Disruption of the Mouse {micro}-Calpain Gene Reveals an Essential Role in Platelet Function

doi:10.1128/MCB.21.6.2213-2220.2001

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Molecular and Cellular Biology, March 2001, p. 2213-2220, Vol. 21, No. 6
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.6.2213-2220.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Disruption of the Mouse µ-Calpain Gene Reveals an Essential Role in Platelet Function

Mohammad Azam,¹ Shaida S. Andrabi,¹ Kenneth E. Sahr,¹ Lakshmi Kamath,² Athan Kuliopulos,² and Athar H. Chishti¹^,^*

Section of Hematology-Oncology Research, Departments of Medicine, Anatomy, and Cellular Biology, St. Elizabeth's Medical Center, Tufts University School of Medicine, Boston, Massachusetts 02135,¹ and Division of Hematology-Oncology, New England Medical Center, Departments of Medicine and Biochemistry, Tufts University School of Medicine, Boston, Massachusetts 02111²

Received 15 September 2000/Returned for modification 8 November 2000/Accepted 27 December 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results and Discussion References

Conventional calpains are ubiquitous calcium-regulated cysteine proteases that have been implicated in cytoskeletal organization,cell proliferation, apoptosis, cell motility, and hemostasis.There are two forms of conventional calpains: the µ-calpain, orcalpain I, which requires micromolar calcium for half-maximalactivation, and the m-calpain, or calpain II, which functionsat millimolar calcium concentrations. We evaluated the functionalrole of the 80-kDa catalytic subunit of µ-calpain by genetic inactivationusing homologous recombination in embryonic stem cells. The µ-calpain-deficientmice are viable and fertile. The complete deficiency of µ-calpaincauses significant reduction in platelet aggregation and clotretraction but surprisingly the mutant mice display normal bleedingtimes. No detectable differences were observed in the cleavagepattern and kinetics of calpain substrates such as the $beta$ 3 subunitof $alpha$ IIb $beta$ 3 integrin, talin, and ABP-280 (filamin). However, µ-calpainnull platelets exhibit impaired tyrosine phosphorylation of severalproteins including the $beta$ 3 subunit of $alpha$ IIb $beta$ 3 integrin, correlatingwith the agonist-induced reduction in platelet aggregation. Theseresults provide the first direct evidence that µ-calpain is essentialfor normal platelet function, not by affecting the cleavage ofcytoskeletal proteins but by potentially regulating the stateof tyrosine phosphorylation of the plateletproteins.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results and Discussion References

The calpains are a family of calcium-dependent neutral cysteine proteases present in essentially all tissues of higher animals(8, 34, 37). Calpain homologues distantly related to thecatalytic subunits of conventional calpains are also found inlower organisms such as parasites, insects, nematodes, fungi,and yeast (34). They are believed to play functionally importantroles in diverse biological processes such as reorganization ofcortical cytoskeleton, cell motility, cell proliferation, apoptosis,and hemostasis (9, 27, 31, 39). Calpains are dividedinto two broad classes, ubiquitous and tissue specific. CalpainI (also referred to as µ-calpain) and calpain II (also referredto as m-calpain) are expressed in all tissues in varying amountsand share ~61% sequence identity (20). Both the µ- and m-calpainscontain an 80-kDa catalytic subunit that forms a heterodimer withthe regulatory 30-kDa subunit (34). The 80-kDa catalytic subunitsof the µ- and m-calpains are products of separate but closelyrelated genes (referred to as Capn1 and Capn2, respectively),while the 30-kDa subunit (encoded by the Capn4 gene) is commonto both (34). The µ-calpain is fully active in micromolar concentrationsof calcium, while the m-calpain requires millimolar calcium concentrationsfor full activation. Larger tissue-specific calpains have beencloned from stomach and smooth muscle tissues (35, 37). Mutationsof the muscle-specific Capn3 (calpain 3 gene) have been shownto cause one form of limb-girdle muscular dystrophy type 2A (30).More recently, several groups have identified CAPN10 (calpain10) as the target gene for mutations in the type 2 or non-insulin-dependentdiabetes mellitus, thus underscoring the importance of calpainsin the regulation of fundamental signaling pathways (2, 16,25). Although much biochemical information has been accumulatedon the combined effects of µ- and m-calpains, their individualphysiological functions have not been identified. In order toobtain an in vivo model of µ-calpain deficiency, we disruptedthe µ-calpain catalytic subunit gene (Capn1) in the mouse. Here,we describe the in vivo consequences of disruption of the µ-calpaingene in mice. Our data provide the first unambiguous proof ofthe essential role of µ-calpain in platelet aggregation, clotretraction, and tyrosine phosphorylation of platelet proteins.Since the µ-calpain gene is expressed in many cell types, ourfindings may be of significance not only in blood coagulationand platelet physiology but also in the areas of cell motility,cancer (metastasis), inflammation, and other integrin-dependentprocesses.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results and Discussion References

