpenUrl
↵
1. Pathak T and
2. Trebak M
(2018) Mitochondrial Ca²⁺ signaling. Pharmacol Ther 192:112–123.
OpenUrl CrossRef PubMed
↵
1. Payne BA,
2. Wilson IJ,
3. Hateley CA,
4. Horvath R,
5. Santibanez-Koref M,
6. Samuels DC,
7. Price DA, and
8. Chinnery PF
(2011) Mitochondrial aging is accelerated by anti-retroviral therapy through the clonal expansion of mtDNA mutations. Nat Genet 43:806–810.
OpenUrl CrossRef PubMed
↵
1. Pereira CV,
2. Moreira AC,
3. Pereira SP,
4. Machado NG,
5. Carvalho FS,
6. Sardão VA, and
7. Oliveira PJ
(2009) Investigating drug-induced mitochondrial toxicity: a biosensor to increase drug safety? Curr Drug Saf 4:34–54.
OpenUrl CrossRef PubMed
1. Pereira GC,
2. Pereira SP,
3. Tavares LC,
4. Carvalho FS,
5. Magalhães-Novais S,
6. Barbosa IA,
7. Santos MS,
8. Bjork J,
9. Moreno AJ,
10. Wallace KB et al.
(2016) Cardiac cytochrome c and cardiolipin depletion during anthracycline-induced chronic depression of mitochondrial function. Mitochondrion 30:95–104.
OpenUrl CrossRef PubMed
↵
1. Pessayre D,
2. Fromenty B,
3. Berson A,
4. Robin MA,
5. Lettéron P,
6. Moreau R, and
7. Mansouri A
(2012) Central role of mitochondria in drug-induced liver injury. Drug Metab Rev 44:34–87.
OpenUrl CrossRef PubMed
↵
1. Pu L,
2. Govindaraj RG,
3. Lemoine JM,
4. Wu HC, and
5. Brylinski M
(2019) DeepDrug3D: classification of ligand-binding pockets in proteins with a convolutional neural network. PLOS Comput Biol 15:e1006718.
OpenUrl
↵
1. Quintanilla RA,
2. Jin YN,
3. von Bernhardi R, and
4. Johnson GV
(2013) Mitochondrial permeability transition pore induces mitochondria injury in Huntington disease. Mol Neurodegener 8:45.
OpenUrl CrossRef PubMed
↵
1. Ramachandran A,
2. Umbaugh DS, and
3. Jaeschke H
(2021) Mitochondrial dynamics in drug-induced liver injury. MDPI: Livers 1:102–115.
OpenUrl
↵
1. Ramachandran A,
2. Visschers RGJ,
3. Duan L,
4. Akakpo JY, and
5. Jaeschke H
(2018) Mitochondrial dysfunction as a mechanism of drug-induced hepatotoxicity: current understanding and future perspectives. J Clin Transl Res 4:75–100.
OpenUrl
↵
1. Rana P,
2. Aleo MD,
3. Gosink M, and
4. Will Y
(2019) Evaluation of in vitro mitochondrial toxicity assays and physicochemical properties for prediction of organ toxicity using 228 pharmaceutical drugs. Chem Res Toxicol 32:156–167.
OpenUrl
↵
1. Rao VK,
2. Carlson EA, and
3. Yan SS
(2014) Mitochondrial permeability transition pore is a potential drug target for neurodegeneration. Biochim Biophys Acta 1842:1267–1272.
OpenUrl CrossRef PubMed
↵
1. Ren J,
2. Xie L,
3. Li WW, and
4. Bourne PE
(2010) SMAP-WS: a parallel web service for structural proteome-wide ligand-binding site comparison. Nucleic Acids Res 38:W441-4.
OpenUrl
↵
1. Riley JS and
2. Tait SW
(2020) Mitochondrial DNA in inflammation and immunity. EMBO Rep 21:e49799.
OpenUrl CrossRef PubMed
↵
1. Ritschel T,
2. Schirris TJ, and
3. Russel FG
(2014) KRIPO–a structure-based pharmacophores approach explains polypharmacological effects. J Cheminform 6(Suppl 1):O26.
OpenUrl
↵
1. Rodenburg RJ
(2011) Biochemical diagnosis of mitochondrial disorders. J Inherit Metab Dis 34:283–292.
OpenUrl CrossRef PubMed
1. Rodriguez RJ and
2. Acosta Jr D
(1996) Inhibition of mitochondrial function in isolated rate liver mitochondria by azole antifungals. J Biochem Toxicol 11:127–131.
OpenUrl CrossRef PubMed
↵
1. Rolland T,
2. Taşan M,
3. Charloteaux B,
4. Pevzner SJ,
5. Zhong Q,
6. Sahni N,
7. Yi S,
8. Lemmens I,
9. Fontanillo C,
10. Mosca R et al.
(2014) A proteome-scale map of the human interactome network. Cell 159:1212–1226.
OpenUrl CrossRef PubMed
↵
1. Rolo AP,
2. Palmeira CM,
3. Holy JM, and
4. Wallace KB
(2004) Role of mitochondrial dysfunction in combined bile acid-induced cytotoxicity: the switch between apoptosis and necrosis. Toxicol Sci 79:196–204.
OpenUrl CrossRef PubMed
↵
1. Roth KG,
2. Mambetsariev I,
3. Kulkarni P, and
4. Salgia R
(2020) The mitochondrion as an emerging therapeutic target in cancer. Trends Mol Med 26:119–134.
OpenUrl CrossRef PubMed
↵
1. Rowland Adams J and
2. Stefanovska A
(2021) Modeling cell energy metabolism as weighted networks of non-autonomous oscillators. Front Physiol 11:613183.
OpenUrl
↵
1. Saada A
(2011) The use of individual patient’s fibroblasts in the search for personalized treatment of nuclear encoded OXPHOS diseases. Mol Genet Metab 104:39–47.
OpenUrl CrossRef PubMed
↵
1. Salentin S,
2. Haupt VJ,
3. Daminelli S, and
4. Schroeder M
(2014) Polypharmacology rescored: protein-ligand interaction profiles for remote binding site similarity assessment. Prog Biophys Mol Biol 116:174–186.
OpenUrl CrossRef PubMed
↵
1. Salimi A,
2. Gholamifar E,
3. Naserzadeh P,
4. Hosseini MJ, and
5. Pourahmad J
(2017) Toxicity of lithium on isolated heart mitochondria and cardiomyocyte: a justification for its cardiotoxic adverse effect. J Biochem Mol Toxicol 31:21836.
OpenUrl
1. Salimi A,
2. Neshat MR,
3. Naserzadeh P, and
4. Pourahmad J
(2019) Mitochondrial permeability transition pore sealing agents and antioxidants protect oxidative stress and mitochondrial dysfunction induced by naproxen, diclofenac and celecoxib. Drug Res (Stuttg) 69:598–605.
OpenUrl
1. Santos NA,
2. Catão CS,
3. Martins NM,
4. Curti C,
5. Bianchi ML, and
6. Santos AC
(2007) Cisplatin-induced nephrotoxicity is associated with oxidative stress, redox state unbalance, impairment of energetic metabolism and apoptosis in rat kidney mitochondria. Arch Toxicol 81:495–504.
OpenUrl CrossRef PubMed
1. Satapathy SK,
2. Kuwajima V,
3. Nadelson J,
4. Atiq O, and
5. Sanyal AJ
(2015) Drug-induced fatty liver disease: an overview of pathogenesis and management. Ann Hepatol 14:789–806.
