Pyrrolopyrimidines: Novel Brain-Penetrating Antioxidants with Neuroprotective Activity in Brain Injury and Ischemia Models

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Vol. 281, Issue 2, 895-904, 1997

Pyrrolopyrimidines: Novel Brain-Penetrating Antioxidants with Neuroprotective Activity in Brain Injury and Ischemia Models

E. D. Hall, P. K. Andrus, S. L. Smith, T. J. Fleck, H. M. Scherch, B. S. Lutzke, G. A. Sawada, J. S. Althaus, P. F. Vonvoigtlander, G. E. Padbury, P.G. Larson, J. R. Palmer and G. L. Bundy

CNS Diseases Research (E.D.H., P.K.A., S.L.S., T.J.F., H.M.S., B.S.L., J.S.A., P.F.V.), Drug Delivery Systems Research (G.A.S.), Drug Metabolism Research (G.E.P., P.G.L.) and Medicinal Chemistry Research (J.R.P., G.L.B.), Pharmacia & Upjohn, Inc., Kalamazoo, Michigan

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

A novel group of antioxidant compounds, the pyrrolopyrimidines, has been discovered recently. Many of these possess significantlyimproved oral bioavailability (56-70% in rats), increased efficacyand potency in protecting cultured neurons against iron-inducedlipid peroxidative injury and as much as a 5-fold increase inbrain uptake compared with the 21-aminosteroid antioxidant compound,tirilazad mesylate (U-74006F), described earlier. They appearto quench lipid peroxidation reactions by electron-donating and/orradical-trapping mechanisms. Several compounds in the series,such as U-101033E and U-104067F, demonstrate greater ability thantirilazad to protect the hippocampal CA1 region in the gerbiltransient (5-min) forebrain ischemia model. Delaying treatmentuntil 4 hr after the ischemic insult still results in significantCA1 neuronal protection. U-101033E is still effective in salvaginga portion of the CA1 neuronal population when the ischemic durationis extended to 10 min. In addition, U-101033E has been found tobe protective in the context of focal cerebral ischemia, reducinginfarct size in the mouse permanent middle cerebral artery occlusionmodel, in contrast to tirilazad which is minimally effective.These results suggest that antioxidant compounds with improvedbrain parenchymal penetration are better able to limit certaintypes of ischemic brain damage than those which are localizedin the cerebral microvasculature. However, the activity of U-101033Ein improving early post-traumatic recovery in mice subjected tosevere concussive head injury is similar to that of tirilazad.Last, the oral bioavailability of many pyrrolopyrimidines suggeststhat they may be useful for certain chronic neurodegenerativedisorders in which lipid peroxidation plays a role.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

There is now a significant amount of information that supports a role of oxygen radical-induced LP in the pathophysiologyof acute CNS injury and ischemia (Braughler and Hall, 1989; Halland Braughler, 1989; Siesjo et al., 1989). The 21-aminosteroid(lazaroid), tirilazad, has been demonstrated to be a potent inhibitorof LP that acts by a combination of chemical radical scavengingand membrane stabilization mechanisms. It has been shown to reducetraumatic and ischemic damage in several experimental models,and a correlation has been demonstrated between attenuation ofoxygen radical levels and/or LP and the neuroprotective effectin several instances (see review by Hall et al., 1994). Currently,tirilazad is being actively investigated in phase III clinicaltrials in head and spinal cord injury, ischemic stroke and SAH.Results from a multinational European/Australian/New Zealand trialin SAH have demonstrated a highly significant reduction in 3-monthmortality and improvement in the incidence of "Good" recovery(Glasgow Outcome Scale) in patients treated with tirilazad (Kassellet al., 1996).

Tirilazad appears to act, in large part, on the CNS microvascular endothelium (Audus et al., 1991; Raub et al., 1993; Hallet al., 1994) and consequently has been shown to protect the BBB,to maintain cerebral or spinal cord blood flow autoregulatorymechanisms and/or to reduce delayed vasospasm in multiple models(Hall et al., 1994). Therefore, its ability to protect neuraltissue from traumatic or ischemic insult in many models may belargely indirect. Indeed, tirilazad, most likely because of itslimited penetration into brain parenchyma, has generally failedto affect delayed neuronal damage in the selectively vulnerablehippocampal CA1 and striatal regions (Beck and Bielenburg, 1990;Buchan et al., 1992; Sutherland et al., 1993), although it hassome ability to protect cortical neurons (Sutherland et al., 1993).Moreover, in models of permanent focal ischemia in which microvasculareffects may be less important than in temporary ischemia paradigms,the compound's ability to affect infarct size, although demonstratedin some experiments (Beck and Bielenburg, 1991; Park and Hall,1994), has been inconsistent (Xue et al., 1992).