Generation of targeted embryonic stem cells and mutant mice. A 2.3-kb mouse µ-calpain cDNA was amplified by reverse transcriptase PCR (RT-PCR) using a total spleen RNA as a template.Total RNA was first reverse transcribed using a random hexamerprimer (Promega) and Moloney murine leukemia virus reverse transcriptase(Gibco BRL). Overlapping cDNA fragments were then amplified usingthe Expand Long Template PCR system (Boehringer Mannheim). Thefollowing primers were designed based on the rat and mouse µ-calpaincDNA sequences: Cal 1 (263 to 282, 5'-CTACGGAACTGCTGTCAAAC) andCal 2 (970 to 989, 5'-TCCATCTTGACCCTCAGCTG); Cal 6 (1872 to 1892,5'-GTTCACCATGCTGCGGCACGA) and Cal 7 (941 to 958, 5'-GGAACAAAGTGGACCCCT).A genomic clone of 28 kb was isolated by screening a 129-Sv genomiclibrary (Stratagene) and was characterized. An XbaI fragment (5.5kb) containing exons 1 to 3 (upstream arm) was cloned at the XbaIsite in the pPNT targeting vector. A SalI fragment (2.4 kb) containingexon 5 and a segment of exon 4 was cloned at the XhoI site asthe downstream arm. The vector was linearized using SspI and electroporatedinto the R1 ES cell line. Six correctly targeted clones were identifiedby PCR and confirmed by Southern blotting. PCR analysis was performedusing primers specific for Neo on the 5' end and exon 6 on the3' end. Two separate ES cell clones heterozygous for disruptedalleles were microinjected into the blastocysts of C57BL/6J mice.Male chimeras were then bred with female C57BL/6J mice to confirmgerm line transmission, and the resulting heterozygotes were matedto generate homozygotes for the mutation in the µ-calpain gene.Southern, Northern, and Western blotting and casein zymographywere performed using standard protocols. To ensure that the designof the targeting construct did not result in the expression oflow abundance, truncated µ-calpain transcripts, RT-PCR of µ-calpainwas performed using total RNA pooled from different tissues (Fig.1e). The following primers were used: Cal 1 (exon 1) and Cal 2(exon 7); Cal 10 (exon 2; 5'-ACAGACATCTGCCAGGGAGC) and Cal 19(exon 8; 5'-CCAGTTTGGTGAATTCACGG); Cal 18 (exon 6; 5'-GGGTGAAGTGGAGTGGAAAGGA)and Cal 6 (exon 16; 5'-GTTCACCATGCTGCGGCACGA). The RT-PCR of m-calpain(primers: mCal 1 [5'-GAGGTGGTGGTGGACGACAG] and maCal 2 [5'-TTTCTGCAGGCTTCCTGAAC]),G3PDH (primers: Clonetech 5'-RACE kit), and the 30-kDa regulatorysubunit of calpain (primers: 30K-1 [5'-CTCCGCCTCCACGTAGTCAT] and30K-2 [5'-GCTATCAGGGACTAGCCAGT]) was performed using gene-specificprimers.

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FIG. 1. Targeted disruption of the Capn1 locus and generation of mutant mice. (a) Schematic representation of the genomic locus of mouse µ-calpain drawn to scale. Sequence information for the intron-exon boundaries is shown in Table 1. The restriction sites shown on the map are as follows: BamHI (B), HindIII (H), and SalI (S). (b) The Capn1 locus (wild type; top line), the targeting vector (middle line), and the disrupted Capn1 locus (bottom line). Shown is the expected size of an XbaI and SalI fragment that hybridized with the probe for the wild-type locus (top) and the mutated allele (bottom). Small arrows indicate the positions of calpain primers that were used to conduct the RT-PCR analysis. (c) Southern blot analysis of genomic DNA isolated from the F2 generation of Capn1^+/ mice was digested with XbaI and SalI and was blotted and hybridized with the probe shown in panel b. (d) RT-PCR analysis of mouse µ-calpain using primers Cal 1 and Cal 2. Glyceraldehyde 3-phosphate dehydrogenase (G3PDH) was used as a control to normalize the samples. The calpain regulatory 30-kDa subunit and the m-calpain catalytic subunit were amplified from the total RNA of liver, lung, and kidney of wild-type and Capn1^/ mice using gene-specific primers as described in Materials and Methods. (e) To rule out the possibility that alternate splicing may have occurred and produced low levels of truncated transcripts, RT-PCR analysis was conducted using total RNA pooled from liver, lung, and kidney. Lanes 1 and 2 show the results obtained using primer pair Cal 10 and Cal 19 (upstream transcript), and lanes 3 and 4 show the results obtained with primer pair Cal 18 and Cal 6 (downstream transcript). (f) Northern blot analysis of total RNA isolated from liver and lung of Capn1^+/+ and Capn1^/ mice. The blot was hybridized with a cDNA probe (1.5 kb; exons 2 to 16) of murine µ-calpain. (g) Casein zymogram showing the distribution of µ-calpain and m-calpain in the platelet extract of Capn1^+/+ and Capn1^/ mice. Note that only the µ-calpain activity was lost in the Capn1^/ mice. (h) Western blot analysis of µ-calpain in the whole red blood cell lysate of Capn1^+/+ (left lane) and Capn1^/ (right lane) mice. (i) Casein zymogram of calpain activity in the red blood cell lysate of Capn1^+/+ (left lane) and Capn1^/ (right lane) mice. The dark band represents the position of hemoglobin in the red cell lysate.

