The calpain family of proteases has been implicated in cellular processes such as apoptosis, proliferation and cell migration. Calpains are involved in several key aspects of migration, including: adhesion and spreading; detachment of the rear; integrin- and growth-factor-mediated signaling; and membrane protrusion. Our understanding of how calpains are activated and regulated during cell migration has increased as studies have identified roles for calcium and phospholipid binding, autolysis, phosphorylation and inhibition by calpastatin in the modulation of calpain activity. Knockout and knockdown approaches have also contributed significantly to our knowledge of calpain biology, particularly with respect to the specific functions of different calpain isoforms. The mechanisms by which calpain-mediated proteolysis of individual substrates contributes to cell motility have begun to be addressed, and these efforts have revealed roles for proteolysis of specific substrates in integrin activation, adhesion complex turnover and membrane protrusion dynamics. Understanding these mechanisms should provide avenues for novel therapeutic strategies to treat pathological processes such as tumor metastasis and chronic inflammatory disease.

Keywords:
Calpain, Cell motility, Proteolysis

The importance of cell migration is evident from both the physiological processes that depend on the regulated movement of cells, including embryonic development, immune responses and tissue maintenance and repair, and from the disease states driven by aberrant cell motility, such as chronic inflammation, vascular disease and tumor metastasis. Not surprisingly, immense effort has been directed towards furthering our understanding of this complex process. These efforts have provided us with the current concept of cell migration, which comprises a cycle of several highly coordinated and regulated steps (Lauffenburger and Horwitz, 1996; Ridley et al., 2003). In response to various migratory cues, directional movement is initiated by polarization of the cell, as defined by the spatial segregation of molecular machineries that control the different stages of the migratory cycle. At the front of the cell, actin polymerization drives membrane protrusion to form the leading edge. Subsequently, the leading edge is stabilized by attachment to the extracellular matrix (ECM) through integrin-mediated adhesion complexes, which not only link the ECM to the actin cytoskeleton but also function as signal transduction centers that modulate cell migration. Once coupled to adhesion complexes, the actin cytoskeleton can generate the forces necessary to translocate the cell body forward. Finally, adhesive contacts at the rear of the cell must be disassembled to allow detachment of the rear and to complete the migratory cycle.

Because of their involvement in cell motility, integrin-containing adhesion complexes are necessarily dynamic structures that undergo repeated cycles of formation and disassembly (Webb et al., 2002). Likewise, the activities of the actin-based protrusion and contraction machineries must also be continually regulated to ensure proper timing and localization (Rafelski and Theriot, 2004). The calpain family of proteases has been shown to contribute to the control of cell migration through their ability to regulate the dynamics of both integrin-mediated adhesion and actin-based membrane protrusion (Perrin and Huttenlocher, 2002). Although our current understanding of the mechanisms underlying this regulation remains limited, recent studies have begun to shed light on this subject. Here, we discuss recent advances that have provided insight into where calpains fit into the cell migration cycle, how the activities of calpains are modulated, the roles of individual calpain isoforms in motility, and the molecular basis of their effects during directional cell movement.

The mammalian calpain gene superfamily contains 16 known genes: 14 of these genes encode proteins that contain cysteine protease domains; the other two genes encode smaller regulatory proteins that associate with some of the catalytic subunits to form heterodimeric proteases (Goll et al., 2003; Suzuki et al., 2004). Several calpain isoforms are ubiquitously expressed, whereas many demonstrate tissue-specific expression patterns (Table 1). They are typically thought of as intracellular proteases, although there is some evidence that active calpains are also found in the extracellular space (Nishihara et al., 2001; Xu and Deng, 2004). However, the physiological significance of extracellular calpains is not yet known. Within the cell, the localization patterns of calpains are complex and somewhat variable (Table 2), which means that their subcellular localization might be dynamically regulated and constitutes an important factor in the modulation of their functions.

Table 1.

Expression patterns of calpains

Isoform Pattern Highest Lowest References
Capn1   Ubiquitous   Ac, Dc, Es, Pl, Th, Tr   Te   Farkas et al., 2003  
Capn2   Ubiquitous   Ki, Lu, St, Tc, Tr   Bm, Li, Ov   Farkas et al., 2003  
Capn3   Ubiquitous   Sm   Ov   Farkas et al., 2003  
Capn5   Ubiquitous   Br, Ki, Li, Lu, Te, Tr   He, Sm   Dear et al., 1997; Dear and Boehm, 1999  
Capn6   Tissue specific   Pl, Sm   -   Dear et al., 1997; Dear and Boehm, 1999  
Capn7   Ubiquitous    -   Fran z et al., 1999  
Capn8   Tissue specific   Br, Dt, St, Te   He, Ki   Braun et al., 1999; Sorimachi et al., 1993  
Capn9   Tissue specific   Dt, He, St   -   Markmann et al., 2005; Sorimachi et al., 1993  
Capn10   Ubiquitous   He   -   Horikawa et al., 2000  
Capn11   Tissue specific   St, Te   He, Ki   Dear et al., 1999  
Capn12   Tissue specific   Hf   -   Dear et al., 2000  
Capn13   Tissue specific   Lu, Te   -   Dear and Boehm, 2001  
Capn14   Unknown   -   -   Dear and Boehm, 2001  
Capn15   Ubiquitous   Br   -   Kamei et al., 1998  
CSS1   Ubiquitous   He, Is, Ki, Pa, Pr, Sm, Te   -   Farkas et al., 2003  
CSS2   Tissue specific   Bl, Es, Pr, Tr,   -   Farkas et al., 2003; Ma et al., 2004  
Calpastatin   Ubiquitous   Is   Ov   Farkas et al., 2003  
Isoform Pattern Highest Lowest References
Capn1   Ubiquitous   Ac, Dc, Es, Pl, Th, Tr   Te   Farkas et al., 2003  
Capn2   Ubiquitous   Ki, Lu, St, Tc, Tr   Bm, Li, Ov   Farkas et al., 2003  
Capn3   Ubiquitous   Sm   Ov   Farkas et al., 2003  
Capn5   Ubiquitous   Br, Ki, Li, Lu, Te, Tr   He, Sm   Dear et al., 1997; Dear and Boehm, 1999  
Capn6   Tissue specific   Pl, Sm   -   Dear et al., 1997; Dear and Boehm, 1999  
Capn7   Ubiquitous    -   Fran z et al., 1999  
Capn8   Tissue specific   Br, Dt, St, Te   He, Ki   Braun et al., 1999; Sorimachi et al., 1993  
Capn9   Tissue specific   Dt, He, St   -   Markmann et al., 2005; Sorimachi et al., 1993  
Capn10   Ubiquitous   He   -   Horikawa et al., 2000  
Capn11   Tissue specific   St, Te   He, Ki   Dear et al., 1999  
Capn12   Tissue specific   Hf   -   Dear et al., 2000  
Capn13   Tissue specific   Lu, Te   -   Dear and Boehm, 2001  
Capn14   Unknown   -   -   Dear and Boehm, 2001  
Capn15   Ubiquitous   Br   -   Kamei et al., 1998  
CSS1   Ubiquitous   He, Is, Ki, Pa, Pr, Sm, Te   -   Farkas et al., 2003  
CSS2   Tissue specific   Bl, Es, Pr, Tr,   -   Farkas et al., 2003; Ma et al., 2004  
Calpastatin   Ubiquitous   Is   Ov   Farkas et al., 2003  

