We will study the molecular basis of trans-Golgi-network (TGN) to plasma membrane (PM) trafficking in polarized hepatic cells. We will compare and contrast how diverse apical and basolateral PM proteins, as well as secretory proteins, are packaged, targeted and delivered to the two plasma membranes. Rat hepatocytes in vivo and rat-human WIF-B cells in vitro are our polarized cell models. Many selected PM proteins have been expressed in these cells using recombinant adenovirus.
In Aim #1, we will identify and characterize the post-TGN membrane carriers of selected apical and basolateral PM proteins and soluble proteins. Immunofluorescence detection of combinations of single transmembrane, glycolipid-anchored and polytopic PM proteins as they emerge from the TGN will identify cargoes that are carried separately versus together. We will immuno-isolate selected carrier populations from livers of rats expressing these proteins then compare biochemical properties of the membrane carriers using antibodies to probe for the presence of trafficking molecules (e.g., rabs, t- and v-SNAREs, motors) and mass spectrometric analysis (MALDI-TOF/ electrospray MS) to identify known and novel proteins. This biochemical comparison will extend to vesicles carrying the copper-transporting P-type ATPase (ATP7B), which traffics between the TGN and apical PM of hepatocytes in a copper-regulated manner and, when defective, causes Wilson's disease.
In Aim #2, we will study the roles of cytoplasmic proteins in the targeting/retention of polytopic apical proteins. Several apical proteins of the ABC transporter subfamily C contain C-terminal tripeptides recognized by identified PDZ proteins, whereas their basolateral counterparts lack these motifs. We will use site-directed mutagenesis, cell expression and immunofluorescence to determine the necessity and sufficiency of the motifs for apical protein localization, followed by ectopic expression of selected PDZ domains to test the role of each PDZ candidate in this localization. For the Wilson protein ATPase, we will both express and inhibit different domains to identify which parts are involved in its copper-regulated trafficking.
In Aim #3, we will use live-cell imaging to determine the steps in the post-TGN-to-PM transport of selected carriers that are regulated by known trafficking proteins (eg. rabs 8, 11 and 17 and the t-SNAREs) as well as candidates identified in Aims #1 B and #2. Our overall goal is to understand the molecular basis of PM protein traffic in polarized hepatocytes.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
1R01GM064645-01
Application #
6420652
Study Section
General Medicine A Subcommittee 2 (GMA)
Program Officer
Shapiro, Bert I
Project Start
2002-04-01
Project End
2006-03-31
Budget Start
2002-04-01
Budget End
2003-03-31
Support Year
1
Fiscal Year
2002
Total Cost
$346,620
Indirect Cost
Name
Johns Hopkins University
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
045911138
City
Baltimore
State
MD
Country
United States
Zip Code
21218
Nyasae, L; Bustos, R; Braiterman, L et al. (2007) Dynamics of endogenous ATP7A (Menkes protein) in intestinal epithelial cells: copper-dependent redistribution between two intracellular sites. Am J Physiol Gastrointest Liver Physiol 292:G1181-94
Kallay, Laura M; McNickle, Allison; Brennwald, Patrick J et al. (2006) Scribble associates with two polarity proteins, Lgl2 and Vangl2, via distinct molecular domains. J Cell Biochem 99:647-64
Guo, Y; Nyasae, L; Braiterman, L T et al. (2005) NH2-terminal signals in ATP7B Cu-ATPase mediate its Cu-dependent anterograde traffic in polarized hepatic cells. Am J Physiol Gastrointest Liver Physiol 289:G904-16