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Class I histone deacetylase complex: Structure and functional correlates

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA. 2023-07; 
Xiao Wang, Yannan Wang, Simiao Liu, Yi Zhang, Ke Xu, Liting Ji, Roger D Kornberg, Heqiao Zhang
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Gene Synthesis including Pst2, Clr6, Prw1, Alp13, Cph1, and Cph2, synthesized from GenScript Biotech, were cloned into pFastBac1 vector, respectively. The lysate was further cleared by high-speed centrifugation, purified using anti-Flag resins (GenScript Biotech) To obtain the S. cerevisiae Rpd3S complex, the genes encoding Sin3, bearing a Flag tag at its N terminus, Rpd3, Ume1, Rco1, and Eaf3, all synthesized from GenScript Biotech, were constructed into the pFastBac1 vector, respectively. Get A Quote
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摘要

The Schizosaccharomyces pombe Clr6S complex, a class I histone deacetylase complex, functions as a zinc-dependent enzyme to remove acetyl groups from lysine residues in histone tails. We report here the cryo-EM structure of Clr6S alone and a cryo-EM map of Clr6S in complex with a nucleosome. The active center, revealed at near-atomic resolution, includes features important for catalysis-A water molecule coordinated by zinc, the likely nucleophile for attack on the acetyl-lysine bond, and a loop that may position the substrate for catalysis. The cryo-EM map in the presence of a nucleosome reveals multiple Clr6S-nucleosome contacts and a high degree of relative motion of Clr6S and the nucleosome. Such flexibility... More

关键词

HDAC; cryo-EM; deacetylase; nucleosome; post translational modification