Inverted formin 2 in focal adhesions promotes dorsal stress fiber and fibrillar adhesion formation to drive extracellular matrix assembly

Actin filaments and integrin-based focal adhesions (FAs) form integrated systems that mediate dynamic cell interactions with their environment or other cells during migration, the immune response, and tissue morphogenesis. How adhesion-associated actin structures obtain their functional specificity is unclear. Here we show that the formin-family actin nucleator, inverted formin 2 (INF2), localizes specifically to FAs and dorsal stress fibers (SFs) in fibroblasts. High-resolution fluorescence microscopy and manipulation of INF2 levels in cells indicate that INF2 plays a critical role at the SF–FA junction by promoting actin polymerization via free barbed end generation and centripetal elongation of an FA-associated actin bundle to form dorsal SF. INF2 assembles into FAs during maturation rather than during their initial generation, and once there, acts to promote rapid FA elongation and maturation into tensin-containing fibrillar FAs in the cell center. We show that INF2 is required for fibroblasts to organize fibronectin into matrix fibers and ultimately 3D matrices. Collectively our results indicate an important role for the formin INF2 in specifying the function of fibrillar FAs through its ability to generate dorsal SFs. Thus, dorsal SFs and fibrillar FAs form a specific class of integrated adhesion-associated actin structure in fibroblasts that mediates generation and remodeling of ECM.The dynamic connection between the forces generated in the actomyosin cytoskeleton and integrin-mediated focal adhesions (FAs) to the extracellular matrix (ECM) is essential for many physiological processes including cell migration, vascular formation and function, the immune response, and tissue morphogenesis. These diverse functions are mediated by distinct cellular structures including protruding lamellipodia containing nascent FAs that mediate haptotaxis (1), ventral adhesive actin waves that mediate leukocyte transmigration through endothelia (2, 3), and stress fibers (SFs) and FAs that drive fibrillarization of ECM in developing embryos (4, 5). The coordination and interdependence of actin and integrin-based adhesion in these specialized cellular structures are rooted in their biochemical interdependence. Activation of integrins to their high-affinity ECM binding state requires the actin cytoskeleton (6). In turn, integrin engagement with ECM induces signaling that mediates actin polymerization and contractility downstream of Rho GTPases (6, 7). ECM-engaged integrins also affect cytoskeletal organization by physically linking the contractile actomyosin system to extracellular anchorage points (7). Thus, adhesion-associated actin structures are integrated systems that mediate cellular functions requiring coordination of intracellular cytoskeletal forces with ECM binding.Mesenchymal cells generally possess two main types of adhesion-associated actin structures: protruding lamellipodia containing nascent FAs at the cell edge and linear actin bundles in the cell body connected to FAs. Compared with architecturally invariant lamellipodia, adhesion-associated actin bundle structures, including filopodia, the perinuclear actin cap/transmembrane actin-associated nuclear lines, trailing edge bundles, and dorsal SFs, are more diverse in their morphology and less well understood in their architecture and function (8–10). The most-studied actin bundle structure is perhaps dorsal SFs, noncontractile bundles associated at one end with a ventral FA near the cell edge and that extend radially toward the cell center and join with dorsal actin arcs on their other end. How the functional specificity of dorsal SFs is generated apart from the many other distinct adhesion-associated actin bundle structures is not well understood.The functional specificity of adhesion-associated actin structures could be generated either on the adhesion side by compositional differences in FA proteins or on the actin side by differences in the nucleation mechanism and actin binding proteins. On the adhesion side, it is well known that different integrin family members bind distinct types of ECM (11, 12). However, cells adhered to different ECMs all form common structures including lamellipodia, filopodia, and multiple types of SFs. In addition to different integrins, FA function could be regulated by the process of “maturation” in which FAs undergo stereotypical dynamic changes in composition and morphology driven by actomyosin-mediated cellular tension (13, 14). Nascent FAs contain integrins, focal adhesion kinase (FAK), a-actinin, and paxillin (13, 15). When tension is applied, nascent FAs grow and recruit hundreds of proteins, including talin, vinculin, and zyxin (16). These mature FAs then either disassemble or further mature into tensin-containing fibrillar FAs that are responsible for fibronectin fibrillogenesis (17). Thus, the changes in FA size and protein content that accompany FA maturation could give rise to functional specialization of adhesion/actin systems.On the other hand, actin filaments in migrating cells are generated by two main classes of nucleators: the Arp2/3 complex and formins (18). Different nucleating proteins generate different actin organization and geometries, which could in turn dictate functional specificity of adhesions. Arp2/3 forms the branched network in lamellipodia and is thought to be linked to nascent FAs through interaction with FAK (19–21) or vinculin (22). The formin family of actin nucleators, which generates linear actin bundles (23), is more diverse, although formins share a common actin assembly core domain (24), (25). Recent work has begun to ascribe the generation of particular actin structures to some of the 15 formins in mammalian cells, particularly members of the diaphanous family and FHOD1 (26–29). Specifically regarding dorsal SFs, evidence points strongly to polymerization by a formin family member (23, 30–32) but no formin has ever been localized to these SFs or their associated FAs in motile cells. Thus, although formins are clearly critical for forming distinct actin structures, whether they cooperate with FA proteins to specify the function of adhesion-associated actin structures in the cell is unclear.We hypothesized that inverted formin 2 (INF2), found in our recent FA proteome (33), may play a critical role in the formation and functional specificity of adhesion-associated actin structures. INF2 is expressed in cells in two isoforms, one containing a membrane-targeting CAAX-motif that plays a role in mitochondrial fission (34) and a non-CAAX isoform whose function is not well characterized. INF2 is an unusual formin insofar as it contains, in addition to the FH1–FH2 domains that polymerize actin, a WH2-like domain at the C terminus (35) that binds actin monomers to regulate autoinhibition, and also mediates filament severing (35, 36). INF2 also interacts with and inhibits members of the diaphanous family of formin proteins (37). INF2 therefore could have multiple possible roles at FAs in local modulation of actin.Here we explore the role of INF2 in mouse embryonic fibroblasts (MEFs). We find for the first time to our knowledge strong localization of an endogenous formin to FAs at the distal tips of dorsal SFs where it is required for actin polymerization at FAs to form dorsal SFs. We show that INF2 plays a role in controlling morphological, but not compositional maturation of FAs. Strikingly, INF2 is responsible for the formation of one specific class of FAs, the fibrillar FAs that organize the ECM; disruption of INF2 leads to defects in ECM fibrillogenesis. Thus, our study demonstrates that INF2 mediates the formation of dorsal SFs and fibrillar FAs, which together comprise a specific integrated adhesion-associated actin structure responsible for the fibrillogenesis of ECM by fibroblasts.