Calcium and Calmodulin-dependent Serine/Threonine Protein Kinase Type II (CaMKII)-mediated Intramolecular Opening of Integrin Cytoplasmic Domain-associated Protein-1 (ICAP-1α) Negatively Regulates β1 Integrins*

Background: Integrin affinity is controlled by the recruitment of both activators and inactivators on their cytoplasmic domain. Results: We showed that CamKII phosphorylates the negative regulator ICAP-1α and thereby regulates its interaction with β1 integrins. Conclusion: This phosphorylation is required for proper focal adhesion dynamics and cell adhesion. Significance: Our findings support an important role of this pathway in cell adhesion and cell migration. Focal adhesion turnover during cell migration is an integrated cyclic process requiring tight regulation of integrin function. Interaction of integrin with its ligand depends on its activation state, which is regulated by the direct recruitment of proteins onto the β integrin chain cytoplasmic domain. We previously reported that ICAP-1α, a specific cytoplasmic partner of β1A integrins, limits both talin and kindlin interaction with β1 integrin, thereby restraining focal adhesion assembly. Here we provide evidence that the calcium and calmodulin-dependent serine/threonine protein kinase type II (CaMKII) is an important regulator of ICAP-1α for controlling focal adhesion dynamics. CaMKII directly phosphorylates ICAP-1α and disrupts an intramolecular interaction between the N- and the C-terminal domains of ICAP-1α, unmasking the PTB domain, thereby permitting ICAP-1α binding onto the β1 integrin tail. ICAP-1α direct interaction with the β1 integrin tail and the modulation of β1 integrin affinity state are required for down-regulating focal adhesion assembly. Our results point to a molecular mechanism for the phosphorylation-dependent control of ICAP-1α function by CaMKII, allowing the dynamic control of β1 integrin activation and cell adhesion.


Focal adhesion turnover during cell migration is an integrated cyclic process requiring tight regulation of integrin function.
Interaction of integrin with its ligand depends on its activation state, which is regulated by the direct recruitment of proteins onto the ␤ integrin chain cytoplasmic domain. We previously reported that ICAP-1␣, a specific cytoplasmic partner of ␤1A integrins, limits both talin and kindlin interaction with ␤1 integrin, thereby restraining focal adhesion assembly. Here we provide evidence that the calcium and calmodulin-dependent serine/threonine protein kinase type II (CaMKII) is an important regulator of ICAP-1␣ for controlling focal adhesion dynamics. CaMKII directly phosphorylates ICAP-1␣ and disrupts an intramolecular interaction between the N-and the C-terminal domains of ICAP-1␣, unmasking the PTB domain, thereby permitting ICAP-1␣ binding onto the ␤1 integrin tail. ICAP-1␣ direct interaction with the ␤1 integrin tail and the modulation of ␤1 integrin affinity state are required for downregulating focal adhesion assembly. Our results point to a molecular mechanism for the phosphorylation-dependent control of ICAP-1␣ function by CaMKII, allowing the dynamic control of ␤1 integrin activation and cell adhesion.
In metazoan organisms, cell adhesion to the extracellular matrix is largely mediated by the integrin family and plays a central role in many physiological processes, such as embryonic development, inflammatory response, wound healing, and tissue regeneration (1). These receptors cluster into adhesive sites that connect the microenvironment to actin cytoskeleton and thereby coordinate cell motility. Continuous assembly and disassembly of these adhesive sites is a prerequisite for cell migration (2).
Integrins ectodomains can adopt at least three conformational states: a bent conformation associated with a low affinity state for its extracellular ligand, an incomplete extended form with intermediate affinity for the ligand, and a fully extended conformation corresponding to the ligand-occupied state (3)(4)(5)(6). Conformational change from a bent to an extended form leads to integrin activation and is triggered by the recruitment of intracellular integrin partners on the ␤ cytoplasmic domain, such as talin and kindlin (7)(8)(9)(10)(11)(12)(13). On the other hand, inhibitors, such as sharpin or integrin cytoplasmic domain-associated protein 1␣ (ICAP-1␣), 5 limit the recruitment of those activators (14,15). Conversely, ICAP-1␣ is a ␤1A integrin-specific partner involved in the negative regulation of ␤1 integrin activity by limiting talin and kindlin-2 recruitment (14, 16 -19). More precisely, we demonstrated that ICAP-1␣ maintains the low affinity state of ␤1 integrins to slow down focal adhesion (FA) assembly (20). This feature appears to be critical for cells to sense the extracellular matrix surface density and adapt their migratory and adhesive behavior. Despite growing evidence for the role of ICAP-1␣ during integrin-dependent adhesion, little is known about the signaling pathway controlling ICAP-1␣ activity. Several putative phosphorylation sites for protein kinases, such as CaMKII, PKC, PKG, and PKA, have been identified within ICAP-1␣ (19,21). Although their biological pertinence has not always been accurately verified, previous studies showed that ICAP-1␣ is phosphorylated upon cell adhesion on fibronectin (FN), suggesting a phosphorylation-dependent regulatory mechanism (18,19).
