Amelioration of ischemia-reperfusion injury with cyclic peptide blockade of ICAM-1

doi:10.1152/ajpheart.00840.2002

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Amelioration of ischemia-reperfusion injury with cyclic peptide blockade of ICAM-1

Shakil H. Merchant, Debbie M. Gurule, and Richard S. Larson

Department of Pathology, University of New Mexico Health Science Center, Albuquerque, New Mexico 87131

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Neutrophils are pivotal in the pathogenesis of ischemia-reperfusion (I/R) injury leading to muscle damage. Firm adhesion ofneutrophils to the endothelium is initiated by an interactionbetween intercellular adhesion molecular-1 (ICAM-1) on the endotheliumand $beta$ ₂-integrins on neutrophils. Inhibition of ICAM-1-dependentbinding using monoclonal antibodies has been shown to be efficaciousin ameliorating I/R injury by preventing the influx of neutrophilsinto the ischemic tissue. We recently described a cyclic peptidethat is a potent and selective inhibitor of ICAM-1 (IP25) in vitro.In this study, we tested the hypothesis that IP25-mediated blockadeof ICAM-1 would inhibit neutrophil influx during reperfusion ofischemic tissue and consequently attenuate muscle injury in atourniquet hindlimb murine model of I/R injury. Varying amountsof peptide drug were injected at the beginning of the reperfusionperiod. The neutrophil influx and size of infarction at the endof 2 h of reperfusion were compared with those in untreated controlmice and contralateral nonischemic limbs. Mice receiving IP25immediately before reperfusion showed a 56% reduction in neutrophilinfiltration in the ischemic muscle, accompanied by a 40% reductionin the infarct size. No effect on I/R injury was seen if IP25administration was delayed for 60 min after reperfusion. We concludethat IP25 effectively inhibits ICAM-1-mediated adhesion of neutrophilsto the endothelium in mice leading to a protective effect andsuggests that synthetic peptide antagonists have a potential roleas therapeutictools.

infarction; peptide antagonist; cell adhesion

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

PROLONGED INTERRUPTION of the blood supply to the heart results in cell death and irreversible tissue damage (15, 16,37, 47). In myocardial ischemia, there is a direct correlationbetween the amount of tissue necrosis and the prognosis of thepatient (16). Salvage of the ischemic tissue depends on earlyreperfusion. However, there is evidence that reperfusion leadsto a series of events that significantly worsens the tissue injury(15, 47). Reperfusion injury after ischemia [ischemia-reperfusion(I/R) injury] determines the outcome in several clinical scenariosincluding myocardial infarction, stroke, organ transplant, andskeletal muscle ischemia during abdominal aortic aneurysm surgery(15, 20, 22, 38, 43, 47). A sizable number of observationsindicate that neutrophils [polymorphonuclear cells (PMNs)] playa pathogenetic role in tissue damage after ischemia and reperfusion,including the observations that treatment with monoclonal antibodies(MAb) that inhibit neutrophil (PMNs) activation or influx intothe myocardium result in a significant decrease in the size ofinfarction in experimental animals (8-10, 21, 31, 33, 40-42).

Increased PMN adhesiveness to the endothelium appears to be a critical step early in the sequence of events leading to I/Rinjury. PMN extravasation is dependent on increased adhesive interactionsbetween PMNs and the vascular endothelial cell surface, togetherwith the decreased shear force produced by vascular leakinessat sites of inflammation. Coordinated expression and usage ofadhesion molecules results in physiological events that lead toPMN localization to a tissue or organ (3, 23, 26, 33).Members of the selectin family present on PMNs (L-selectin) andendothelial cells (P-selectin and E-selectin) initially mediatethe transition from rapid flow to rolling (1, 3, 23, 25,55). The loosely interacting (rolling) PMNs are then activatedby chemokines to a more adhesive state (arrest), making the cellmore resistant to being sheared off the endothelial lining bylocal microhemodynamic shear forces. Initial in vitro observationshave suggested that the arrest and transmigration of PMNs wasmediated by two members of the $beta$ ₂-integrin family [LFA-1 (CD11a/CD18)and Mac-1(CD11b/CD18)] binding to intercellular adhesion molecule-1(ICAM-1) on endothelial cells (33). However, more recent evidencesuggests that LFA-1 binding to ICAM-1 alone is sufficient forPMN emigration, because MAb directed at the LFA-1 $alpha$ -subunit completelyblock hypoxia-induced adhesion of neutrophils to endothelial cells(49, 50). Furthermore, PMN from mice genetically deficientin ICAM-1 or LFA-1, but not Mac-1, will not extravasate efficientlyduring inflammatory processes, and I/R injury is ameliorated inthese animals (13, 33, 49).