Thus, we reasoned that LP-inhibiting (antioxidant) compounds with improved brain penetration might possess certain advantagesover the microvascularly localized tirilazad in certain CNS injurysituations. Recently, we have discovered a new group of compounds,the pyrrolopyrimidines (fig. 1; Bundy et al., 1995), which areequal or better antioxidants than tirilazad, but with significantlyimproved ability to penetrate the BBB and gain direct access toneural tissue. The present report details the effects of thesein regard to inhibition of iron-dependent lipid peroxidative injuryto cultured mouse spinal cord neurons and neuroprotective activityin models of focal and global cerebral ischemia and concussivehead injury.

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Fig. 1. Chemical structures of the 21-aminosteroid or "lazaroid" tirilazad (U-74006) and selected pyrrolopyrimidines. Tirilazad isa nonglucocorticoid 21-aminosteroid. The primary chemical antioxidantportion of the molecule is the amino moiety bound to the 21 positionof the steroid side chain. Physicochemical studies indicate thatthe highly lipophilic (i.e., hydrophobic) steroid moiety orientsitself within the fatty acid core of the membrane and is largelyresponsible for the high affinity of the compound for cell (e.g.,endothelium) membranes (Hall et al., 1994

). The more hydrophilicamino substitution exists closer to the surface in juxtapositionto the phosphate head groups of the phospholipids. In contrast,the pyrrolopyrimidines lack the highly lipophilic steroid moiety,but bear some structural resemblance to the bis-pyrrolidinylpyrimidinylpiperazine 21-amino substitution of tirilazad. Lack of the steroidserves to lessen the high affinity for and retention in lipidbilayers.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

All experiments received prior approval by the Institutional Animal Use and Care Committee of Pharmacia & Upjohn, Inc. toensure that they were performed in strict compliance with theNational Institutes of Health Guide for the Care and Use of LaboratoryAnimals.

Iron-dependent lipid peroxidative injury to cultured fetal mouse spinal neurons. Fetal mouse spinal neurons were cultured as described previously (Hall et al., 1991). Spinal neurons were dissected from 13-to 15-day-old embryos of CD-1 virus-free mice. The tissue waschemically and mechanically dissociated. The cells were resuspendedin minimum essential media plus additional nutrients and transferredto 24-well, Falcon Primaria culture plates. The cells were platedat a density of approximately 6 × 10⁵/ml (total volume in well, 1 ml). Plates were maintained at 35°Cin 8% CO₂/95% humidity. Cytosine arabinoside was added at a finalconcentration of 5 µM on day 6 and removed on day 8. Assays wererun on day 15.

Test compounds were dissolved in dimethyl sulfoxide in a 10 mM concentration. They were then diluted to a concentration of100 µM in a solution of fatty acid-free bovine serum albumin inphosphate-buffered saline (30 mg/ml). With use of this stock solution,the compounds were added to the cultures to obtain final concentrationsranging from 0.3 to 100 µM. After 1 hr, the medium containingthe test compound was removed and replaced with degassed, argon-purgedKrebs' buffer containing 5.55 mM glucose and 200 µM ferrous ammoniumsulfate. After 40 min of exposure to the iron-containing medium,viability of the neurons was assessed by uptake of [³H]- $alpha$ -(methylamino)isobutyric acid as described previously (Buxserand Bonventre, 1981

; Hall et al., 1991

). The data represent theuptake (cpm) in iron-exposed cultures as a mean % of parallelnon-iron-exposed cultures. All the determinations were run intriplicate wells for each drug concentration.

Determination of oxidation potential. Electrochemical oxidation followed by HPLC with UV detection was used to study the oxidation potential of the test compounds.The mobile phase consisted of 89% water, 10% methanol and 1% ammoniumacetate. A 10-µl solution (0.3 µg/µl) was injected onto an HPLCsystem. At 1 ml/min, the mobile phase flowed into an ESA (MilliporeCorp.; Milford, MA) guard cell. The guard cell was set at electrochemicalpotentials ranging between 0 and 1000 mV. Next, the mobile phaseflowed into a Waters (Chelmsford, MA) C8 symmetry column whereoxidative by-products could be separated. Flow carried columneffluent into a UV detector that monitored light absorption at230 nm. For each sample, 1 ng of pyrrolopyrimidine was injectedonto the column. One minute after injection, the electrochemicalpotential across the guard cell was turned off until the nextinjection. During this 1-min period of electrochemical oxidation,electrical current output was observed to increase rapidly andthen diminish to base line. The magnitude of current output wasdirectly proportional to the electrochemical potential setting.This suggests that the pyrrolopyrimidines were oxidized in proportionto voltage across the guard cell. Quantitation of the test compoundwas based on the area of peaks which co-eluted with a nonoxidizedsample of the test compound. Peak areas associated with oxidationwere normalized to a peak that was measured under conditions wherethe test compound was not oxidized. The potential that resultedin a 50% loss of starting material was determined.