Our group and others have illustrated the role of serine/threonine protein kinase CaMKII in integrin-mediated cell adhesion. CaMKII activity promotes FA turnover (22) and cell migration (23,24). CaMKII is activated following ␣5␤1 integrin engagement and is required for ␣5␤1-dependent cell migration and phagocytosis (25). In turn, CaMKII activation decreases the affinity state of ␣5␤1 integrin and reduces cell spreading on FN (26), suggesting the existence of a CaMKII-dependent feedback loop regulating ␣5␤1 integrin activity. Although the substrate of CaMKII was not clearly identified from those studies, we previously reported that CaMKII inhibition could be overcome by ectopically expressing a mutant form of ICAP-1␣ in which the threonine 38 of the CaMKII consensus site has been substituted by a non-phosphorylatable alanine (27). This finding suggested that both proteins were involved in the same signaling pathway. To test this hypothesis, we used a combination of ␤1 integrin and ICAP-1␣ mutants and showed that CaMKII controls the capability of ICAP-1␣ to bind to ␤1 integrin and regulate focal adhesion dynamics. ICAP-1␣ phosphorylation on threonine 38 by CaMKII released a cryptic binding site for ␤1 integrin located in the C-terminal part of ICAP-1␣. The resulting opened active form of ICAP-1␣ consequently interacted with the ␤1A integrin tail and negatively regulated ␤1 integrin function by slowing down FA turnover.

EXPERIMENTAL PROCEDURES
Proteins, Reagents, and Antibodies-FN was purified from bovine serum as described previously (49). Vitronectin (VN) was purchased from BD Biosciences. KN-93 was purchased from Sigma-Aldrich.
Cell Treatment and Immunofluorescence-Osteoblast cells were trypsinized, treated with 1 mg/ml soybean trypsin inhibitor (Sigma-Aldrich), washed in PBS, and incubated in serumfree DMEM containing 5% BSA for 30 min at 37°C. To inhibit CaMKII␣ activity, cells in suspension were treated with 10 M KN-93 for 1 h at 37°C. CaMKII␣ T286D -expressing cells or KN-93-treated cells were seeded for either 2 or 16 h at 37°C on glass coverslips coated with either 10 g/ml FN or 5 g/ml VN in FN-free FCS/DMEM-supplemented medium. Cells were then fixed with a 3% paraformaldehyde, 2% sucrose solution for 10 min; permeabilized with 0.2% Triton X-100 for 10 min; blocked with PBS, 3% BSA for 30 min; and incubated with primary antibodies for 45 min at 37°C. After washes in PBS, 3% BSA, 0.05% Tween 20, AlexaFluor-conjugated goat secondary antibodies were added for 45 min at 37°C. Cells were finally mounted in Mowiol solution and imaged on an apotome microscope (Carl Zeiss S.A.S., Le Pecq, France).
Solid Phase Assay-The interaction between the N-and C-terminal regions of ICAP-1␣ was carried out using a solid phase assay. Briefly, a 96-well microplate (Maxisorp, Nunc (Dutscher, Brumath, France)) was coated with either 10 g of recombinant C-terminal ICAP-1␣ or BSA for 16 h at 4°C and blocked with a 3% BSA, PBS solution for 1 h at room temperature. After washes with a 3% BSA, 0.01% Tween 20, PBS solution, increased amounts of either recombinant N-terminal ICAP-1 wild-type , N-terminal ICAP-1 T38A , or N-terminal ICAP-1 T38D (0 -400 ng) were added for 1 h at 37°C. After washes in 3% BSA, 0.01% Tween 20, PBS solution, the monoclonal antibody 9B10H directed against the N-terminal part of ICAP-1 was added for 1 h at 37°C, and then an HRP-conjugated secondary anti-mouse antibody was added for 45 min at 37°C.
After washes in 3% BSA, 0.01% Tween 20, PBS solution, the presence of N-terminal ICAP-1 was detected by adding ABTS reagent and quantified by measuring absorbance at 405 nm.
