Competitive Interactions of Collagen and a Jararhagin-derived Disintegrin Peptide with the Integrin α2-I Domain*

Integrin α2β1 is a major receptor required for activation and adhesion of platelets, through the specific recognition of collagen by the α2-I domain (α2-I), which binds fibrillar collagen via Mg2+-bridged interactions. The crystal structure of a truncated form of the α2-I domain, bound to a triple helical collagen peptide, revealed conformational changes suggestive of a mechanism where the ligand-bound I domain can initiate and propagate conformational change to the full integrin complex. Collagen binding by α2-I and fibrinogen-dependent platelet activity can be inhibited by snake venom polypeptides. Here we describe the inhibitory effect of a short cyclic peptide derived from the snake toxin metalloprotease jararhagin, with specific amino acid sequence RKKH, on the ability of α2-I to bind triple helical collagen. Isothermal titration calorimetry measurements showed that the interactions of α2-I with collagen or RKKH peptide have similar affinities, and NMR chemical shift mapping experiments with 15N-labeled α2-I, and unlabeled RKKH peptide, indicate that the peptide competes for the collagen-binding site of α2-I but does not induce a large scale conformational rearrangement of the I domain.

The integrins constitute a functionally versatile family of integral membrane receptors that mediate cell-cell and cellextracellular matrix interactions through their regulation of cell adhesion, differentiation, migration, and the immune response (1)(2)(3)(4)(5). Signal transduction is bi-directional through both outside-in and inside-out mechanisms. All integrins are heterodimers composed of subunits ␣ and ␤. Different combinations of subunits are expressed on different cell types with the interplay of 19 ␣ and 8 ␤ subunits, generating a family of 25 different heterodimers (3,5).
The integrin receptors share common structural features. The extracellular portions of the ␣ and ␤ subunits combine to form a globular "head" domain that is attached to a pair of membrane-spanning helical "stalks." Signal transduction is believed to involve an allosteric rearrangement characterized by the separation and reorientation of the stalk segments. The bidirectional nature of signal transduction is complex. Extracellular ligands induce outside-in signals by binding to fixed motifs in the head domain, whereas inside-out signaling ensues from intracellular interactions between relatively short structurally plastic control elements and a large repertoire of cellular proteins.
In nine of the human ␣ subunits, ligand recognition is carried out by a 200-residue structurally conserved inserted (I) domain or a von Willebrand factor A domain (3,5). The I and A domains adopt a Rossmann dinucleotide-binding fold, with a 6-stranded ␤-sheet surrounded by seven ␣-helices, and ligand recognition requires the binding of a single Mg 2ϩ ion to a metal ion-dependent adhesion (MIDAS) 2 motif (6,7). The importance of the ␣ I domain for understanding conformational regulation and ligand binding for all integrins has been reviewed recently (5).
Integrin ␣2␤1 is a member of the collagen/laminin receptor family and is a major receptor required for activation and adhesion of platelets, through the specific recognition of collagen by the ␣2-I domain (␣2-I) (8), which binds fibrillar collagen via Mg 2ϩ -bridged interactions, supported by the MIDAS motif residues Asp-151, Ser-153, Thr-221, and Asp-254. The crystal structure of the ␣2-I domain, bound to a triple helical collagen peptide, revealed conformational changes from an unbound "closed" form to a bound "open" form, suggestive of a mechanism where the ligand-bound I domain can initiate and propagate conformational change to the full integrin complex (9).
Collagen binding and fibrinogen-dependent platelet activity can be inhibited by snake venom polypeptide toxins, enhancing the effects of hemorrhagic venom metalloproteases. These socalled disintegrins are functional homologues of the Arg-Gly-Asp (RGD) motif found in extracellular matrix proteins. Integrin ␣2␤1 associates with Jararhagin, a 52-kDa metalloprotease isolated from the venom of the Brazilian pit viper Bothrops jararaca, that targets multiple components in hemostasis, including von Willebrand factor, fibrinogen, and platelet aggregation. Anti-platelet activity is thought to stem from its specificity for the ␣2␤1 integrin (10 -14).