OpenUrl
↵
1. Schenone M,
2. Dančík V,
3. Wagner BK, and
4. Clemons PA
(2013) Target identification and mechanism of action in chemical biology and drug discovery. Nat Chem Biol 9:232–240.
OpenUrl CrossRef PubMed
↵
1. Schirris TJ,
2. Renkema GH,
3. Ritschel T,
4. Voermans NC,
5. Bilos A,
6. van Engelen BG,
7. Brandt U,
8. Koopman WJ,
9. Beyrath JD,
10. Rodenburg RJ et al.
(2015a) Statin-induced myopathy is associated with mitochondrial complex III inhibition. Cell Metab 22:399–407.
OpenUrl CrossRef PubMed
↵
1. Schirris TJ,
2. Ritschel T,
3. Herma Renkema G,
4. Willems PH,
5. Smeitink JA, and
6. Russel FG
(2015b) Mitochondrial ADP/ATP exchange inhibition: a novel off-target mechanism underlying ibipinabant-induced myotoxicity. Sci Rep 5:14533.
OpenUrl
1. Scruggs ER and
2. Dirks Naylor AJ
(2008) Mechanisms of zidovudine-induced mitochondrial toxicity and myopathy. Pharmacology 82:83–88.
OpenUrl CrossRef PubMed
↵
1. Seachrist JL,
2. Loi CM,
3. Evans MG,
4. Criswell KA, and
5. Rothwell CE
(2005) Roles of exercise and pharmacokinetics in cerivastatin-induced skeletal muscle toxicity. Toxicol Sci 88:551–561.
OpenUrl CrossRef PubMed
↵
1. Segawa M,
2. Sekine S,
3. Sato T, and
4. Ito K
(2018) Increased susceptibility to troglitazone-induced mitochondrial permeability transition in type 2 diabetes mellitus model rat. J Toxicol Sci 43:339–351.
OpenUrl
↵
1. Seo JB,
2. Riopel M,
3. Cabrales P,
4. Huh JY,
5. Bandyopadhyay GK,
6. Andreyev AY,
7. Murphy AN,
8. Beeman SC,
9. Smith GI,
10. Klein S et al.
(2019) Knockdown of ANT2 reduces adipocyte hypoxia and improves insulin resistance in obesity. Nat Metab 1:86–97.
OpenUrl
1. Seydi E,
2. Servati T,
3. Samiei F,
4. Naserzadeh P, and
5. Pourahmad J
(2020) Toxicity of pioglitazone on mitochondria isolated from brain and heart: an analysis for probable drug-induced neurotoxicity and cardiotoxicity. Drug Res (Stuttg) 70:112–118.
OpenUrl
↵
1. Shannon CE,
2. Ragavan M,
3. Palavicini JP,
4. Fourcaudot M,
5. Bakewell TM,
6. Valdez IA,
7. Ayala I,
8. Jin ES,
9. Madesh M,
10. Han X et al.
(2021) Insulin resistance is mechanistically linked to hepatic mitochondrial remodeling in non-alcoholic fatty liver disease. Mol Metab 45:101154.
OpenUrl
↵
1. Sharma H,
2. Singh A,
3. Sharma C,
4. Jain SK, and
5. Singh N
(2005) Mutations in the mitochondrial DNA D-loop region are frequent in cervical cancer. Cancer Cell Int 5:34.
OpenUrl PubMed
↵
1. Sharma N,
2. Pasala MS, and
3. Prakash A
(2019) Mitochondrial DNA: epigenetics and environment. Environ Mol Mutagen 60:668–682.
OpenUrl CrossRef PubMed
↵
1. Shchepinova MM,
2. Cairns AG,
3. Prime TA,
4. Logan A,
5. James AM,
6. Hall AR,
7. Vidoni S,
8. Arndt S,
9. Caldwell ST,
10. Prag HA et al.
(2017) MitoNeoD: a mitochondria-targeted superoxide probe. Cell Chem Biol 24:1285–1298.e12.
OpenUrl
↵
1. Shi W,
2. Lemoine JM,
3. Shawky AA,
4. Singha M,
5. Pu L,
6. Yang S,
7. Ramanujam J, and
8. Brylinski M
(2020) BionoiNet: ligand-binding site classification with off-the-shelf deep neural network. Bioinformatics 36:3077–3083.
OpenUrl
↵
1. Sidarala V,
2. Zhu J,
3. Levi-D’Ancona E,
4. Pearson GL,
5. Reck EC,
6. Walker EM,
7. Kaufman BA, and
8. Soleimanpour SA
(2022) Mitofusin 1 and 2 regulation of mitochondrial DNA content is a critical determinant of glucose homeostasis. Nat Commun 13:2340.
OpenUrl CrossRef
1. Silva MF,
2. Aires CC,
3. Luis PB,
4. Ruiter JP,
5. IJIst L,
6. Duran M,
7. Wanders RJ, and
8. Tavares de Almeida I
(2008) Valproic acid metabolism and its effects on mitochondrial fatty acid oxidation: a review. J Inherit Metab Dis 31:205–216.
OpenUrl CrossRef PubMed
↵
1. Silva Ramos E,
2. Motori E,
3. Brüser C,
4. Kühl I,
5. Yeroslaviz A,
6. Ruzzenente B,
7. Kauppila JHK,
8. Busch JD,
9. Hultenby K,
10. Habermann BH et al.
(2019) Mitochondrial fusion is required for regulation of mitochondrial DNA replication. PLoS Genet 15:e1008085.
OpenUrl CrossRef
↵
1. Sivitz WI and
2. Yorek MA
(2010) Mitochondrial dysfunction in diabetes: from molecular mechanisms to functional significance and therapeutic opportunities. Antioxid Redox Signal 12:537–577.
OpenUrl CrossRef PubMed
↵
1. Smith AJ,
2. Hancock MK,
3. Bi K,
4. Andrews J,
5. Harrison P, and
6. Vaughan TJ
(2012) Feasibility of implementing cell-based pathway reporter assays in early high-throughput screening assay cascades for antibody drug discovery. J Biomol Screen 17:713–726.
OpenUrl CrossRef PubMed
↵
1. Soler-López M,
2. Zanzoni A,
3. Lluís R,
4. Stelzl U, and
5. Aloy P
(2011) Interactome mapping suggests new mechanistic details underlying Alzheimer’s disease. Genome Res 21:364–376.
OpenUrl Abstract/FREE Full Text
↵
1. Sun BB,
2. Maranville JC,
3. Peters JE,
4. Stacey D,
5. Staley JR,
6. Blackshaw J,
7. Burgess S,
8. Jiang T,
9. Paige E,
10. Surendran P et al.
(2018) Genomic atlas of the human plasma proteome. Nature 558:73–79.
OpenUrl CrossRef PubMed
↵
1. Suomalainen A,
2. Elo JM,
3. Pietiläinen KH,
4. Hakonen AH,
5. Sevastianova K,
6. Korpela M,
7. Isohanni P,
8. Marjavaara SK,
9. Tyni T,
10. Kiuru-Enari S et al.
(2011) FGF-21 as a biomarker for muscle-manifesting mitochondrial respiratory chain deficiencies: a diagnostic study. Lancet Neurol 10:806–818.
OpenUrl CrossRef PubMed
↵
1. Swain SM,
2. Whaley FS, and
3. Ewer MS
(2003) Congestive heart failure in patients treated with doxorubicin: a retrospective analysis of three trials. Cancer 97:2869–2879.
OpenUrl CrossRef PubMed
↵
1. Tang H,
2. Tao A,
3. Song J,
4. Liu Q,
5. Wang H, and
6. Rui T
(2017) Doxorubicin-induced cardiomyocyte apoptosis: role of mitofusin 2. Int J Biochem Cell Biol 88:55–59.
OpenUrl
↵
1. Tang X,
2. Wang Z,