Determination of brain uptake in mice. Female CF-1 mice (Charles River; Portage, MI) were injected via a tail vein with 23 µmol/kg (approximately 10 mg/kg) of testcompound in propylene glycol (5 mg/ml). At either 5 or 60 minafter the dose, the mice were deeply anesthetized with methoxyfluranefollowed by intracardiac perfusion with 10 ml of 0.9% saline.The brain samples were placed in a volume of acetonitrile equalto five times the brain weight and kept on ice during processing.The samples were sonicated for 20 sec, followed by centrifugationat 2060 × g for 15 min at 4°C. The supernatants were analyzedby HPLC on a reverse phase column (Zorbax SB-CN, 250 × 4.6 mm,5 µm particle size, Dupont, Chadds Ford, PA) with an autoinjector(Perkin Elmer ISS 100) with 100-µl injections and a flow rateof 1 ml/min. The isocratic mobile phase used consisted of variousproportions of 100:1 (v/v) acetonitrile/trifluoroacetic acid and100:0.115 (v/v) water/trifluoroacetic acid. UV detection (AppliedBiosystems Spectroflow 783 Foster City, CA) was used for all compounds.However, fluorescence detection (Applied Biosystems 980) was foundto be more sensitive for quantifying some of the pyrrolopyrimidinecompounds, with excitation set at 320 nm and an emission cutofffilter at 389 nm. For others that were not fluorescent, electrochemicaldetection (Waters 460 with a glassy carbon electrode and Ag/AgClreference electrode) was used at 700 mV.

Other mice were sacrificed, but not perfused. In these, the harvested, unperfused brains were bisected medially and fixedin 10% buffered formalin for 10 to 20 min at 25°C. The tissueswere then frozen and 7-µm-thick cryosections were quickly dried,coverslipped and viewed by confocal scanning laser microscopyat 4°C. Sections excited with a 100-mW laser at 352 to 358 nmemitted fluorescence between 457 and 600 nm. The fluorescenceintensity was transformed into a pseudo-color image.

Determination of oral bioavailability in rats. Male Sprague-Dawley rats (Charles River; Portage, MI) weighing 250 to 300 g were surgically implanted with a dosing/samplingcannula in their superior vena cava and allowed a 1-week recoveryperiod. The animals had access to water ad libitum and were fastedovernight before and for 4 hr after each treatment. Three animalswere used for the determination of oral bioavailability. Theywere administered approximately a 10 mg/kg i.v. bolus and a 25mg/kg oral solution by gavage in a cross-over design, with a minimumof a week between doses. Serial blood samples (250 µl) were obtainedat defined time points from before dosing through 48 hr postdosing.

After centrifugation (14,000 × g for 3-4 min) of the blood samples, a 100-µl aliquot of plasma was transferred to a 1.5-mltube and plasma proteins precipitated with 0.5 ml of acetonitrilecontaining an internal standard. After vortexing and recentrifugation,the supernatant was transferred to an injection vial and 100 µlinjected into the HPLC. The prepared samples were chromatographedon a Zorbax RX-C8 reversed phase column (4.6 mm inside diameter× 250 mm, 5-µm particle size) with a Brownlee RP-8 Newguard (3.2mm inside diameter × 15 mm, 7-µm particle size) guard column.The mobile phase consisted of 65 to 72% (v/v) acetonitrile and35 to 28% water containing 0.3% (v/v) triethylamine and adjustedto pH 5 with glacial acetic acid, and was delivered at a flowrate of 1 ml/min. The column effluent was monitored by UV detectionat a wavelength of 250 nm. Concentration of the test compoundwas determined by calculating the ratio of the peak height forthe test compound to that for an internal standard and by comparingthe ratio to a linear standard curve.

Oral bioavailability was calculated by dividing the integrated area under the 48-hr plasma elimination curve after oral dosingby the area under the curve after i.v. dosing, correcting firstfor the fact that a 2.5 times higher dose was used for the oraladministration.

Gerbil forebrain ischemia model. Male Mongolian gerbils (Tumblebrook Farms; West Brookfield, MA) weighing 45 to 55 g were anesthetized with methoxyflurane.A 1- to 2-cm midline throat incision provided access to both carotidarteries, which were occluded with microaneurysm clips. After5 min of near-complete ischemia, the clips were removed and reperfusionallowed for 5 days. The animals were placed in a warming box withan ambient temperature maintained at 37°C during the ischemicinsult and then until the animals regained their righting reflexafter reperfusion. Previous studies from this laboratory havedemonstrated that this warming procedure successfully maintainsboth rectal and brain temperatures of the animals at 35.5°C whilethe animals are kept in the chamber (Hall et al., 1993). Typically,the test compound was administered p.o. (3, 10 or 30 mg/kg) 30min before induction of ischemia and again at 2 hr after reperfusion,followed by additional single oral doses at 24, 48 and 72 hr.The concentration of drug in the vehicle (40% hydroxypropyl cyclodextrin)was adjusted such that the oral administration volume was heldconstant at 0.1 ml.