Currently, effective intervention strategies for modulating clinically relevant I/R injury do not exist. Yet, pharmacologicalmodulation of the reperfusion injury may be beneficial in severalscenarios, including reducing myocardial infarct size. Severalinvestigators have shown that MAb directed against ICAM-1 or $beta$ ₂-integrinreduce PMN infiltration and consequently infarct size in experimentalanimals (26, 28, 29, 49, 50, 54). However, anaphylacticreactions and secondary physiological effects have hampered theclinical use of these antibodies in humans. Thus we have recentlydeveloped a small peptide antagonist of ICAM-1 that inhibits ICAM-1/LFA-1-dependentcell adhesion. An initial weaker nonapeptide ICAM-1 antagonist(IP04) was identified using phase display (44). IP04 was shownto specifically block ICAM-1/LFA-1 binding, ICAM-1-dependent homotypicaggregation of human and mouse cells, and neutrophil binding tothe activated endothelium under flow conditions in a parallelplate flow chamber. With the use of alanine and homologous aminoacid substitutions, IP04 was further mutagenized to increase itspotency for inhibition of homotypic aggregation as well as PMNbinding to the endothelium in vitro under flow conditions in aparallel plate flow chamber (IP25) (Refs. 4 and 44 and E.J. Burks, L. O. Sillerud, M. J. Wester, D. C. Brown, and R. S.Larson, unpublished observations). Recently, we have solved thetertiary structures of IP04 and IP25 and proposed a model forhow these antagonists bind to ICAM-1 (Ref. 4; E. J. Burks,L. O. Sillerud, M. J. Wester, D. C. Brown, and R. S. Larson, unpublishedobservations). In this model, IP25 binds to ICAM-1 proximal tothe binding site of the native ligand LFA-1 as defined by mutagenesisstudies (6, 48), thus competing with LFA-1 to bind ICAM-1.Because of the small size and ability to block cell-cell adhesion,we postulated that IP25 may be a useful tool in the pharmacologicalmodulation of reperfusion injury by blocking emigration of PMNsto the ischemic segments. The purpose of the study was to evaluatethe usefulness of the peptide antagonist of ICAM-1 in reducingI/R injury. With the use of a mouse model of tourniquet hindlimbskeletal muscle I/R injury, we evaluated the hypotheses that 1)the peptide antagonist of ICAM-1 reduces PMN infiltration in theareas of infarction, and 2) the attenuation of PMN infiltrationinto muscle is associated with a decrease in infarctsize.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Reagents

Blocking MAb against murine ICAM-1 (clone 3E2B) was purchased from Endogen (Woburn, MA) and used in the in vivo blocking studies.MAb directed against murine ICAM-1 (MEM111) was purchased fromCaltag (Uden, The Netherlands) and used in immunoperoixidase studies.The disulfide-linked cyclic nonapeptide IP25 (CLLRMKSAC) was synthesizedby Biopeptide (San Diego, CA). The purity (95%) was verified byHPLC, and the structure was verified by mass spectroscopy andtwo-dimensional NMR as part of concurrent structural studies (Refs.4 and 44 and E. J. Burks, L. O. Sillerud, M. J. Wester, D.C. Brown, and R. S. Larson, unpublishedobservations).

Animals

Female BALB/c mice (Harlan Sprague Dawley) weighing between 20 and 25 g were used for all experiments. The mice were maintainedat the animal care facilities of the University of New Mexico(Albuquerque,NM).