Notably, a short cyclic peptide derived from the jararhagin metalloprotease domain, containing the specific amino acid sequence RKKH, is sufficient to prevent binding of type I collagen to ␣2-I in a competitive manner and is capable of disrupting cell adhesion to type I collagen (15). The cyclic RKKH peptidebinding site coincides with the collagen-binding site, near the I domain MIDAS motif (16). The inhibitory effects of the RKKH peptides on the homologous ␣1␤1 integrin have been suggested to reflect the ability of the peptide to mimic the natural type I collagen ligand by inducing or stabilizing a conformational transition from the closed to the open form of the I domain (17).
In this study we characterize the conformational dynamics of the ␣2-I domain and its interactions with collagen and RKKH peptides. Our studies show that the RKKH peptide binds the ␣2-I domain and inhibits its association with type I collagen, without inducing a conformational change in the ␣2-I domain.

EXPERIMENTAL PROCEDURES
Materials-The pET-28b expression plasmid was from Invitrogen. ( 15 NH 4 ) 2 SO 4 , [ 13 C]glucose, and D 2 O were purchased from Cambridge Isotopes Laboratories. Nickel-nitrilotriacetic acid-agarose was from Qiagen. The reverse phase Delta Pak C18 HPLC column (300 ϫ 7.8 mm; 300 Å) was obtained from Waters. The 24-residue type I collagen peptide with the GFOGER recognition sequence (O ϭ hydroxyproline, Hyp) was purchased in HPLC-purified powder form from Biomer Technology (Hayward, CA). The partially purified RKKH peptide was purchased from Genscript (Piscataway, NJ). The peptide sequences are shown in Fig. 1.
Expression and Purification of Integrin ␣2-I Domain-The recombinant ␣2-I domain used in these studies corresponds to residues 144 -334 of the human sequence (NCBI accession number NP_002194). The DNA coding for the sequence was inserted into the NdeI/XhoI site of the pET-28b expression plasmid (Invitrogen). For eventual chemical derivatization, Ser-334, at the C terminus, was mutated to Cys. Site-directed mutagenesis was used to convert Cys-150 to Leu. The resulting plasmid, pNHis-␣2-I(144 -334)C150L, has a His 6 tag at the N terminus for purification. The sequence of the expressed protein is shown in Fig. 1.
Recombinant ␣2-I domain was expressed in Escherichia coli strain BL21(DE3). To prepare 15 N-and 13 C-labeled protein for NMR experiments, cells bearing pNHis-␣2-I(144 -334)C150L were grown in minimal M9 media containing ( 15 NH 4 ) 2 SO 4 and/or [ 13 C]glucose. Induction at A 600 ϭ 1 with 1 mM isopropyl 1-thio-␤-D-galactopyranoside for 2 h at 37°C gave high level expression of the protein in the soluble fraction. Cells were lysed using a French press in buffer D (50 mM Tris, pH 8.0, 1 M NaCl, 30 mM imidazole), and the ␣2-I domain was purified by nickel-affinity chromatography on nickel-nitrilotriacetic acidagarose, in buffer C (50 mM Tris, pH 7, 1 M NaCl, 300 mM imidazole). The purified protein solution was dialyzed against two changes of buffer A (50 mM Tris, pH 8.0, 150 mM NaCl) with 1 mM EDTA, followed by two changes of buffer B (50 mM PO 4 , pH 7.0, 150 mM NaCl, 5 mM MgSO 4 ) with 1 mM dithiothreitol, using dialysis membranes with a molecular weight cutoff of 10,000. The final yield of purified protein was 20 mg/liter of cell culture. For NMR experiments, the protein solution was concentrated by ultrafiltration to 0.7 mM (⑀ ϭ 17330 cm Ϫ1 M Ϫ1 ).
For experiments with the RKKH peptide, the surface-exposed C-terminal Cys residue of the ␣2-I domain was alkylated with iodoacetamide as follows. Purified protein was dialyzed against four changes of buffer A. The protein was removed from the dialysis bag, reacted with 10 mM iodoacetamide for 10 h at 4°C, dialyzed against two changes of buffer B, and concentrated by ultrafiltration.