Preparation of washed platelets and PRP. Blood was collected from the inferior vena cava of mice anesthetized with the pentobarbitol sodium (Nembutal)-ketamine mixture.Blood (~700 µl) was withdrawn into a syringe containing 25 µlof heparin (1,000 U/ml) and 5 U of apyrase/ml. Blood was pooledfrom several mice in a 15-ml tube, and an equal volume of phosphate-bufferedsaline was added. The sample was centrifuged at 1,000 × g for10 min and the resulting platelet-rich plasma (PRP) was centrifugedat 3,000 × g for 7 min. Sedimented platelets were resuspendedin Tyrode's buffer (10 mM HEPES [pH 7.4], 5.56 mM glucose, 137mM NaCl, 12 mM NaHCO₃, 2.7 mM KCl, 0.36 mM NaH₂PO₄, 1 mM MgCl₂),counted, and diluted to 1.5 × 10⁸/ml. All steps were performed at 25 to 30°C.

Platelet aggregation and tail-bleeding measurements. Aggregation and ATP secretion of washed and recalcified (2.0 mM) platelets were measured by light scattering in a Chrono-loglumiaggregometer (Model 560VS/490-2D). Platelets were inducedto aggregate by the addition of thrombin (Hematologic Technologies,Inc.), ADP (Sigma), collagen (Sigma), and A23187 ionophore(Sigma) with stirring at 37°C. For tail-bleeding experiments,8- to 12-week-old Capn1^+/+ (36 mice) and Capn1^/ (52 mice) mice were anesthetized and 6 min later their tailswere transected 0.2 cm from the tip with a scalpel blade. Thetail was placed in a solution of phosphate-buffered saline at37°C, and the time taken for the blood flow to cease was recorded.Where necessary, experiments were terminated by cauterizationat 600 s to preventdeath.

Clot retraction assay. Clot retraction was measured essentially as described before (15) by mixing the following: 200 µl of PRP from Capn1 nulland wild-type mice, 750 µl of 53 µM Na₂HPO₄-12 µM KH₂PO₄, 5 µlof erythrocytes (to enhance clot contrast for photography), and50 µl of thrombin (1 or 10 nM). A glass rod was placed in eachglass test tube and incubated at ambient temperature for 1 to12 h. Clot formation and subsequent clot retraction were recordedvisually at various time intervals prior tophotography.

Cleavage of talin, filamin, and $beta$ 3 integrin and tyrosine phosphorylation. Purified platelets (200 µl at 5 × 10⁸ platelets/ml) were calcified (1.0 mM CaCl₂) and stimulated using calcium ionophore A23187(1.0 µM) and thrombin (10 nM) at 37°C with constant stirring.Samples were withdrawn at the indicated time intervals, immediatelysolubilized in the 5× gel-loading buffer (250 mM Tris-HCl [pH6.8], 5 mM sodium vanadate, 10 mM EDTA, 5 mM phenylmethylsulfonylfluoride, 10 mM benzimidine, 25% glycerol, 15% sodium dodecylsulfate [SDS], 2.5% $beta$ -mercaptoethanol), and boiled at 95°C for5 min. Proteins were analyzed by SDS-polyacrylamide gel electrophoresis(PAGE) (6% gel) and visualized by Coomassie staining of the gel.Cleavage of talin was analyzed by Western blotting using a monoclonalanti-talin 8d4 antibody (Sigma), and $beta$ 3 integrin was detectedusing a polyclonal anti- $beta$ 3C antibody (raised against the C-terminal20 amino acids of the $beta$ 3 integrin cytoplasmic domain) (10).Another polyclonal antibody, anti-N $beta$ 3 (N-20), raised against theN-terminal domain of $beta$ 3 integrin (Santa Cruz) was used to normalizethe amount of $beta$ 3 integrin in the Western blots. For antiphosphotyrosineblots, total platelet protein extract was analyzed by SDS-PAGE(7% gel), transferred to the nitrocellulose, and immunoblottedwith an antiphosphotyrosine monoclonal antibody 4G10 (UpstateBiotechnology Inc.).

Immunoprecipitation assays. Equal numbers of platelets from wild-type and Capn1^/ mice were activated with either 10 nM thrombin or 1 µM calcium ionophoreA23187 for 30 s, 1 min, and 3 min. Platelets were solubilizedwith an equal volume of double-strength modified RIPA buffer (50mM Tris-HCl [pH 7.5], 150 mM NaCl, 4 mM EDTA, 4 mM EGTA, 20 µgof aprotinine/ml, 2 mM phenylmethylsulfonyl fluoride, 200 µM leupeptin,4 mM sodium orthovanadate, 4 mM benzamidine, 2 mM sodium fluoride,2 mM sodium pyrophosphate, and 0.2% sodium deoxycholate). Immunoprecipitationswere performed using biotin-conjugated anti-integrin $beta$ 3 antibody(Becton Dickinson) for 12 h at 4°C, followed by incubation withstreptavidin-conjugated agarose beads (Pierce) for 2 h at 4°C.Immunoprecipitates were washed with two volumes of RIPA buffer(as described above) and analyzed by SDS-PAGE (8% gel). Immunoprecipitateswere transferred to nitrocellulose, and immunoblotting was performedusing an antiphosphotyrosine antibody, 4G10 (Upstate BiotechnologyInc.). The same blot was stripped and reprobed with an anti- $beta$ 3integrin antibody, N $beta$ 3 (Santa Cruz), to ensure an equal amountof $beta$ 3 integrin in eachlane.

