Joseph S. Wolenski

Brain myosin-V is a two-headed unconventional myosin with motor activity

Chicken myosin-V is a member of a recently recognized class of myosins distinct from both the myosins-I and the myosins-II. We report here the purification, electron microscopic visualization, and motor properties of a protein of this class. Myosin-V molecules consist of two heads attached to an approximately 30 nm stalk that ends in a globular region of unknown function. Myosin-V binds to and decorates F-actin, has actin-activated magnesium-ATPase activity, and is a barbed-end-directed motor capable of moving actin filaments at rates of up to 400 nm/s. Myosin-V does not form filaments. Each myosin-V heavy chain is associated with approximately four calmodulin light chains as well as two less abundant proteins of 23 and 17 kd.

Function of myosin-V in filopodial extension of neuronal growth cones.

The molecular mechanisms underlying directed motility of growth cones have not been determined. The role of myosin-V, an unconventional myosin, in growth cone dynamics was examined by chromophore-assisted laser inactivation (CALI). CALI of purified chick brain myosin-V absorbed onto nitrocellulose-coated cover slips inhibited the ability of myosin-V to translocate actin filaments. CALI of myosin-V in growth cones of chick dorsal root ganglion neurons resulted in rapid filopodial retraction. The rate of filopodial extension was significantly decreased, whereas the rate of filopodial retraction was not affected, which suggests a specific role for myosin-V in filopodial extension.

The Light Chain Composition of Chicken Brain Myosin-Va: Calmodulin, Myosin-II Essential Light Chains, and 8-kDa Dynein Light Chain/PIN

Class V myosins are a ubiquitously expressed family of actin-based molecular motors. Biochemical studies on myosin-Va from chick brain indicate that this myosin is a two-headed motor with multiple calmodulin light chains associated with the regulatory or neck domain of each heavy chain, a feature consistent with the regulatory effects of Ca(2+) on this myosin. In this study, the identity of three additional low molecular weight proteins of 23-,17-, and 10 kDa associated with myosin-Va is established. The 23- and 17-kDa subunits are both members of the myosin-II essential light chain gene family, encoded by the chicken L23 and L17 light chain genes, respectively. The 10-kDa subunit is a protein originally identified as a light chain (DLC8) of flagellar and axonemal dynein. The 10-kDa subunit is associated with the tail domain of myosin-Va.

Regulation of calmodulin-binding myosins

Myosins constitute a diverse superfamily of actin-based mechanoenzymes that are involved in many essential cellular motilities. In addition to conventional muscle myosin II, ten other classes of unconventional myosins are known. Many unconventional myosins bind multiple calmodulin light chains and Ca2+, which can dramatically alter their mechanochemical and enzymatic activity. Calmodulin-binding myosins can also be regulated by phospholipid binding, phosphorylation of the heavy chain and actin-binding proteins. The molecular details linking unconventional-myosin regulation and function are just beginning to emerge.

Chapter 3 Structural and Functional Dissection of a Membrane-Bound Mechanoenzyme: Brush Border Myosin I

Publisher Summary The only vertebrate myosin I that has been thoroughly characterized is termed brush border (BB) myosin I and is expressed within the microvilli of the intestinal epithelial cell. This chapter discusses the structural and functional properties of brush border myosin I— the subunit composition, the protein domain structure, and the primary structure of its heavy chain— with compliment of multiple calmodulin (CM) light chains. The chapter also discusses the acid binding properties— that is, stoichiometry and Ca 2+ dependence and actin filament cross-linking by brush border Myosin I. It describes the adenosine triphosphate (ATP)ase properties of the brush border myosin I, its mechanochemistry, the function of brush border myosin I calmodulin light chains, the role of calmodulin light chains as repressors rather than activators of brush border myosin I Mg 2+ -ATPase. The chapter discusses the interaction of brush border myosin I, with the microvillar membrane, with acidic phospholipids, the evidence for a microvillar membrane “Docking” protein for brush border myosin I and notions regarding brush border myosin I function. A ∼140-kDa glycoprotein (GP-140) binds to the heavy chain of BB myosin I. GP-140 is the linker protein that tethers BB myosin I to the microvillus (MV) membrane. The disk-bound BB myosin I molecules are tethered to the membrane by their tails. The bound BB myosin I retain all the activities, associated with the free molecule, including actin binding and mechanochemical activity. BB myosin I might participate in the biogenesis and recycling of the apical membrane, by transporting vesicles, up through the terminal web. BB myosin I could cause a relative downward or perhaps rotational movement of the core within the MV membrane and could promote bulk movement of the membrane upward along the MV axis, as a part of an active vesicular shedding mechanism.

Viral membrane fusion and nucleocapsid delivery into the cytoplasm are distinct events in some flaviviruses.

Flaviviruses deliver their genome into the cell by fusing the viral lipid membrane to an endosomal membrane. The sequence and kinetics of the steps required for nucleocapsid delivery into the cytoplasm remain unclear. Here we dissect the cell entry pathway of virions and virus-like particles from two flaviviruses using single-particle tracking in live cells, a biochemical membrane fusion assay and virus infectivity assays. We show that the virus particles fuse with a small endosomal compartment in which the nucleocapsid remains trapped for several minutes. Endosomal maturation inhibitors inhibit infectivity but not membrane fusion. We propose a flavivirus cell entry mechanism in which the virus particles fuse preferentially with small endosomal carrier vesicles and depend on back-fusion of the vesicles with the late endosomal membrane to deliver the nucleocapsid into the cytoplasm. Virus entry modulates intracellular calcium release and phosphatidylinositol-3-phosphate kinase signaling. Moreover, the broadly cross-reactive therapeutic antibody scFv11 binds to virus-like particles and inhibits fusion.

Usp25m protease regulates ubiquitin-like processing of TUG proteins to control GLUT4 glucose transporter translocation in adipocytes

Insulin stimulates the exocytic translocation of specialized vesicles in adipocytes, which inserts GLUT4 glucose transporters into the plasma membrane to enhance glucose uptake. Previous results support a model in which TUG (Tether containing a UBX domain for GLUT4) proteins trap these GLUT4 storage vesicles at the Golgi matrix and in which insulin triggers endoproteolytic cleavage of TUG to translocate GLUT4. Here, we identify the muscle splice form of Usp25 (Usp25m) as a protease required for insulin-stimulated TUG cleavage and GLUT4 translocation in adipocytes. Usp25m is expressed in adipocytes, binds TUG and GLUT4, dissociates from TUG-bound vesicles after insulin addition, and colocalizes with TUG and insulin-responsive cargoes in unstimulated cells. Previous results show that TUG proteolysis generates the ubiquitin-like protein, TUGUL (for TUG ubiquitin-like). We now show that TUGUL modifies the kinesin motor protein, KIF5B, and that TUG proteolysis is required to load GLUT4 onto these motors. Insulin stimulates TUG proteolytic processing independently of phosphatidylinositol 3-kinase. In nonadipocytes, TUG cleavage can be reconstituted by transfection of Usp25m, but not the related Usp25a isoform, together with other proteins present on GLUT4 vesicles. In rodents with diet-induced insulin resistance, TUG proteolysis and Usp25m protein abundance are reduced in adipose tissue. These effects occur soon after dietary manipulation, prior to the attenuation of insulin signaling to Akt. Together with previous data, these results support a model whereby insulin acts through Usp25m to mediate TUG cleavage, which liberates GLUT4 storage vesicles from the Golgi matrix and activates their microtubule-based movement to the plasma membrane. This TUG proteolytic pathway for insulin action is independent of Akt and is impaired by nutritional excess.