Abbreviations: Ac, ascending colon; Bl, bladder; Bm, bone marrow; Br, brain; Dc, descending colon; Dt, digestive tract; Es, eso phagus; He, heart; Hf, hair follicle; Is, interventricular septum; Ki, kidne y; Li, liver; Lu, lung; Ov, ovary; Pa, pancreas; Pl, placenta; Pr, prostate; Sm, skeletal muscle; St, stomach; Tc, transverse colon; Te, testis; Th, thyroid; Tr, trachea.

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Table 2.

Localization of calpains

Localization Isoform References
Adhesion comple xes   Capn2   Beckerle et al., 1987  
Caveolae   Capn2   Kifor et al., 2003  
Diffuse cytoplasmic   Capn1, 2, 5, 7, 10, CSS1   Gafni et al., 2004; Gil-Parrado et al., 2003; Lane et al., 1992; Raynaud et al., 2004  
Endoplasmic reticulum   Capn1, 2, CSS1   Hood et al., 2004; Hood et al., 2003; Sakai et al., 1989  
Extracellular   Capn1, 2   Nishihara et al., 2001; Raynaud et al., 2004; Xu and Deng, 2004  
Golgi   Capn1, 2, CSS1   Hood et al., 2004; Hood et al., 2003  
Lipid rafts   Capn2   Morford et al., 2002; P. Nuzzi and A.H., unpublished data  
Nuclear   Capn1, 2, 5, 7, 10, CSS1   Gafni et al., 2004; Gil-Parrado et al., 2003; Mellgren and Lu, 1994; Raynaud et al., 2004; Tremper-Wells and Vallano, 2005  
Plasma membrane   Capn1, CSS1   Gil-Parrado et al., 2003; Lane et al., 1992; Sakai et al., 1989  
Localization Isoform References
Adhesion comple xes   Capn2   Beckerle et al., 1987  
Caveolae   Capn2   Kifor et al., 2003  
Diffuse cytoplasmic   Capn1, 2, 5, 7, 10, CSS1   Gafni et al., 2004; Gil-Parrado et al., 2003; Lane et al., 1992; Raynaud et al., 2004  
Endoplasmic reticulum   Capn1, 2, CSS1   Hood et al., 2004; Hood et al., 2003; Sakai et al., 1989  
Extracellular   Capn1, 2   Nishihara et al., 2001; Raynaud et al., 2004; Xu and Deng, 2004  
Golgi   Capn1, 2, CSS1   Hood et al., 2004; Hood et al., 2003  
Lipid rafts   Capn2   Morford et al., 2002; P. Nuzzi and A.H., unpublished data  
Nuclear   Capn1, 2, 5, 7, 10, CSS1   Gafni et al., 2004; Gil-Parrado et al., 2003; Mellgren and Lu, 1994; Raynaud et al., 2004; Tremper-Wells and Vallano, 2005  
Plasma membrane   Capn1, CSS1   Gil-Parrado et al., 2003; Lane et al., 1992; Sakai et al., 1989  
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The enzymatically active (large) calpains each comprise up to four domains (Fig. 1) (Hosfield et al., 1999; Pal et al., 2003; Sorimachi and Suzuki, 2001; Strobl et al., 2000). Domain I is a single α-helix present at the N-terminus of some calpains; it can interact with domain VI of the non-catalytic (small) subunits and may be important for stability. Domain II comprises the protease domain, which contains the active site catalytic triad Cys105, His262 and Asn286. Interestingly, the alignment and spacing of these residues in the inactive molecule is such that catalytic activity is not permitted, indicating that a structural change must take place to activate calpains. Domain III consists of eight β-strands arranged in a β-sandwich configuration similar to that of C2 domains. The C2 domain was first discovered in protein kinase C as a stretch of approximately 130 amino acids that binds phospholipids in a calcium-dependent manner (Newton and Johnson, 1998). Since then, C2-like domains have been identified in nearly 100 proteins, and they are usually involved in binding calcium and phospholipids (Rizo and Sudhof, 1998). Domain III can bind phospholipids in a calcium-dependent fashion (Tompa et al., 2001), which further suggests that it is a C2-like domain. Domains IV and VI in the large and small subunits, respectively, each contain five EF-hand motifs, the fifth EF hand from each subunit interacting with the other to assemble heterodimers (Blanchard et al., 1997; Hosfield et al., 1999; Lin et al., 1997). Domain V of the small subunits appears to have a very flexible structure as a consequence of being glycine rich, which is probably why, unlike the other domains, it remains unresolved by crystallography.