	RESULTS AND DISCUSSION

Top Abstract Introduction Materials and Methods Results and Discussion References

Although numerous attempts have been made to delineate the biological function of µ-calpain and m-calpain using cysteine proteaseinhibitors, the results have often been confounded due to thelack of specificity of these inhibitors. We set out to determinethe specific function of µ-calpain by genetic inactivation ofits expression in mice. Overlapping mouse µ-calpain large subunitcDNA clones were isolated by RT-PCR of BALB/c mouse spleen RNA.The overlapping cDNA sequence (GenBank accession number AF084459)extends 2,311 nucleotides and encodes a protein of 713 amino acidsconsistent with the reported cDNA sequence of the mouse µ-calpaincatalytic subunit (26). A mouse 129 strain $lambda$ genomic library(Stratagene) was screened, and the complete genomic structureof the µ-calpain large subunit was assembled using establishedmethods. The mouse µ-calpain large subunit gene spans ~28 kb andconsists of 21 exons (Fig. 1a and Table 1). A targeting vectorwas constructed that will delete the 5' segment of exon 4 (aminoacids 153 to 160: LWQFGEWV) as well as disrupt the gene by insertingthe pGK-Neo cassette (Fig. 1b). Exon 4 encodes a critical partof the catalytic domain of µ-calpain (17, 36). Two embryonicstem cell clones bearing the targeted allele were used to generatechimeric mice, which were then mated to generate heterozygousanimals. Wild-type, heterozygous, and homozygous mice were borneat the expected Mendelian ratio from the heterozygous mating.A Neo-specific probe was used to confirm unique integration inthe genome. Correct targeting of Capn1 was confirmed by Southernblotting (Fig. 1c) using a probe derived from exons 6 and 7 (Fig.1b). Northern blot analysis of liver and lung tissues indicateda complete absence of µ-calpain transcript (~2.8 kb) when probedwith a cDNA fragment of 1.5 kb from exons 2 to 16 of Capn1 (Fig.1f). The absence of µ-calpain transcript in the homozygous mutantmice was further confirmed by RT-PCR analysis of liver, lung,and kidney tissues (Fig. 1d). In order to check any differentiallyspliced transcript, RT-PCR was carried out from the regions upstreamand downstream of pGK-Neo insertion (Fig. 1e). The transcriptsencoding m-calpain and the regulatory 30-kDa subunit were unalteredin the µ-calpain null tissues (Fig. 1d).

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TABLE 1. Mouse µ-calpain large subunit gene exon donor and acceptor sequences

The enzyme activity of µ-calpain was measured in the platelets of mutant mice by casein zymography. Casein zymograms of wild-typeplatelets showed an asymmetric distribution of calpain activity:~80% µ-calpain and ~20% m-calpain (Fig. 1g). In the µ-calpainnull platelets, the band corresponding to µ-calpain activity wasabsent whereas the m-calpain activity remained essentially unaltered(Fig. 1g). Because the available monoclonal antibody reacts withall isoforms of calpains, we could not perform Western blottingon µ-calpain null platelets since both µ- and m-calpains migrateat the same position during electrophoresis under denaturing conditions.Alternatively, we examined the mature erythrocytes from µ-calpainnull mice by Western blotting using the same monoclonal antibodythat reacts with both calpains. As shown in Fig. 1h, neither µ-calpainnor m-calpain was present in the mature erythrocytes. Indeed,the casein zymography confirmed that the mature erythrocytes fromwild-type mice contain the µ-calpain exclusively, whereas theµ-calpain null erythrocytes are completely devoid of any calpainactivity (Fig. 1i). Taken together, these results demonstratethe development of a murine model system that selectively lacksthe µ-calpain activitysystemically.

Because ~80% of the total calpain activity in mouse platelets is contributed by the µ-calpain (Fig. 1g) and the calpains areknown to play a major role in platelet physiology, we evaluatedthe effects of µ-calpain deficiency on platelet function. Activationof platelets involves a sequence of cytoskeletal reorganizationevents that include release of granule contents, engagement ofintegrins to form platelet-platelet aggregrates, and eventualformation of a stable hemostatic plug (33). Calcium-dependentcalpains proteolyze a wide range of cytoskeletal proteins, includingthe $beta$ 3 subunit of $alpha$ IIb $beta$ 3 integrin, that have been proposed toplay an essential role in platelet granule secretion, aggregation,and retraction of fibrin-bound blood clots (9, 10, 31,32, 41). Therefore, we examined the effects of µ-calpain deficiencyon platelet function. Platelet aggregation was reduced by 50 to60% in response to thrombin (10 nM), ADP (20 µM), collagen (20µg/ml), and calcium ionophore A23187 (1.0 µM) (Fig. 2, toppanels). In separate experiments (data not shown), a comparablediminution in the platelet aggregation (~55%) was observed ata lower concentration of the calcium ionophore A23187 (0.1µM). In contrast, relatively small differences were observed inthe ATP secretion from dense granules upon thrombin and collagenactivation whereas no detectable differences were apparent inthe ADP- and calcium ionophore A23187-treated platelets (Fig.2, bottom panels). We then measured the bleeding time in Capn1^/ mice using the transected tail method. The bleeding times wereessentially normal (Fig. 3a). The platelet numbers in the peripheralblood of 8- to 12-week-old mice were comparable between wild-type(1.13 × 10⁶/µl) and homozygous (1.07 × 10⁶/µl) mice. Significantly, however, the Capn1^/ platelets were defective in retracting clots, especially whenthe clot formation was induced with 1.0 nM thrombin (Fig. 3b).Since the clot retraction is an important part of thrombus consolidationand is dependent upon $alpha$ IIb $beta$ 3 integrin function (18, 21, 40),our results suggest that µ-calpain plays a role in $alpha$ IIb $beta$ 3 integrin-mediatedsignaling in murine platelets.