Formation of Collagen Triple Helix-To obtain a collagen triple helix, the 24-residue collagen peptide powder was suspended in buffer B at 1 mM concentration, heated to 45°C, and then allowed to equilibrate at 4°C for at least 12 h, as described previously (18).
Formation of Cyclic RKKH Peptide-Formation of cyclic peptide was obtained by forming a disulfide link between the terminal Cys residues as described (15). The peptide was dissolved at 1 mg/ml concentration in 0.1 M NH 4 CO 3 and incubated at 4°C for 24 h. The reaction was flash-frozen and the water removed by lyophilization. The cyclized peptide was resuspended in HPLC grade water and purified by reverse phase HPLC. Peak fractions were combined, frozen, and lyophilized to powder. A colorimetric assay using 5,5Ј-dithiobis(2-nitrobenzoic acid), to test for the presence of free thiol, showed complete conversion to the cyclized product within the limits of detection. The cyclized peptide was suspended in buffer B immediately before experiments.
NMR Spectroscopy-NMR experiments were performed on Bruker AVANCE 600-and 800-MHz spectrometers. The standard 1 H/ 15 N fast HSQC pulse sequence was used for experiments with peptides (19). Backbone resonance assignments were made using a standard CBCA(CO)NH experiment (20) and by comparison with the assignments reported previously by Elshorst et al. (21) for the same polypeptide. The chemical shifts are referenced to the 1 H 2 O resonance, set to its expected position of 4.87 ppm at 20°C (22). The NMR data were processed using NMRPipe (23), and the spectra were assigned and analyzed using Sparky (24). All experiments were performed at millimolar concentrations of collagen or the RKKH to obtain saturation of the ␣2-I domain, for a single site binding model of interaction and the measured affinity of the peptides for ␣2-I (see below).
Isothermal Titration Calorimetry (ITC)-The ␣2-I domain, the triple helix collagen peptide, and the cyclized RKKH peptide were all dissolved in buffer B. The pH of each solution was measured to ensure that no changes were produced by the polypeptide components. For the collagen binding experiments the concentration of ␣2-I domain in the cell was 100 M and that of the collagen peptide solution 1 mM. For the RKKH binding experiments, the ␣2-I domain was Cysalkylated with iodoacetamide, and its concentration in the sample cell was 100 M. The concentration of cyclized RKKH was 1 mM.
ITC experiments were performed with a Microcal VP-ITC calorimeter. Measurements were made by titration of collagen or RKKH peptide into the ␣2-I domain at a temperature of 10°C. For titration experiments, the ␣2-I domain was degassed and placed in the 1.4-ml reaction cell. The collagen or RKKH peptides were loaded in the 250-l injection syringe, and a series of 8-l injections over 16 s were made, with a spacing of 500 s between injections over 300 min. The reference power was set to 20 cal/s, and the stirring speed was 300 rpm. Parallel control experiments, to correct for the heat of mixing, were performed by adding the peptide to a sample cell containing only buffer without ␣2-I domain.
The thermodynamic data were processed with the ORIGIN program (Microcal) to extract the enthalpic, entropic, and equilibrium constants. Nonlinear least squares fitting was done using a single site binding model.
Size Exclusion Chromatography-Size exclusion chromatography was performed at 4 or 22°C, using an Acta

Association of ␣2-I with Type I Collagen Peptide and RKKH
Disintegrin Peptide-In activated platelets ␣2␤1 integrin has a high affinity for soluble collagen with an associated K d of 35-90 nM (25), whereas the affinity of the ␣2-I domain for type I collagen measured by surface plasmon resonance is weaker, with a K d in the low micromolar range (26,27). Recognition by ␣2␤1 resides totally within the collagen sequence GFOGER, where Glu cannot be replaced by Asp, and sequence recognition is entirely dependent upon the presence of a triple helical conformation (28). To determine the affinity of ␣2-I for the triple helical type I collagen peptide, we performed ITC experiments where the 26-residue collagen peptide, containing the GFOGER recognition sequence (Fig. 1B), was titrated into the ␣2-I domain. This peptide sequence is similar to that which was co-crystallized with ␣2-I (9).