Calpain activity is highly regulated in vivo by multiple mechanisms (Fig. 2A), although the details are only now beginning to be defined. The best-studied mechanism is activation by calcium - hence the name calpain (Guroff, 1964). In fact, calpain 1 and calpain 2 are commonly referred to by their in vitro requirements for calcium: calpain 1 (μ-calpain) is activated by micromolar calcium concentrations and calpain 2 (m-calpain) requires millimolar concentrations (Suzuki et al., 1981b). Because calpains contain calcium-binding EF-hand motifs in domains IV and VI and, because domain IV of calpain 1 and domain IV of calpain 2 are different, these were originally presumed to be responsible for the calcium-dependent activation of calpains. However, structural data suggest that conformational changes caused by calcium occupancy of the EF hands alone are insufficient to align the active site catalytic residues properly. Furthermore, functional studies have demonstrated that domain II alone exhibits calcium-dependent protease activity (Hata et al., 2001) and that non-EF-hand calcium-binding sites within the protease domain act as a calcium switch to align the catalytic triad (Hata et al., 2001; Moldoveanu et al., 2002; Moldoveanu et al., 2004).

Fig. 1.
Fig. 1. Schematic representation of the domain architecture of the classical calpains. The 80 kDa large subunits can be divided into four domains, plus a short linker that might be important for transducing conformational changes throughout the molecule upon calcium binding (T). The N-terminal α-helix makes up domain I, which interacts with the small subunits before undergoing intermolecular autolysis on activation. Protease activity is contained within domain II, which is further divided into subdomains (IIa and IIb) that make up the two halves of the active site. Domain III comprises a C2-like domain that harbors sites for phosphorylation and phospholipid binding. Five consecutive EF-hand motifs make up domain IV and contribute to the calcium binding of the large subunits and to dimerization with the small subunits. Domain VI of the small subunits has a similar arrangement; the first four EF hands participate in calcium binding and the last motif interacts with the large subunit. The small subunits also contain a highly flexible, glycine-rich region called domain V. Calpain 1 and calpain 2 large subunits are phosphorylated at several sites in domains I-III; some of these residues are conserved and some are isoform specific.
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Schematic representation of the domain architecture of the classical calpains. The 80 kDa large subunits can be divided into four domains, plus a short linker that might be important for transducing conformational changes throughout the molecule upon calcium binding (T). The N-terminal α-helix makes up domain I, which interacts with the small subunits before undergoing intermolecular autolysis on activation. Protease activity is contained within domain II, which is further divided into subdomains (IIa and IIb) that make up the two halves of the active site. Domain III comprises a C2-like domain that harbors sites for phosphorylation and phospholipid binding. Five consecutive EF-hand motifs make up domain IV and contribute to the calcium binding of the large subunits and to dimerization with the small subunits. Domain VI of the small subunits has a similar arrangement; the first four EF hands participate in calcium binding and the last motif interacts with the large subunit. The small subunits also contain a highly flexible, glycine-rich region called domain V. Calpain 1 and calpain 2 large subunits are phosphorylated at several sites in domains I-III; some of these residues are conserved and some are isoform specific.

Fig. 1.
Fig. 1. Schematic representation of the domain architecture of the classical calpains. The 80 kDa large subunits can be divided into four domains, plus a short linker that might be important for transducing conformational changes throughout the molecule upon calcium binding (T). The N-terminal α-helix makes up domain I, which interacts with the small subunits before undergoing intermolecular autolysis on activation. Protease activity is contained within domain II, which is further divided into subdomains (IIa and IIb) that make up the two halves of the active site. Domain III comprises a C2-like domain that harbors sites for phosphorylation and phospholipid binding. Five consecutive EF-hand motifs make up domain IV and contribute to the calcium binding of the large subunits and to dimerization with the small subunits. Domain VI of the small subunits has a similar arrangement; the first four EF hands participate in calcium binding and the last motif interacts with the large subunit. The small subunits also contain a highly flexible, glycine-rich region called domain V. Calpain 1 and calpain 2 large subunits are phosphorylated at several sites in domains I-III; some of these residues are conserved and some are isoform specific.
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Schematic representation of the domain architecture of the classical calpains. The 80 kDa large subunits can be divided into four domains, plus a short linker that might be important for transducing conformational changes throughout the molecule upon calcium binding (T). The N-terminal α-helix makes up domain I, which interacts with the small subunits before undergoing intermolecular autolysis on activation. Protease activity is contained within domain II, which is further divided into subdomains (IIa and IIb) that make up the two halves of the active site. Domain III comprises a C2-like domain that harbors sites for phosphorylation and phospholipid binding. Five consecutive EF-hand motifs make up domain IV and contribute to the calcium binding of the large subunits and to dimerization with the small subunits. Domain VI of the small subunits has a similar arrangement; the first four EF hands participate in calcium binding and the last motif interacts with the large subunit. The small subunits also contain a highly flexible, glycine-rich region called domain V. Calpain 1 and calpain 2 large subunits are phosphorylated at several sites in domains I-III; some of these residues are conserved and some are isoform specific.

Fig. 2.
Fig. 2. (A) Some of the mechanisms involved in regulating calpain activity. (B) Possible pathway for growth-factor-induced, calpain-mediated cell migration. Binding of epidermal growth factor (EGF) to its receptor (EGFR) activates a MAP kinase cascade that eventually activates ERK. The scaffolding function of FAK brings ERK and calpain 2 into a complex, resulting in phosphorylation of calpain 2. This ERK-mediated phosphorylation leads to activation of calpain 2, which can be counteracted by phosphorylation of calpain 2 by PKA. Active calpain 2 can then cleave talin 1, leading to adhesion complex turnover and cell migration.
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(A) Some of the mechanisms involved in regulating calpain activity. (B) Possible pathway for growth-factor-induced, calpain-mediated cell migration. Binding of epidermal growth factor (EGF) to its receptor (EGFR) activates a MAP kinase cascade that eventually activates ERK. The scaffolding function of FAK brings ERK and calpain 2 into a complex, resulting in phosphorylation of calpain 2. This ERK-mediated phosphorylation leads to activation of calpain 2, which can be counteracted by phosphorylation of calpain 2 by PKA. Active calpain 2 can then cleave talin 1, leading to adhesion complex turnover and cell migration.