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FIG. 2. Effects of µ-calpain deficiency on platelet aggregation and granule secretion. Aggregation (top panel) and granule secretion (bottom panel) responses of washed platelets (1.5 × 10⁸/ml) from Capn1^+/+ (black) and Capn1^/ (gray) mice are shown. (a) Thrombin, 10 nM. (b) ADP, 20 µM. (c) Collagen, 20 µg/ml. (d) Calcium ionophore A23187, 1 µM. In separate experiments, calcium ionophore at 0.1 µM was also used and produced an aggregation response consistent with other agonists. All measurements of platelet aggregation and granule secretion (19) were performed on the apyrase-treated (5 U/ml) platelets. Data are representative of four experiments.

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FIG. 3. Effects of µ-calpain deficiency on hemostasis and clot retraction. (a) Bleeding time was measured as described in Materials and Methods. Each symbol represents bleeding time measurement on a single Capn1^+/+ mouse (left) and Capn1^/ mouse (right). (b) Photographs show the extent of in vitro clot retraction using PRP from wild-type and calpain null mice. Samples were treated with either 1.0 or 10 nM thrombin. As mentioned in Materials and Methods, 5 µl of red blood cells was added to enhance the color contrast for photography. The defective clot retraction in the µ-calpain null platelets was not influenced by the addition of red blood cells. Each photograph is representative of three independent experiments.

It is noteworthy here that the ~50% impaired platelet-platelet aggregate formation occurs under saturating agonist concentrationsfor thrombin, ADP, and collagen. In other words, the additionof more agonist does not overcome this deficient aggregation,demonstrating that impairment cannot be overcome by eventual activationof m-calpain. Thus, the most obvious biological function of µ-calpainis its role in controlling the very late events of platelet aggregation.Remarkably, early events of platelet activation such as shapechange, granule release, and the initial rate of platelet aggregationare unaffected (the initial slopes start out identically); however,the final extent of platelet aggregation and clot retraction areboth severely deficient. Therefore, it is quite clear that thehigh-affinity µ-calpain isoform is essential for the proper functioningof the later calcium-dependent cytoskeletal, integrin, and contractilityapparatus in murineplatelets.

To further investigate the molecular basis of µ-calpain-mediated signaling in platelets, we examined the proteolysis of knowncalpain substrates such as $beta$ 3 integrin, filamin, and talin inµ-calpain null platelets. Talin (270 kDa) and filamin (280 kDa)link the cytoplasmic domain of $beta$ 3 integrin to the actin cytoskeletonand are cleaved upon platelet activation (3, 9, 12). Similarly,the cytoplasmic domain of $beta$ 3 integrin itself undergoes calpain-dependentproteolysis upon platelet activation (10). Surprisingly, thetime courses of proteolysis of talin (Fig. 4a to d), filamin (Fig.4a and b), and the $beta$ 3 integrin cytoplasmic domain (Fig. 4c andd) were indistinguishable in Capn1^+/+ and Capn1^/ platelets. This result suggests that the dysfunctions of Capn1^/ platelets are not due to the cleavage of the $beta$ 3 cytoplasmic domainof $alpha$ IIb $beta$ 3 integrin. These results also suggest either that µ-calpainis not essential for this thrombin- and ionophore (A23187)-inducedcleavage or that a possible compensation of µ-calpain activityby m-calpain occurs in the Capn1^/ platelets. Alternatively, these proteins may not be authenticsubstrates of µ-calpain in murine platelets and an independentproteolytic mechanism might exist that mediates cleavage of theseproteins upon agonist-dependent activation of mouse platelets.