To maintain the collagen peptide in its active triple helical form, the ITC cell temperature was kept at 10°C, below the predicted melting temperature of about 20°C (9). The results are shown in Fig. 2A, and the free energy parameters are reported in Table 1. Fitting the ITC data to a single-site binding curve (Fig. 2C) yields a K d of 7.8 M.
ITC was also performed to determine the affinity of ␣2-I for a cyclic RKKH peptide whose sequence had been previously identified to have the most potent inhibitory effect on ␣2-I ( Fig.  1C) (15). To enable direct comparison with the affinity determined for collagen, this study was also performed at 10°C. Fig.  2B shows the titration profile, and the thermodynamic parameters are reported in Table 1. The data fit to a single-site binding model (Fig. 2D) with a K d of 8.0 M, consistent with the IC 50 of 1.2 M, estimated in competition assays for the inhibition of collagen binding (15).
Characterization of the ␣2-I-Collagen Complex-To further characterize the formation of the ␣2-I-collagen complex, we performed size exclusion chromatography at temperatures below or above the melting transition of the collagen triple helix (Fig. 3, A and B). Isolated ␣2-I elutes with an apparent molecular mass near 30 kDa at both temperatures (peak a), whereas the collagen peptide elutes near 20 kDa (peak b). We attribute the differences between these observed values and those expected from the calculated molecular weights of the proteins (23 kDa for ␣2-I; 6.8 kDa for triple helical collagen peptide; 2.3 kDa for monomeric collagen peptide) to the hydrodynamic radii of the molecules, which govern the elution profiles. In particular, the elution of collagen is likely to be dominated by the rod-like shape of the triple helix. However, it is interesting to note that the peptide elutes at a slightly higher apparent molecular weight at 4 than 22°C, reflecting triple helix formation below the melting temperature. This is further corroborated by the elution profiles of premixed ␣2-I and collagen. At 22°C, the elution profile is identi-   cal to that of the individual components, with two resolved peaks corresponding to either ␣2-I (Fig. 3A, peak a) or collagen ( Fig. 3A, peak b). However, when the molecules are combined and eluted at 4°C, a new peak appears at a higher apparent molecular mass of about 45 kDa (Fig. 3B, peak c), indicating complex formation with triple helical collagen. These results are consistent with specific recognition by ␣2-I of the GFOGER sequence properly displayed in triple helical collagen (28). The size exclusion results in Fig. 3 further show that the ␣2-I domain and collagen form a stable long lived complex and help explain the NMR results, where the extreme broadening observed in the presence of collagen reflects the formation of a large slowly tumbling biomolecular species (see below).
Effects of Mg 2ϩ and Collagen on ␣2-I-The ␣2-I domain possesses high affinity for type I collagen in the presence of the divalent metal cation Mg 2ϩ . The metal-binding site consists of MIDAS motif residues Asp-151, Ser-153, Ser-155, Thr-221, Asp-254, and Glu-256 which form an octahedral coordination sphere composed of direct and water-bridged interactions. The structural role of Mg 2ϩ has been examined using both x-ray and NMR methods in the CD11a/LFA-1 I domain (29 -32), where Mg 2ϩ was found to play a role in ligand binding, and its removal did not cause large scale structural change in the CD11a/LFA-1 I domain.
The crystal structure of ␣2-I bound to triple helical collagen suggests that collagen binding is accompanied by a large conformational rearrangement of the C-terminal helix, coupled with changes in the coordination the Mg 2ϩ metal (9). Collagen binding causes three concerted changes in the I domain; the loops of the MIDAS motif are perturbed because of a rearrangement upon insertion of a collagen Glu side chain into the metal coordination sphere; helices h6 and h7 rearrange to open up the top surface; and helix h7 moves downward to the opposite pole of the MIDAS motif. The rearrangement of helix h7 is thought to produce the large scale conformational changes experienced by the integrin heterodimer during signaling. To see if the protein dynamics and conformation associated with Mg 2ϩ and collagen binding could be characterized in solution, we examined the 1 H/ 15 N HSQC NMR spectrum of ␣2-I in the presence or absence of metal and collagen.