Microinjection-NIH3T3 cells were seeded for 16 h at 37°C onto 10 g/ml FN-coated glass coverslips. Microinjections were carried out with a micromanipulator model 5171 connected to an Eppendorf microinjector unit (Transjector 5246). The cells were microinjected with a KCl (120 mM), HEPES (10 mM), pH 7, solution containing 100 M tetramethyl rhodaminedextran amine (M r 3000; Molecular Probes, Interchim) and 1 mg/ml purified recombinant fragment C-terminal ICAP-1␣ alone or in combination with either N-terminal ICAP-1 T38A or N-terminal ICAP-1 T38D . 30 min after microinjection, cells were fixed and immunostained for vinculin localization using a mouse anti-vinculin antibody and an Alexa488-conjugated anti-mouse IgG antibody. Cells were imaged using a wide field epifluorescence microscope (Olympus Provis AX70), and each rhodamine-positive cell was used to count for FA-positive or -negative.
CaMKII Phosphorylation Assay-The CaMKII phosphorylation assay was performed using CaMKII extracted from rat brain. Brains were homogenized in extraction buffer (50 mM Tris-HCl, pH 7.5, 10% ethylene glycol, 250 mM sucrose, 4 mM EDTA, 2 mM EGTA, 1 mM DTT, protease inhibitors). After centrifugation at 100,000 ϫ g for 45 min at 4°C, the lysate was clarified with a non-immune IgG2A serum coupled to protein A-conjugated Sepharose beads (GE Healthcare) for 2 h at 4°C. Then supernatant was incubated with mouse monoclonal anti-␣CaMKII (CB␣-2) for 1 h at 4°C, and CaMKII was purified using the protein A-coupled Sepharose beads. After 1 h at 4°C, beads were washed once in extraction buffer and twice in kinase assay buffer (10 mM Tris-HCl, pH 7.4, 150 mM NaCl, 10 mM MgCl 2 , 0.5 mM DTT). Then the phosphorylation reaction was performed in the presence of 1 mg/ml N-terminal ICAP-1 fragment, 100 M ATP, 2.5 Ci of [␥-32 P]ATP, 100 M CaCl 2 , and 10 g/ml calmodulin. The reaction was stopped after 30 min at 37°C by adding reducing Laemmli sample buffer, and samples were run on 10% SDS-PAGE. The gel was stained with Coomassie Blue and then digitized and dried before the autoradiography was processed at Ϫ80°C. For control experiments, phosphorylation reactions were performed without either calmodulin or N-terminal ICAP-1 or in the presence of 1 mM EGTA.
Alternatively, for ICAP-1 WT and its T38A mutant, ICAP-1 phosphorylation was assayed using recombinant CaMKII. Briefly, before use, CaMKII (New England Biolabs, Evry, France) was activated by autophosphorylation as follows. CaMKII (500 units) was first incubated in the presence of ATP (200 M), calmodulin (1.2 M), and CaCl 2 (2 mM) for 10 min at 30°C, and then 5 l of recombinant protein His-ICAP-1 immobilized on nickel-nitrilotriacetic acid beads were added in the presence 3 Ci of [␥-32 P]ATP, MgCl 2 , and CaCl 2 for 1 h at 30°C. The reaction was stopped by adding 5ϫ Laemmli buffer and heating at 95°C for 10 min. CaMKII-mediated ICAP-1 phosphorylation was visualized on an SDS-polyacrylamide gel after autoradiography and Coomassie Blue staining.
Time Lapse Videomicroscopy-Time lapse recordings were processed on osteoblast cells (␤1 Ϫ/Ϫ or Icap-1 Ϫ/Ϫ ) expressing either eGFP-VASP or mRFP-VASP together with ICAP-1␣ wild-type , ICAP-1␣ T38A , ICAP-1␣ T38D , ␤1 wild-type , ␤1 D759A , or ␤1 V787T . Cells treated or not with 10 M KN-93 were trypsinized, blocked using a soybean trypsin inhibitor-containing solution (1 mg/ml), washed in PBS, and resuspended in serum-free DMEM containing 5% BSA. After 1 h at 37°C, cells were seeded in LabTek I chambers (Nunc) coated with 1 g/ml FN. Cells were allowed to spread in FN-free FCS/DMEM supplemented or not with 10 M KN-93 for 2 or 16 h, and time lapse recordings were assessed as described previously (20). Briefly, records were done in a 5% CO 2 humidified atmosphere at 37°C using an inverted microscope (Axiovert 200 M, Carl Zeiss) and a live cell imaging plan apochromat ϫ63, numerical aperture 1.2 water immersion objective (Carl Zeiss). For each condition, 20 cells were randomly chosen, and images were taken simultaneously every 4 min using a motorized stage and a cooled CCD camera (CoolSNAP HQ2; Roper Scientific). Photobleaching events were minimized with a FluoArc system and an ND75 filter (Carl Zeiss), which reduce the excitation light of a 100-watt mercury lamp. FAs located at the leading edge were selectively chosen, and their turnover was quantified using Metamorph software (Molecular Devices, Sunnyvale, CA) as described previously (20). Briefly, mature FAs were manually outlined as well as their surrounding cytoplasmic area, and adhesions were manually tracked from their nucleation to their disassembly. The mean fluorescence intensity in the adhesion area was subtracted from the cytoplasmic background value. From these data, a shaped bell curve denoting FA turnover was obtained, allowing the measurements of FA assembly and disassembly rates as well as FA lifetime.
