Coordinated membrane actin remodeling are integral to a number of cellular functions including (i) cell movement, (ii) endocytosis and exocytosis and (iii) mitosis. A number of signaling molecules that control either or both membrane and actin remodeling include phosphoinositides, Arf family GTP binding proteins and Rho family GTP-binding proteins. The main objective of the work in our laboratory is to elucidate the mechanisms that regulate the signals mediated by Arf family proteins. The work has led to the identification of a family of Arf GTPase-activating proteins, the ASAPs, that may integrate at least four signaling pathways, providing coordinated responses in membranes and actin necessary for particular cellular behaviors. The ASAPs are comprised of four subfamilies: ASAP1/2, ACAP1/2/3, AGAP1/2/3 and ARAP1/2/3. Studies with two general goals are being conducted. One emphasis of the laboratory is to examine specific molecular mechanisms by which Arf GAPs interact with Arf and impact Arf activities. We have found that the PH domain of one Arf GAP, ASAP1, is an allosteric site regulating catalysis through the Arf GAP domain. In those studies, we also found that ASAP1 contains localization domains that function independently of the PH domain. Using the coat adaptor protein, GGA, as a model, we have also found that interaction of Arf GAP with Arf requires that Arf dissociate from its effector proteins. Based on these data, we have proposed that Arf GAPs bind to the site of Arf action, and senses, through changes in the lipid environment for instance, when Arf should be inactivated. Continuing studies are designed to define the site of interaction between Arf and Arf GAP as well as between Arf and GGA. In addition, we are examining the potential role of Arf GAP - Arf interactions in cargo sorting that occurs during membrane trafficking events such as protein secretion and exocytosis. A second emphasis of the laboratory is an examination of the specific cellular roles of ASAP family members. We have started by examining representative members of each subfamily. ASAP1 has been found to localize to and control the turnover of focal adhesion, structures that anchor cells to the substratum and which must be remodeled for cell movement to occur. ACAP1 has been found to regulate Arf6 dependent actin-rich protrusion formation, an event thought to be involved in cell spreading and movement. ARAP1 has been also found to regulate both membrane trafficking and the actin cytoskeleton, functioning as a node in a signaling network that regulates cell movement. PIP3 binds to ARAP1, activating the Arf GAP, thereby inactivating Arf and controlling Golgi function. In addition, ARAP1 both induces the activation of Cdc42 and the inactivation of Rho. Reciprocal regulation of these two proteins has been found to induce cell migration. Therefore, in general the ASAP family of Arf GAPs appear to regulate events involved in cell migration. Continuing studies are designed to (i) further delineate the role of Arf GAPs in signaling, (ii) identify specific biological events dependent on signaling through Arf GAPs, eg. Development and function of immunological cells and (iii) evaluate a possible involvement in pathological processes, particularly tumor cell invasion and metastasis. Z01 BC 07365-03 LBC to LCO

Agency
National Institute of Health (NIH)
Institute
Division of Basic Sciences - NCI (NCI)
Type
Intramural Research (Z01)
Project #
1Z01BC007365-07
Application #
6761994
Study Section
(LCO)
Project Start
Project End
Budget Start
Budget End
Support Year
7
Fiscal Year
2002
Total Cost
Indirect Cost
Name
Basic Sciences
Department
Type
DUNS #
City
State
Country
United States
Zip Code
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