Cytosolic chaperones mediate quality control of higher-order septin assembly in budding yeast

Author:

Johnson Courtney R.1,Weems Andrew D.1,Brewer Jennifer M.2,Thorner Jeremy2,McMurray Michael A.1

Affiliation:

1. Department of Cell and Developmental Biology, University of Colorado Anschutz Medical Campus, Aurora, CO 80045

2. Department of Molecular and Cell Biology, University of California, Berkeley, Berkeley, CA 94720

Abstract

Septin hetero-oligomers polymerize into cytoskeletal filaments with essential functions in many eukaryotic cell types. Mutations within the oligomerization interface that encompasses the GTP-binding pocket of a septin (its “G interface”) cause thermoinstability of yeast septin hetero-oligomer assembly, and human disease. When coexpressed with its wild-type counterpart, a G interface mutant is excluded from septin filaments, even at moderate temperatures. We show that this quality control mechanism is specific to G interface mutants, operates during de novo septin hetero-oligomer assembly, and requires specific cytosolic chaperones. Chaperone overexpression lowers the temperature permissive for proliferation of cells expressing a G interface mutant as the sole source of a given septin. Mutations that perturb the septin G interface retard release from these chaperones, imposing a kinetic delay on the availability of nascent septin molecules for higher-order assembly. Un­expectedly, the disaggregase Hsp104 contributes to this delay in a manner that does not require its “unfoldase” activity, indicating a latent “holdase” activity toward mutant septins. These findings provide new roles for chaperone-mediated kinetic partitioning of non-native proteins and may help explain the etiology of septin-linked human diseases.

Publisher

American Society for Cell Biology (ASCB)

Subject

Cell Biology,Molecular Biology

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