Image Analysis-Cells were imaged on a nonlinear optics LSM510 inverted confocal and biphoton laser-scanning microscope equipped with a ϫ63, numerical aperture 1.4 oil immersion plan apochromat objective (Carl Zeiss, Inc.). The images were manually thresholded, and FAs were automatically selected using MetaMorph software. Number and surface of ␤1 integrin-, ␤3 integrin-, and vinculin-containing FAs were quantified. Experiments were performed in triplicate, and at least 15 cells were analyzed per condition.

RESULTS
CaMKII Negatively Regulates ␤1 Integrin-dependent FA Assembly and Turnover Upstream of ICAP-1␣-Immortalized osteoblast cells derived from Icap-1 knock-out or control mice were used to analyze whether the inhibition or activation of CaMKII could differentially affect ICAP-1␣-dependent FA formation and dynamics (16). The constitutively active mutant ␣CaMKII T286D (28 -30) was stably expressed into Icap-1 ϩ/ϩ and Icap-1 Ϫ/Ϫ osteoblast cells. Increasing CaMKII activity leads to a strong reduction in FA size in control cells spread on FN (a ␤1 integrin-dependent matrix) (Fig. 1, a and b). In contrast, on a VN matrix (to engage ␤3 integrin) or in Icap-1 null background, ␣CaMKII T286D did not mediate any deleterious effect on FA growth, suggesting that CaMKII acts on ␤1 integrin-specific adhesion sites through ICAP-1␣ (Fig. 1, a and c). Consistent with those data, pharmacological inhibition of CaMKII activity with KN-93 leads to a rapid (within 2 h) increase in FA size in Icap-1 ϩ/ϩ cells spread on FN but had no effect on VN or in Icap-1 Ϫ/Ϫ cells (Fig. 1, d-f). Re-expression of ICAP-1␣ in Icap-1 Ϫ/Ϫ cells restored the effect of KN-93 treatment on FA growth observed in Icap-1 ϩ/ϩ cells, indicating that CaMKII controls ␤1 integrin-dependent adhesion complex formation in an ICAP-1␣-dependent manner (Fig. 1, d-f).
To characterize how CaMKII activity influences the dynamics of FN-induced adhesion complexes in Icap-1 ϩ/ϩ and Icap-1 Ϫ/Ϫ cells, live cell imaging was performed using cells expressing an eGFP-tagged VASP widely used as an adhesion marker. Because FA dynamics largely depend on their relative location within the cells (leading edges or trailing end) (31), the measurement of adhesion dynamics was assessed on FAs located at the cell front. Four different parameters of FA dynamics were measured: assembly and disassembly rates, the steady state duration, and the total lifetime. Consistent with an increased growth upon KN-93 treatment, the dynamics of adhesion complexes in Icap-1 ϩ/ϩ cells were decreased by short term inhibition of CaMKII. The assembly rate was faster, whereas the disassembly rate was lower, and the resulting steady state as well as the lifetime were longer (Fig. 2, a and b). Again, none of those dynamic parameters appeared to be affected in Icap-1-deficient cells, indicating that CaMKII functions through an ICAP-1␣dependent pathway (Fig. 2b). We previously showed that Icap-1 deficiency promotes the formation of centrally located ␤1 integrin-containing focal adhesions (20). To identify whether CaMKII also constrains the assembly and distribution of adhesion complexes, control and Icap-1 Ϫ/Ϫ cells were treated overnight with KN-93 to measure focal adhesion distribution and dynamics in a permanently inhibited CaMKII cell context. Inhibition of CaMKII with KN93 in control cells stimulated the formation of ␤1 integrin-positive FAs, mimicking the Icap-1 null phenotype (Fig. 2, c and d). Moreover, the high number of FAs in Icap-1 null cells was not further affected upon CaMKII inhibition. Quantification of focal adhesion assembly and disassembly rates as well as lifetime showed that long term CaMKII inhibition accelerated focal adhesion assembly without modifying the disassembly rate, thereby leading to an overall reduction in adhesion lifetime (Fig. 2e). Interestingly, CaMKII inhibition in control cells reproduced the adhesion dynamics of Icap-1 Ϫ/Ϫ cells. Here again, KN-93 treatment in Icap-1 Ϫ/Ϫ cells did not further modify FA dynamics. These data indicated that CaMKII negatively regulated FA assembly and turnover upstream of ICAP-1␣.