3. Hu S, and
4. Zhou B
(2022) Assessing drug-induced mitochondrial toxicity in cardiomyocytes: implications for preclinical cardiac safety evaluation. Pharmaceutics 14:1313.
OpenUrl
↵
1. Tebani A,
2. Abily-Donval L,
3. Afonso C,
4. Marret S, and
5. Bekri S
(2016a) Clinical metabolomics: the new metabolic window for inborn errors of metabolism investigations in the post-genomic era. Int J Mol Sci 17:1167.
OpenUrl
↵
1. Tebani A,
2. Afonso C,
3. Marret S, and
4. Bekri S
(2016b) Omics-based strategies in precision medicine: toward a paradigm shift in inborn errors of metabolism investigations. Int J Mol Sci 17:1555.
OpenUrl
↵
1. Teusink B,
2. Passarge J,
3. Reijenga CA,
4. Esgalhado E,
5. van der Weijden CC,
6. Schepper M,
7. Walsh MC,
8. Bakker BM,
9. van Dam K,
10. Westerhoff HV et al.
(2000) Can yeast glycolysis be understood in terms of in vitro kinetics of the constituent enzymes? Testing biochemistry. Eur J Biochem 267:5313–5329.b
OpenUrl CrossRef PubMed
1. Thai PN,
2. Ren L,
3. Xu W,
4. Overton J,
5. Timofeyev V,
6. Nader CE,
7. Haddad M,
8. Yang J,
9. Gomes AV,
10. Hammock BD et al.
(2021) Chronic diclofenac exposure increases mitochondrial oxidative stress, inflammatory mediators, and cardiac dysfunction. Cardiovasc Drugs Ther. DOI:10.1007/s10557-021-07253-4 [published ahead of print].
↵
1. Thakur S,
2. Daley B,
3. Gaskins K,
4. Vasko VV,
5. Boufraqech M,
6. Patel D,
7. Sourbier C,
8. Reece J,
9. Cheng SY,
10. Kebebew E,
11. Agarwal S, and
12. Klubo-Gwiezdzinska J
(2018) Metformin targets mitochondrial glycerophosphate dehydrogenase to control rate of oxidative phosphorylation and growth of thyroid cancer in vitro and in vivo. Clin Cancer 24:4030–4043.
OpenUrl
↵
1. Theunissen TEJ,
2. Nguyen M,
3. Kamps R,
4. Hendrickx AT,
5. Sallevelt SCEH,
6. Gottschalk RWH,
7. Calis CM,
8. Stassen APM,
9. de Koning B,
10. Mulder-Den Hartog ENM et al.
(2018) Whole exome sequencing is the preferred strategy to identify the genetic defect in patients with a probable or possible mitochondrial cause. Front Genet 9:400.
OpenUrl CrossRef PubMed
↵
1. Thiele I,
2. Swainston N,
3. Fleming RM,
4. Hoppe A,
5. Sahoo S,
6. Aurich MK,
7. Haraldsdottir H,
8. Mo ML,
9. Rolfsson O,
10. Stobbe MD et al.
(2013) A community-driven global reconstruction of human metabolism. Nat Biotechnol 31:419–425.
OpenUrl CrossRef PubMed
↵
1. Thistlethwaite LR,
2. Li XQ,
3. Burrage LC,
4. Riehle K,
5. Hacia JG,
6. Braverman N,
7. Wangler MF,
8. Miller MJ,
9. Elsea SH, and
10. Milosavljevic A
(2022) Clinical diagnosis of metabolic disorders using untargeted metabolomic profiling and disease-specific networks learned from profiling data. Sci Rep 12:6556.
OpenUrl
↵
1. Tiku V,
2. Tan MW, and
3. Dikic I
(2020) Mitochondrial functions in infection and immunity. Trends Cell Biol 30:263–275.
OpenUrl CrossRef PubMed
↵
1. Tilokani L,
2. Nagashima S,
3. Paupe V, and
4. Prudent J
(2018) Mitochondrial dynamics: overview of molecular mechanisms. Essays Biochem 62:341–360.
OpenUrl Abstract/FREE Full Text
↵
1. Tirmenstein MA,
2. Hu CX,
3. Gales TL,
4. Maleeff BE,
5. Narayanan PK,
6. Kurali E,
7. Hart TK,
8. Thomas HC, and
9. Schwartz LW
(2002) Effects of troglitazone on HepG2 viability and mitochondrial function. Toxicol Sci –131–138.
↵
1. Totten SP,
2. Im YK,
3. Cepeda Cañedo E,
4. Najyb O,
5. Nguyen A,
6. Hébert S,
7. Ahn R,
8. Lewis K,
9. Lebeau B,
10. La Selva R et al.
(2021) STAT1 potentiates oxidative stress revealing a targetable vulnerability that increases phenformin efficacy in breast cancer. Nat Commun 12:3299.
OpenUrl
1. Tuquet C,
2. Dupont J,
3. Mesneau A, and
4. Roussaux J
(2000) Effects of tamoxifen on the electron transport chain of isolated rat liver mitochondria. Cell Biol Toxicol 16:207–219.
OpenUrl CrossRef PubMed
↵
1. Turner RM,
2. Park BK, and
3. Pirmohamed M
(2015) Parsing interindividual drug variability: an emerging role for systems pharmacology. Wiley Interdiscip Rev Syst Biol Med 7:221–241.
OpenUrl PubMed
↵
1. Umbaugh DS,
2. Nguyen NT,
3. Jaeschke H, and
4. Ramachandran A
(2021) Mitochondrial membrane potential drives early change in mitochondrial morphology after acetaminophen exposure. Toxicol Sci –186–195.
↵
1. Unsay JD,
2. Cosentino K,
3. Subburaj Y, and
4. García-Sáez AJ
(2013) Cardiolipin effects on membrane structure and dynamics. Langmuir 29:15878–15887.
OpenUrl CrossRef PubMed
↵
1. Uppal K,
2. Ma C,
3. Go YM,
4. Jones DP, and
5. Wren J
(2018) xMWAS: a data-driven integration and differential network analysis tool. Bioinformatics 34:701–702.
OpenUrl PubMed
1. Uyemura SA,
2. Santos AC,
3. Mingatto FE,
4. Jordani MC, and
5. Curti C
(1997) Diclofenac sodium and mefenamic acid: potent inducers of the membrane permeability transition in renal cortex mitochondria. Arch Biochem Biophys 342:231–235.
OpenUrl CrossRef PubMed
↵
1. Valko M,
2. Leibfritz D,
3. Moncol J,
4. Cronin MT,
5. Mazur M, and
6. Telser J
(2007) Free radicals and antioxidants in normal physiological functions and human disease. Int J Biochem Cell Biol 39:44–84.
OpenUrl CrossRef PubMed
↵
1. Valm AM,
2. Oldenbourg R, and
3. Borisy GG
(2016) Multiplexed spectral imaging of 120 different fluorescent labels. PLoS One 11:e0158495.
OpenUrl CrossRef
↵
1. van den Heuvel L,
2. Ruitenbeek W,
3. Smeets R,
4. Gelman-Kohan Z,
5. Elpeleg O,
6. Loeffen J,
7. Trijbels F,
8. Mariman E,
9. de Bruijn D, and
10. Smeitink J
(1998) Demonstration of a new pathogenic mutation in human complex I deficiency: a 5-bp duplication in the nuclear gene encoding the 18-kD (AQDQ) subunit. Am J Hum Genet 62:262–268.
OpenUrl CrossRef PubMed
↵
1. van der Stel W,
2. Carta G,
3. Eakins J,
4. Darici