Fig. 2.
Fig. 2. (A) Some of the mechanisms involved in regulating calpain activity. (B) Possible pathway for growth-factor-induced, calpain-mediated cell migration. Binding of epidermal growth factor (EGF) to its receptor (EGFR) activates a MAP kinase cascade that eventually activates ERK. The scaffolding function of FAK brings ERK and calpain 2 into a complex, resulting in phosphorylation of calpain 2. This ERK-mediated phosphorylation leads to activation of calpain 2, which can be counteracted by phosphorylation of calpain 2 by PKA. Active calpain 2 can then cleave talin 1, leading to adhesion complex turnover and cell migration.
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(A) Some of the mechanisms involved in regulating calpain activity. (B) Possible pathway for growth-factor-induced, calpain-mediated cell migration. Binding of epidermal growth factor (EGF) to its receptor (EGFR) activates a MAP kinase cascade that eventually activates ERK. The scaffolding function of FAK brings ERK and calpain 2 into a complex, resulting in phosphorylation of calpain 2. This ERK-mediated phosphorylation leads to activation of calpain 2, which can be counteracted by phosphorylation of calpain 2 by PKA. Active calpain 2 can then cleave talin 1, leading to adhesion complex turnover and cell migration.

Except under pathological conditions associated with cell death, such as axonal transection, neurodegeneration and tissue ischemia, the levels of calcium required to activate calpains maximally in vitro do not exist within living cells. This apparent paradox has led researchers towards the idea that other regulatory mechanisms can lower this requirement in vivo. Several different modes of regulation have been identified, although their contributions in vivo have not yet been determined. The large subunits of some calpains are autolyzed on activation, which removes domain I and abolishes the N-terminal link between the large and small subunits, thereby allowing movement of domain II (Baki et al., 1996; Cong et al., 1989; Elce et al., 1997; Guttmann et al., 1997; Imajoh et al., 1986; Molinari et al., 1994; Suzuki and Sorimachi, 1998; Suzuki et al., 1981a). The truncated large subunit is catalytically active and has a lower requirement for calcium (Baki et al., 1996; Imajoh et al., 1986; Suzuki and Sorimachi, 1998; Suzuki et al., 1981b). However, this event is clearly not required for catalytic activity (Cong et al., 1989; Elce et al., 1997; Guttmann et al., 1997; Molinari et al., 1994), which suggests that it functions more in the progression of activation than in its initiation.

The binding of phospholipids also decreases the calcium requirement for calpains in vitro (Arthur and Crawford, 1996; Melloni et al., 1996; Saido et al., 1992; Suzuki et al., 1992; Tompa et al., 2001), but the in vivo relevance of this is unknown. Similarly, regulation of protein-protein interactions changes the calcium requirements of calpains (Melloni et al., 2000a; Melloni et al., 2000b; Melloni et al., 1998; Melloni et al., 2000c; Michetti et al., 1991; Salamino et al., 1993), but their roles in activation are not clear. Finally, calpains are regulated by their best-known interacting partner, the endogenous calpain inhibitor calpastatin (Wendt et al., 2004). Although overexpression of calpastatin in cells can decrease calpain activity, escape from calpastatin is not sufficient to activate calpains. Furthermore, structural and biochemical data indicate that calpastatin might bind preferentially to calcium-activated calpains (Barnoy et al., 1999; Tullio et al., 1999), suggesting that this is an attenuation mechanism rather than a preventive one.

Friedrich has recently provided an explanation for this apparent paradox (Friedrich, 2004). He proposes that the calpain system developed this high requirement for calcium during evolution as a safety device to prevent potentially destructive hyperactivity of calpains, and that it is preferable for calpains to work at much less than half-maximal activity. Several pieces of evidence support this idea, including structural considerations, the need for spatial and temporal regulation of calpains and the benefits of a large separation between normal and pathological function.

In addition, phosphorylation at several sites controls the activities of calpains. Calpain 2 is activated by phosphorylation of Ser50 by the ERK mitogen-activated protein (MAP) kinase (Glading et al., 2004) during migration of fibroblasts and in keratinocytes stimulated with epidermal growth factor (EGF; Glading et al., 2000; Satish et al., 2005). Phosphorylation of calpain 2 at this site is particularly interesting since calpain 1, which does not contain a phosphorylatable site in this region, does not seem to play a major role in EGF-mediated motility (Glading et al., 2000; Satish et al., 2005). Instead, calpain 1 is important for IP-9-induced motility, which requires intracellular calcium flux (Satish et al., 2005). By contrast, EGF-mediated activation of calpain 2 by phosphorylation occurs in the absence of increased calcium levels. Furthermore, calpain 3 has a glutamic acid residue at this position that could act as an activating phosphomimetic, which might explain why calpain 3 lacks a requirement for increased calcium levels. Together, these data suggest that calcium and growth-factor-mediated phosphorylation can independently activate calpains in an isoform-specific fashion. Interestingly, only membrane-proximal calpain 2 is activated by ERK-mediated phosphorylation (Glading et al., 2001), which suggests that there are alternative modes of activation for certain calpain 2 subpopulations.

Unsurprisingly, the MAP kinase kinase MEKK1 is required for normal calpain 2 activity (Cuevas et al., 2003). MEKK1 associates with focal adhesion kinase (FAK) in adhesion complexes and appears to act upstream of ERK in the regulation of calpain 2 activation and subsequent detachment of the rear of the cell during migration. Note that the adaptor function of FAK mediates the assembly of an ERK-calpain 2 complex at peripheral adhesion sites (Carragher et al., 2003). The formation of this complex and the activity of ERK are both required for normal calpain 2 activity and for processes dependent on calpain 2 such as adhesion complex turnover, transformation and cell migration. There is thus a novel signaling pathway by which growth factors regulate cell migration via phosphorylation-dependent activation of calpains (Fig. 2B).