CaMKII-mediated Down-regulation of ␤1A Integrin Activation Requires ICAP-1␣ Binding onto the ␤1A Tail-We previously showed that ICAP-1␣ reduced FA assembly by restraining ␤1 integrin in a low affinity state for its extracellular ligand (20). On the other hand, we also previously demonstrated that the disruption of the salt bridge between the ␣ and ␤1 subunits by the ␤1 D759A mutation reproduced the FA pattern and dynamics observed upon ICAP-1␣ loss. To identify whether CaMKII regulates FA formation and dynamics by controlling the ␤1 integrin affinity state, CaMKII activity was either increased using the active form of CaMKII␣ (␣CaMKII T286D ) or inhibited upon KN-93 treatment in ␤1 Ϫ/Ϫ osteoblasts expressing the ␤1 D759A preactivated mutant. Although the expression of ␣CaMKII T286D affected FA growth in control cells (␤1 wild-type ), no significant difference was observed in  ␤1 D759A -expressing cells (Fig. 3, a and b). As shown previously, short term treatment of KN93 (2 h) increased FA size in control cells, whereas ␤1 D759A expression rendered FAs insensitive to CaMKII inhibition (Fig. 3, c and d). As shown previously (20), quantification of FA assembly and disassembly rates as well as lifetime in eGFP-VASP-expressing ␤1 WT and ␤1 D759A cells showed an increased FA assembly rate together with a reduced lifetime in ␤1 D759A cells compared with ␤1 wild-type cells, mimicking Icap-1 loss (Fig. 3e). Long term inhibition of CaMKII (overnight) accelerated adhesion assembly and reduced lifetime in ␤1 wild-type cells to a similar extent as in ␤1 D759A cells. Again, KN-93 did not significantly modify FA turnover in ␤1 D759A cells, indicating that the expression of a preactivated ␤1 integrin phenocopied the effect of CaMKII inhibition and ICAP-1␣ loss. These findings suggested that CaMKII controls ␤1 integrin activation state and thereby FA assembly and turnover.
Phosphorylation of ICAP-1␣ at Threonine 38 Regulates FA Dynamics in a CaMKII-dependent Manner-We previously reported that CaMKII regulates ␣5␤1-dependent cell adhesion through a predicted CaMKII phosphorylation site on ICAP-1 threonine 38 (27). To identify whether this putative CaMKII phosphorylation site found in ICAP-1␣ might participate in FA dynamics, the phosphomimetic T38D and a non-phosphorylatable T38A mutant form of ICAP-1 (27) were expressed in Icap-1 null cells, respectively, and FA formation and dynamics were analyzed. Whereas the expression of ICAP-1␣ T38A had no significant effect on FAs formation, the ICAP-1␣ T38D mutant strongly reduced it, suggesting that phosphorylation of threonine 38 negatively regulates FA formation (Fig. 4, a and b). Consequently, ICAP-1␣ T38D cells were less spread compared with control cells (Fig. 4c). CaMKII inhibition by KN-93 did not significantly modify FA formation in cells expressing both ICAP-1␣ phosphomutants (Fig. 4, a and b). As previously, we conducted dynamic analysis of FA behavior in cells expressing ICAP-1␣ wild-type , ICAP-1␣ T38A , or ICAP-1␣ T38D . Whereas ICAP-1␣ loss accelerated FA assembly rate and consequently shortened lifetime, the few remaining adhesions in ICAP-1␣ T38D cells displayed much slower dynamics with decreased assembly and disassembly rates, leading to a longer lifetime (Fig. 4d). Conversely, ICAP-1␣ T38A cells displayed a faster assembly phase and a reduced lifetime similar to Icap-1 Ϫ/Ϫ cells or control cells after inhibition of CaMKII, indicating that the deleterious effect of ICAP-1␣ Thr-38 phosphorylation on adhesion formation depends on CaMKII activity.