After 5 days, the animals were deeply re-anesthetized with methoxyflurane and perfused intracardially with phosphate-bufferedsaline (pH 7.2) until the effluent was cleared of blood (2 min),followed by perfusion with 10% formaldehyde, 10% acetic acid and80% methanol (FAM). The brains were removed and stored overnightin FAM. They were then blocked and embedded in paraffin. Five-micron-thickcross-sections were taken through the dorsal hippocampus (1.4-3.0mm posterior to Bregma), mounted on gelatin-coated slides andstained with cresyl violet (Hall and Pazara, 1988

). The numberof hippocampal CA1 neurons was counted under light microscopy(magnification ×320). All normal-appearing CA1 pyramidal neuronsin a 315-µ length of the CA1 region were counted bilaterally andaveraged. Two sections were examined per animal and the countsaveraged. Animals which showed significant asymmetry in regardto the CA1 neuronal counts (>50% difference between hemispheres)were discarded. All analyses were carried out in a blinded fashionin relation to the identification of vehicle versus pyrrolopyrimidine-treatedgerbils.

All data were expressed as mean ± standard error. Statistical evaluation was performed by an analysis of variance, followedby a Student's t test with Bonferroni correction for multiplecomparisons (i.e., three dose groups or three treatment initiationtimes).

Mouse focal cerebral ischemia model. Male CD-1 mice (Charles River; Portage, MI), weighing 18 to 22 g, were used. They had access to water and chow ad libitum.Under methoxyflurane anesthesia, an incision was made over thetemporoparietal region, and the skull was exposed by retractionof the musculature and parietal gland. A small burr hole exposedthe MCA. The MCA was cauterized in two places 2 mm apart and thencut, just above the origin of the lenticulostriate arteries byuse of bipolar diathermy.

At 5 min and again at 60 min postocclusion, the mice received an i.v. (tail vein) injection of vehicle (0.02 M citric acid)or test compound (0.03, 0.1, 0.3, 1.0 or 3.0 mg/kg). The injectionvolume was kept constant at 0.05 ml.

At 6 hr postocclusion, the mice were re-anesthetized and perfused intracardially with 5 ml of a 4% solution of 2,3,5-triphenyltetrazoliumchloride and brains removed and fixed overnight in 10% bufferedformalin at room temperature in the dark. After the overnightfixation, the brains were cross-sectioned into eight 2-mm slices.The most anterior and posterior sections were discarded. The remainingsix sections were placed in a 6-well culture dish and each coveredwith distilled water to prevent drying. 2,3,5-Triphenyltetrazoliumchloride reacts with mitochondrial cytochrome oxidases in viabletissue and produces a deep red color, whereas the infarcted, deadtissue does not stain. With an Image 1 Analysis System (UniversalImaging Corporation; West Chester, PA), the infarct area of eachbrain slice was quantitated and expressed as a percent of thetotal area. The percent infarct areas were averaged to give anestimate of the total infarct volume per brain.

Differences between infarct size were compared between vehicle- and U-101033E-treated mice by analysis of variance, followedby Student's t test (two-tailed).

Mouse head injury model. Details of the mouse head injury model have been published in detail elsewhere (Hall et al., 1988). Male CF-1 mice (CharlesRiver; Portage, MI) weighing 17 to 20 g were used. Each mousethat survived the injury received vehicle (0.05 N HCl) or testdrug in a 0.1-ml volume as an i.v. bolus within 5 min postinjury.Groups of 20 to 25 mice were injured in rapid succession. Eachtrial was carried out in a blinded fashion, with a vehicle groupand three groups receiving either 0.1, 1 or 10 mg/kg of test compound.

At 1 hr postinjury, the neurological status of the injured mice was blindly evaluated by a grip test. The mean time that theinjured mice could remain on the grip string was measured (30sec maximum), and comparisons between vehicle- and drug-treatedmice made with an analysis of variance followed by Student's ttest (two-tailed).

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Comparison of inhibition of iron-dependent lipid peroxidative neuronal injury. Table 1 shows the IC₅₀ values and maximum percent protection of cultured fetal mouse spinal neurons from iron-induced lipidperoxidative injury (system described in detail elsewhere; Hallet al., 1991; Zhang et al., 1996) for tirilazad and the pyrrolopyrimidines.Protection of cellular viability was measured in terms of preservationof amino acid uptake (i.e., uptake of ³H-aminoisobutyric acid) as described and validated by Buxser andBonventre (1981). As seen, the pyrrolopyrimidines are consistentlymore potent and efficacious in this in vitro model. Figure 2 showsfull concentration-response graphs for the pyrrolopyrimidinesU-89843E and U-101033E versus tirilazad (U-74006F). U-89843D,and even more so U-101033E, are more potent and more efficaciousthan U-74006F. Figure 3 shows similar graphs for U-104067E andits para-hydroxylated metabolite U-106311E. U-106311E is significantlymore potent and efficacious than U-104067E, which has a concentration-responserelationship quite similar to that of U-74006F (compare with fig.2). It should be noted that neither tirilazad nor any of the pyrrolopyrimidinesaffected the base-line level of ³H-aminoisobutyric acid uptake (i.e., in the absence of iron; datanot shown).