Calpain activity can also be inhibited by phosphorylation. Cyclic-AMP-mediated activation of protein kinase A (PKA) can block EGF-induced activation of calpain 2 and fibroblast migration (Shiraha et al., 2002). This appears to occur through phosphorylation of calpain 2 by PKA, which probably restricts calpain 2 to an inactive conformation (Shiraha et al., 2002; Smith et al., 2003). The residues in calpain 2 (Ser369 and Thr370) that appear to be the PKA targets are conserved in other calpains, which suggests that phosphorylation of domain III represents yet another mechanism for regulating calpain activity.

Among the >100 proteins identified as calpain substrates are transcription factors, transmembrane receptors, signaling enzymes and cytoskeletal proteins. Although calpains can lead to extensive degradation of some of these substrates, most are cleaved in a limited fashion, resulting in stable protein fragments that can have functions different from those of their intact forms. Such limited proteolysis might be correlated with a highly specific recognition sequence. However, no single consensus sequence has been found to have significant value for predicting whether a protein can be proteolyzed by calpains or even where calpains cleave a known substrate. Instead, recognition and proteolysis seem to be controlled by multiple determinants, including but not limited to secondary structure and PEST score (Tompa et al., 2004). This suggests that calpains cleave their substrates in disordered regions between structured domains. Nevertheless, despite this complex set of determinants, there is a significant preference for particular sequences immediately surrounding the site of proteolysis, and studies that have elucidated these preferences have provided valuable tools with which the calpain systems may be specifically and efficiently manipulated (Tompa et al., 2004).

PEST score is a calculation of the quality of potential PEST motifs [characterized by high local concentrations of the amino acids proline (P), glutamic acid (E), serine (S), threonine (T) and, to a lesser extent, aspartic acid (D)], which can reduce the half-lives of proteins by serving as signals for proteolysis. PEST score=0.55 × DPEST - 0.5 × (10 × Kyte-Doolittle hydropathy index + 45); where DPEST represents the corresponding amino acids expressed in mass % (w/w) and corrected for one equivalent of D or E, one of P and one of S or T.

One obvious clue as to how calpains might affect cell motility comes from the fact that numerous adhesion complex components and migration-related proteins are substrates for calpains (Table 3) (Glading et al., 2002; Goll et al., 2003). Although proteolysis of most of these adhesion-related substrates has been demonstrated in vitro as well as in cell culture, several issues have made it difficult to determine which are relevant to calpain-mediated pathways in vivo. The specificity and extent of proteolysis of adhesion complex components can vary between cell types (S.J.F. and A.H., unpublished). Further complicating the issue is the fact that most of these substrates can be proteolyzed in vitro equally well by either calpain 1 or calpain 2, which can have widely differing subcellular localizations and cell-type-specific expression patterns even in culture.

Table 3.

Motility-related calpain substrates

Calpain substrate In vitro Cell culture In vitro isoforms* Cell culture isoforms References
α-actinin   No   Yes   -   ND   Goll et al., 1991; Selliah et al., 1996  
β integrins   Yes   Yes   Capn2   ND   Du et al., 1995; Pfaff et al., 1999  
β-catenin   Yes   Yes   Capn1   Capn2   Rios-Doria et al., 2004  
Cadherins   Yes   Yes   Capn1, 2   ND   Covault et al., 1991; Rios-Doria et al., 2003  
Cortactin   Yes   Yes   Capn1, 2   Capn2   Huang et al., 1997  
EGFR   Yes   Yes   ND   ND   Gates and King, 1983; King and Gates, 1985; Stoscheck et al., 1988  
FAK   Yes   Yes   Capn1, 2   Capn2   Carragher et al., 1999; Cooray et al., 1996; Franco et al., 2004a  
Filamin   Yes   Yes   Capn1, 2, 3   Capn2, 3   Huff-Lonergan et al., 1996; Kwak et al., 1993; Verhallen et al., 1987  
MARCKS   Yes   Yes   Capn2   Capn1, 2   Dedieu et al., 2003; Dulong et al., 2004a  
MLCK   Yes   Yes   ND   ND   Kambayashi et al., 1986; Kosaki et al., 1983  
Paxillin   Yes   Yes   Capn1, 2   Capn2   Carragher et al., 1999; Franco et al., 2004a  
PTP-1B   Yes   Yes   Capn1   ND   Frangioni et al., 1993; Schoenwaelder et al., 1997  
RhoA   Yes   Yes   Capn1   ND   Kulkarni et al., 2002  
Spectrin   Yes   Yes   Capn1, 2   Capn2   Croall et al., 1986; Fox et al., 1987; Franco et al., 2004a  
Src   ND   Yes   ND   ND   Oda et al., 1993  
Talin 1   Yes   Yes   Capn1, 2   Capn2   Carragher et al., 1999; Franco et al., 2004a  
Vinculin   ND   Yes   ND   ND   Serrano and Devine, 2004  
Calpain substrate In vitro Cell culture In vitro isoforms* Cell culture isoforms References
α-actinin   No   Yes   -   ND   Goll et al., 1991; Selliah et al., 1996  
β integrins   Yes   Yes   Capn2   ND   Du et al., 1995; Pfaff et al., 1999  
β-catenin   Yes   Yes   Capn1   Capn2   Rios-Doria et al., 2004  
Cadherins   Yes   Yes   Capn1, 2   ND   Covault et al., 1991; Rios-Doria et al., 2003  
Cortactin   Yes   Yes   Capn1, 2   Capn2   Huang et al., 1997  
EGFR   Yes   Yes   ND   ND   Gates and King, 1983; King and Gates, 1985; Stoscheck et al., 1988  
FAK   Yes   Yes   Capn1, 2   Capn2   Carragher et al., 1999; Cooray et al., 1996; Franco et al., 2004a  
Filamin   Yes   Yes   Capn1, 2, 3   Capn2, 3   Huff-Lonergan et al., 1996; Kwak et al., 1993; Verhallen et al., 1987  
MARCKS   Yes   Yes   Capn2   Capn1, 2   Dedieu et al., 2003; Dulong et al., 2004a  
MLCK   Yes   Yes   ND   ND   Kambayashi et al., 1986; Kosaki et al., 1983  
Paxillin   Yes   Yes   Capn1, 2   Capn2   Carragher et al., 1999; Franco et al., 2004a  
PTP-1B   Yes   Yes   Capn1   ND   Frangioni et al., 1993; Schoenwaelder et al., 1997  
RhoA   Yes   Yes   Capn1   ND   Kulkarni et al., 2002  
Spectrin   Yes   Yes   Capn1, 2   Capn2   Croall et al., 1986; Fox et al., 1987; Franco et al., 2004a  
Src   ND   Yes   ND   ND   Oda et al., 1993  
Talin 1   Yes   Yes   Capn1, 2   Capn2   Carragher et al., 1999; Franco et al., 2004a  
Vinculin   ND   Yes   ND   ND   Serrano and Devine, 2004  
*