Experimental Protocol

The model for tourniquet hindlimb ischemia and reperfusion was preformed as described previously (3). In brief, mice wereanesthetized using an inhalant anesthetic (1.5% Halothane, HalocarbonLaboratories; River Edge, NJ) and placed on a circulating hotwater blanket (Baxter; Deerfield, IL) to maintain a constant bodyand muscle temperature. Latex O-rings (Miltex Instruments; Bethpage,NY) were applied above the greater trochanter using a McGivneyhemorrhoidal ligator (Miltex Instrument; Bethpage, NY) to interruptthe arterial blood supply to the hindlimbs. After 2 h of hindlimbischemia, the O-rings were removed, initiating hindlimb reperfusion.Reperfusion of the previously occluded artery was confirmed byvisualinspection.

Exclusions

All animals surviving the full I/R protocol were included in the data analysis. There were no deaths during the experimentalprotocol in the IP25-treatedmice.

Animal Groups

In all, 53 mice were used in this study. The experimental protocol was divided into two different sets ofexperiments.

Assessment of the time course of I/R injury. The animals were randomized in two groups: group A (n = 5) mice remained anesthetized for the entire duration of the study(4 h) but did not go through the I/R protocol, and group B (n= 20) mice underwent 2 h of ischemia and varying periods of reperfusion(ranging from 1 to 4 h). Each experiment was performed with fivemice: one mouse from group A and 4 mice from group B (group Bmice underwent 1, 2, 3, and 4 h of reperfusion,respectively).

Peptide blockade of ICAM-1 on I/R injury. Animals were randomized into five groups: group A (n = 11) animals underwent 2 h of ischemia, followed by 2 h of reperfusion(untreated mice); group B (n = 15) animals underwent 2 h of ischemiafollowed by 2 h of reperfusion and additionally received varyingamounts of the peptide drug IP25 (0.025-0.114 mg/g body wt inthree divided doses every 30 min, beginning at the start of thereperfusion period); group C (n = 4) animals underwent 2 h ofischemia, followed by 2 h of reperfusion and additionally receiveda peptide drug with a scrambled IP25 sequence (identical aminoacid composition as IP25 but with a fixed randomized sequence);and group D (n = 4) animals underwent 2 h of ischemia, followedby 2 h of reperfusion and additionally received blocking MAb directedagainst ICAM-1 (2 mg/kg body wt) at the start of the reperfusionperiod. Group E (n = 3) animals were administered 0.114 mg/g IP25in three doses at 60, 75, and 90 min after reperfusion. The contralateralnonischemic hindlimb of each animal served as a paired control;0.114 mg/g was the maximum dose that could be given due to peptidesolubility. Because the serum half-life of peptide antagonistsis typically short, three injections were given to maintain theserum concentration of the peptide antagonist. Each experimentin this set was performed using at least one mouse from groupsA, C, and D and multiple mice from group B (receiving differentamounts of the peptide drugIP25).

Tissue Collection

At the end of the reperfusion period, the animals were euthanized and blood samples were collected by heart puncture. Serumwas used to measure lactate dehydrogenase (LDH) levels. Skeletalmuscles (quadriceps and hamstrings) were harvested from bothhindlimbs.

Histological and Immunohistochemical Evaluation of Area of Infarction, PMN Infiltration, and Myocyte Damage

The quadriceps were fixed in 10% neutral buffered formalin, processed for paraffin embedding, sectioned, and stained withhematoxylin and eosin (H-E) for routine histological studies.Immunohistochemical studies were performed on formalin-fixed,paraffin-embedded tissue sections using the avidin-biotin-peroxidasecomplex (ABC) method in a Dako Autostainer (Carpinteria, CA).Immunohistochemical staining for the infarcted area was performedusing rabbit anti-human myoglobin polyclonal antibody (Dako) asa primary antibody and anti-rabbit IgG biotinylated MAb as a secondaryantibody (Vectastain, ABC Kit Elite Rabbit IgG PK-6101, VectorLaboratories; Burlingame, CA). To determine the expression ofICAM-1, immunohistochemical staining using MAb against ICAM-1(clone MEM111, dilution 1:100, Monosan; Uden, The Netherlands)was performed. The pathologists (R. S. Larson and S. H. Merchant)were blinded to the treatment of the animals until all the datawereanalyzed.