[1] ↵
Abdelwahid E
(2017) Mitochondrial dynamics regulate myocardial contractility and vice versa. Int J Cardiol 247:35.
OpenUrl

[2] Abdelwahid E

[3] ↵
AbdulHameed MDM,
Pannala VR, and
Wallqvist A
(2019) Mining public toxicogenomic data reveals insights and challenges in delineating liver steatosis adverse outcome pathways. Front Genet 10:1007.
OpenUrl

[4] AbdulHameed MDM,

[5] Pannala VR, and

[6] Wallqvist A

[7] ↵
Agren R,
Bordel S,
Mardinoglu A,
Pornputtapong N,
Nookaew I, and
Nielsen J
(2012) Reconstruction of genome-scale active metabolic networks for 69 human cell types and 16 cancer types using INIT. PLOS Comput Biol 8:e1002518.
OpenUrl CrossRef PubMed

[8] Agren R,

[9] Bordel S,

[10] Mardinoglu A,

[11] Pornputtapong N,

[12] Nookaew I, and

[13] Nielsen J

[14] Ahadpour M,
Eskandari MR,
Mashayekhi V,
Haj Mohammad Ebrahim Tehrani K,
Jafarian I,
Naserzadeh P, and
Hosseini MJ
(2016) Mitochondrial oxidative stress and dysfunction induced by isoniazid: study on isolated rat liver and brain mitochondria. Drug Chem Toxicol 39:224–232.
OpenUrl CrossRef

[15] Ahadpour M,

[16] Eskandari MR,

[17] Mashayekhi V,

[18] Haj Mohammad Ebrahim Tehrani K,

[19] Jafarian I,

[20] Naserzadeh P, and

[21] Hosseini MJ

[22] Aires CC,
Ijlst L,
Stet F,
Prip-Buus C,
de Almeida IT,
Duran M,
Wanders RJ, and
Silva MF
(2010) Inhibition of hepatic carnitine palmitoyl-transferase I (CPT IA) by valproyl-CoA as a possible mechanism of valproate-induced steatosis. Biochem Pharmacol 79:792–799.
OpenUrl CrossRef PubMed

[23] Aires CC,

[24] Ijlst L,

[25] Stet F,

[26] Prip-Buus C,

[27] de Almeida IT,

[28] Duran M,

[29] Wanders RJ, and

[30] Silva MF

[31] ↵
Alam MA and
Rahman MM
(2014) Mitochondrial dysfunction in obesity: potential benefit and mechanism of co-enzyme Q10 supplementation in metabolic syndrome. J Diabetes Metab Disord 13:60.
OpenUrl

[32] Alam MA and

[33] Rahman MM

[34] ↵
Albert R
(2007) Network inference, analysis, and modeling in systems biology. Plant Cell 19:3327–3338.
OpenUrl FREE Full Text

[35] Albert R

[36] ↵
Alexeyev M,
Shokolenko I,
Wilson G, and
LeDoux S
(2013) The maintenance of mitochondrial DNA integrity—critical analysis and update. Cold Spring Harb Perspect Biol 5:a012641.
OpenUrl Abstract/FREE Full Text

[37] Alexeyev M,

[38] Shokolenko I,

[39] Wilson G, and

[40] LeDoux S

[41] ↵
Amacher DE
(2005) Drug-associated mitochondrial toxicity and its detection. Curr Med Chem 12:1829–1839.
OpenUrl CrossRef PubMed

[42] Amacher DE

[43] ↵
Amoedo ND,
Obre E, and
Rossignol R
(2017) Drug discovery strategies in the field of tumor energy metabolism: limitations by metabolic flexibility and metabolic resistance to chemotherapy. Biochim Biophys Acta Bioenerg 1858:674–685.
OpenUrl

[44] Amoedo ND,

[45] Obre E, and

[46] Rossignol R

[47] ↵
Arndt S,
Baeza-Garza CD,
Logan A,
Rosa T,
Wedmann R,
Prime TA,
Martin JL,
Saeb-Parsy K,
Krieg T,
Filipovic MR et al.
(2017) Assessment of H₂S in vivo using the newly developed mitochondria-targeted mass spectrometry probe MitoA. J Biol Chem 292:7761–7773.
OpenUrl Abstract/FREE Full Text

[48] Arndt S,

[49] Baeza-Garza CD,

[50] Logan A,

[51] Rosa T,

[52] Wedmann R,

[53] Prime TA,

[54] Martin JL,

[55] Saeb-Parsy K,

[56] Krieg T,

[57] Filipovic MR et al.

[58] Atashbar S,
Jamali Z,
Khezri S, and
Salimi A
(2022) Celecoxib decreases mitochondrial complex IV activity and induces oxidative stress in isolated rat heart mitochondria: an analysis for its cardiotoxic adverse effect. J Biochem Mol Toxicol 36:e22934.
OpenUrl

[59] Atashbar S,

[60] Jamali Z,

[61] Khezri S, and

[62] Salimi A

[63] ↵
Babaei H,
Razmaraii N,
Assadnassab G,
Mohajjel Nayebi A,
Azarmi Y,
Mohammadnejad D, and
Azami A
(2020) Ultrastructural and echocardiographic assessment of chronic doxorubicin-induced cardiotoxicity in rats. Arch Razi Inst 75:55–62.
OpenUrl

[64] Babaei H,

[65] Razmaraii N,

[66] Assadnassab G,

[67] Mohajjel Nayebi A,

[68] Azarmi Y,

[69] Mohammadnejad D, and

[70] Azami A

[71] ↵
Bai JP and
Abernethy DR
(2013) Systems pharmacology to predict drug toxicity: integration across levels of biological organization. Annu Rev Pharmacol Toxicol 53:451–473.
OpenUrl CrossRef PubMed

[72] Bai JP and

[73] Abernethy DR

[74] Ball AL,
Kamalian L,
Alfirevic A,
Lyon JJ, and
Chadwick, AE
(2016) Identification of the additional mitochondrial liabilities of 2-hydroxyflutamide when compared with its parent compound, flutamide in HepG2 cells. Toxicol Sci 153:341–351.
OpenUrl CrossRef PubMed

[75] Ball AL,

[76] Kamalian L,

[77] Alfirevic A,

[78] Lyon JJ, and

[79] Chadwick, AE

[80] ↵
Bayraktar EC,
Baudrier L,
Özerdem C,
Lewis CA,
Chan SH,
Kunchok T,
Abu-Remaileh M,
Cangelosi AL,
Sabatini DM,
Birsoy K et al.
(2019) MITO-tag mice enable rapid isolation and multimodal profiling of mitochondria from specific cell types in vivo. Proc Natl Acad Sci USA 116:303–312.
OpenUrl Abstract/FREE Full Text

[81] Bayraktar EC,

[82] Baudrier L,

[83] Özerdem C,

[84] Lewis CA,

[85] Chan SH,

[86] Kunchok T,

[87] Abu-Remaileh M,

[88] Cangelosi AL,

[89] Sabatini DM,

[90] Birsoy K et al.

