Affiliation:
1. Department of Molecular and Cell Biology and California Institute of Quantitative Biology, University of California Berkeley, Berkeley, California, USA
Abstract
ABSTRACT
We used the budding yeasts
Saccharomyces cerevisiae
and
Torulaspora delbrueckii
to examine the evolution of Sir-based silencing, focusing on Sir1, silencers, the molecular topography of silenced chromatin, and the roles of
SIR
and RNA interference (RNAi) genes in
T. delbrueckii
. Chromatin immunoprecipitation followed by deep sequencing (ChIP-Seq) analysis of Sir proteins in
T. delbrueckii
revealed a different topography of chromatin at the
HML
and
HMR
loci than was observed in
S. cerevisiae. S. cerevisiae
Sir1, enriched at the silencers of
HML
α and
HMR
a
, was absent from telomeres and did not repress subtelomeric genes. In contrast to
S. cerevisiae
SIR1
's partially dispensable role in silencing, the
T. delbrueckii
SIR1
paralog
KOS3
was essential for silencing.
KOS3
was also found at telomeres with
T. delbrueckii
Sir2 (Td-Sir2) and Td-Sir4 and repressed subtelomeric genes. Silencer mapping in
T. delbrueckii
revealed single silencers at
HML
and
HMR
, bound by Td-Kos3, Td-Sir2, and Td-Sir4. The
KOS3
gene mapped near
HMR
, and its expression was regulated by Sir-based silencing, providing feedback regulation of a silencing protein by silencing. In contrast to the prominent role of Sir proteins in silencing,
T. delbrueckii
RNAi genes
AGO1
and
DCR1
did not function in heterochromatin formation. These results highlighted the shifting role of silencing genes and the diverse chromatin architectures underlying heterochromatin.
Funder
HHS | National Institutes of Health
Publisher
American Society for Microbiology
Subject
Cell Biology,Molecular Biology
Cited by
10 articles.
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