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dissection and design of yeast prions酵母朊病毒的解剖和设计
PLoS BIOLOGY
Dissection and Design of Yeast Prions
1,2* 2 2 1
Lev Z. Osherovich , Brian S. Cox , Mick F. Tuite , Jonathan S. Weissman
1 Department of Cellular and Molecular Pharmacology and Howard Hughes Medical Institute, University of California, San Francisco, California, United States of America,
2 Department of Biosciences, University of Kent, Canterbury, United Kingdom
Many proteins can misfold into b-sheet-rich, self-seeding polymers (amyloids). Prions are exceptional among such
aggregates in that they are also infectious. In fungi, prions are not pathogenic but rather act as epigenetic regulators
of cell physiology, providing a powerful model for studying the mechanism of prion replication. We used prion-forming
domains from two budding yeast proteins (Sup35p and New1p) to examine the requirements for prion formation and
inheritance. In both proteins, a glutamine/asparagine-rich (Q/N-rich) tract mediates sequence-specific aggregation,
while an adjacent motif, the oligopeptide repeat, is required for the replication and stable inheritance of these
aggregates. Our findings help to explain why although Q/N-rich proteins are relatively common, few form heritable
aggregates: prion inheritance requires both an aggregation sequence responsible for self-seeded growth and an
element that permits chaperone-dependent replication of the aggregate. Using this knowledge, we have designed
novel artificial prions by fusing the replication element of Sup35p to aggregation-prone sequences from other
proteins, including pathogenically expanded polyglutamine.
Introduction
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