[91] ↵
Beeson CC,
Beeson GC, and
Schnellmann RG
(2010) A high-throughput respirometric assay for mitochondrial biogenesis and toxicity. Anal Biochem 404:75–81.
OpenUrl CrossRef PubMed

[92] Beeson CC,

[93] Beeson GC, and

[94] Schnellmann RG

[95] ↵
Begriche K,
Massart J,
Robin MA,
Borgne-Sanchez A, and
Fromenty B
(2011) Drug-induced toxicity on mitochondria and lipid metabolism: mechanistic diversity and deleterious consequences for the liver. J Hepatol 54:773–794.
OpenUrl CrossRef PubMed

[96] Begriche K,

[97] Massart J,

[98] Robin MA,

[99] Borgne-Sanchez A, and

[100] Fromenty B

[101] ↵
Bellance N,
Furt F,
Melser S,
Lalou C,
Thoraval D,
Maneta-Peyret L,
Lacombe D,
Moreau P, and
Rossignol R
(2020) Doxorubicin inhibits phosphatidylserine decarboxylase and modifies mitochondrial membrane composition in HeLa cells. Int J Mol Sci 21:1317.
OpenUrl

[102] Bellance N,

[103] Furt F,

[104] Melser S,

[105] Lalou C,

[106] Thoraval D,

[107] Maneta-Peyret L,

[108] Lacombe D,

[109] Moreau P, and

[110] Rossignol R

[111] ↵
Belousov VV,
Fradkov AF,
Lukyanov KA,
Staroverov DB,
Shakhbazov KS,
Terskikh AV, and
Lukyanov S
(2006) Genetically encoded fluorescent indicator for intracellular hydrogen peroxide. Nat Methods 3:281–286.
OpenUrl CrossRef PubMed

[112] Belousov VV,

[113] Fradkov AF,

[114] Lukyanov KA,

[115] Staroverov DB,

[116] Shakhbazov KS,

[117] Terskikh AV, and

[118] Lukyanov S

[119] Benzer F,
Kandemir FM,
Kucukler S,
Comaklı S, and
Caglayan C
(2018) Chemoprotective effects of curcumin on doxorubicin-induced nephrotoxicity in Wistar rats: by modulating inflammatory cytokines, apoptosis, oxidative stress and oxidative DNA damage. Arch Physiol Biochem 124:448–457.
OpenUrl

[120] Benzer F,

[121] Kandemir FM,

[122] Kucukler S,

[123] Comaklı S, and

[124] Caglayan C

[125] Bereiter-Hahn J and
Vöth M
(1994) Dynamics of mitochondria in living cells: shape changes, dislocations, fusion, and fission of mitochondria. Microsc Res Tech 27:198–219.
OpenUrl CrossRef PubMed

[126] Bereiter-Hahn J and

[127] Vöth M

[128] ↵
Bisson WH,
Cheltsov AV,
Bruey-Sedano N,
Lin B,
Chen J,
Goldberger N,
May LT,
Christopoulos A,
Dalton JT,
Sexton PM et al.
(2007) Discovery of antiandrogen activity of nonsteroidal scaffolds of marketed drugs. Proc Natl Acad Sci USA 104:11927–11932.
OpenUrl Abstract/FREE Full Text

[129] Bisson WH,

[130] Cheltsov AV,

[131] Bruey-Sedano N,

[132] Lin B,

[133] Chen J,

[134] Goldberger N,

[135] May LT,

[136] Christopoulos A,

[137] Dalton JT,

[138] Sexton PM et al.

[139] ↵
Blanchet L,
Smeitink JA,
van Emst-de Vries SE,
Vogels C,
Pellegrini M,
Jonckheere AI,
Rodenburg RJ,
Buydens LM,
Beyrath J,
Willems PH et al.
(2015) Quantifying small molecule phenotypic effects using mitochondrial morpho-functional fingerprinting and machine learning. Sci Rep 5:8035.
OpenUrl CrossRef PubMed

[140] Blanchet L,

[141] Smeitink JA,

[142] van Emst-de Vries SE,

[143] Vogels C,

[144] Pellegrini M,

[145] Jonckheere AI,

[146] Rodenburg RJ,

[147] Buydens LM,

[148] Beyrath J,

[149] Willems PH et al.

[150] Bloom MW,
Hamo CE,
Cardinale D,
Ky B,
Nohria A,
Baer L,
Skopicki H,
Lenihan DJ,
Gheorghiade M,
Lyon AR et al.
(2016) Cancer therapy-related cardiac dysfunction and heart failure: part 1: definitions, pathophysiology, risk factors, and imaging. Circ Heart Fail 9:e002661.
OpenUrl Abstract/FREE Full Text

[151] Bloom MW,

[152] Hamo CE,

[153] Cardinale D,

[154] Ky B,

[155] Nohria A,

[156] Baer L,

[157] Skopicki H,

[158] Lenihan DJ,

[159] Gheorghiade M,

[160] Lyon AR et al.

[161] ↵
Bludau I and
Aebersold R
(2020) Proteomic and interactomic insights into the molecular basis of cell functional diversity. Nat Rev Mol Cell Biol 21:327–340.
OpenUrl CrossRef PubMed

[162] Bludau I and

[163] Aebersold R

[164] ↵
Boelsterli UA and
Lim PL
(2007) Mitochondrial abnormalities—a link to idiosyncratic drug hepatotoxicity? Toxicol Appl Pharmacol 220:92–107.
OpenUrl CrossRef PubMed

[165] Boelsterli UA and

[166] Lim PL

[167] ↵
Bogenhagen DF
(2012) Mitochondrial DNA nucleoid structure. Biochim Biophys Acta 1819:914–920.
OpenUrl CrossRef PubMed

[168] Bogenhagen DF

[169] Bolaji OKE
(2018) Dynamic modelling of mitochondrial metabolism. IFAC Papers Online 51:126–127.
OpenUrl

[170] Bolaji OKE

[171] Bonte R,
Bongaerts M,
Demirdas S,
Langendonk JG,
Huidekoper HH,
Williams M,
Onkenhout W,
Jacobs EH,
Blom HJ, and
Ruijter GJG
(2019) Untargeted metabolomics-based screening method for inborn errors of metabolism using semi-automatic sample preparation with an UHPLC-Orbitrap-MS platform. Metabolites 9:289.
OpenUrl

[172] Bonte R,

[173] Bongaerts M,

[174] Demirdas S,

[175] Langendonk JG,

[176] Huidekoper HH,

[177] Williams M,

[178] Onkenhout W,

[179] Jacobs EH,

[180] Blom HJ, and

[181] Ruijter GJG

[182] ↵
Bova MP,
Tam D,
McMahon G, and
Mattson MN
(2005) Troglitazone induces a rapid drop of mitochondrial membrane potential in liver HepG2 cells. Toxicol Lett 155:41–50.
OpenUrl CrossRef PubMed

[183] Bova MP,

[184] Tam D,

[185] McMahon G, and

[186] Mattson MN

[187] Brandão SR,
Reis-Mendes A,
Domingues P,
Duarte JA,
Bastos ML,
Carvalho F,
Ferreira R, and
Costa VM
(2021) Exploring the aging effect of the anticancer drugs doxorubicin and mitoxantrone on cardiac mitochondrial proteome using a murine model. Toxicology 459:152852.
OpenUrl