Proteolysis by unlisted isoforms has not been determined. ND, not determined.

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Recent studies have begun to identify the motility-related substrates that are most readily and consistently cleaved by calpains, as well as the isoforms responsible in living cells. Knockout of calpain small subunit 1 (CSS1 or Capn4) in mice (Arthur et al., 2000) leads to reduced expression and activities of both calpain 1 and calpain 2 (Dourdin et al., 2001). Embryonic fibroblasts isolated from these mice exhibit decreased proteolysis of several reported substrates, including FAK, paxillin, spectrin, cortactin and talin 1. However, others do not appear to be consistently cleaved in mouse embryonic fibroblasts, including vinculin, RhoA, α-actinin and Src (Dourdin et al., 2001) (S.J.F. and A.H., unpublished). The relevance of these findings remains to be determined, but, together with other reports, they indicate that some calpain substrates are more readily cleaved than others in certain cell types. However, this cell line cannot reveal which calpain isoform is responsible in each case, since the activities of both calpain 1 and calpain 2 are reduced in these cells.

Studies of cells isolated from calpain-1-knockout mice reveal that, despite the absence of calpain 1, these cells can proteolyze many substrates normally, including FAK, paxillin, spectrin and talin 1 (Azam et al., 2001). However, other calpain isoforms could be compensating for calpain 1 deficiency in these cells. More recently, RNA interference (RNAi) technology has been employed to knockdown expression of individual calpain isoforms (Franco et al., 2004a). Interestingly, knockdown of calpain 2 results in decreased proteolysis of FAK, paxillin, spectrin, cortactin and talin 1, while knockdown of calpain 1 has no effect on proteolysis of these proteins (Franco et al., 2004a) (B. Perrin and A.H., unpublished). Therefore, it seems that many motility-related proteins require calpain 2 for proteolysis and are either not cleaved by calpain 1 in living cells or are cleaved by compensatory mechanisms in the absence of calpain 1.

Calpains were first implicated in cell migration by studies showing that pharmacological inhibition of calpains results in reduced integrin-mediated cell migration (Huttenlocher et al., 1997; Palecek et al., 1998). This inhibition leads to stabilization of adhesion complexes and therefore an increase in adhesiveness, thus reducing the rate of detachment of the rear of the cell and decreasing cell migration. Knockout studies support these findings: embryonic fibroblasts from CSS1-deficient mice display a similar reduction in integrin-mediated motility (Dourdin et al., 2001). Since inhibition of calpains by several means results in formation of large peripheral adhesion complexes, calpains were initially thought to regulate cell motility primarily by destabilizing adhesion to the ECM and promoting rear detachment. However, subsequent studies have demonstrated roles for calpains in many aspects of migration, such as cell spreading, membrane protrusion, chemotaxis, and adhesion complex formation and turnover (Fig. 3).

Cell spreading

Cell spreading on ECM components is a complex process involving dynamic reorganization of the actin cytoskeleton in response to integrin-mediated signaling through various pathways. Roles for calpains during cell spreading have been demonstrated in several different systems, but these studies do not reveal one clear function for calpains during this process. Inhibition of the primary calpain in platelets, calpain 1, reduces the ability of these cells to spread, possibly by decreasing proteolysis of adhesion complex proteins (Croce et al., 1999). Inhibition of calpains also reduces spreading in T cells, vascular smooth muscle cells and pancreatic β cells (Parnaud et al., 2005; Paulhe et al., 2001; Rock et al., 2000).

In fibroblasts, overexpression of calpastatin leads to decreased levels of calpain 2 and a decrease in cell spreading and spreading-related actin rearrangements (Potter et al., 1998). This might be caused by an increase in the steady-state levels of the ERM protein ezrin; calpains can proteolyze ezrin and regulate its mRNA levels by an unknown mechanism (Potter et al., 1998). By contrast, spreading of bovine aortic endothelial (BAE) cells is reported to depend specifically on calpain 1, since overexpression of calpain 1 leads to increased cell spreading and a dominant-negative calpain 1 reduces spreading (Kulkarni et al., 1999). However, in the same cell type, calpain 1 can proteolyze RhoA, thereby generating a dominant-negative fragment that inhibits cell spreading (Kulkarni et al., 2002). Studies showing that calpain 1 is important for the formation of early clusters of adhesion molecules that might be sites of Rac1 activation in the early stages of spreading in BAE cells support the idea that calpain 1 positively regulates spreading (Bialkowska et al., 2000). By contrast, knockdown of calpain 1 in several fibroblast cell lines does not affect the ability of these cells to spread (Franco et al., 2004a). Further complicating the issue is the fact that inhibition of calpains in neutrophils might increase spreading of these cells (Lokuta et al., 2003).