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TABLE 1
Comparison of the potency and efficacy of U-74006F and selected pyrrolopyrimidines in regard to protection against lipid peroxidativeimpairment of viability (i.e., attenuation of ³H-AIB uptake) in cultured fetal mouse spinal neurons by 200 µMferrous ammonium sulfate application for 40 min
Cultures were pretreated with test compound in varying concentrations for 1 hr. The medium containing the compound was thenremoved, and the treated cultures were exposed to 200 µM ferrousammonium sulfate for 1 hr, followed by determination of ³H-AIB uptake. Potentials required to oxidize 50% of the test compoundwere determined as described under "Methods."

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Fig. 2. Protection of the viability (uptake of ³H-AIB) of cultured fetal mouse spinal cord neurons against iron-induced lipid peroxidativeinjury by tirilazad (U-74006F) or the three pyrrolopyrimidinesU-89843E, U-94430E or U-101033E. Values are means ± standard errorfor triplicate determinations. Cultures were pretreated with testcompound in varying concentrations for 1 hr. The medium containingthe compound was then removed and the treated cultures exposedto 200 µM ferrous ammonium sulfate for 40 min, followed by determinationof ³H-AIB uptake. The absolute level of uptake-related radioactivityin iron-exposed, non-drug-treated cultures ranged from 729 ± 65to 1640 ± 238 cpm. CON, control.

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Fig. 3. Protection of the viability (uptake of ³H-AIB) cultured fetal mouse spinal cord neurons against iron-induced lipid peroxidativeinjury by the pyrrolopyrimidines U-104067F or U-106311E. Valuesare means ± standard error for triplicate determinations. Cultureswere pretreated with test compound in varying concentrations for1 hr. The medium containing the compound was then removed andthe treated cultures were exposed to 200 µM ferrous ammonium sulfatefor 40 min, followed by determination of ³H-AIB uptake. The absolute level of uptake-related radioactivityin iron-exposed, non-drug-treated cultures ranged from 483 ± 30to 3629 ± 987 cpm. CON, control.

Figure 4 presents the hypothetical antioxidant (i.e., LP-inhibiting) mechanisms of the pyrrolopyrimidines. Mechanism I, relatingto U-87663, U-89843, U-94430 and U-101033, involves a scenarioof initial electron donation and consequent quenching of eithera lipid alkoxyl (LO·), lipid peroxyl (LOO·) or hydroxyl (·OH)radical followed by peroxyl radical trapping. Circumstantial evidencefor the intermediacy of radical cations I and II in the reactionof the pyrrolopyrimidines with lipid peroxides is provided bypreparative scale electrochemical experiments. Electrochemicaloxidation of U-87663 under very mild conditions, in either methanolor acetic acid, affords the chemically labile 5-methoxy and 5-acetoxyderivatives, respectively, in good yield (data not shown). Theseproducts are therefore rationalized by invoking solvent captureof radical cations I and II. Further evidence is provided by thefinding that chemical oxidation of U-87663 under radical cation-producingconditions (e.g., benzoyl peroxide) provides the corresponding5-benzoyloxy derivative, presumably via a similar mechanism. Incontrast, mechanism II requires the metabolic para-hydroxylationof U-104067 to U-106311, which can then act as a phenolic-likeperoxyl radical scavenger. The significant, albeit less potentand less efficacious, antioxidant neuroprotective action of theparent compound, U-104067, is likely caused by a physicochemicalmembrane-stabilizing mechanism that is perhaps similar to thatdemonstrated for U-74006F (Hall et al., 1994

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Fig. 4. Probable antioxidant mechanisms of the pyrrolopyrimidines. Antioxidant mechanism I, which is relevant to U-87663, U-89843,U-94430 and U-101033, involves reaction of an alkoxyl (LO·), peroxyl(LOO·) or hydroxyl (·OH) radical in which the pyrrolidine nitrogenquenches the radical species via the transfer of an electron.The pyrrolopyrimidine, in turn, becomes a radical cation. Thecationic center is transferred to the 5-position of the pyrrolopyrimidinewhich can then react with (i.e., trap) a second radical species,most likely a peroxyl radical. This particular scenario is unlikelyin U-104067. Rather, its antioxidant capacity is probably dependenton para-hydroxylation of the aromatic ring, resulting in a phenolic-typeelectron-donating antioxidant (U-106311). Indeed, U-106311 hasa much lower oxidation potential than U-104067 (see table 1).

Comparison of brain uptake. The comparative brain uptake of tirilazad (U-74006F) and the pyrrolopyrimidines in mice after i.v. administration of molarequivalent doses (approximately 10 mg/kg) is shown in figure 5.Each of the pyrrolopyrimidines produced significantly higher brainlevels 5 min after injection compared with tirilazad. For U-87663E,U-89843E, U-94430E, U-101033E and U-104067F, the brain levelsat the initial time point were 4.7, 3.2, 3.7, 2.8 and 5.1 timeshigher, respectively, than the levels of tirilazad. For U-87663E,the brain levels were still 2.3 times higher than tirilazad at60 min postinjection. It is also clear that the brain levels seemto fall off faster for the pyrrolopyrimidines as a further reflectionof their greater membrane permeabilities (Sawada et al., 1995a,b). In other words, they diffuse into the brain and, in the absenceof repeated dosing, they may diffuse out of the brain more quicklythan tirilazad. Additionally, we have taken advantage of the intrinsicfluorescent properties of U-87663E to demonstrate unequivocallyby fluorescence microscopy that this prototype pyrrolopyrimidineefficiently penetrates the BBB in mice after i.v. dosing (fig.6). Moreover, it concentrates in brain parenchyma and not thecerebrovascular endothelium (fig. 6, inset).

