Abstract

The internal organization and dynamics of eukaryotic cells is largely determined by the framework of cytoskeletal elements and molecular motors that transport organelles and macromolecular complexes to specific destinations in the cell. Long range transport is generally mediated by microtubule-based motors, and short range transport and capture by the actin-based motors, myosins. The myosin-V family of molecular motors is evolutionarily highly conserved between animals, plants and fungi, and defects in vertebrate myosin-Vs can cause disease. Many different organelles are transported by myosin-Vs, but how they recognize specific cargo, transport and release it at its destination is poorly understood. To address these questions, the researchers use budding yeast where the essential myosin-V, encoded by Myo2, transports secretory vesicles for growth as its major cargo, but also transports peroxisomes, compartments of the secretory pathway, and the vacuole for segregation during the cell cycle, and microtubule ends for nuclear orientation prior to mitosis. These transport events are all mediated by organelle-specific receptors, many of which are known. Here the researchers explore three fundamental aspects of the Myo2 secretory vesicle delivery cycle. In the first aim, they use quantitative live-cell imagining to quantify the number of motors per secretory vesicle and establish how this is determined, and the kinetics of the delivery cycle and how this is integrated with tethering and fusion of the vesicles at their destination. They also explore mechanisms for recycling and regulation of Myo2. In the second aim, they use genetic and live cell imaging methods to explore the function of two proteins, Mmr1 and Smy1, that bind the tail of Myo2 and seem to play a role in its delivery cycle. In the third aim, they first propose to exploit genetic and biochemical approaches to extend their studies on the receptor by which Myo2 identifies and binds secretory vesicles. They also explore the relationship between binding sites on the Myo2 cargo-binding tail by identifying specific mutations that compromise the interactions with individual receptors, and also exploring how binding to one receptor affects binding to another. Finally, they propose to set up an in vitro assay to reconstitute the binding of Myo2 to secretory vesicles based on the genetic, biochemical and cell biological information collected in the earlier aims. Overall, this study will provide unprecedented insights into the delivery cycle of Myo2, which will be of broad relevance due to the high conservation between fungal and vertebrate myosin-Vs as well as their dysfunction in diseases such as Griscelli's syndrome.

Public Health Relevance

All non-infectious diseases are caused by cellular defects that translate into dysfunction of organ(s). As molecular motors selectively ferry organelles and macromolecular complexes to specific sites in the cell to provide the appropriate cellular organization, this project studies in detail how an evolutionarily conserved motor, myosin-V, picks up, transports and drops off many different specific organelles. This is of crucial importance as the regulated transport of specific cargos, including critical membrane proteins like growth factor receptors, proteins involved in nutrient uptake, and adhesion molecules determine the functions of cells, and defects in these processes contribute to many diseases, including cancer.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM039066-25
Application #
8723236
Study Section
Nuclear and Cytoplasmic Structure/Function and Dynamics Study Section (NCSD)
Program Officer
Gindhart, Joseph G
Project Start
1988-02-01
Project End
2015-08-31
Budget Start
2014-09-01
Budget End
2015-08-31
Support Year
25
Fiscal Year
2014
Total Cost
Indirect Cost

  Institution

Name
Cornell University
Department
Type
Organized Research Units
DUNS #
City
Ithaca
State
NY
Country
United States
Zip Code
14850

  Publications

Shin, Myungjoo; van Leeuwen, Jolanda; Boone, Charles et al. (2018) Yeast Aim21/Tda2 both regulates free actin by reducing barbed end assembly and forms a complex with Cap1/Cap2 to balance actin assembly between patches and cables. Mol Biol Cell 29:923-936
Lwin, Kyaw Myo; Li, Donghao; Bretscher, Anthony (2016) Kinesin-related Smy1 enhances the Rab-dependent association of myosin-V with secretory cargo. Mol Biol Cell 27:2450-62
Donovan, Kirk W; Bretscher, Anthony (2015) Head-to-tail regulation is critical for the in vivo function of myosin V. J Cell Biol 209:359-65
Donovan, Kirk W; Bretscher, Anthony (2015) Tracking individual secretory vesicles during exocytosis reveals an ordered and regulated process. J Cell Biol 210:181-9
Xu, Li; Bretscher, Anthony (2014) Rapid glucose depletion immobilizes active myosin V on stabilized actin cables. Curr Biol 24:2471-9
Wayt, Jessica; Bretscher, Anthony (2014) Cordon Bleu serves as a platform at the basal region of microvilli, where it regulates microvillar length through its WH2 domains. Mol Biol Cell 25:2817-27
Viswanatha, Raghuvir; Bretscher, Anthony; Garbett, Damien (2014) Dynamics of ezrin and EBP50 in regulating microvilli on the apical aspect of epithelial cells. Biochem Soc Trans 42:189-94
Bretscher, Anthony (2013) Deconstructing formin-dependent actin cable assembly. Proc Natl Acad Sci U S A 110:18744-5
Chernyakov, Irina; Santiago-Tirado, Felipe; Bretscher, Anthony (2013) Active segregation of yeast mitochondria by Myo2 is essential and mediated by Mmr1 and Ypt11. Curr Biol 23:1818-24
Liu, Wenyu; Santiago-Tirado, Felipe H; Bretscher, Anthony (2012) Yeast formin Bni1p has multiple localization regions that function in polarized growth and spindle orientation. Mol Biol Cell 23:412-22

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