[188] Brandão SR,

[189] Reis-Mendes A,

[190] Domingues P,

[191] Duarte JA,

[192] Bastos ML,

[193] Carvalho F,

[194] Ferreira R, and

[195] Costa VM

[196] Brandolini L,
Antonosante A,
Giorgio C,
Bagnasco M,
d’Angelo M,
Castelli V,
Benedetti E,
Cimini A, and
Allegretti M
(2020) NSAIDs-dependent adaption of the mitochondria-proteasome system in immortalized human cardiomyocytes. Sci Rep 10:18337.
OpenUrl

[197] Brandolini L,

[198] Antonosante A,

[199] Giorgio C,

[200] Bagnasco M,

[201] d’Angelo M,

[202] Castelli V,

[203] Benedetti E,

[204] Cimini A, and

[205] Allegretti M

[206] ↵
Bridges HR,
Jones AJ,
Pollak MN, and
Hirst J
(2014) Effects of metformin and other biguanides on oxidative phosphorylation in mitochondria. Biochem J 462:475–487.
OpenUrl Abstract/FREE Full Text

[207] Bridges HR,

[208] Jones AJ,

[209] Pollak MN, and

[210] Hirst J

[211] Brinkman K and
Kakuda TN
(2000) Mitochondrial toxicity of nucleoside analogue reverse transcriptase inhibitors: a looming obstacle for long-term antiretroviral therapy? Curr Opin Infect Dis 13:5–11.
OpenUrl CrossRef PubMed

[212] Brinkman K and

[213] Kakuda TN

[214] ↵
Brinkman K,
ter Hofstede HJM,
Burger DM,
Smeitink JA, and
Koopmans PP
(1998) Adverse effects of reverse transcriptase inhibitors: mitochondrial toxicity as common pathway. AIDS 12:1735–1744.
OpenUrl CrossRef PubMed

[215] Brinkman K,

[216] ter Hofstede HJM,

[217] Burger DM,

[218] Smeitink JA, and

[219] Koopmans PP

[220] ↵
Brunk E,
Sahoo S,
Zielinski DC,
Altunkaya A,
Dräger A,
Mih N,
Gatto F,
Nilsson A,
Preciat Gonzalez GA,
Aurich MK et al.
(2018) Recon3D enables a three-dimensional view of gene variation in human metabolism. Nat Biotechnol 36:272–281.
OpenUrl CrossRef PubMed

[221] Brunk E,

[222] Sahoo S,

[223] Zielinski DC,

[224] Altunkaya A,

[225] Dräger A,

[226] Mih N,

[227] Gatto F,

[228] Nilsson A,

[229] Preciat Gonzalez GA,

[230] Aurich MK et al.

[231] ↵
Buzkova J,
Nikkanen J,
Ahola S,
Hakonen AH,
Sevastianova K,
Hovinen T,
Yki-Järvinen H,
Pietiläinen KH,
Lönnqvist T,
Velagapudi V et al.
(2018) Metabolomes of mitochondrial diseases and inclusion body myositis patients: treatment targets and biomarkers. EMBO Mol Med 10:e9091.
OpenUrl Abstract/FREE Full Text

[232] Buzkova J,

[233] Nikkanen J,

[234] Ahola S,

[235] Hakonen AH,

[236] Sevastianova K,

[237] Hovinen T,

[238] Yki-Järvinen H,

[239] Pietiläinen KH,

[240] Lönnqvist T,

[241] Velagapudi V et al.

[242] ↵
Calvano SE,
Xiao W,
Richards DR,
Felciano RM,
Baker HV,
Cho RJ,
Chen RO,
Brownstein BH,
Cobb JP,
Tschoeke SK et al.
(2005) A network-based analysis of systemic inflammation in humans. Nature 437:1032–1037.
OpenUrl CrossRef PubMed

[243] Calvano SE,

[244] Xiao W,

[245] Richards DR,

[246] Felciano RM,

[247] Baker HV,

[248] Cho RJ,

[249] Chen RO,

[250] Brownstein BH,

[251] Cobb JP,

[252] Tschoeke SK et al.

[253] ↵
Calvo SE,
Clauser KR, and
Mootha VK
(2016) MitoCarta2.0: an updated inventory of mammalian mitochondrial proteins. Nucleic Acids Res 44(D1):D1251–D1257.
OpenUrl CrossRef PubMed

[254] Calvo SE,

[255] Clauser KR, and

[256] Mootha VK

[257] ↵
Campbell CT,
Kolesar JE, and
Kaufman BA
(2012) Mitochondrial transcription factor A regulates mitochondrial transcription initiation, DNA packaging, and genome copy number. Biochim Biophys Acta 1819:921–929.
OpenUrl CrossRef PubMed

[258] Campbell CT,

[259] Kolesar JE, and

[260] Kaufman BA

[261] ↵
Canta A,
Pozzi E, and
Carozzi VA
(2015) Mitochondrial dysfunction in chemotherapy-induced peripheral neuropathy (CIPN). Toxics 3:198–223.
OpenUrl

[262] Canta A,

[263] Pozzi E, and

[264] Carozzi VA

[265] ↵
Chan K,
Truong D,
Shangari N, and
O’Brien PJ
(2005) Drug-induced mitochondrial toxicity. Expert Opin Drug Metab Toxicol 1:655–669.
OpenUrl CrossRef PubMed

[266] Chan K,

[267] Truong D,

[268] Shangari N, and

[269] O’Brien PJ

[270] ↵
Chang RL,
Xie L,
Bourne PE, and
Palsson BO
(2013) Antibacterial mechanisms identified through structural systems pharmacology. BMC Syst Biol 7:102.
OpenUrl

[271] Chang RL,

[272] Xie L,

[273] Bourne PE, and

[274] Palsson BO

[275] ↵
Chen H,
Vermulst M,
Wang YE,
Chomyn A,
Prolla TA,
McCaffery JM, and
Chan DC
(2010) Mitochondrial fusion is required for mtDNA stability in skeletal muscle and tolerance of mtDNA mutations. Cell 141:280–289.
OpenUrl CrossRef PubMed

[276] Chen H,

[277] Vermulst M,

[278] Wang YE,

[279] Chomyn A,

[280] Prolla TA,

[281] McCaffery JM, and

[282] Chan DC

[283] Chen PI,
Cao A,
Miyagawa K,
Tojais NF,
Hennigs JK,
Li CG,
Sweeney NM,
Inglis AS,
Wang L,
Li D et al.
(2017a) Amphetamines promote mitochondrial dysfunction and DNA damage in pulmonary hypertension. JCI Insight 2:e90427.
OpenUrl

[284] Chen PI,

[285] Cao A,

[286] Miyagawa K,

[287] Tojais NF,

[288] Hennigs JK,

[289] Li CG,

[290] Sweeney NM,

[291] Inglis AS,

[292] Wang L,

[293] Li D et al.