Threonine 38 Phosphorylation Disrupts ICAP-1␣ N-to C-terminal Interaction and Controls Its Binding to ␤1
Integrins-ICAP-1␣ regulates FA dynamics by directly interacting with ␤1 integrins, and this regulation is at least partly dependent on the phosphorylation status of the threonine 38. Next, we investigated whether ICAP-1␣ phosphorylation is a prerequisite to its binding to ␤1 integrins. We used an in vitro pull-down assay to estimate the capability of the wild-type form of ICAP-1␣ to interact with the ␤1A or ␤3 integrin cytoplasmic tail, either in the presence of phosphatase inhibitors or alkaline phosphatase. As shown in Fig. 5a (left), whereas phosphatase inhibitors promoted the specific ICAP-1␣ binding onto the ␤1A cytoplasmic tail, alkaline phosphatase treatment strongly reduced it. Subsequently, we investigated the binding capability of the T38A or T38D ICAP-1␣ mutants to the cytoplasmic tail of ␤1A, using the ␤3 integrin tail as a negative control. ICAP-1␣ T38D and ICAP-1␣ wild-type displayed a stronger interaction with ␤1 cytoplasmic tail compared with ICAP-1␣ T38A (Fig. 5a, left). Those data are highly suggestive that ICAP-1␣ recruitment onto the ␤1A tail is regulated by its phosphorylation status. We previously demonstrated that ICAP-1␣ association with ␤1 integrins prevents the recruitment of integrin activators such as kindlins, thereby maintaining integrins in their low affinity state for extracellular ligands (17). As shown in Fig. 5b, the expression of ICAP-1 T38D reduced kindlin-2 binding on the ␤1 integrin tail, indicating that the threonine 38 phosphorylation state modulates kindlin-2 association with integrins and their subsequent activation. ICAP-1␣ is composed of an N-terminal moiety (amino acids 1-58), which is devoid of any structural motif but enriched in serine and threonine residues and encompasses several potential phosphorylation sites (including the CaMKII consensus site), and a C-terminal domain (amino acids 59 -200), which folds into a PTB motif containing the ␤1 integrin binding site (32,34) (Fig. 7). To test whether ICAP-1␣ activity may be regulated by a head to tail interaction, we used a solid phase assay to probe this putative intramolecular interaction. Indeed, a specific and dose-dependent interaction was detected between the N-terminal (residues 1-99) and C-terminal (residues 100 -200) moieties of ICAP-1␣ (Fig. 5c). To check whether this interaction could be modulated by the Thr-38 phosphorylation, the ability of the N-terminal region of ICAP-1␣ containing either a T38A or T38D mutation to interact with the C-terminal domain was measured. Although the T38A mutation did not affect the interaction between the N-and the C-terminal domains of ICAP-1, the phosphomimetic mutation of the threonine by an aspartic acid residue abolished it (T38D) (Fig. 5c). FIGURE 5. ICAP-1␣ exists in a close, inactive conformation opened upon threonine 38 phosphorylation. a, pull-down assays between ICAP-1␣ and ␤1A integrin cytodomain. Left, CHO cell lysates expressing ICAP-1␣ wild-type and treated with phosphatase inhibitors or alkaline phosphatase were incubated with either GST alone or fused to the cytoplasmic tail of ␤1A or ␤3 integrin. Alternatively (bottom), CHO cell lysates expressing either ICAP-1␣ wild-type , ICAP-1␣ T38A , or ICAP-1␣ T38D mutants were incubated with GST alone or GST-integrin tail fusion proteins. Bound fraction of ICAP-1␣ was revealed by immunoblotting. b, pull-down assays between kindlin-2 and ␤1A integrin cytodomain. HEK 293 cells were transiently transfected with pcDNA3.1-ICAP wt or pcDNA3.1-ICAP T38D , respectively, and kindlin-2 associated with ␤1A and ␤3 integrin tails fused to GST or GST alone were visualized by Western blotting. c, solid phase assay of the intramolecular interaction between N-and C-terminal ICAP-1␣. Increased amounts of either N-terminal ICAP-1 wild-type , N-terminal ICAP-1 T38A , or N-terminal ICAP-1 T38D (1-400 ng) were added to C-terminal ICAP-1 (10 g) coated onto a 96-well microplate. After washes, the interaction between ICAP-1 fragments was revealed with an anti-ICAP-1 antibody (9B10H) that recognizes the N-terminal region. As a negative control, BSA-coated wells were used to estimate the nonspecific binding of N-terminal ICAP-1. Error bars, S.D. of three independent experiments. d, cells were co-microinjected with the recombinant C-terminal ICAP-1 (residues 100 -200) and dextran rhodamine alone or with N-terminal ICAP-1 bearing the Thr-38 phosphomimetic mutations (amino acids 1-99). Cells were fixed and stained for vinculin to visualize adhesion sites. Numbers of cells devoid or not of FAs were counted, and FA disruption efficiency was expressed as a percentage of total cells.
