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抑制子筛选揭示了在 condensin 和 cohesin 中常见的 kleisin-hinge 相互作用,但调节方式不同。

Suppressor screening reveals common kleisin-hinge interaction in condensin and cohesin, but different modes of regulation.

机构信息

G0 Cell Unit, Okinawa Institute of Science and Technology Graduate University, Onna-son, 904-0495 Okinawa, Japan.

G0 Cell Unit, Okinawa Institute of Science and Technology Graduate University, Onna-son, 904-0495 Okinawa, Japan

出版信息

Proc Natl Acad Sci U S A. 2019 May 28;116(22):10889-10898. doi: 10.1073/pnas.1902699116. Epub 2019 May 9.

Abstract

Cohesin and condensin play fundamental roles in sister chromatid cohesion and chromosome segregation, respectively. Both consist of heterodimeric structural maintenance of chromosomes (SMC) subunits, which possess a head (containing ATPase) and a hinge, intervened by long coiled coils. Non-SMC subunits (Cnd1, Cnd2, and Cnd3 for condensin; Rad21, Psc3, and Mis4 for cohesin) bind to the SMC heads. Here, we report a large number of spontaneous extragenic suppressors for fission yeast condensin and cohesin mutants, and their sites were determined by whole-genome sequencing. Mutants of condensin's non-SMC subunits were rescued by impairing the SUMOylation pathway. Indeed, SUMOylation of Cnd2, Cnd3, and Cut3 occurs in midmitosis, and Cnd3 K870 SUMOylation functionally opposes Cnd subunits. In contrast, cohesin mutants and were rescued by loss of the RNA elimination pathway (Erh1, Mmi1, and Red1), and loader mutant was rescued by loss of Hrp1-mediated chromatin remodeling. In addition, distinct regulations were discovered for condensin and cohesin hinge mutants. Mutations in the N-terminal helix bundle [containing a helix-turn-helix (HTH) motif] of kleisin subunits (Cnd2 and Rad21) rescue virtually identical hinge interface mutations in cohesin and condensin, respectively. These mutations may regulate kleisin's interaction with the coiled coil at the SMC head, thereby revealing a common, but previously unknown, suppression mechanism between the hinge and the kleisin N domain, which is required for successful chromosome segregation. We propose that in both condensin and cohesin, the head (or kleisin) and hinge may interact and collaboratively regulate the resulting coiled coils to hold and release chromosomal DNAs.

摘要

黏合蛋白和凝聚蛋白分别在姐妹染色单体黏合和染色体分离中起基本作用。它们都由结构维持染色体的异二聚体 Smc 亚基组成,这些亚基具有一个头(包含 Atpase)和一个铰链,铰链中间是长的螺旋线圈。非 Smc 亚基(凝聚蛋白的 Cnd1、Cnd2 和 Cnd3;黏合蛋白的 Rad21、Psc3 和 Mis4)与 Smc 头结合。在这里,我们报告了大量裂殖酵母凝聚蛋白和黏合蛋白突变体的自发外显子抑制因子,其位点通过全基因组测序确定。通过破坏 SUMO 化途径,非 Smc 亚基的凝聚蛋白突变体得到了拯救。事实上,Cnd2、Cnd3 和 Cut3 的 SUMO 化发生在有丝分裂中期,并且 Cnd3 K870 的 SUMO 化在功能上与 Cnd 亚基相对立。相比之下,黏合蛋白突变体 和 被 RNA 消除途径(Erh1、Mmi1 和 Red1)缺失所拯救,而 loader 突变体 被 Hrp1 介导的染色质重塑缺失所拯救。此外,还发现了凝聚蛋白和黏合蛋白铰链突变体的不同调控。黏合蛋白和凝聚蛋白 kleisin 亚基(Cnd2 和 Rad21)的 N 端螺旋束(包含螺旋-转角-螺旋(HTH)模体)中的突变分别拯救了几乎相同的铰链界面突变。这些突变可能调节 kleisin 与 Smc 头部的螺旋线圈的相互作用,从而揭示了铰链和 kleisin N 结构域之间的共同但以前未知的抑制机制,这对于成功的染色体分离是必需的。我们提出,在凝聚蛋白和黏合蛋白中,头部(或 kleisin)和铰链可能相互作用,并协同调节产生的螺旋线圈,以保持和释放染色体 DNA。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8306/6561158/8b38e1afd00a/pnas.1902699116fig01.jpg

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