Immunoperoxidase staining was done using the LSAB2 peroxidase kit (Dako). Briefly, deparaffinized sections were placed ina thermoresistant container filled with citrate buffer solution(pH 6.0), steamed for 45 min, and then cooled for 20 min beforebeing stained. The antigen-antibody reaction was visualized using3,3'-diaminobenzidine as achromogen.

We evaluated four aspects of histological changes related to reperfusion injury: 1) total area of infarction, 2) PMN infiltration,3) degree of myocyte damage, and 4) ICAM-1 expression. The histologicalaspects were evaluated as follows. The total surface area of theskeletal muscle in each section was measured, and the area ofinfarction was measured from the H-E-stained histological sectionsand confirmed by immunohistochemical stains for myoglobin (infarctedarea seen as loss of myoglobin staining in the infarcted area).The infarcted areas were measured using a measuring grid and expressedas the percentage of the total surface area of the skeletal muscle.PMNs were counted manually using an Axioskop microscope at a powerof ×400 in a blinded fashion (by S. H. Merchant), and the PMNnumbers in each section were expressed PMNs per millimeter squaredof section. A histopathology score to assess the presence of myocytedamage was recorded (performed blinded by S. H. Merchant) andranged from 0 to 5 (Table 1). Finally, ICAM-1 expression in theendothelium and myocytes in the infarcted zone, border zone, andviable tissue was recorded.

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Table 1. Histopathology scoring system to assess myocyte damage

Serum LDH

Blood was collected by heart puncture at the end of the reperfusion period. Serum LDH levels were measured using a spectrophotometricassay on an Ektachem 250 analyzer (Ortho-Clinical Diagnostics;Rochester, NY), and results are expressed in units perliter.

Statistical Analysis

We tested the differences in myocyte damage, LDH levels, infarct size, and neutrophils influx using ANOVA and Student's t-tests.One-way ANOVA was used first to show statistical differences amongthe groups, and Student's t-test showed differences between specificgroups. A P value of <0.05 was considered statistically significant.Statistical calculations were performed using GraphPad statisticalsoftware (San Diego,CA).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Time Course of I/R Injury

To examine I/R injury and determine the earliest time period at which measurable alterations were evident, animals were evaluatedat the end of varying periods of reperfusion ranging from 1 to4h.

Skeletal Muscle Histology

Morphometric estimation of the infarct zone size showed an increase in the size of infarct as a function of time of reperfusion(Fig. 1). The infarct was evident at 1 h and increased over the4-h reperfusion period. The skeletal muscle also showed a dramaticincrease in PMNs beginning at 1 h and increasing over the 4 hof reperfusion (P < 0.05 compared with control at all time periods)(Figs. 1 and 2). The PMN infiltration correlated with the presenceof myocyte injury and was seen as preferentially localized inthe border zones surrounding the area of myocyte damage. PMNswere observed in the interstitium and infiltrating the skeletalmuscle fibers (Fig. 2).

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Fig. 1. Relationship of area of infarct, neutrophil influx, and myocyte damage at increasing times of reperfusion (R). A: area of infarction (percentage of total muscle) and PMNs per millimeter squared (means ± SE) were measured at various intervals of reperfusion as described in METHODS (n = 4 for each time point; statistically significant differences were seen between the control group and each of other groups by Student's t-test, P < 0.05). Area of infarction and myocyte damage were measured as described in METHODS. C: serum lactate dehydrogenase (LDH) levels (means ± SE) at various intervals of reperfusion (n = 4 for each time point). Control mice underwent 4 h of anesthesia without the ischemia-reperfusion (I/R) protocol. There was a significant increase in LDH levels after 2 h of reperfusion (*P = 0.004) compared with controls. $delta$ represents both control mice that underwent 4 h of anesthesia without the I/R protocol as well as the contralateral limb of mice undergoing I/R (n = 16). ANOVA analysis indicated that differences among groups in each of A-C were statistically significant. No significant difference was seen among the two control groups.