Next, we investigated the functional effect of ICAP-1␣ intramolecular association on FA assembly. A complementation strategy was used to investigate whether the co-injection of the N-terminal moiety of ICAP-1␣ prevented the deleterious effect on FA formation induced by the C-terminal domain (14) (Fig.  5d). As previously published (14), microinjection of the ICAP-1␣ C-terminal moiety alone led to the disappearance of FA sites in 66% of microinjected cells as visualized by vinculin staining. Co-injection of the ICAP-1 T38A N-terminal moiety together with the C-terminal part of the protein strongly blocked its effect on FA disassembly, with only 27% of microinjected cells showing disrupted adhesion structures. On the other hand, co-injection of the ICAP-1 T38D N terminus with the C terminus did not significantly modify FA disassembly induced by the C-terminal fragment (76% versus 66%, respectively). These results suggested that the N-terminal region masks the integrin binding site when ICAP-1␣ is unphosphorylated on threonine 38.

ICAP-1␣ Is a Substrate of CaMKII␣ in Vitro-
The finding that ICAP-1␣ phosphorylation on threonine 38, a residue located within a putative CaMKII consensus site, and ICAP-1␣ binding onto ␤1 integrin were required for CaMKII-mediated down-regulation of FA assembly and turnover suggested that ICAP-1␣ was directly regulated by CaMKII. To further demonstrate that ICAP-1␣ is a direct target of CaMKII, we carried out co-immunoprecipitation experiments after expression of one or both proteins (ICAP-1␣ and/or CaMKII␣) using standard lysis conditions (radioimmune precipitation assay or glycerol buffer). Under those conditions, we obtained non-reproducible co-immunoprecipitations (2 positives over 5 tentatives), probably due to a labile and transient interaction that has often been reported between protein kinases and their substrates. Therefore, we decided to express into CHO cells ICAP-1␣ either alone or with CaMKII␣ T286D and to use a cross-linking reagent before immunoenrichment to stabilize the interaction. Indeed, treating the cells before lysis with a cell-permeable cross-linker greatly increased the level and efficiency of co-immunoprecipitation of ICAP-1␣ with CaMKII␣ (ectopically or endogenously expressed) (Fig. 6a). Such experiments were also performed in Icap-1 Ϫ/Ϫ osteoblasts and gave similar results (data not shown). Next, an in vitro phosphorylation assay using immunoprecipitated CaMKII␣ and the purified recombinant ICAP-1␣ N-terminal moiety in the presence of Ca 2ϩ and calmodulin (two cofactors essential for CaMKII activity) revealed that ICAP-1␣ can be phosphorylated by CaMKII (Fig. 6b), confirming that ICAP-1␣ is an actual substrate of CaMKII. To directly visualize the phosphorylation of the Thr-38 residue by CaMKII, we performed comparative in vitro CaMKII phosphorylation assays with wild-type ICAP-1␣ or its mutant (ICAP-1 T38A ). Indeed, we showed that the T38A mutation strongly diminished the ability of CaMKII to phosphorylate ICAP-1 compared with the wild-type form of ICAP-1 (Fig. 6c). Altogether, these results indicated that CaMKII phosphorylates ICAP-1␣ on threonine 38.

DISCUSSION
In this study, we dissected the signaling pathway regulating the function of ICAP-1␣, a negative regulator of ␤1 integrin activation. We showed that ICAP-1␣ phosphorylation by CaMKII enabled its interaction with the ␤1A integrin cytosolic tail by allowing the accessibility to the PTB domain and thereby regulating FA dynamics (Fig. 7).
Regulation of the capability of proteins to interact with effectors by unmasking cryptic binding sites through a phosphorylation-dependent process has been identified in several adhesion proteins, such as vinculin (35,36), talin (37,38), and ERM (ezrin, radixin, and moesin) proteins (39,40). Recently, the ICAP-1␣ structure has been solved, and in line with the previous hypothesized model, ICAP-1␣ contains a PTB domain (which starts at residue 58) that is preceded by a presumably unstructured N-terminal part enriched in serine and threonine residues and containing most of the phosphorylation sites (32, FIGURE 6. In vitro phosphorylation of ICAP-1␣ by CaMKII␣. a, ICAP-1␣ association with ␣CaMKII was analyzed by immunoprecipitation of FLAG-ICAP-1␣ in CHO cells expressing or not expressing ␣CaMKIIT286D. Interaction between CaMKII and ICAP was analyzed after immunoprecipitation of FLAG-ICAP-1, and the presence of CaMKII was detected by Western blotting analysis using polyclonal CaMKII antibody. FLAG-ICAP co-immunoprecipitated ectopically expressed CaMKII (left) or endogenous CaMKII (middle), whereas control immunoprecipitation (when FLAG-ICAP was not expressed) did not immunoprecipitate CaMKII as expected (right). b, CaMKII␣ immunoprecipitated from rat brain