Abstract
Anti-inflammatory properties of pentoxifylline (PTX) have recently been described. Spontaneously hypertensive stroke-prone rats (SHRSP) constitute an animal model that develops an inflammatory condition that precedes the appearance of brain abnormalities. The aim of the present investigation was to assess: 1) the efficacy of PTX treatment in protecting the neural system in SHRSP, and 2) how its anti-inflammatory properties might be involved in this effect. Male SHRSP fed with a permissive diet received no drug or PTX (100 or 200 mg/kg/day). Brain abnormalities detected by magnetic resonance imaging developed spontaneously in control rats after 42 ± 3 days, whereas in rats treated with 100 mg/kg/day PTX, abnormalities developed in only 80% of the animals and only after 70 to 80 days. Treatment with a higher dose of PTX (200 mg/kg/day) completely protected the brain from abnormal development. The drug treatment prevented the accumulation of macrophages or CD4+ positive cells, the activation of glia in brain tissues, and the appearance of inflammatory proteins and thiobarbituric acid-reactive substances in body fluids. PTX treatment did induce a greater increase of serum tumor necrosis factor-α (TNF-α), but not of interleukin (IL)-1β and IL-6 induced by in vivo administration of lipopolysaccharide (LPS), which suggests a protective role for TNF-α. PTX also exerted protective effects when it was administered after the first occurrence of proteinuria (>40 mg/day). These data indicate that PTX treatment dose-dependently prevents the occurrence of spontaneous brain damage by reducing inflammatory events. We also hypothesize that the increase of TNF-α by PTX treatment represents a protective mechanism in SHRSP.
Pentoxifylline (PTX), a methylxanthine derivative and nonspecific type 4 phosphodiesterase inhibitor, is a drug widely used in the management of peripheral arterial disease and, in particular, for intermittent claudication (Labs et al., 1997; Creager, 2001). The mechanism underlying its beneficial effects appears to be related to the improvement of cellular functions and modifications in the plasma that improve microcirculatory perfusion in both peripheral and cerebral vascular beds (Seiffge, 1997; Windmeier and Gressner, 1997).
In recent years, in vitro and in vivo experiments indicated an additional therapeutic potential for PTX as an anti-inflammatory and immunomodulator agent (Teixeira et al., 1997; Laurat et al., 2001; Haddad et al., 2002). This newly described pharmacological effect can be ascribed to an inhibition of the functional responses of circulating mononuclear phagocytes, neutrophils, and T lymphocytes and the decreased synthesis of several proinflammatory cytokines (Dong et al., 1997; Neuner et al., 1997; Marcinkiewicz et al., 2000; Bahra et al., 2001; Laurat et al., 2001; Samardzic et al., 2001). Studies of the anti-inflammatory effects of PTX in vivo have focused attention on tissue injury after ischemia. Thus, in vivo PTX treatment reduced ischemia-reperfusion injury in the lung (Thabut et al., 2001), intestine (Sener et al., 2001), liver (Iwamoto et al., 2002), kidney (Kim et al., 2001), spinal cord (Savas et al., 2002), and brain of different animal species including rats, mice, and dogs (Toung et al., 1994; Sirin et al., 1998; Eun et al., 2000). Inflammatory processes accompany tissue injury regardless of the organ system involved, and chronic inflammation may predispose to ischemia in peripheral organs and to brain damage (Lindsberg and Grau, 2003).
We have previously reported (Sironi et al., 2001; Guerrini et al., 2002) that spontaneously hypertensive stroke-prone rats (SHRSP) subjected to salt loading develop an inflammatory condition characterized by the accumulation of acutephase proteins in plasma and urine, and this event precedes and predicts the appearance of brain abnormalities. This seems to be a suitable experimental model to explore if the effect of PTX on tissue damage depends on anti-inflammatory properties. This study was designed to: 1) evaluate the neuroprotective effect of PTX in salt-loaded SHRSP, and 2) to understand whether its anti-inflammatory properties are involved. We used the salt-loaded SHRSP, a spontaneous model of cerebral damage, and measured the onset and development of brain damage and increase in survival time after PTX treatment in either prophylactic or rescue mode. We found that both regimens delay brain damage and attenuate the associated inflammatory responses.