The 1 H and 15 N chemical shifts from protein backbone amide groups are very sensitive to changes in protein conformation or chemical environment and can be used to monitor the equilibrium exchange between states arising from free and ligand-bound protein (22). If the exchange rate is faster than the difference between the chemical shifts measured for the two states, then the system is in fast exchange, and one peak is observed at the population-weighted average chemical shift of the two states. NMR can be used to detect weak binding or minor conformational rearrangements, and chemical shift changes as small as 0.02 ppm have been reported for minor local effects on protein structure resulting from binding of small molecules or modifications, whereas much larger changes (Ͼ1 ppm) can reflect major conformational rearrangements (33)(34)(35)(36).
A sample of metal-free ␣2-I domain (isotopically enriched with 15 N) was prepared by exhaustive dialysis against EDTA. The 1 H-15 N HSQC spectra of the metal-free and Mg 2ϩbound forms of the ␣2-I domain are shown in Fig. 4A. Several peaks undergo measurable frequency changes reflecting metal binding. A plot of the total change in 1 H and 15 N chemical shifts against amino acid number shows that the peaks with the largest frequency changes are localized to residues involved in direct coordination of Mg 2ϩ in the MIDAS motif (Fig. 5). This is further highlighted by mapping the frequency changes on the previously determined crystal structure of the ␣2-I domain (Fig. 6C). However, most of the peaks from other residues throughout the protein structure do not change, indicating that Mg 2ϩ binding does not induce a large scale conformational change of the ␣2-I domain in solution. This is similar to the results reported for LFA-1 (31).
A potential indicator of close association between the metalbinding site and conformational change in helix h7 is the chemical shift change observed for Glu-318 in the spectra from metal-bound and unbound ␣2-I. Glu-318 is located in the loop preceding the C-terminal helix and is characterized by a distinctive downfield chemical shift ( 1 H ϳ 11.5 ppm). In the comparison of the structures of the collagen-bound and unbound forms of the ␣2-I domain, it was noted that Glu-318 in the unbound form of ␣2-I domain is engaged in a salt bridge interaction with Arg-288, which is not present in the collagenbound form (9). In addition, Glu-318 and Asp-317 are observed to undergo a pronounced torsion angle change associated with the displacement of helix h7. The observed change in Glu-318 chemical shift upon addition of Mg 2ϩ indicates close association of this residue with the MIDAS-binding site. However, other residues in helix h7, including Asp-317, do not change upon addition of metal, indicating that metal binding alone does not induce the conformational transition from the closed to the open state of the I domain.
To probe conformational changes of the ␣2-I domain upon binding to type I collagen, a series of NMR titration experiments were performed with a 26-residue collagen peptide containing the GFOGER recognition sequence, similar to that previously co-crystallized with the ␣2-I domain (Fig. 1B). The melting temperature for triple helix formation of this peptide is predicted to be around 20°C (9). The collagen triple helix was allowed to form for 12 h at 6°C and then combined with ␣2-I solution at 10°C for NMR studies, which were also performed at 10°C to maintain the triple helical conformation.
Additions of increasing concentrations of triple helical collagen lead to a dramatic progressive loss of signal intensity for all peaks in the NMR spectrum of ␣2-I (Fig. 4B), reflecting the formation of a large slowly tumbling complex and/or slow conformational exchange on the NMR time scale. The formation of a large complex is consistent with the size exclusion data at low temperature. The reduced peak intensity is also exacerbated by slower molecular tumbling rates due the need to perform experiments at 10°C. Further addition of collagen to ␣2-I, above 1:1 molar ratio, causes the NMR signals to disappear completely (data not shown). The apparent lack of concomitant line broadening for the remaining peaks (see Fig. 8, A-D) suggests that complex formation leads to the complete disappearance of the signals from ␣2-I/collagen, rather than a reduction in local backbone dynamics.
A few peaks are also seen to undergo a change in chemical shift frequencies (Fig. 7), and for some of these, the presence of two distinct resonances, one shifted and the other at the same frequencies as free ␣2-I, may reflect slow exchange between the bound and unbound forms of ␣2-I. Interestingly, these peaks map to residues situated in (Gly-329) or near (Asp-145, Val-194, Thr-202, Ser-236, Ala-245, Glu-309, and Glu-318) the C-terminal helix (Fig. 6C) and may reflect the conformational change indicated by the crystal structure of collagen-bound ␣2-I. We note that in the crystal structure the last 13 amino acids in the C terminus, including seven residues in helix h7, were not visible.
