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姐妹染色单体黏连所需的替代型Ctf18-Dcc1-Ctf8-复制因子C复合物将增殖细胞核抗原加载到DNA上。

The alternative Ctf18-Dcc1-Ctf8-replication factor C complex required for sister chromatid cohesion loads proliferating cell nuclear antigen onto DNA.

作者信息

Bermudez Vladimir P, Maniwa Yoshimasa, Tappin Inger, Ozato Keiko, Yokomori Kyoko, Hurwitz Jerard

机构信息

Molecular Biology Program, Memorial Sloan-Kettering Cancer Center, 1275 York Avenue, New York, NY 10021, USA.

出版信息

Proc Natl Acad Sci U S A. 2003 Sep 2;100(18):10237-42. doi: 10.1073/pnas.1434308100. Epub 2003 Aug 20.

Abstract

The linkage of sister chromatids after DNA replication ensures the faithful inheritance of chromosomes by daughter cells. In budding yeast, the establishment of sister chromatid cohesion requires Ctf8, Dcc1, and Ctf18, a homologue of the p140 subunit of the replication factor C (RFC). In this report we demonstrate that in 293T cells, Flag-tagged Ctf18 forms a seven-subunit cohesion-RFC complex comprised of Ctf18, Dcc1, Ctf8, RFCp40, RFCp38, RFCp37, and RFCp36 (Ctf18-RFC). We demonstrate that a stoichiometric heteroheptameric Ctf18-RFC complex can be assembled by coexpressing the seven proteins in baculovirus-infected insect cells. In addition, the two other stable subcomplexes were formed, which include a pentameric complex comprised of Ctf18, RFCp40, RFCp38, RFCp37, and RFCp36 and a dimeric Dcc1-Ctf8. Both the five- and seven-subunit Ctf18-RFC complexes bind to single-stranded and primed DNAs and possess weak ATPase activity that is stimulated by the addition of primed DNA and proliferating cell nuclear antigen (PCNA). These complexes catalyzed the ATP-dependent loading of PCNA onto primed and gapped DNA but not onto double-stranded nicked or single-stranded circular DNAs. Consistent with these observations, both Ctf18-RFC complexes substituted for the replicative RFC in the PCNA-dependent DNA polymerase delta-catalyzed DNA replication reaction. These results support a model in which sister chromatid cohesion is linked to DNA replication.

摘要

DNA复制后姐妹染色单体的连接确保了子细胞对染色体的忠实遗传。在芽殖酵母中,姐妹染色单体黏连的建立需要Ctf8、Dcc1和Ctf18,后者是复制因子C(RFC)的p140亚基的同源物。在本报告中,我们证明在293T细胞中,带有Flag标签的Ctf18形成了一个由Ctf18、Dcc1、Ctf8、RFCp40、RFCp38、RFCp37和RFCp36组成的七亚基黏连-RFC复合物(Ctf18-RFC)。我们证明,通过在杆状病毒感染的昆虫细胞中共表达这七种蛋白质,可以组装出化学计量的异源七聚体Ctf18-RFC复合物。此外,还形成了另外两种稳定的亚复合物,其中包括一个由Ctf18、RFCp40、RFCp38、RFCp37和RFCp36组成的五聚体复合物以及一个二聚体Dcc1-Ctf8。五亚基和七亚基的Ctf18-RFC复合物都能结合单链和引发的DNA,并具有微弱的ATP酶活性,添加引发的DNA和增殖细胞核抗原(PCNA)可刺激该活性。这些复合物催化了PCNA依赖ATP加载到引发的和有缺口的DNA上,但不能加载到双链切口或单链环状DNA上。与这些观察结果一致,两种Ctf18-RFC复合物在PCNA依赖的DNA聚合酶δ催化的DNA复制反应中替代了复制性RFC。这些结果支持了一个模型,即姐妹染色单体黏连与DNA复制相关联。

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