Materials and Methods
Animal Model of Brain Damage. Male SHRSP (8–10 weeks old), purchased from Charles River Italica (Calco, Como, Italy), were fed a permissive diet containing 18.7% protein, 0.63% potassium, 0.37% sodium (Laboratorio Dr. Piccioni, Milano, Italy), and 1% NaCl in drinking water (salt-loaded) ad libitum. Their food and liquid intakes were measured weekly, as was proteinuria. T2-weighted MRI assessments were repeated every other day in rats after 24-h proteinuria exceeded 40 mg/day and daily after a brain abnormality had been detected (Sironi et al., 2001). Three days after brain damage was detected, the rats were anesthetized with chloral hydrate (400 mg/kg i.p.), and the brain was removed for immunohistochemical analysis. At the same time, PTX-treated rats with no sign of brain abnormalities were also sacrificed. Procedures involving animals and their care were in accordance with the Guide for the Care and Use of Laboratory Animals.
Drug Treatment. In each experiment, animals were matched for age and weight and randomly divided into the different treatment groups. Pentoxifylline [PTX; 3,7 dimethyl-1-(5-oxohexyl) xanthine], obtained from Sigma-Aldrich (St. Louis, MO), was dissolved daily in a small amount of drinking water to achieve doses of 100 (n = 12) or 200 mg/kg/day (n = 12). Each rat was kept in a separate cage, and an operator ensured that each animal drank the entire drug solution daily, after which the animal had free access to 1% NaCl. Control rats (n = 12) received the vehicle in the same way as PTX.
Drug treatments were started simultaneously with the permissive diet in the prophylactic experiment and soon after proteinuria exceeded 40 mg/day in the rescue therapy. Rats were weighed weekly, and their arterial blood pressure was measured, then housed individually in metabolic cages for 24 h, and urine was collected for measurement of proteinuria and for proteomic studies.
MRI Evaluations of Brain Damage. The rats were anesthetized with 2% isofluorane in 70% N2/30% O2, fixed to an animal holder by means of a rod beneath the teeth, and placed inside the magnet (4.7T, vertical 15-cm bore) of a Bruker spectrometer (AMX3 with micro-imaging accessory; Bruker Biospin, Karlsruhe, DE). A 6.4-cm diameter birdcage coil was used for the imaging. A T2 multislice image was obtained after a 3-orthogonal plane gradient echo scout. Sixteen contiguous 1-mm thick slices were analyzed caudally to the olfactory bulb using a field of view of 4 × 4 cm2. A turbo spin echo sequence was used with 16 echoes per excitation, 10 ms of interecho time, 85 ms of equivalent echo time, and 4 s of repetition time. The images were 128 × 128 points (zero filled to 256 × 256), and eight images were averaged in 8′30″. The occurrence of lesions was identified as the presence of areas of high signal intensity on T2-weighted MRI.
Immunohistochemistry of Brain Tissue. For histological examination, the brains were fixed in Carnoy reagent (Merck, Darmstadt, Germany), embedded in Paraplast (Sigma-Aldrich), and coronal sections (5 μm) were stained with hematoxylin/eosin and examined by light microscopy. For immunohistochemical studies, paraffin-embedded brain coronal sections were dewaxed in xylene and dehydrated. Endogenous peroxidase was blocked by adding 1% H2O2 in 50% methanol. Nonspecific binding sites were saturated with goat serum. The sections were incubated overnight at 4°C with the primary antibodies, then with biotinylated secondary antibodies, and streptavidine peroxidase (LSAB2 kit; DAKO, Glostrup, Denmark). Horseradish peroxidase was detected with H2O2 and diaminobenzidine (Sigma-Aldrich). The primary antibodies used were: anti-CD4 which react with T helper cells (1:10; Cymbus Biotechnologies, Chandlers Ford, Hants, UK), anti-ED1 which react with myeloid cells (1:20; Serotec, Oxford, UK), and anti-ED2 which react with resident macrophages (1:20; Serotec). Microglia were specifically visualized by lectin histochemistry using peroxidase-labeled isolectin B4 from Griffonia simplicifolia seeds (Sigma-Aldrich).
