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核小体 DNA 解缠绕不会影响原型泡沫病毒的整合效率或整合位点选择。

Nucleosome DNA unwrapping does not affect prototype foamy virus integration efficiency or site selection.

机构信息

Department of Cancer Biology and Genetics, The Ohio State University College of Medicine, Columbus, OH, United States of America.

Department of Chemistry and Biochemistry, The Ohio State University, Columbus, OH, United States of America.

出版信息

PLoS One. 2019 Mar 13;14(3):e0212764. doi: 10.1371/journal.pone.0212764. eCollection 2019.

Abstract

Eukaryotic DNA binding proteins must access genomic DNA that is packaged into chromatin in vivo. During a productive infection, retroviral integrases (IN) must similarly interact with chromatin to integrate the viral cDNA genome. Here we examine the role of nucleosome DNA unwrapping in the retroviral integrase search for a target site. These studies utilized PFV intasomes that are comprised of a tetramer of PFV IN with two oligomers mimicking the viral cDNA ends. Modified recombinant human histones were used to generate nucleosomes with increased unwrapping rates at different DNA regions. These modifications included the acetylmimetic H3(K56Q) and the chemically engineered H4(K77ac, K79ac). While transcription factors and DNA damage sensors may search nucleosome bound DNA during transient unwrapping, PFV intasome mediated integration appears to be unaffected by increased nucleosome unwrapping. These studies suggest PFV intasomes do not utilize nucleosome unwrapping to search nucleosome targets.

摘要

真核生物 DNA 结合蛋白必须能够接触到在体内与染色质包装在一起的基因组 DNA。在有效的感染过程中,逆转录病毒整合酶(IN)也必须与染色质相互作用,以整合病毒 cDNA 基因组。在这里,我们研究了核小体 DNA 解旋在逆转录病毒整合酶寻找靶位点中的作用。这些研究利用了由四聚体 PFV IN 与两个模拟病毒 cDNA 末端的寡聚体组成的 PFV 整合酶核心酶,来生成不同 DNA 区域具有更高解旋速率的核小体。这些修饰包括乙酰模拟的 H3(K56Q)和化学工程化的 H4(K77ac、K79ac)。虽然转录因子和 DNA 损伤传感器可能在短暂解旋期间搜索与核小体结合的 DNA,但 PFV 整合酶核心酶介导的整合似乎不受核小体解旋增加的影响。这些研究表明,PFV 整合酶核心酶不会利用核小体解旋来搜索核小体靶标。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ec4a/6415784/db81e9dc6509/pone.0212764.g001.jpg

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