[294] Chen Q,
Cui Y,
Ding G,
Jia Z,
Zhang Y,
Zhang A, and
Huang S
(2017b) PEA3 protects against gentamicin nephrotoxicity: role of mitochondrial dysfunction. Am J Transl Res 9:2153–2162.
OpenUrl

[295] Chen Q,

[296] Cui Y,

[297] Ding G,

[298] Jia Z,

[299] Zhang Y,

[300] Zhang A, and

[301] Huang S

[302] ↵
Chen WW,
Freinkman E,
Wang T,
Birsoy K, and
Sabatini DM
(2016) Absolute quantification of matrix metabolites reveals the dynamics of mitochondrial metabolism. Cell 166:1324–1337.e11.
OpenUrl CrossRef PubMed

[303] Chen WW,

[304] Freinkman E,

[305] Wang T,

[306] Birsoy K, and

[307] Sabatini DM

[308] ↵
Clish CB
(2015) Metabolomics: an emerging but powerful tool for precision medicine. Csh Mol Case Stud 1:a000588.
OpenUrl

[309] Clish CB

[310] ↵
Cochemé HM,
Quin C,
McQuaker SJ,
Cabreiro F,
Logan A,
Prime TA,
Abakumova I,
Patel JV,
Fearnley IM,
James AM et al.
(2011) Measurement of H2O2 within living Drosophila during aging using a ratiometric mass spectrometry probe targeted to the mitochondrial matrix. Cell Metab 13:340–350.
OpenUrl CrossRef PubMed

[311] Cochemé HM,

[312] Quin C,

[313] McQuaker SJ,

[314] Cabreiro F,

[315] Logan A,

[316] Prime TA,

[317] Abakumova I,

[318] Patel JV,

[319] Fearnley IM,

[320] James AM et al.

[321] Coe KJ,
Jia Y,
Ho HK,
Rademacher P,
Bammler TK,
Beyer RP,
Farin FM,
Woodke L,
Plymate SR,
Fausto N et al.
(2007) Comparison of the cytotoxicity of the nitroaromatic drug flutamide to its cyano analogue in the hepatocyte cell line TAMH: evidence for complex I inhibition and mitochondrial dysfunction using toxicogenomic screening. Chem Res Toxicol 20:1277–1290.
OpenUrl CrossRef PubMed

[322] Coe KJ,

[323] Jia Y,

[324] Ho HK,

[325] Rademacher P,

[326] Bammler TK,

[327] Beyer RP,

[328] Farin FM,

[329] Woodke L,

[330] Plymate SR,

[331] Fausto N et al.

[332] ↵
Coene KLM,
Kluijtmans LAJ,
van der Heeft E,
Engelke UFH,
de Boer S,
Hoegen B,
Kwast HJT,
van de Vorst M,
Huigen MCDG,
Keularts IMLW et al.
(2018) Next-generation metabolic screening: targeted and untargeted metabolomics for the diagnosis of inborn errors of metabolism in individual patients. J Inherit Metab Dis 41:337–353.
OpenUrl

[333] Coene KLM,

[334] Kluijtmans LAJ,

[335] van der Heeft E,

[336] Engelke UFH,

[337] de Boer S,

[338] Hoegen B,

[339] Kwast HJT,

[340] van de Vorst M,

[341] Huigen MCDG,

[342] Keularts IMLW et al.

[343] ↵
Comte J,
Maïsterrena B, and
Gautheron DC
(1976) Lipid composition and protein profiles of outer and inner membranes from pig heart mitochondria. Comparison with microsomes. Biochim Biophys Acta 419:271–284.
OpenUrl CrossRef PubMed

[344] Comte J,

[345] Maïsterrena B, and

[346] Gautheron DC

[347] ↵
Console L,
Scalise M,
Giangregorio N,
Tonazzi A,
Barile M, and
Indiveri C
(2020) The link between the mitochondrial fatty acid oxidation derangement and kidney injury. Front Physiol 11:794.
OpenUrl CrossRef

[348] Console L,

[349] Scalise M,

[350] Giangregorio N,

[351] Tonazzi A,

[352] Barile M, and

[353] Indiveri C

[354] ↵
Cordes H,
Thiel C,
Baier V,
Blank LM, and
Kuepfer L
(2018) Integration of genome-scale metabolic networks into whole-body PBPK models shows phenotype-specific cases of drug-induced metabolic perturbation. NPJ Syst Biol Appl 4:10.
OpenUrl

[355] Cordes H,

[356] Thiel C,

[357] Baier V,

[358] Blank LM, and

[359] Kuepfer L

[360] ↵
Cortassa S,
Aon MA, and
Sollott SJ
(2019) Control and regulation of substrate selection in cytoplasmic and mitochondrial catabolic networks. A systems biology analysis. Front Physiol 10:201.
OpenUrl

[361] Cortassa S,

[362] Aon MA, and

[363] Sollott SJ

[364] de Arriba G,
Calvino M,
Benito S, and
Parra T
(2013) Cyclosporine A-induced apoptosis in renal tubular cells is related to oxidative damage and mitochondrial fission. Toxicol Lett 218:30–38.
OpenUrl CrossRef PubMed

[365] de Arriba G,

[366] Calvino M,

[367] Benito S, and

[368] Parra T

[369] ↵
de Wolf FA,
Staffhorst RW,
Smits HP,
Onwezen MF, and
de Kruijff B
(1993) Role of anionic phospholipids in the interaction of doxorubicin and plasma membrane vesicles: drug binding and structural consequences in bacterial systems. Biochemistry 32:6688–6695.
OpenUrl CrossRef PubMed

[370] de Wolf FA,

[371] Staffhorst RW,

[372] Smits HP,

[373] Onwezen MF, and

[374] de Kruijff B

[375] ↵
DiMauro S,
Bonilla E, and
De Vivo DC
(1999) Does the patient have a mitochondrial encephalomyopathy? J Child Neurol 14(Suppl 1):S23–S35.
OpenUrl CrossRef PubMed

[376] DiMauro S,

[377] Bonilla E, and

[378] De Vivo DC

[379] ↵
Dimauro S,
Tay S, and
Mancuso M
(2004) Mitochondrial encephalomyopathies: diagnostic approach. Ann N Y Acad Sci 1011:217–231.
OpenUrl CrossRef PubMed

[380] Dimauro S,

[381] Tay S, and

[382] Mancuso M

[383] ↵
Divakaruni AS,
Wiley SE,
Rogers GW,
Andreyev AY,
Petrosyan S,
Loviscach M,
Wall EA,
Yadava N,
Heuck AP,
Ferrick DA et al.
(2013) Thiazolidinediones are acute, specific inhibitors of the mitochondrial pyruvate carrier. Proc Natl Acad Sci USA 110:5422–5427.
OpenUrl Abstract/FREE Full Text

[384] Divakaruni AS,

[385] Wiley SE,

[386] Rogers GW,

[387] Andreyev AY,

[388] Petrosyan S,

[389] Loviscach M,

[390] Wall EA,

[391] Yadava N,

[392] Heuck AP,

[393] Ferrick DA et al.

[394] ↵
Dolce V,
Fiermonte G,
Runswick MJ,
Palmieri F, and
Walker JE
(2001) The human mitochondrial deoxynucleotide carrier and its role in the toxicity of nucleoside antivirals. Proc Natl Acad Sci USA 98:2284–2288.
OpenUrl Abstract/FREE Full Text

[395] Dolce V,

[396] Fiermonte G,

[397] Runswick MJ,

[398] Palmieri F, and

[399] Walker JE

[400] ↵
Du K,
Ramachandran A,
McGill MR,
Mansouri A,
Asselah T,
Farhood A,
Woolbright BL,
Ding WX, and
Jaeschke H
(2017) Induction of mitochondrial biogenesis protects against acetaminophen hepatotoxicity. Food Chem Toxicol 108(Pt A):339–350.
OpenUrl

[401] Du K,

[402] Ramachandran A,

[403] McGill MR,

[404] Mansouri A,

[405] Asselah T,

[406] Farhood A,

[407] Woolbright BL,

[408] Ding WX, and

[409] Jaeschke H

[410] ↵
Düssmann H,
Perez-Alvarez S,
Anilkumar U,
Papkovsky DB, and
Prehn JH
(2017) Single-cell time-lapse imaging of intracellular O₂ in response to metabolic inhibition and mitochondrial cytochrome-c release. Cell Death Dis 8:e2853.
OpenUrl

[411] Düssmann H,

[412] Perez-Alvarez S,

[413] Anilkumar U,

[414] Papkovsky DB, and

[415] Prehn JH

[416] Dykens J and
Will Y
(2008) Drug‐Induced Mitochondrial Dysfunction, John Wiley, Hoboken, NJ.