Myeloperoxidase (MPO) Tissue Activity. MPO activity was measured by a modification of the Hillegass technique (Hillegass et al., 1990). Briefly, 0.1 g of rat brain tissue was homogenized in 4 ml of 50 mM potassium phosphate buffer, pH 6.0 and centrifuged at 16,000 rpm for 30 min at 4°C. The pellet was resuspended in the same buffer with 0.5% hexadecyltrimethylammonium bromide. The samples were alternately frozen and thawed three times and sonicated between cycles before another centrifugation (16,000 rpm at 4°C). For the measurement, 0.1 ml of supernatant was mixed with 0.1 ml of tetramethylbenzidine, 16 mM in dimethylsulfoxide, and 0.8 ml of H2O2 0.3 mM. Absorbance was measured at 655 nm for 5 min. The MPO activity values were expressed as percentage of change in optical density per minute per gram over tissues from that in nonsalt-loaded rats (100%).
Determination of Urinary Thiobarbituric Acid Reacting Substances (TBARS). TBARS were measured by the method of Valenzuela (1991). Briefly, 500 μl of urine was combined with 500 μl of a 0.67% thiobarbituric acid (TBA) aqueous solution and 500 μl of 20% trichloroacetic acid solution. The samples were vortexed and incubated at 100°C for 1 h, and the absorbance at 532 nm was measured spectrophotometrically. The quantity of TBARS is proportional to the amount of malondialdehyde (MDA), a lipid peroxidation product generated by the oxidation of membrane lipids by reactive oxygen species. The concentration of MDA was calculated by the absorbance coefficient of the MDA-TBA complex (absorbance coefficient ϵ = 1.56 × 105 cm-1 M-1) and expressed as percentage of increase over that in nonsalt-loaded rat urine.
Lipopolysaccharide Induction of Serum TNF-α, IL-1β, and IL-6. SHRSPs subjected to the permissive diet were not treated (n = 8) or treated with PTX (200 mg/kg/day; n = 8). Three days after detection of brain abnormalities in control rats, all the animals were injected with LPS (dissolved in sterile pyrogen-free saline at 5 mg/kg) to trigger the formation of inflammatory cytokines. Three hours later, blood samples were collected, serum was prepared by centrifugation at 1200g for 10 min at 4°C, and stored at -80°C until assay. TNF-α, IL-1β, and IL-6 levels were determined using an enzyme-linked immunosorbent assay kit (NIBSC, Hertfordshire, UK) following the manufacturer's instructions.
Proteomic Studies. Urine proteins were concentrated by trichloroacetic acid-acetone precipitation. One-dimensional electrophoresis was run on urine proteins in the presence of SDS, without sample reduction, in a discontinuous buffer system on a 4 to 20% polyacrylamide gradient. The sample load was 3.75 μg per lane. Proteins were stained with 0.3% w/v Coomassie Blue, and the protein patterns were digitalized with a scanner.
Statistical Analysis. Data are expressed as mean ± S.D. Differences between groups were computed by analysis of variance for repeated measurements, followed by Bonferroni's post hoc test. p < 0.05 was taken as statistically significant.
Results
Effects of Pentoxifylline on Physiological Parameters. Body weight increased similarly in the three groups of salt-loaded SHRSPs up to the sixth week of treatment (Table 1). After that, body weight decreased in control rats only. In PTX-treated animals, the growth curves constantly increased over the entire experimental period (not shown). The severe hypertension that developed in salt-loaded SHRSPs was not influenced by either dose of PTX used (Table 1).
Effects of Pentoxifylline on Proteinuria and Inflammatory Proteins in Urine. In control rats, proteinuria progressively increased and rose sharply after 4 weeks of salt loading, reaching a maximum of 166 ± 31.7 mg/day on the 42nd day of treatment. At either dose of PTX, proteinuria was lower than in the untreated animals. The lower dose (n = 12) resulted in a delayed rise in proteinuria (not shown), whereas the higher dose (n = 12) virtually prevented the loss of protein (Fig. 1A). The mixture of proteins excreted by control SHRSP and by those given 200 mg/kg/day of PTX, was identified by running the urine on one-dimensional gels (example in Fig. 1B). The appearance of high molecular weight proteins, markers of an inflammatory response in control animals, were dramatically delayed in the drug-treated rats.