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FIG. 4. Proteolysis and tyrosine phosphorylation of platelet proteins. Washed platelets were activated by either calcium ionophore A23187 (1 µM) or thrombin (10 nM) at 37°C with stirring, and samples were taken out at indicated times for gel electrophoresis. (a) SDS-PAGE and Coomassie blue-stained 6% gel of total platelet lysate (40 µl). Calcium ionophore A23187 was used as an agonist. Arrows indicate the positions of intact filamin and talin. The 190-kDa fragment of talin (solid arrowhead) and the 130- and 93-kDa cleavage products of filamin (open arrowheads) are shown. (b) SDS-PAGE and Coomassie blue-stained 6% gel of total platelet lysate (40 µl). Thrombin was used as an agonist. Other symbols are the same as shown in the previous panel. (c and d) Western blot analysis of total platelet protein samples shown in panels a and b. (c) Calcium ionophore A23187 treatment. (d) Thrombin-treated platelets. An equal amount of platelet lysate, normalized by protein concentration, was analyzed by SDS-PAGE (7% gel), transferred to nitrocellulose, and probed with an antiphosphotyrosine monoclonal antibody (4G10). Note that the asterisk at p110 indicates the position of the $beta$ 3 subunit of $alpha$ IIb $beta$ 3 integrin. The same blots were stripped and reprobed to examine the proteolysis of $beta$ 3 integrin and talin using defined antibodies. The bottom three panels show the results of Western blots using antibodies against $beta$ 3 integrin and talin. The anti-N $beta$ 3 antibody is specific for the N-terminal region of $beta$ 3 integrin and was used to determine the total amount of $beta$ 3 integrin in each lane. The anti- $beta$ 3C antibody is cleavage sensitive and detects only the intact C terminus of $beta$ 3 integrin (10). The anti-talin 8d4 antibody (Sigma) recognized the intact talin and cleaved the 190-kDa fragment but not the 50-kDa fragment. The same results were obtained in four independent experiments.

Studies with pharmacological inhibitors of tyrosine kinases have shown that the platelet agonists trigger inside-out signalingvia $alpha$ IIb $beta$ 3 integrin by tyrosine phosphorylation of proteins inthe molecular mass range of 54, 60, 64, 75, and 130 to 140 kDa(6, 7, 13, 14). Moreover, the cytoplasmic domain of $beta$ 3 integrin is itself tyrosine phosphorylated as a consequenceof outside-in signaling and plays an important role in the regulationof integrin-myosin interaction during clot retraction (18, 22).Most agonists, except collagen, activate platelets by bindingto G protein coupled receptors, and the agonist-induced plateletaggregation and secretion parallel this activity with a concomitantincrease in the tyrosine phosphorylation of multiple proteins(24, 33). These phosphorylation events occur in distinct temporalwaves. The early tyrosine phosphorylation of proteins such asp21^ras GAP (4), cortactin (11), p60^src (5), and RAFTK/Pyk2 (29) follows engagement of $alpha$ IIb $beta$ 3 integrinwith fibrinogen resulting in platelet aggregation-dependent tyrosinephosphorylation of several proteins, such as focal adhesion kinase,p72^syk, vinculin, paxillin, and the cytoplasmic domain of $beta$ 3 integrinitself (7, 22, 23, 28, 38). Calpain-dependent proteolysisof phosphotyrosine phosphatase 1B has also been implicated inthe regulation of tyrosine phosphorylation following plateletaggregation (41).

We explored the mechanism of µ-calpain-mediated signaling by Western blotting using antiphosphotyrosine antibodies. Time courseanalysis revealed that the level of tyrosine phosphorylation ofseveral proteins was significantly reduced (~70% reduction) inµ-calpain null platelets upon their activation with either calciumionophore or thrombin (Fig. 4c and d). Striking differences intyrosine phosphorylation were seen at 30 s after the additionof ionophore or thrombin, the time period that encompasses theinitiation of platelet aggregation. The most notable phosphorylationdifference was observed for the band corresponding to the $beta$ 3 subunitof $alpha$ IIb $beta$ 3 integrin (~70% reduction), although several other asyet unidentified polypeptides ranging in molecular mass from 54to 150 kDa were also underphosphorylated during the initial phaseof platelet activation (Fig. 4c and d). To confirm that the $beta$ 3integrin cytoplasmic domain is underphosphorylated, we immunoprecipitatedthe $beta$ 3 integrin from wild-type and µ-calpain null platelets andimmunoblotted with antiphosphotyrosine antibodies. Indeed, the $beta$ 3 subunit of $alpha$ IIb $beta$ 3 integrin is significantly underphosphorylatedat tyrosine residues as a consequence of µ-calpain deficiency(Fig. 5a and b). We suggest that the underphosphorylation of $beta$ 3integrin at one or both tyrosine residues in its cytoplasmic domainmay lead to defective platelet aggregation and clot retraction(18, 21). Together, our results provide the first direct evidencefor the functional requirement of µ-calpain in the agonist-inducedactivation of tyrosine phosphorylation during platelet activation.How the µ-calpain activity modulates tyrosine phosphorylationof platelet proteins, including $beta$ 3 integrin, remains an issueof fundamental importance and requires an extensive biochemicalanalysis of the µ-calpain-deficient platelets in terms of definedeffects of µ-calpain on specific modulatory molecules and signalingpathways.

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FIG. 5. Immunoprecipitation and tyrosine phosphorylation of the $beta$ 3 subunit of $alpha$ IIb $beta$ 3 integrin. The $beta$ 3 integrin was immunoprecipitated using biotin-conjugated anti-mouse antibody against the integrin $beta$ 3 chain. Immunoprecipitates (IP) were analyzed by SDS-PAGE (8% gel), transferred to a nitrocellulose membrane, and blotted (IB) an antiphosphotyrosine antibody, 4G10 (upper panel). The same blot was stripped and blotted with an anti-N $beta$ 3 antibody to normalize the amount of $beta$ 3 integrin in each lane (lower panel).