[417] Dykens J and

[418] Will Y

[419] ↵
Dykens J and
Will Y
(2018) Mitochondrial Dysfunction Caused by Drugs and Environmental Toxicants, John Wiley, Hoboken, NJ.

[420] Dykens J and

[421] Will Y

[422] ↵
Dykens JA,
Jamieson JD,
Marroquin LD,
Nadanaciva S,
Xu JJ,
Dunn MC,
Smith AR, and
Will Y
(2008) In vitro assessment of mitochondrial dysfunction and cytotoxicity of nefazodone, trazodone, and buspirone. Toxicol Sci 103:335–345.
OpenUrl CrossRef PubMed

[423] Dykens JA,

[424] Jamieson JD,

[425] Marroquin LD,

[426] Nadanaciva S,

[427] Xu JJ,

[428] Dunn MC,

[429] Smith AR, and

[430] Will Y

[431] ↵
Dykens JA,
Marroquin LD, and
Will Y
(2007) Strategies to reduce late-stage drug attrition due to mitochondrial toxicity. Expert Rev Mol Diagn 7:161–175.
OpenUrl CrossRef PubMed

[432] Dykens JA,

[433] Marroquin LD, and

[434] Will Y

[435] ↵
Dykens JA and
Will Y
(2007) The significance of mitochondrial toxicity testing in drug development. Drug Discov Today 12:777–785.
OpenUrl CrossRef PubMed

[436] Dykens JA and

[437] Will Y

[438] ↵
Dykens JA,
Wiseman RW, and
Hardin CD
(1996) Preservation of phosphagen kinase function during transient hypoxia via enzyme abundance or resistance to oxidative inactivation. J Comp Physiol B 166:359–368.
OpenUrl CrossRef PubMed

[439] Dykens JA,

[440] Wiseman RW, and

[441] Hardin CD

[442] ↵
El-Gharbawy A and
Vockley J
(2018) Inborn errors of metabolism with myopathy: defects of fatty acid oxidation and the carnitine shuttle system. Pediatr Clin North Am 65:317–335.
OpenUrl

[443] El-Gharbawy A and

[444] Vockley J

[445] Elimadi A,
Morin D,
Albengres E,
Chauvet-Monges AM,
Allain V,
Crevat A, and
Tillement JP
(1997) Differential effects of zidovudine and zidovudine triphosphate on mitochondrial permeability transition and oxidative phosphorylation. Br J Pharmacol 121:1295–1300.
OpenUrl

[446] Elimadi A,

[447] Morin D,

[448] Albengres E,

[449] Chauvet-Monges AM,

[450] Allain V,

[451] Crevat A, and

[452] Tillement JP

[453] ↵
Fannin RD,
Russo M,
O’Connell TM,
Gerrish K,
Winnike JH,
Macdonald J,
Newton J,
Malik S,
Sieber SO,
Parker J et al.
(2010) Acetaminophen dosing of humans results in blood transcriptome and metabolome changes consistent with impaired oxidative phosphorylation. Hepatology 51:227–236.
OpenUrl CrossRef PubMed

[454] Fannin RD,

[455] Russo M,

[456] O’Connell TM,

[457] Gerrish K,

[458] Winnike JH,

[459] Macdonald J,

[460] Newton J,

[461] Malik S,

[462] Sieber SO,

[463] Parker J et al.

[464] ↵
Fasano M,
Monti C, and
Alberio T
(2016) A systems biology-led insight into the role of the proteome in neurodegenerative diseases. Expert Rev Proteomics 13:845–855.
OpenUrl

[465] Fasano M,

[466] Monti C, and

[467] Alberio T

[468] Fau D,
Eugene D,
Berson A,
Letteron P,
Fromenty B,
Fisch C, and
Pessayre D
(1994) Toxicity of the antiandrogen flutamide in isolated rat hepatocytes. J Pharmacol Exp Ther 269:954–962.
OpenUrl Abstract/FREE Full Text

[469] Fau D,

[470] Eugene D,

[471] Berson A,

[472] Letteron P,

[473] Fromenty B,

[474] Fisch C, and

[475] Pessayre D

[476] ↵
Ferreira LG,
Dos Santos RN,
Oliva G, and
Andricopulo AD
(2015) Molecular docking and structure-based drug design strategies. Molecules 20:13384–13421.
OpenUrl CrossRef

[477] Ferreira LG,

[478] Dos Santos RN,

[479] Oliva G, and

[480] Andricopulo AD

[481] ↵
Ferrick DA,
Neilson A, and
Beeson C
(2008) Advances in measuring cellular bioenergetics using extracellular flux. Drug Discov Today 13:268–274.
OpenUrl CrossRef PubMed

[482] Ferrick DA,

[483] Neilson A, and

[484] Beeson C

[485] ↵
Forkink M,
Smeitink JA,
Brock R,
Willems PH, and
Koopman WJ
(2010) Detection and manipulation of mitochondrial reactive oxygen species in mammalian cells. Biochim Biophys Acta 1797:1034–1044.
OpenUrl CrossRef PubMed

[486] Forkink M,

[487] Smeitink JA,

[488] Brock R,

[489] Willems PH, and

[490] Koopman WJ

[491] ↵
Fosslien E
(2001) Mitochondrial medicine–molecular pathology of defective oxidative phosphorylation. Ann Clin Lab Sci 31:25–67.
OpenUrl Abstract/FREE Full Text

[492] Fosslien E

[493] ↵
Furberg CD and
Pitt B
(2001) Withdrawal of cerivastatin from the world market. Curr Control Trials Cardiovasc Med 2:205–207.
OpenUrl CrossRef PubMed

[494] Furberg CD and

[495] Pitt B

[496] Gai Z,
Gui T,
Kullak-Ublick GA,
Li Y, and
Visentin M
(2020) The role of mitochondria in drug-induced kidney injury. Front Physiol 11:1079.
OpenUrl

[497] Gai Z,

[498] Gui T,

[499] Kullak-Ublick GA,

[500] Li Y, and

[501] Visentin M

Main menu

User menu

Search

Time to Change: A Systems Pharmacology Approach to Disentangle Mechanisms of Drug-Induced Mitochondrial Toxicity

Visual Overview

Abstract

I. Mitochondrial Dysfunction as a Major Determinant in Adverse Drug Reactions

II. Current Methods to Identify Drug-Induced Mitochondrial Dysfunction

III. Application of Systems Pharmacology to Investigate Drug-Induced Mitochondrial Dysfunction

IV. A Tiered Approach to Implement Mitochondrial Systems Pharmacology in Drug Development

A. Tier 1: Phenotypic Screening During Hit Identification

B. Tier 2: Key Metabolic Profiling During Lead Development

C. Tier 3: Mechanistic Studies During Lead Optimization

D. Tier 4: Functional In Situ Studies Versus In Vivo Efficacy and Safety Studies

V. Concluding Remarks and Future Perspectives

Acknowledgments

Authorship Contributions

Footnotes

Abbreviations

References