Awardee OrganizationUNIVERSITY OF CALIFORNIA BERKELEY
Description
Abstract Text
Clathrin-coated vesicles and membranes have been implicated in a variety of
intracellular transport processes in eukaryotic cells. The precise
funciton of clathrin in cell growth and protein transport will be addressed
by evaluation of yeast mutants defective in production of clathrin heavy
and light subunits. Polyclonal antiserum was used to identify a clone of
the yeast heavy chain gene (CHC1) expressed in a Lambdagtll genomic
library. The identity of this insert was confirmed by hybrid-selected
translation of heavy chain mRNA followed by immune precipitation. A
fragment of the insert was then used to generate deletions of the
chromosomal CHC1 locus. Surprisingly, viable deletion mutant strains were
produced which have no detectable immunoreactive heavy chain, and which
produce vesicles that also lack clathrin light chain. Although clathrin
deletion mutant cells grow slowly, secretion of the glycoprotein invertase
is nearly normal. Deletion mutant cells will now be examined for the rate
and fidelity of transport and sorting of proteins to various destinations.
Structural analogues of clathrin will be sought using sensitive nucleic
acid hybridization procedures and by examining alternative associations
formed with clathrin light chain in heavy chain deletion mutant cells.
Cloning and deletion analysis of the light chain gene will be used to
detect any independent role that light chains may play in protein transport.
No Sub Projects information available for 1R01GM036881-01
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