and recombinant N-terminal ICAP-1 (residues 1-99) were incubated with calmodulin, Ca 2ϩ , and [␥-32 P]ATP. ICAP-1 phosphorylation was revealed by autoradiography. EGTA was added as a negative control of CaMKII-dependent ICAP-1 phosphorylation. c, schematic representation of ICAP-1␣ N-and C-terminal structures illustrating ICAP-1 head domain with the kinase phosphorylation sites and the PTB domain containing the ␤1A integrin binding site. c, His-ICAP-1 wild-type or mutated form T38A, immobilized on nickel-nitrilotriacetic acid beads, was incubated with purified CaMKII in the presence of [␥-32 P]ATP. GST protein immobilized on glutathione-Sepharose beads was used as control. CaMKII-induced phosphorylation was analyzed by autoradiography (top). The amount of recombinant proteins was determined with Coomassie staining (bottom). 34). Our findings suggested that this region might block the accessibility of the PTB domain to the ␤1A integrin tail, thereby regulating ICAP-1␣ function. Phosphorylation at threonine 38 releases the cis-interaction and promotes ICAP-1␣ binding to ␤1A integrin. Although our study focused on CaMKII phosphorylation of ICAP-1␣ threonine 38, at this stage, we cannot rule out that phosphorylation at residues other than threonine 38 may also be involved in the regulation of ICAP-1␣ activity as well as the involvement of other protein kinases, such as PKC, PKG, or PKA. Indeed, a phosphomapping of Krit-1-associated ICAP-1␣ in the U2OS cell line did not identify the threonine 38, whereas a high throughput MS analysis of phosphorylated proteins has identified Thr-38 as a phosphorylation site (41,42). This suggests the existence of other redundant phosphorylation sites or an integrin-specific regulation of ICAP-1␣ by CaMKII. Interestingly, in a very recent study (34), it has been proposed that Krit1 antagonizes the inactivating effect of ICAP-1␣ toward ␤1 integrins. This observation added a new way to regulate ICAP-1␣ inhibitory function and could be complementary to the phosphorylation control because ICAP-1␣/ Krit1 interaction is Thr-38 phosphorylation-independent.
Whereas PKC inhibition does not alter the ability of ␣5␤1 integrin to bind FN (26), PKA has been shown to be involved in ␣v␤3 and ␣5␤1 cross-talk by regulating VASP phosphorylation (43). Determination of whether PKA also controls ICAP-1␣ phosphorylation and function requires more work, but this could be an attractive hypothesis to explain how ␤3 integrins negatively cross-talk with ␤1 integrins.
In this study, we have accumulated a large body of evidence to show that CaMKII and ICAP-1␣ regulate focal adhesion dynamics in a linear pathway. CaMKII function in the control of cell adhesion has been demonstrated in several previous reports. CaMKII inhibition accelerates cell spreading on FN, whereas its constitutive activation decreases cell adhesion and destabilizes FAs (22,26). CaMKII activity is largely controlled by an increase in cytoplasmic calcium content within the cell (44). Interestingly, a close relationship between integrins and calcium channels has been shown. Whereas ␣5␤1 integrin engagement with FN induces a release of intracellular calcium stores, ␣v␤3 integrin binding to VN strongly reduces the intracellular calcium flux (45,46). Moreover, ␣v␤3 and ␣5␤1 engagement differentially regulates CaMKII activity. CaMKII activation upon ␣5␤1 integrin ligation is inhibited by ␣v␤3 integrin binding to VN (25). Our present work opens the possibility that ICAP-1␣ plays an important role in integrin crosstalk and could provide the missing link between CaMKII and ␤1 integrin. In line with this, CaMKII activity was shown to be concentrated at the leading edge of cells, and this spatial distribution promotes cell motility and polarization (47). ICAP-1␣ is also localized in lamellipodia during the early stage of cell spreading together with ␤1 integrin (48). Thus, CaMKII activation at the leading edge may limit ICAP-1␣ activity to the lamellipodia, where adhesion assembly initially takes place.
ICAP-1␣ was previously reported to restrict the recruitment of talin and kindlin-2 onto ␤1 tail and to reduce FA assembly by maintaining the ␤1 integrin low affinity state (14,20). Interestingly, CaMKII inhibition and ICAP-1␣ depletion as well as blocking ICAP-1␣ interaction onto the ␤1 tail strongly reproduced the ex vivo phenotype of the preactivated mutant ␤1 D759A (20). CaMKII-induced ICAP-1␣ binding to ␤1 integrin might keep this integrin in its inactive form by limiting kindlin and talin recruitment and subsequently reducing the initiation of FA assembly (Fig. 7). Clearly, more work is still needed to further clarify the precise interplay between talin, kindlins, and ICAP-1␣ as well as the biological significance of such a dynamic process.