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Fig. 5. Comparison of the mouse brain levels of U-74006F and selected pyrrolopyrimidines at 5 or 60 min after a 23 µM/kg (approximately10 mg/kg) i.v. bolus. Mice were perfused with saline at sacrificeto eliminate any contribution of blood to the measured levels.Values are means ± standard error for n = 3. Asterisk indicatesP < .05 versus U-74006F at the same time point.

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Fig. 6. Low magnification fluorescence photomicrograph of a slice of mouse cerebral cortex, with dura mater intact, showing penetrationof the pyrrolopyrimidine U-87663 into brain parenchyma after a23 µM/kg (approximate 10 mg/kg) i.v. bolus. The color scale showsrelative drug-associated fluorescence pseudocolor intensity (white= highest concentration). The black holes represent brain microvessels.The circular structure on the right is a pial artery. Note thatvessel walls show relatively low drug-related fluorescence comparedto parenchyma (higher magnification inset).

Comparison of oral bioavailability. Table 2 shows the comparative oral bioavailability and terminal plasma half-lives of tirilazad (U-74006F) versus severalpyrrolopyrimidines. The bioavailability of the included pyrrolopyrimidinesranges from a low of 20.7% (U-106311E) to a high of 84.6% (U-89843E).The terminal half-lives range from 2.7 hr (U-106311E) to 22.1hr (U-87663E). These values are considerably higher than thosefor the 21-aminosteroid U-74006F.

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TABLE 2
Oral bioavailability and terminal plasma half-lives of tirilazad (U-74006F) and pyrrolopyrimidines in Sprague-Dawley rats

Pyrrolopyrimidine neuronal protection in transient forebrain ischemia. As noted above, tirilazad has been demonstrated to have very limited ability to attenuate selective hippocampal CA1 vulnerabilityin models of transient forebrain ischemia (Beck and Bielenburg,1990; Buchan et al., 1992; Sutherland et al., 1993). This is mostlikely caused by its limited BBB penetration in the context ofmodels where BBB permeability is minimally compromised. In contrast,figure 7 illustrates that oral preischemic treatment (plus repeatedpostreperfusion treatment) with any of the BBB-permeable pyrrolopyrimidines(U-94430E, U-101033E and U-104067F) produces significantly moreCA1 neuronal protection than that observed in vehicle-treatedanimals. Figure 8 shows the dose-response curve for the abilityof U-101033E to protect the CA1 region. Dose levels of 10 or 30mg/kg (×5) are significantly effective, but doses as low as 1and 3 mg/kg appear to have some effect. Figure 9 displays thetherapeutic window for the efficacy of U-101033E in regard toCA1 protection in the gerbil 5-min forebrain ischemia model. Theinitiation of dosing 30 min before ischemia (plus repeated postreperfusiondosing) is the most effective. However, a delay in dosing to 4hr after reperfusion still provides a statistically significantneuroprotective effect.

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Fig. 7. Attenuation of hippocampal CA1 neuronal loss of the pyrrolopyrimidines U-94430E, U-101033E and U-104067F at 5 days after a5-min episode of bilateral carotid occlusion in male Mongoliangerbils. n = 10 animals/group. Gerbils were dosed with 30 mg/kgp.o. preischemia plus 2 hr after reperfusion and once daily ondays 2, 3 and 4. Asterisk indicates P < .05 versus the vehicle-treatedgroup (Veh).

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Fig. 8. Dose response for the effect of U-101033E to salvage hippocampal CA1 neurons at 5 days after a 5-min episode of bilateralcarotid occlusion in male Mongolian gerbils. n = 10 animals/group.Gerbils were dosed with each dose level p.o. preischemia plus2 hr after reperfusion and once daily on days 2, 3 and 4. Asteriskindicates P < .05 versus the vehicle-treated group (Veh).

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Fig. 9. Therapeutic window for the effect of U-101033E to salvage hippocampal CA1 neurons at 5 days after a 5-min episode of bilateralcarotid occlusion in male Mongolian gerbils. n = 10 animals/group.Gerbils were dosed beginning at each time point with 30 mg/kgp.o. plus 2 hr later and on the subsequent days. Asterisk indicatesP < .05 versus the vehicle-treated group (Veh).