The biological function of calpains has been extensively investigated using synthetic inhibitors of calpain activity. Becausethe calpain inhibitors cannot distinguish between µ- and m-calpains,the specific role of each calpain remains to be established inplatelet secretion, aggregation, and spreading (9). Our findingsbegin to resolve some of these questions, and the Capn1^/ mice would be useful in evaluating the function of µ-calpainin apoptosis, cell shape regulation, the pathogenesis of Alzheimer'sdisease, and numerous other cellular processes. Recently, thegenetic disruption of the small regulatory subunit of murine calpain(Capn4) has been reported (1). The small subunit is requiredfor the activity of µ-calpains as well as m- calpains, and theCapn4^/ embryos die at midgestation with defects in vasculogenesis anderythropoiesis (1). Since our µ-calpain null mice have no apparentembryological defects, this would suggest that m-calpain compensatesfor µ-calpain in Capn1^/ mice. The future generation of m-calpain-deficient mice may alsoallow assessment of the individual and specific contributionsof both µ-and m-calpains in a diverse array of biologically importantprocesses. Combined with the availability of mice specificallylacking µ-calpain, as reported here, we may finally begin to comprehendthe biological function of conventional calpains in mammalianphysiology.

	ACKNOWLEDGMENTS

This work was partially supported by grants from the National Institutes of Health to A.H.C. and A.K.

We thank Toshihiko Hanada, Hani Hassoun, and David Liu for many helpful suggestions during the course of these studies. Weare also grateful to D. Marie-Mironchuk for help with the artwork,Xiaoping Du of the University of Illinois, Chicago, for the giftof the anti- $beta$ 3C antibody, and Gary Sclar for help with the microinjectionexperiments.

M.A. and S.S.A. contributed equally to thiswork.

	FOOTNOTES

^* Corresponding author. Mailing address: Biomedical Research, CBR 404, St. Elizabeth's Medical Center, 736 Cambridge St., Boston,MA 02135. Phone: (617) 789-3118. Fax: (617) 789-3111. E-mail:Athar_Chishti{at}cchcs.org.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References

1. Arthur, J. S. C., J. S. Elce, C. Hegadorn, K. Williams, and P. A. Greer. 2000. Disruption of the murine calpain small subunit gene, Capn4: calpain is essential for embryonic development but not for cell growth and division. Mol. Cell. Biol. 20:4474-4481[Abstract/Free Full Text].

2. Baier, L. J., P. A. Permana, X. Yang, R. E. Pratley, R. L. Hanson, G. Q. Shen, D. Mott, W. C. Knowler, N. J. Cox, Y. Horikawa, N. Oda, G. I. Bell, and C. Bogardus. 2000. A calpain-10 gene polymorphism is associated with reduced muscle mRNA levels and insulin resistance. J. Clin. Investig. 106:R69-R73.

3. Calderwood, D. A., R. Zent, R. Grant, D. J. Rees, R. O. Hynes, and M. H. Ginsberg. 1999. The Talin head domain binds to integrin beta subunit cytoplasmic tails and regulates integrin activation. J. Biol. Chem. 274:28071-28074[Abstract/Free Full Text].

4. Cichowski, K., F. McCormick, and J. S. Brugge. 1992. p21rasGAP association with Fyn, Lyn, and Yes in thrombin-activated platelets. J. Biol. Chem. 267:5025-5028[Abstract/Free Full Text].

5. Clark, E. A., and J. S. Brugge. 1993. Redistribution of activated pp60c-src to integrin-dependent cytoskeletal complexes in thrombin-stimulated platelets. Mol. Cell. Biol. 13:1863-1871[Abstract/Free Full Text].

6. Clark, E. A., S. J. Shattil, and J. S. Brugge. 1994. Regulation of protein tyrosine kinases in platelets. Trends Biochem. Sci. 19:464-469[CrossRef][Medline].

7. Clark, E. A., S. J. Shattil, M. H. Ginsberg, J. Bolen, and J. S. Brugge. 1994. Regulation of the protein tyrosine kinase pp72syk by platelet agonists and the integrin alpha IIb beta 3. J. Biol. Chem. 269:28859-28864[Abstract/Free Full Text].

8. Croall, D. E., and G. N. DeMartino. 1991. Calcium-activated neutral protease (calpain) system: structure, function, and regulation. Physiol. Rev. 71:813-847[Free Full Text].

9. Croce, K., R. Flaumenhaft, M. Rivers, B. Furie, B. C. Furie, I. M. Herman, and D. A. Potter. 1999. Inhibition of calpain blocks platelet secretion, aggregation, and spreading. J. Biol. Chem. 274:36321-36327[Abstract/Free Full Text].

10. Du, X., T. C. Saido, S. Tsubuki, F. E. Indig, M. J. Williams, and M. H. Ginsberg. 1995. Calpain cleavage of the cytoplasmic domain of the integrin beta 3 subunit. J. Biol. Chem. 270:26146-26151[Abstract/Free Full Text].

11. Fox, J. E., L. Lipfert, E. A. Clark, C. C. Reynolds, C. D. Austin, and J. S. Brugge. 1993. On the role of the platelet membrane skeleton in mediating signal transduction. Association of GP IIb-IIIa, pp60c-src, pp62c-yes, and the p21ras GTPase-activating protein with the membrane skeleton. J. Biol. Chem. 268:25973-25984[Abstract/Free Full Text].