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Fig. 2. Representative histological sections (hematoxylin and eosin stain, ×400) of skeletal muscle. A: control limbs; B: 2-h ischemia and 1-h reperfusion; C: 2-h ischemia and 4-h reperfusion. No polymorphonuclear neutrophil (PMN) infiltration is seen in control limbs. At 1 h of reperfusion, early PMN influx with tagging of muscle sarcolemmal membranes is seen. At 4 h of reperfusion, there is dense accumulation of PMNs in the interstitium.

Morphological examination to assess qualitative myocyte damage (using morphological criteria, as listed in Table 1) revealedevidence of myocyte damage within 1 h of reperfusion (Figs. 1and 2). Myocyte damage scores only assessed the presence of myocyteinjury, not the size of infarction. Because the highest degreeof myocyte damage was evident within 1 h of reperfusion, withincreasing time of reperfusion, the myocyte damage scores remainedconstant, although these changes were seen spreading to largerzones of the skeletal muscle over the period of reperfusion. Necrosisor extravasated PMNs were not observed in any muscle from thecontrol mice or the contralaterallegs.

Serum LDH Studies

Serum LDH enzyme levels were used as an indicator of skeletal muscle damage and to confirm the histological observations.The serum LDH levels at the end of the I/R protocol were markedlyincreased compared with control mice (Fig. 1). Statistically significantelevation in the serum LDH levels was observed within 2 h of reperfusion(17,984 ± 2,814 U/dl, P = 0.004) compared with control mice (3,912± 1,101 U/dl).

ICAM-1 Expression

The expression of ICAM-1 in vascular endothelium and myocytes was observed in the same experimental animals described aboveusing the MAb against ICAM-1 for immunostaining. Expression ofICAM-1 was observed in capillary, venous, and arterial endotheliumof all skeletal muscle sections of all experimental animals, includingcontrol mice not exposed to I/R injury. No ICAM expression wasidentified in the myocytes from control mice (Fig. 3A). At eachtime point after injury, there was a qualitative increase in myocyteexpression of ICAM-1 (Fig. 3B), but ICAM-1 expression in endotheliumdid not appreciably increase. Myocyte staining was limited tothe small foci of myocytes, which were often concentrated adjacentto the necrotic areas (Fig. 3B). Additionally, infiltrating neutrophilswere often concentrated in the ischemic regions in the vicinityof vessels and myoctyes staining for ICAM-1, indicating neutrophilemigration occurs in ischemic muscle concurrent with the inductionof ICAM-1 expression.

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Fig. 3. Representative immunoperoxidase staining for ICAM-1 (×400) as described in METHODS. A: normal skeletal muscle in control mice. Inset, ICAM-1 staining in the endothelium of the vessel. ICAM-1 expression is not seen in myocytes. B: ischemic muscle in mice undergoing the I/R protocol. Inset, area indicated by arrow. Dense membrane staining of damaged myocytes is seen. Immunoreaction is restricted to the endothelium in nonischemic muscles, whereas intense staining is evident in the ischemic myoctes.

Effect of IP25 on I/R Injury

To evaluate the in vivo effect of IP25 on I/R injury, varying amounts of drug were injected in the tail vein beginning immediatelybefore the reperfusion period, and the results were compared withthose in untreatedanimals.

PMN Influx, Infarct Area, LDH Levels, and Histology

The area of infarction and PMN influx were significantly decreased in mice receiving IP25 (16 ± 2% of muscle and 3.2 ± 0.6PMNs/mm², respectively, using the 0.114 mg/g dose) compared with untreatedmice at the end of the 2-h period of reperfusion (27 ± 3% of muscleand 7.2 ± 1.3 PMNs/mm², P = 0.0034 and P = 0.037, respectively, n = 4 in each group)(Figs. 4A and 5). In addition, there was a linear dose responsefrom 0 to 0.102 mg/g IP25, in that with increasing concentrationsof IP25, smaller infarct areas, lower LDH levels, and lower PMNinflux were observed (Fig. 4, B and C). Increasing the dose from0.102 to 0.114 mg/g IP25 did not alter infarct size or PMN influx.The results obtained with IP25 doses >0.102 mg/g were comparablewith those obtained by MAb blockage of ICAM-1 (Fig. 4A). No decreasein the size of infarction or PMN infiltration was obtained whena peptide with a scrambled IP25 sequence or, alternatively, nopeptide was used (Fig. 4A). In contrast to the reduction in PMNand area of infarction, myocyte damage scores were not reducedin mice receiving IP25 (data not shown). This reflects the presenceof some muscle damage (i.e., wavy fibers) still present in foci(Fig. 5). We also administered the peptide blockade after 1 hof reperfusion (Fig. 4A). Statistically significant reductionsin neutrophil influx or the size of infarct were not observed.