Pyrrolopyrimidine neuroprotection in permanent focal ischemia. U-101033E has also been examined for the ability to limit brain infarct volume in mice subjected to permanent MCA occlusion.Mice received two doses of test compound, one at 5 min and a secondat 60 min postocclusion. As observed in figure 10, U-101033E potentlyreduced infarct volume by as much as 27% at a dose of only 0.1mg/kg (×2) i.v. In addition, U-87663E and U-89843E have also beenfound to be significantly effective in the mouse permanent MCAocclusion model, whereas tirilazad (0.1-3.0 mg/kg × 2) has shownonly nonsignificant trends toward infarct reduction (data notshown).

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Fig. 10. Dose-response for U-101033E reduction of 6 hr infarct size in male CF-1 mice subjected to permanent unilateral occlusion ofthe right MCA. The mice received one dose of compound i.v. at5 min postocclusion and a second dose at 1 hr. Values are percentreduction in mean infarct volume (summation of eight cross-sectionsthrough the infarct) compared with a vehicle-treated group ofanimals. n = 8 to 13 animals/group. Asterisk indicates P < .05versus vehicle.

Pyrrolopyrimidine enhancement of early neurological recovery in brain-injured mice. Figure 11 demonstrates the ability of acutely administered (5 min postinjury) intravenous U-101033E to enhance the early (1hr) neurological recovery of male CF-1 mice subjected to a severeconcussive head injury. A dose-related effect is seen over therange of 0.1 to 10 mg/kg. A similar magnitude of effect has beenreported for several other pyrrolopyrimidines (Bundy et al., 1995)and for tirilazad (Hall et al., 1988, 1992).

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Fig. 11. Dose-response for the effect of U-101033E to improve the early (1 hr) neurological recovery of male CF-1 mice after a severeconcussive head injury. n = 6 to 9 mice in the U-101033E-treatedgroups and 23 mice in the vehicle-treated group (V). The dataare presented as percent decrease in infarct size. However, thestatistical analysis was actually performed using the raw percentinfarct size values.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

This report describes a novel group of potent inhibitors of iron-dependent LP in neural tissue, the pyrrolopyrimidines (e.g.,U-87663E, U-89843D, U-101033E). Members of the series have alsobeen reported to inhibit in vitro neuronal injury by peroxynitrite(Fici et al., 1996). With both iron and peroxynitrite-inducedcellular injury, the pyrrolopyrimidines show increased potencyand efficacy compared with the 21-aminosteroid tirilazad. In addition,the pyrrolopyrimidines possess improved BBB permeability and brainparenchymal penetration compared with tirilazad which remainslargely localized in the cerebral microvascular endothelium (Raubet al., 1993; Hall et al., 1994). In previously reported experiments,the comparative brain uptake of tirilazad and selected pyrrolopyrimidineshas also been evaluated in rats in terms of first-pass extractionof radiolabeled compounds after intracarotid injection (Sawadaet al., 1995b; Hall et al., 1995). With this technique, tirilazadis only 6% extracted, which is not much better than the extractionof sucrose or thiourea to which the BBB is essentially nonpermeable.In contrast, the pyrrolopyrimidine U-87663E is 83% extracted onthe first pass through the cerebral circulation, and U-89843Eis 88% extracted. These extraction values are very near that measuredfor the freely BBB-diffusible butanol. Thus, the pyrrolopyrimidinesappear to permeate the BBB quite readily. Confocal laser microscopyhas also been used to show that U-87663E readily gains accessto the intracellular space of cultured cells (Sawada et al., 1995a,b). As a result of the greater brain and perhaps intracellularpenetration, compounds like U-101033E have neuroprotective efficacyin attenuating selective neuronal damage in highly vulnerableregions, such as the CA1 area of the hippocampus, after a transientepisode of forebrain ischemia. In contrast, tirilazad is largelyineffective in salvaging CA1 neurons in rodent forebrain ischemiaparadigms (Beck and Bielenburg, 1990; Buchan et al., 1992; Sutherlandet al., 1993; Hall et al., 1995).

Other purportedly brain-penetrable antioxidants have been described previously with neuroprotective efficacy in transientforebrain ischemia models in either gerbils or rats, includingLY-178002 (Clemens et al., 1991), PBN (Phillis and Clough-Helfman,1990) and dimethylthiourea (Pahlmark et al., 1993). However, muchhigher doses of all of these compounds are required to achieveneuroprotection, whereas U-101033E is significantly effectiveat oral dose levels as low as 10 mg/kg. This suggests that theseearlier described and studied compounds either may not be as brain-penetrableas thought or perhaps they are not as effective in attenuatingoxygen radical-induced, iron-catalyzed LP as the pyrrolopyrimidines.In addition, U-101033E has been shown to have at least a 4-hrpostischemic therapeutic window. In contrast, PBN $'$ s ability toprotect CA1 neurons in the identical gerbil forebrain ischemiamodel, which requires higher mg/kg doses (100 mg/kg) than thosepresently used, is lost by 2 hr after reperfusion (Phillis andClough-Helfman, 1990). Nevertheless, further study of U-101033Eand other pyrrolopyrimidines is necessary before an exact assessmentof their neuroprotective potency and efficacy can be establishedin comparison with the earlier described antioxidant compounds.