12. Hayashi, M., H. Suzuki, S. Kawashima, T. C. Saido, and M. Inomata. 1999. The behavior of calpain-generated N- and C-terminal fragments of talin in integrin-mediated signaling pathways. Arch. Biochem. Biophys. 371:133-141[CrossRef][Medline].

13. Hers, I., J. Donath, P. E. M. H. Litjens, G. van Willigen, and J. W. Akkerman. 2000. Inhibition of platelet integrin $alpha$ _IIb $beta$ ₃ by peptides that interfere with protein kinases and the $beta$ ₃ tail. Arterioscler. Thromb. Vasc. Biol. 20:1651-1660[Abstract/Free Full Text].

14. Hers, I., J. Donath, G. van Willigen, and J. W. Akkerman. 1998. Differential involvement of tyrosine and serine/threonine kinases in platelet integrin alphaIIbbeta3 exposure. Arterioscler. Thromb. Vasc. Biol. 18:404-414[Abstract/Free Full Text].

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1.	Arthur, J. S. C., J. S. Elce, C. Hegadorn, K. Williams, and P. A. Greer. 2000. Disruption of the murine calpain small subunit gene, Capn4: calpain is essential for embryonic development but not for cell growth and division. Mol. Cell. Biol. 20:4474-4481[Abstract/Free Full Text].
2.	Baier, L. J., P. A. Permana, X. Yang, R. E. Pratley, R. L. Hanson, G. Q. Shen, D. Mott, W. C. Knowler, N. J. Cox, Y. Horikawa, N. Oda, G. I. Bell, and C. Bogardus. 2000. A calpain-10 gene polymorphism is associated with reduced muscle mRNA levels and insulin resistance. J. Clin. Investig. 106:R69-R73.
3.	Calderwood, D. A., R. Zent, R. Grant, D. J. Rees, R. O. Hynes, and M. H. Ginsberg. 1999. The Talin head domain binds to integrin beta subunit cytoplasmic tails and regulates integrin activation. J. Biol. Chem. 274:28071-28074[Abstract/Free Full Text].
4.	Cichowski, K., F. McCormick, and J. S. Brugge. 1992. p21rasGAP association with Fyn, Lyn, and Yes in thrombin-activated platelets. J. Biol. Chem. 267:5025-5028[Abstract/Free Full Text].
5.	Clark, E. A., and J. S. Brugge. 1993. Redistribution of activated pp60c-src to integrin-dependent cytoskeletal complexes in thrombin-stimulated platelets. Mol. Cell. Biol. 13:1863-1871[Abstract/Free Full Text].
6.	Clark, E. A., S. J. Shattil, and J. S. Brugge. 1994. Regulation of protein tyrosine kinases in platelets. Trends Biochem. Sci. 19:464-469[CrossRef][Medline].
7.	Clark, E. A., S. J. Shattil, M. H. Ginsberg, J. Bolen, and J. S. Brugge. 1994. Regulation of the protein tyrosine kinase pp72syk by platelet agonists and the integrin alpha IIb beta 3. J. Biol. Chem. 269:28859-28864[Abstract/Free Full Text].
8.	Croall, D. E., and G. N. DeMartino. 1991. Calcium-activated neutral protease (calpain) system: structure, function, and regulation. Physiol. Rev. 71:813-847[Free Full Text].
9.	Croce, K., R. Flaumenhaft, M. Rivers, B. Furie, B. C. Furie, I. M. Herman, and D. A. Potter. 1999. Inhibition of calpain blocks platelet secretion, aggregation, and spreading. J. Biol. Chem. 274:36321-36327[Abstract/Free Full Text].
10.	Du, X., T. C. Saido, S. Tsubuki, F. E. Indig, M. J. Williams, and M. H. Ginsberg. 1995. Calpain cleavage of the cytoplasmic domain of the integrin beta 3 subunit. J. Biol. Chem. 270:26146-26151[Abstract/Free Full Text].
11.	Fox, J. E., L. Lipfert, E. A. Clark, C. C. Reynolds, C. D. Austin, and J. S. Brugge. 1993. On the role of the platelet membrane skeleton in mediating signal transduction. Association of GP IIb-IIIa, pp60c-src, pp62c-yes, and the p21ras GTPase-activating protein with the membrane skeleton. J. Biol. Chem. 268:25973-25984[Abstract/Free Full Text].
12.	Hayashi, M., H. Suzuki, S. Kawashima, T. C. Saido, and M. Inomata. 1999. The behavior of calpain-generated N- and C-terminal fragments of talin in integrin-mediated signaling pathways. Arch. Biochem. Biophys. 371:133-141[CrossRef][Medline].
13.	Hers, I., J. Donath, P. E. M. H. Litjens, G. van Willigen, and J. W. Akkerman. 2000. Inhibition of platelet integrin $alpha$ _IIb $beta$ ₃ by peptides that interfere with protein kinases and the $beta$ ₃ tail. Arterioscler. Thromb. Vasc. Biol. 20:1651-1660[Abstract/Free Full Text].
14.	Hers, I., J. Donath, G. van Willigen, and J. W. Akkerman. 1998. Differential involvement of tyrosine and serine/threonine kinases in platelet integrin alphaIIbbeta3 exposure. Arterioscler. Thromb. Vasc. Biol. 18:404-414[Abstract/Free Full Text].
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