Abstract

The long-term goal of the research is to understand the mechanisms used by cells to impart specificity to signal transducers through compartmentalization and restricted localization. In particular we are interested in the Rab GTPase subfamily of the Ras superfamily. Rab GTPases are important signal transducers and essential elements of the membrane trafficking machinery. Like other Ras-related GTPases, Rab proteins are prenylated and exist in both a soluble pool and on the cytosolic surface of an organelle. A characteristic feature of Rab proteins is that each Rab is localized to a distinct subcellular membrane. Only once recruited to a membrane can Rab GTPases exert their regulatory function, through activation by guanine-nucleotide exchange factors (GEFs) and the subsequent recruitment of effector proteins. The mechanisms that serve to attach Rab proteins to membranes and regulate the activation event are presently unknown. Our studies will address this question, with a combination of several different approaches, including mutant analyses, genomic studies, biochemical, and cell biological techniques and will focus on the model organism S. cerevisiae. The proposed studies are divided into two specific aims.
Specific Aim 1 involves studies of a Rab binding partner, Yip1p, that we feel represents an excellent candidate for playing a fundamental role in membrane localization of Rab proteins.
In Specific Aim 2, we take a converse approach and examine the features of individual Rabs that confer specificity to a given organelle. Overall, we believe the combination of these two aims will help elucidate the long-standing problem of how Rab proteins become recruited onto specific organelles.
Aim 1 : Examine the role of Yip1p, an essential Rab-interacting membrane protein and its influence on Rab function.
Aim 2 : Identify and characterize the specificity determinants responsible for the restricted localization of Rab proteins. A central issue in cell biology has been to understand the mechanisms of membrane transport, and the pathophysiological significance of disrupted transport. Understanding how cells correctly localize and activate Rab GTPases will provide an important missing piece to the puzzle of how these proteins function and how abnormalities in these fundamental processes may contribute to, and be the cause of human disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM069596-04
Application #
7431606
Study Section
Cell Development and Function Integrated Review Group (CDF)
Program Officer
Shapiro, Bert I
Project Start
2005-03-01
Project End
2010-02-28
Budget Start
2008-03-01
Budget End
2009-02-28
Support Year
4
Fiscal Year
2008
Total Cost
$252,557
Indirect Cost

  Institution

Name
Cornell University
Department
Other Basic Sciences
Type
Schools of Veterinary Medicine
DUNS #
872612445
City
Ithaca
State
NY
Country
United States
Zip Code
14850

  Publications

Lepore, Dante; Spassibojko, Olya; Pinto, Gabrielle et al. (2016) Cell cycle-dependent phosphorylation of Sec4p controls membrane deposition during cytokinesis. J Cell Biol 214:691-703
Rinaldi, Fabio C; Packer, Michael; Collins, Ruth (2015) New insights into the molecular mechanism of the Rab GTPase Sec4p activation. BMC Struct Biol 15:14
Wang, Mengqiao; Collins, Ruth N (2014) A lysine deacetylase Hos3 is targeted to the bud neck and involved in the spindle position checkpoint. Mol Biol Cell 25:2720-34
Heger, Christopher D; Wrann, Christiane D; Collins, Ruth N (2011) Phosphorylation provides a negative mode of regulation for the yeast Rab GTPase Sec4p. PLoS One 6:e24332
DeRegis, Carol J; Rahl, Peter B; Hoffman, Gregory R et al. (2008) Mutational analysis of betaCOP (Sec26p) identifies an appendage domain critical for function. BMC Cell Biol 9:3
Nokes, Rita L; Fields, Ian C; Collins, Ruth N et al. (2008) Rab13 regulates membrane trafficking between TGN and recycling endosomes in polarized epithelial cells. J Cell Biol 182:845-53