Effects of Pentoxifylline on the Appearance of Brain Damage. All control rats (n = 12) developed brain abnormalities after 42 ± 3 days of permissive diet, whereas in the group treated with PTX (100 mg/kg/day, n = 12), the abnormalities developed in 80% of the animals after 70 to 80 days. Treatment with the higher dose of PTX (n = 12) completely protected the brain (animals free from MRI-detectable lesions after 4 months) (Fig. 2).
Effects of Pentoxifylline on the Appearance of Inflammatory Cells in the Brain. In control rats, inflammatory cells were found in the damaged brain hemisphere 3 days after MRI first detected the damage. ED1- and ED2-positive macrophages, CD4+ T-lymphocytes, and activated microglia (isolectin B4 positive) accumulated significantly (Fig. 3). ED2-positive cells localized preferentially around the vessels, whereas ED1-positive cells, CD4+ T lymphocytes, and activated microglia, were spread over the whole damage tissue. Conversely, in PTX-treated animals sacrificed at the same time as the controls, no inflammatory, immunocompetent, or activated cells could be detected (Fig. 3). In brain homogenates of control rats, we documented increased MPO activity (188 ± 27% versus nonsalt-loaded SHRSP), an index of accumulation of polymorphonuclear neutrophils; this was not attenuated by PTX treatment (218 ± 16% versus nonsalt-loaded SHRSP).
Effects of Pentoxifylline on Inflammatory Parameters. Three hours after in vivo administration of LPS, the induction of TNF-α was significantly greater in PTX-treated rats (n = 8) than in controls (n = 8) (Fig. 4). However, the induction of IL-1β and IL-6 was not affected by PTX treatment (Fig. 4). The urinary increase in TBARS found in control rats after the detection of damage (257 ± 12.2% versus nonsalt-loaded SHRSP) was almost nullified by PTX treatment (114 ± 24.7% versus nonsalt-loaded SHRSP).
Effects of Pentoxifylline Administered after Increase of Proteinuria. To determine whether the PTX reversed the increase in proteinuria, SHRSPs subjected to salt loading and permissive diet (n = 10) were treated with drug (200 mg/kg/day; n = 10) after >40 mg protein/day were lost in the urine. This treatment also protected the animals from loss in weight, any further increase in proteinuria, and from the development of MRI-detectable brain lesions (not shown).
Discussion
We have shown here that prophylactic treatment with PTX delays, in a dose-dependent manner, the onset and development of brain damage and increases survival in salt-loaded SHRSP. These effects are independent of blood pressure and are linked to a mitigation of the local and systemic inflammatory responses always associated with brain damage in this animal model. Similar results were obtained when PTX administration was delayed.
We have reported earlier that the gray matter of rat brain that develops damage after salt loading is markedly spongy with loss of neurons, accumulation of astrocytes, and deposition of fibrinoid-eosinophilic material (Sironi et al., 2001, 2003; Guerrini et al., 2002). Now, we have shown a local response close to the brain-damaged area of salt-loaded SHRSP, with the accumulation of inflammatory as well as immunocompetent cells. Resident macrophages (ED2) in the damaged area may be activated by proinflammatory cytokines, which in turn may alter the biochemical and physical properties of the blood-brain barrier. Circulating macrophages (ED1) migrate through the vasculature of the impaired blood-brain barrier and surround the damaged tissue, thus favoring local progression of the ischemic process. CD4+ T lymphocytes and neutrophils are also recruited into the inflammatory brain area. PTX treatment suppressed recruitment within the brain of inflammatory cells, with the exception of polymorphonuclear neutrophils, and maintained thiobarbituric acid-reactive substances at their normal level.