CSS1 also appears to play a role in cell spreading through its interaction with the guanine nucleotide exchange factor (GEF) αPIX (Rosenberger et al., 2005). αPIX binds to and colocalizes with calpains in small integrin-containing clusters during the early stages of cell spreading in CHO-K1 cells. Treatment of these cells with calpain inhibitors reduces spreading, which can be overcome by overexpression of αPIX. Interestingly, an αPIX mutant that cannot bind CSS1 does not rescue the spreading defect, but a GEF-deficient αPIX mutant does. αPIX therefore appears to have a GEF-independent role in cell spreading downstream of calpains.

Fig. 3.
Fig. 3. Motility-related processes known to be affected by calpains and the substrates or binding partners acting as effectors. Calpain 2 can cleave adhesion complex proteins such as FAK, paxillin and talin 1, possibly resulting in integrin activation, adhesion complex turnover or detachment of the cell rear. Proteolysis of the actin-regulating protein cortactin might lead to inhibition of membrane protrusion. Cleavage of integrin β-tails might be important for the formation of small integrin clusters during the early stages of cell spreading, whereas proteolysis of the small GTPase RhoA negatively regulates cell spreading. Interaction of αPIX with calpain small subunit 1 (CSS1) can also mediate cell spreading. Proteolysis of the adaptor protein MARCKS might also regulate cell migration in myoblasts, possibly by promoting adhesion formation. The isoforms required for proteolysis of integrins, RhoA and MARCKS remain to be determined, as do the processes affected by proteolysis of nearly 100 other calpain substrates.
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Motility-related processes known to be affected by calpains and the substrates or binding partners acting as effectors. Calpain 2 can cleave adhesion complex proteins such as FAK, paxillin and talin 1, possibly resulting in integrin activation, adhesion complex turnover or detachment of the cell rear. Proteolysis of the actin-regulating protein cortactin might lead to inhibition of membrane protrusion. Cleavage of integrin β-tails might be important for the formation of small integrin clusters during the early stages of cell spreading, whereas proteolysis of the small GTPase RhoA negatively regulates cell spreading. Interaction of αPIX with calpain small subunit 1 (CSS1) can also mediate cell spreading. Proteolysis of the adaptor protein MARCKS might also regulate cell migration in myoblasts, possibly by promoting adhesion formation. The isoforms required for proteolysis of integrins, RhoA and MARCKS remain to be determined, as do the processes affected by proteolysis of nearly 100 other calpain substrates.

Fig. 3.
Fig. 3. Motility-related processes known to be affected by calpains and the substrates or binding partners acting as effectors. Calpain 2 can cleave adhesion complex proteins such as FAK, paxillin and talin 1, possibly resulting in integrin activation, adhesion complex turnover or detachment of the cell rear. Proteolysis of the actin-regulating protein cortactin might lead to inhibition of membrane protrusion. Cleavage of integrin β-tails might be important for the formation of small integrin clusters during the early stages of cell spreading, whereas proteolysis of the small GTPase RhoA negatively regulates cell spreading. Interaction of αPIX with calpain small subunit 1 (CSS1) can also mediate cell spreading. Proteolysis of the adaptor protein MARCKS might also regulate cell migration in myoblasts, possibly by promoting adhesion formation. The isoforms required for proteolysis of integrins, RhoA and MARCKS remain to be determined, as do the processes affected by proteolysis of nearly 100 other calpain substrates.
View largeDownload slide

Motility-related processes known to be affected by calpains and the substrates or binding partners acting as effectors. Calpain 2 can cleave adhesion complex proteins such as FAK, paxillin and talin 1, possibly resulting in integrin activation, adhesion complex turnover or detachment of the cell rear. Proteolysis of the actin-regulating protein cortactin might lead to inhibition of membrane protrusion. Cleavage of integrin β-tails might be important for the formation of small integrin clusters during the early stages of cell spreading, whereas proteolysis of the small GTPase RhoA negatively regulates cell spreading. Interaction of αPIX with calpain small subunit 1 (CSS1) can also mediate cell spreading. Proteolysis of the adaptor protein MARCKS might also regulate cell migration in myoblasts, possibly by promoting adhesion formation. The isoforms required for proteolysis of integrins, RhoA and MARCKS remain to be determined, as do the processes affected by proteolysis of nearly 100 other calpain substrates.

Membrane protrusion

Many studies of calpains and cell spreading also suggest that calpains regulate actin-based mechanisms involved in membrane protrusion. Inhibition of calpains by calpastatin or pharmacological inhibitors leads to formation of abnormal lamellipodia and filopodia (Potter et al., 1998). Likewise, embryonic fibroblasts from CSS1-knockout mice exhibit altered morphologies, displaying thin membrane projections (Dourdin et al., 2001). These cells also exhibit global increases in transient membrane protrusiveness and faster and more-frequent, but less-stable, leading edge protrusions (Franco et al., 2004a). Calpain 2 appears to be the isoform responsible, since knocking it down reproduces the protrusion defects of CSS1-deficient cells. The actin-regulatory protein cortactin is a calpain substrate and probably an important downstream target of calpain 2 in the regulation of membrane protrusions (B. Perrin and A.H., unpublished), because expression of a calpain-resistant form of cortactin leads to membrane defects similar to those seen in calpain-2-knockdown cells. Further support for calpains negatively regulating membrane protrusion comes from studies showing that calcium transients in filopodia of neuronal growth cones act through calpains to reduce lamellipodial protrusion (Robles et al., 2003).