Effect of Cyclic RKKH Peptide on ␣2-I-The ability of recombinant ␣2-I domain to recapitulate the interaction of the integrin ␣2␤1 heterodimer with RKKH has been demonstrated (15) and provides the basis for the experiments described below. Mutational studies with ␣2-I indicate that cyclic RKKH peptides bind near the MIDAS motif ␣2-I (15,16), suggesting a mechanism of direct competition for the collagen-binding site, and the interaction of cyclic RKKH with ␣1I has been suggested to induce or stabilize a conformational transition from the closed to the open form of integrin (17). To characterize the ␣2-I-RKKH interaction, we examined the influence of an RKKH sequence, previously identified to inhibit the association of ␣2-I with type I collagen (15), on the solution NMR spectra of ␣2-I.
The effect of RKKH on the 1 H/ 15 N HSQC spectrum of ␣2-I is shown in Fig. 4C. Favorable linewidths and chemical shift dispersion allowed 172 of the expected 188 ␣2-I resonances to be analyzed. The addition of RKKH (1.5:1 RKKH:␣2-I, molar ratio) causes almost no changes in the HSQC spectrum of ␣2-I, with the exception of four peaks that undergo very small but measurable frequency changes (⌬N Ͻ 0.01 ppm; ⌬H Ͻ 0.01 ppm). Three of these peaks correspond to residues (Asn-189, Thr-221, and Asn-222) that map to the MIDAS motif of ␣2-I, near the predicted collagen-binding site (Fig. 6C), whereas a fourth peak corresponds to His-272, situated on the opposite  pole far from the other perturbed residues, which is susceptible to slight changes in buffer conditions.
Notably, Thr-221 in the MIDAS motif is absolutely critical for collagen binding to the recombinant ␣2-I domain, as well as for ligand binding in the ␣M-I and ␣L-I domains (9,37,38). The finding that this is the residue most affected by cyclic RKKH peptide indicates that it also plays a role in mediating the interaction of ␣2-I with RKKH. Thr-221 is near Asp-219, which is also critical for collagen binding (9). Asp-219 was predicted to play a role in RKKH peptide binding (16); however, mutating this residue to Arg caused RKKH to bind with higher affinity (16), and the NMR data showed no effect on Asp-219 because of RKKH binding.
Aside for the small changes observed for these few residues, the near lack of changes in the NMR spectrum does not support the notion of a structural transition induced in the ␣2-I domain by the RKKH peptide. Instead, the high content of charged residues in the RKKH sequence suggests that charge-charge side chain interactions are responsible for mediating the association between ␣2-I and RKKH.
To characterize the inhibitory effect of cyclic RKKH on ␣2-I/ collagen binding, we examined the effect of RKKH peptide on the intensity of NMR signals from the ␣2-I/collagen complex. Addition of RKKH to the ␣2-I/collagen sample restores some of the ␣2-I signal intensity which had been lost upon collagen binding. This is illustrated for four isolated NMR peaks in Fig. 8  (A-D), however, the effect is uniform across the spectrum of ␣2-I, reflecting the effective inhibition of the ␣2-I/collagen interaction by RKKH. The effect of RKKH on peak intensity increases with increasing peptide concentration up to a 2:1 molar ratio of RKKH to ␣2-I, beyond which no further changes are observed (Fig. 8E). Taken together with the small frequency changes observed upon RKKH binding, these results suggest that RKKH inhibits by competing for the collagen-binding site on ␣2-I.
To further test whether RKKH and collagen compete for the same binding site on ␣2-I, we examined the effects of RKKH on ␣2-I peak intensity in samples where collagen was added to ␣2-I after RKKH (Fig. 8F). Although the addition of collagen to ␣2-I (1:1, collagen:␣2-I, molar ratio) dramatically reduces the ␣2-I signal intensity by as much as 84%, the addition of RKKH to free ␣2-I (1.5:1, RKKH:␣2-I, molar ratio) causes no changes in intensity. When ␣2-I is combined first with RKKH and then collagen is added, the peak intensity decreases only by 22%, in a manner distinctly different from the addition of collagen alone. Further addition of collagen peptide up to 2:1 (collagen:␣2-I, molar ratio) shows that as the RKKH concentration is exceeded, the peak heights are reduced to a level similar to that of the addition of collagen alone.
