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PRC1 Catalytic Activity Is Central to Polycomb System Function.

Molecular cell (2019-12-31)
Neil P Blackledge, Nadezda A Fursova, Jessica R Kelley, Miles K Huseyin, Angelika Feldmann, Robert J Klose
ZUSAMMENFASSUNG

The Polycomb repressive system is an essential chromatin-based regulator of gene expression. Despite being extensively studied, how the Polycomb system selects its target genes is poorly understood, and whether its histone-modifying activities are required for transcriptional repression remains controversial. Here, we directly test the requirement for PRC1 catalytic activity in Polycomb system function. To achieve this, we develop a conditional mutation system in embryonic stem cells that completely removes PRC1 catalytic activity. Using this system, we demonstrate that catalysis by PRC1 drives Polycomb chromatin domain formation and long-range chromatin interactions. Furthermore, we show that variant PRC1 complexes with DNA-binding activities occupy target sites independently of PRC1 catalytic activity, providing a putative mechanism for Polycomb target site selection. Finally, we discover that Polycomb-mediated gene repression requires PRC1 catalytic activity. Together these discoveries provide compelling evidence that PRC1 catalysis is central to Polycomb system function and gene regulation.

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(Z)-4-Hydroxytamoxifen, ≥98% Z isomer
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Proteinase K aus Tritirachium album, buffered aqueous glycerol solution, for molecular biology, ≥800 units/mL
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Indol-3-essigsäure Natriumsalz, BioReagent, suitable for plant cell culture, ≥98%
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Di(N-succinimidyl)-Glutarat, ≥97.0% (CHN)
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Anti-Histon H2A-Antikörper (saure Stelle), serum, Upstate®
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Anti-DEDAF-Antikörper, Chemicon®, from rabbit
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Anti-Cbx7-Antikörper, from rabbit, purified by affinity chromatography