Chemotaxis

Calpains also negatively regulate membrane protrusion in neutrophils. High levels of calpain activity exist in resting neutrophils, and inhibition of these enzymes promotes membrane protrusion and rapid chemokinesis (Lokuta et al., 2003). This contrasts with most other cell types, in which calpain inhibition reduces cell migration. In cell types in which calpains inhibit cell migration, the underlying mechanism might involve negative regulation of the Rho GTPases Cdc42 and Rac1, since calpain inhibition promotes activation of Cdc42 and Rac in neutrophils. The effects are comparable with treatment with chemoattractants such as N-formyl-methionyl-luecyl-phenylalanine (fMLP), which increase chemokinesis (Lokuta et al., 2003). Interestingly, whereas inhibition of calpains promotes random migration of neutrophils, it reduces the directional migration of neutrophils up a gradient of chemoattractant (Lokuta et al., 2003). Spatial regulation of calpain activity might therefore be required for optimum chemotaxis of neutrophils, and calpains could play a role in directional sensing or cell polarization during directed cell migration.

Adhesion complex regulation

Because dynamic regulation of adhesion to the ECM is required for cell migration, the mechanisms by which adhesion complexes are formed and subsequently disassembled are key to cell motility. For some time, inhibition of calpains has been known to alter the morphology and stability of adhesion complexes, but only now are we beginning to elucidate the details of calpain-mediated regulation of adhesion complexes. Although a role for calpains in the disassembly of adhesion sites has been well documented, whether calpains are important for the formation of adhesion complexes remains unclear. As previously mentioned, calpains appear to be important for induction of small, integrin-containing protein clusters at the early stages of spreading (Bialkowska et al., 2000; Bialkowska et al., 2005). However, these clusters do not seem to be precursors of typical adhesion complexes; so their significance is not known. Calpain-mediated proteolysis of talin 1 might be involved in assembling adhesion complexes, since proteolysis of talin 1 by calpains promotes its binding to integrin β-tails, which is known to be crucial for inside-out activation of integrins (Calderwood, 2004; Calderwood et al., 2002; Calderwood et al., 1999; Yan et al., 2001). Proteolysis of the actin-binding protein myristoylated alanine-rich protein kinase C substrate (MARCKS) might also play a role in the formation of adhesion complexes, since inhibition of calpains in myoblasts leads to defects in new adhesion formation and migration coincident with an accumulation of MARCKS (Dedieu et al., 2004). However, several lines of evidence indicate that adhesion complexes can form normally when calpain activity is reduced; so calpains do not appear to be required for assembly of adhesion complexes in most cell types.

As discussed above, calpains can cleave many adhesion complex proteins and downregulation of calpain activity results in large adhesion complexes and inhibits cell detachment. Calpains could therefore be important for destabilization/disassembly of adhesion complexes. Inhibition of calpains by calpastatin or pharmacological agents blocks microtubule-mediated turnover of adhesion complexes after nocodazole washout. This suggests that calpains act downstream of microtubules to mediate adhesion complex disassembly (Bhatt et al., 2002). Knockdown of calpain 2 by RNAi slows the rate at which adhesion complexes disassemble, leading to formation of large, elongated adhesion complexes (Franco et al., 2004b). Furthermore, expression of a calpain-resistant talin 1 mutant in talin-1-null cells also decreases adhesion complex disassembly rates. This indicates that calpain-2-mediated proteolysis of talin 1 regulates adhesion turnover. How talin 1 proteolysis results in adhesion disassembly is not known, but it is likely that this affects both the structural and signaling functions of talin 1 within adhesion complexes. Since talin 1 is cleaved more readily than most other calpain 2 substrates (S.J.F. and A.H., unpublished), its proteolysis might represent the major mode of calpain-2-mediated adhesion disassembly. Future studies will have to determine whether proteolysis of other substrates is also involved.

Calpains have been connected to a variety of pathological conditions (Zatz and Starling, 2005), including stroke and ischemia (Vanderklish and Bahr, 2000), susceptibility to non-insulin diabetes mellitus (Horikawa et al., 2000) and in the pathogenesis of muscular dystrophies (Ono et al., 1998; Sorimachi et al., 2000). Calpain activity appears to play a central role in the movement of immune cells (Lokuta et al., 2003; Stewart et al., 1998), thereby participating in the development of inflammation in normal and pathological conditions such as chronic inflammatory disease (Cuzzocrea et al., 2000; Shields and Banik, 1998; Shields et al., 1998). Furthermore, calpain 2 expression is upregulated in some cancers and has recently been associated with disease progression in patients with breast cancer (Rios-Doria et al., 2003; Wang et al., 2005; Carragher et al., 2004; Huber et al., 2004). The coordinate regulation of adhesion structures by calpains and Src tyrosine kinases places calpains in a crucial role at the interface of kinase and protease cascades that regulate migration of tumor cells and their invasive properties (Carragher et al., 2001; Carragher and Frame, 2002; Carragher et al., 2002; Mamoune et al., 2003). Pathways involving calpains might thus represent an attractive therapeutic target. Future investigations should delineate whether information about the roles of calpains in motility can facilitate development of drugs to treat a variety of human diseases, including cancer and chronic inflammatory disease.

Limited proteolysis by calpains has emerged as a key signal-transducing mechanism that probably functions at the interface of integrin- and growth-factor-mediated signaling to regulate cell migration. The regulation of calpains by calcium, phosphoinositides, and phosphorylation by MAP kinase and PKA pathways places calpains at the center of different signaling pathways controlling many basic cellular processes in addition to cell motility. Crucial to calpain function is the tight regulation of its proteolytic activity, which must be both temporally and spatially controlled during cell migration. Substantial evidence suggests that calpains are activated in a highly localized manner and can be targeted to discrete regions within the cell. However, despite recent progress, our understanding of calpain function during cell migration remains limited. This might be partly attributed to the number and diversity of calpain isoforms; of the 16 known calpain isoforms, only calpain 1, calpain 2 and CSS1 have been studied with respect to migration. Furthermore, there are >100 substrates that can be cleaved by calpains, which makes it difficult to dissect how calpains orchestrate their effects during cell migration. Generation of calpain-resistant substrates will provide important mechanistic clues, but it is important to consider that calpains, like Src-mediated signaling pathways, probably operate by targeting multiple substrates to modify specific stages of the cell motility cycle. Establishing the details involved will require the combination of sophisticated imaging and proteomics-based approaches in both in vitro and in vivo systems.

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