The pyrrolopyrimidines similarly outperform tirilazad in the context of permanent focal cerebral ischemia. In the face ofpermanent vascular occlusion, a successful neuroprotective compoundmust intuitively be able to penetrate the underperfused ischemicpenumbral zone to be optimally effective in salvaging the stillviable, but potentially doomed, neural tissue. Although not directlydetermined in the current study, it is likely that U-101033E isable to penetrate the ischemic penumbra more effectively thanthe microvascularly localized tirilazad. Although tirilazad hasbeen reported to reduce infarct volume in the setting of permanentMCA occlusion in Sprague-Dawley (Park and Hall, 1994) and Fischer(Beck and Bielenburg, 1991) rats, it has not been shown to beefficacious in the same model in the spontaneously hypertensiverat strain (Xue et al., 1992). Likewise, tirilazad is only marginallyeffective in the mouse permanent MCA model (Hall et al., 1995).Similarly, another antioxidant, dihydrolipoate, has not shownactivity in the mouse permanent MCA occlusion model (Prehn etal., 1992). In contrast, the nitrone spin-trapping agent PBN iseffective in reducing infarct size in the rat permanent MCA occlusionmodel although high doses (100 mg/kg i.p.) are required (Cao andPhillis, 1994). However, PBN $'$ s protective efficacy in the mousemodel has not been evaluated.

A greater efficacy of the pyrrolopyrimidines has also been seen in the context of temporary focal ischemia. Rats subjectedto 90 min of MCA occlusion showed a 47% smaller brain infarct7 days later when pretreated with a 3 mg/kg i.v. dose of U-101033E,plus 3 mg/kg i.v. 15 min before and 1 hr after reperfusion. Equivalentdosing with the 21-aminosteroid U-74389G (16-desmethyl tirilazad)only achieved a 17% mean infarct size reduction, which was notstatistically significant. U-101033E, but not U-74389G, also improvedearly postreperfusion neurological recovery (Schmid-Elsaesseret al., 1996). Similarly, PBN has been reported to reduce infarctsize significantly in the rat temporary MCA occlusion model (Zhaoet al., 1994).

Interestingly, in regards to severe concussive brain injury, the degree of acute neurological recovery enhancement observedwith U-101033E is similar to, but not greater than, that reportedfor tirilazad (Hall et al., 1988, 1992). However, in the mouseconcussive injury model, significant BBB disruption is observedas early as 5 min postinjury (Hall et al., 1992). Thus, tirilazadis better able to penetrate into brain parenchyma and thereforegain access to the endangered central neurons, perhaps as wellas U-101033E. Indeed, the uptake of tirilazad is greater in injuredthan in noninjured mouse brain (Hall et al., 1992). Nevertheless,despite this greater posttraumatic BBB penetration, much of tirilazad'sneuroprotective action may still be mediated at the microvascularlevel (Hall et al., 1994). Secondary microvascular damage in braininjury, and its potential attenuation by the microvascularly localizedtirilazad, may be as important as parenchymal neuronal injurymechanisms which would be most efficiently countered by the brain-penetrablepyrrolopyrimidines. In any event, it will be interesting to investigatethe combination of tirilazad, which is largely localized in thebrain microvascular endothelium (Audus et al., 1991; Raub et al.,1993; Hall et al., 1994), with U-101033E, which permeates thevascular wall and exerts direct neuroprotection. Although it islikely that, within the overall spectrum of traumatic and ischemicCNS insults, antioxidant compounds that localize in brain microvasculatureor that penetrate the brain parenchyma will have specific therapeuticroles to play, in some cases they may be complementary.

It has been increasingly recognized that oxygen radical-induced neuronal damage may also have an important role in the pathogenesisof the major chronic neurodegenerative diseases. These includeamyotrophic lateral sclerosis (Rosen et al., 1993; Gurney et al.,1996), Parkinson's disease (Cohen, 1986; Jenner et al., 1992;Youdim et al., 1993) and Alzheimer's disease (Subbarao et al.,1990; Smith et al., 1994). Thus, the pyrrolopyrimidines may beuseful in slowing the progression of these disorders by virtueof their excellent oral bioavailability, brain penetrability andantioxidant neuroprotective efficacy.

	Footnotes

Accepted for publication January 30, 1997.

Received for publication September 16, 1996.

Send reprint requests to: Edward D. Hall, Ph.D., CNS Diseases Research 7251-209-407, Pharmacia & Upjohn, Inc., Kalamazoo, MI 49001.

	Abbreviations

LP, lipid peroxidation; SAH, subarachnoid hemorrhage; BBB, blood-brain barrier; MCA, middle cerebral artery; PBN, N-tert-butyl- $alpha$ -phenylnitrone; HPLC, high-performance liquid chromatography; CNS, central nervous system; ³H-AIB, [³H]- $alpha$ (methylamino)isobutyric acid.

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