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Fig. 4. A: comparison of the area of infarction and PMN influx at the end of 2 h of ischemia and 2 h of reperfusion in mice receiving drug (0.114 mg/g IP25) with mice receiving sham PBS injection (no peptide), control peptide with scrambled sequence (0.114 mg/g), and MAb against ICAM-1 (2 mg/kg 3E2B). Bars indicate SE; n = 4 in each group. ANOVA shows statistically significant differences among all groups, and subsequent Student t-tests compared with the control group indicate differences between groups indicated by asteriks and the control group (P < 0.05). B: dose-response graph showing the area of infarction and PMN influx at the end of 2 h of ischemia and 2 h of reperfusion in mice receiving the amounts of IP25 indicated. Equivalent volumes of PBS were injected in control mice not receiving any drug (n = 4 for each group, see METHODS for details). Bars indicate SE. ANOVA analysis showed statistically significant differences among groups (P < 0.05). C: serum LDH values in control mice (sham PBS injection) and indicated doses of IP25. Bars indicate SE. ANOVA analysis of groups indicated statistically significant differences (P < 0.05).

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Fig. 5. Comparison of skeletal muscle histology (hematoxylin and eosin stain, ×400) in mice undergoing 2-h ischemia/2-h reperfusion (A) with mice receiving the maximal dose of IP25 (B). Control mice received sham injection. There was a dramatic reduction in PMN influx, but presence of myocyte damage (wavy fibers, see Table 1), in mice receiving IP25.

ICAM-1 Expression in IP25-Treated Mice

Similar to the untreated mice described above (Fig. 4), ICAM-1 expression was not identified in the myocytes but was presentin endothelium from the control group. Regardless of treatment,ICAM-1 expression in myocytes was induced during reperfusion,whereas the expression of ICAM-1 as detected with immunoperoxidasedid not qualitatively change. No significant differences in ICAM-1expression in myocytes or endothelium were seen at any time pointsamong the different treatment groups (data notshown).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Experimental studies have shown that inflammatory tissue damage due to I/R is caused primarily by PMNs (41, 42). ICAM-1is an adhesive glycoprotein receptor expressed on endothelialcells and required for PMN emigration from blood into tissue (3,23, 26, 33, 54). MAb directed against ICAM-1 or its ligand, $beta$ ₂-integrin, as well as studies using animals genetically deficientin ICAM-1 or integrin receptors have shown that the extent ofreperfusion injury is attenuated through ICAM-1 blockade or absenceas assessed by 1) decreased myocardial necrosis, 2) a reductionin neutrophil accumulation in I/R myocardium, 3) recovery of endothelium-dependentvasorelaxation in regional ischemia models, and 4) improvementof cardiac function and myocardial energy status in global ischemiamodels (3, 17, 23, 26, 28, 29, 34, 50, 54).We previously described a novel cyclic peptide that is a potent,selective inhibitor of ICAM-1-dependent cell adhesion in vitro(Refs. 4 and 44 and E. J. Burks, L. O. Sillerud, M. J. Wester,D. C. Brown, and R. S. Larson, unpublished observations). Themain aim of the present study was to demonstrate the in vivo efficacyof IP25 by employing a mouse model of tourniquet hindlimb I/Rinjury. This study provides direct evidence for the in vivo protectiveeffect of IP25 by demonstrating an attenuation of infarct size(40% reduction) and PMN influx (56% reduction) after experimentalischemia and reperfusion. Thus inhibition of ICAM-1-dependentbinding after reperfusion of the ischemic myocytes has been investigatedextensively, but this is the first study to show the efficacyof a peptide antagonist in amelioration of I/R injury. Our resultswere comparable with those obtained by MAb blockade of ICAM-1in parallel experiments, indicating that the use of this cyclicpeptide in humans may be therapeuticallybeneficial.