Several complementary anti-inflammatory effects of PTX could be responsible for its neuroprotective effect. One possible mechanism is the inhibition of cellular functions involved in inflammatory and immune diseases, inhibition of adhesion and activation of peripheral blood T-lymphocytes, suppression of T-cell proliferation and differentiation, and inhibition of polarization and migration of human leukocytes and neutrophils (Dong et al., 1997; Gonzalez-Amaro et al., 1998; Laurat et al., 2001; Dominguez-Jiménez et al., 2002). A second neuroprotective mechanism of PTX probably includes the inhibition of the generation of oxygen radicals. Oxidative stress may damage different tissues such as the brain and the kidney in SHRSP (Tanito et al., 2004). It has been documented that PTX protects against lipid peroxidation in in vitro and in vivo models of ischemia (Bhat and Madyastha, 2001).
Lipopolysaccharide injection induced higher levels of TNF-α (but not of IL-1β or IL-6) in PTX-treated rats than in controls. TNF-α has been implicated in brain damage, but also in neuroprotective effects in stroke (Hallenbeck, 2002), and several recent studies postulate an important role for TNF-α in ischemic preconditioning (Ginis et al., 2002). Ischemic tolerance associated with increased plasma levels of TNF-α has recently been reported in human stroke (Castillo et al., 2003). On this basis, we hypothesize that the propensity of PTX-treated rats to produce TNF-α may represent a protective mechanism.
The appearance of brain damage in salt-loaded SHRSP is always preceded by proteinuria and the accumulation of several inflammatory markers in plasma and urine (Sironi et al., 2001). Most of the acute phase proteins (transferrin, hemopexin, albumin, and thiostatin) found in serum are also detected in urine, and their levels increase over time until stroke occurs. The total amount and the composition of proteins in the urine changes during the 2 weeks preceding an ischemic event (Sironi et al., 2001). We therefore tried treating the salt-loaded SHRSPs with PTX immediately after the appearance of inflammatory proteins in the urine. Even this delayed administration protected the animals from the development of brain damage as well as from the linear increase of urinary protein, which suggests that PTX may “cure or reverse” the kidney abnormalities reported in this animal model (Abumiya et al., 1996). Indeed, a nephroprotective effect of PTX in experimentally induced renal failure (Kim et al., 2001) and an antiproteinuric effect in patients with nephropathy (Ducloux et al., 2001) has been reported.
Methylxanthine derivatives are of potential interest in the treatment of vascular diseases, in general, and of stroke, in particular, because of their vasodilating properties (Kruuse et al., 2000). PTX has been reported to increase peripheral blood flow and walking distance in those with arterial disease (Creager, 2001). Results on the effect of PTX on cerebral blood flow are not consistent; the discrepancies could be ascribed either to the different dosages or routes of administration (Kruuse et al., 2000). Preclinical studies suggest that pentoxifylline and propentofylline reduce neural damage following ischemia (Labs et al., 1997; Teixeira et al., 1997). Similarly, uncontrolled open trials have suggested that PTX may improve stroke outcome in humans (Bath et al., 2000). A recent meta-analysis that included five trials with methylxanthines, administered either intravenously or orally, found insufficient evidence to assess the effectiveness and safety of methylxanthines after acute ischemic stroke (Bath et al., 2000). However, a collaborative group is being formed to further assess the effects of methylxanthine derivatives in stroke patients in view of their multiple pharmacological properties as anti-inflammatories, inhibitors of free radical production, neuroprotectors, vasodilators, and antiplatelet agents (Bath et al., 2000).
Footnotes
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This work was supported by a grant from the University of Milan and Italian Ministry of Education, University and Research (FIRB 2001: Project no. RBNE01BNFK).
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Article, publication date, and citation information can be found at http://jpet.aspetjournals.org.
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doi:10.1124/jpet.104.067090.
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ABBREVIATIONS: PTX, pentoxifylline; SHRSP, spontaneously hypertensive stroke-prone rats; MRI, magnetic resonance imaging; MPO, myeloperoxidase; TBA, thiobarbituric acid; TBARS, TBA reacting substances; MDA, malondialdehyde; TNF-α, tumor necrosis factor-α; IL, interleukin; LPS, lipopolysaccharide.
- Received February 17, 2004.
- Accepted June 15, 2004.
- The American Society for Pharmacology and Experimental Therapeutics