Thus we conclude that the mechanism of RKKH inhibition involves direct binding of RKKH to ␣2-I. Both RKKH and collagen compete for the same binding site on the ␣2-I domain, with RKKH exchanging more rapidly than triple helical colla- B, residues in red correspond to peaks that move in Fig. 7. C, residues in red have peaks that undergo minor but measurable frequency changes. gen; however, RKKH binding does not induce a conformational change in the ␣2-I domain.

DISCUSSION
The collagen binding activity of the ␣2␤1 integrin resides entirely in the I domain and provides the basis for the development of integrin signaling inhibitors. Such inhibitors include the jararhagin RKKH peptide that is the focus of this study. The RKKH inhibitors were originally identified by screening short cyclic peptides for their ability to bind the recombinant ␣2-I domain and disrupt collagen binding (15).
Our findings confirm the inhibitory properties of the cyclic RKKH peptide. However, they point to a mechanism where the RKKH cyclic peptide inhibits collagen binding without causing a conformational change of the ␣2-I domain. The jararhagin toxin possesses multiple domains that can inhibit ␣2␤1 integrin, and these activities are required to enhance metalloprotease-mediated cleavage of the ␤1 subunit (13,14) with the net effect of inhibition of collagen-induced activation of platelets. Jararhagin disintegrin possesses multiple motifs, and its activity is complex. Evidence supports an ability to induce ␣2␤1-mediated integrin signaling in platelets and fibroblasts. However, neither the RKKH motif nor the parent jararhagin metalloprotease domain has been demonstrated to induce activation of ␣2␤1. Rather, if the RKKH motif anchors the jararhagin metalloprotease to the ␣2 subunit, it may serve to facilitate other jararhagin motifs to play more direct roles in integrin activation.
Our results also indicate a mechanism of direct competition of the RKKH ligand for the collagen-binding site. The ␣2-I residue MIDAS Thr-221 is involved in Mg 2ϩ metal coordination and is slightly perturbed by RKKH, suggesting that the RKKH-binding site coincides with the MIDAS motif and the collagen-binding site. The NMR perturbation data do not offer structural restraints for docking the RKKH ligand on ␣2-I. However, the small chemical shift change for a residue that directly coordinates Mg 2ϩ metal suggests that the interaction of RKKH with ␣2-I is mediated by charge-charge or water-bridged contacts to the metal-binding site.
In contrast, the NMR results do not support the conclusions of a previous study that suggested that RKKH binding causes a conformational change in the ␣1-I domain (17). A model of RKKH docked on the crystal structure of recombinant ␣1-I predicted that the cyclic peptide could make extensive interactions with ␣1-I residues Arg-218, Glu-255, Ser-256, His-257, Asn-259, Ser-291, Glu-297, Glu-298, and Ser-301, near the MIDAS motif and in helix h6 (17). However, we did not detect any NMR peak perturbations for the corresponding residues in the homologous ␣2-I domain.
The inhibition of collagen binding by RKKH is metal dependent, and clearly the RKKH ligand does not displace Mg 2ϩ , because the removal of Mg 2ϩ has comparatively dramatic effects on the NMR spectrum of ␣2-I (Fig. 4). Water-bridged or charge-charge contacts with the binding site would also account for the ability of RKKH to inhibit collagen binding to the free ␣2-I domain, and its inability to disrupt the ␣2-I-collagen complex once formed.
Although the thermodynamic data show that the affinities of cyclic RKKH and collagen are comparable, the types of molecular interactions and possible conformational changes experienced by the ␣2-I domain may contribute to a disparity in the apparent off rate. The ability to mimic triple helical collagen with a simpler ligand would offer a powerful tool to study integrin signaling in solution and pave the way to drug development (42,43).