In vitro and in vivo studies have clearly demonstrated that the adhesion and transmigration of PMNs through the endotheliuminto tissue is dependent on $beta$ ₂-integrin binding to ICAM-1 duringI/R injury (3, 23, 26, 33). In addition, after emigrationinto tissue, it is well appreciated that PMN-mediated myocardialcell injury may also involve $beta$ ₂-integrin-ICAM-1 interaction (3,26, 28, 29). In agreement with these previous observations,ICAM-1 expression was detected in the endothelium and myocytesin our study as well (3, 24, 53). ICAM-1 expression inendothelial cells was easily detected by immunoperoxidase stainingin normal and infarcted tissue. However, the increased expressionof ICAM-1 in the endothelium in the areas of infarction was noteasily appreciated. With the use of immunoperoxidase staining,other investigators have also seen similar results, and this likelyrelates to the fact that this staining technique is not sensitiveto increasing expression of antigens (24). In contrast, theinduced expression of ICAM-1 is easily appreciated in myocytes,because ICAM-1 is not detected before ischemia. ICAM-1 expressionin myocytes is most intense within the areas of infarction andin viable myocytes at the border zones of infarction. Immunostainingwas evident within 1 h of reperfusion in the form of bright membranousstaining of the myocytes (Fig. 4B). Our findings and those ofothers (3) of ICAM-1 expression in skeletal muscle I/R injuryare similar to those observed in cardiac myocytes during I/R injury.In these previous cardiac I/R studies, ICAM-1 mRNA expressionwas induced as early as 1 h after reperfusion and increased over24 h, although ICAM-1 protein expression on myocytes was not seenuntil 24 h (24, 53). ICAM-1 mRNA expression was most intensein the cardiac myocytes in the ischemic viable "border zone" withinthe first few hours of reperfusion. From these current observationson ICAM-1 expression and neutrophil influx inhibition, as wellas our previous studies (Refs. 4 and 44 and E. J. Burks,L. O. Sillerud, M. J. Wester, D. C. Brown, and R. S. Larson, unpublishedobservations), it is clear that IP25 inhibits neutrophil bindingto and transmigration through the endothelium. However, whetherIP25 may directly antagonize PNM-myocyte interaction, althoughexpected, is not demonstrated. Inhibition of leukocyte-myocytebinding after I/R injury has been shown to improve rat cardiacmyocyte contractitlity (46).

Previous studies also have indicated that PMN influx is most intense and increases during the first 4 h of ischemia, in agreementwith our findings (8, 41, 42). We were able to detect PMNat 1 h, but the most intense PMN influx occured at 3-4 h. ThePMN influx is most intense in the border zones of infarction andis of greater magnitude in larger areas of infarct. Myocyte damagewas also detectable within 1 h of I/R injury. However, focal myocytedamage was present even when neutrophil influx was inhibited andcould not be detected, suggesting that some myocyte damage maybe independent of ICAM-1-dependent mechanisms, and includes complementand endothelial cell-derived factors as suggested by others (2,12, 35). Although there was a reduction in the area of infarctand LDH levels with IP25 treatment, LDH levels were elevated inIP25-treated mice compared with control mice, consistent withthe histological observation of some persistent muscle damageand infarct in the absence of neutrophilinflux.

Our studies show the efficacy of IP25 in inhibiting PMN influx and reducing infarct size after 2-h ischemia and 2-h reperfusion.Previous studies with dogs and rodents have indicated that theremay be only a "window of time" in which it is possible to reduceI/R injury by neutrophil influx inhibition (3, 7, 21).This may be due to the ischemia injury being so severe that thetissue is necrotic before reperfusion and therefore not amenableto reperfusion injury. We chose to study the efficacy of IP25after 2 h of ischemia, because significant PMN and myocyte changeswere readily evident to examine the efficacy of IP25, and we wereconcerned about the potential short half-life of peptide drugs.However, our studies do not fully address the effects of ischemiaduration and how it related to neutrophil influx inhibition. Furthermore,it is unclear whether it will be beneficial to inhibit for 24h or more, because the suppression of PMN influx at later timesafter reperfusion may prevent myocardial healing, as has beenobserved with glucocorticoids (45). In contrast, others haveshown that ICAM-1 inhibition has no protective role in myocardialremodeling at later stages (30, 36). In addition, the effectivenessof IP25 may also be enhanced by constant infusion or repetitivebolusadministration.

There does appear to be a shift in the selectin used for the initial PMN rolling in that P-selectin is utilized during thefirst 60 min of reperfusion, whereas at later times (>4 h) E-selectinis preferentially utilized (1, 3, 25, 55). Thus alterationin selectin utilization and the value of selectin blockade appearsto relate to the change in expression of the various selectinsin the endothelium at different time points after reperfusion.In contrast, ICAM-1 is expressed before ischemia, and its expressionincreases with reperfusion. In our studies, injection of IP25after 1 h of reperfusion did not alter I/R injury. This laterfinding is consistent with the concept that neutrophil influxbegins within minutes of reperfusion and the effects of earlyinfiltration cannot be reversed with later ICAM-1 blockade orthat later infiltration is not ICAM-1dependent.

Ischemia-reperfusion injury is of significant clinical interest. Although there is overwhelming evidence that MAbs directedagainst $beta$ ₂-integrins or ICAM-1 reduce PMN infiltration and consequentlyinfarct size in experimental animals (17, 36, 50, 54),several clinical trials directed at blocking adhesion moleculebinding in humans have not shown efficacy (11, 39, 51).There are a number of potential explanations. First, the designof the trials may not have been adequate, because two of thesestudies had mortality rates in all groups lower than the reportedrates in similar populations, making the studies too small todraw any statistically significant information. Second, currentanimal models may not adequately reflect I/R in humans. This mayrelate to the presence of non-adhesion-related pathways playinga more dominant role in humans or that the dominant pathway isdramatically influenced by the length of ischemia. In supportof this notion, a recent study (19) demonstrated that myocyteinjury in longer ischemia times became increasingly dominatedby a caspase-dependent apoptotic pathway. Finally, the clinicaltrials used MAb therapy. The clinical application of MAbs is hamperedby potential therapeutic hazards, including life-threatening anaphylacticreactions. In addition, some anti-ICAM-1 or integrin MAb thatblock function in vitro have actually been found to activate neutrophilsin vivo and are therefore inappropriate to use in clinical trials(53). Small peptide inhibitors such as IP25 would be less immunogenicand circumvent the secondary physiological effects of antibodies(14, 19, 27, 32). In addition, the short half-life ofpeptide inhibitors is likely to be beneficial if ICAM-1-dependentevents at later time points of myocardial healing are adverseto healing (30, 36). One of the chief difficulties in treatingI/R injury is its multifactorial etiology, although a significantcomponent is mediated by PMN infiltration. Endothelial cell-derivedmediators (including arachidonic acid metabolites, endothelin,and endothelium-derived relaxing factor), complement, and apoptosisinhibitors are among the other more well-characterized factorsthat have shown to be intimately involved with reperfusion injury(2, 12, 15, 18, 35). Modulations of these factors havealso been shown to reduce infarct size in experimental animals(2, 12, 15, 35). Because the mechanism of action of thesemediators are different at different time points after reperfusion,future studies will evaluate whether modulation of one of thesefactors in combination with peptide-mediated blockade of ICAM-1has a synergistic effect in preventing I/R injury. In all, theresults of the present study indicate the potential of syntheticchemically modified peptides as an alternative therapeutic approachto I/Rinjury.

	ACKNOWLEDGEMENTS

The authors thank Dr. Dan Theele of the animal care facility at the University of New Mexico for the assistance and supportduring the experimentalprotocols.

	FOOTNOTES

This study was supported in part by American Heart Association Grant 9960318Z and American Cancer Society Grant RPG-00-096-01-LBC.

Address for reprint requests and other correspondence: R. S. Larson, Univ. of New Mexico Cancer Research Facility, Rm. 223,2325 Camino de Salud, Albuquerque, NM 87131 (E-mail: rlarson{at}salud.unm.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

First published December 19, 2002;10.1152/ajpheart.00840.2002

Received 20 September 2002; accepted in final form 12 December 2002.

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TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

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