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人核提取物中大片段插入/缺失异源双链的修复由5'单链断裂引导,且与错配修复系统无关。

Repair of large insertion/deletion heterologies in human nuclear extracts is directed by a 5' single-strand break and is independent of the mismatch repair system.

作者信息

Littman S J, Fang W H, Modrich P

机构信息

Department of Biochemistry, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

J Biol Chem. 1999 Mar 12;274(11):7474-81. doi: 10.1074/jbc.274.11.7474.

Abstract

The repair of 12-, 27-, 62-, and 216-nucleotide unpaired insertion/deletion heterologies has been demonstrated in nuclear extracts of human cells. When present in covalently closed circular heteroduplexes or heteroduplexes containing a single-strand break 3' to the heterology, such structures are subject to a low level repair reaction that occurs with little strand bias. However, the presence of a single-strand break 5' to the insertion/deletion heterology greatly increases the efficiency of rectification and directs repair to the incised DNA strand. Because nick direction of repair is independent of the strand in which a particular heterology is placed, the observed strand bias is not due to asymmetry imposed on the heteroduplex by the extrahelical DNA segment. Strand-specific repair by this system requires ATP and the four dNTPs and is inhibited by aphidicolin. Repair is independent of the mismatch repair proteins MSH2, MSH6, MLH1, and PMS2 and occurs by a mechanism that is distinct from that of the conventional mismatch repair system. Large heterology repair in nuclear extracts of human cells is also independent of the XPF gene product, and extracts of Chinese hamster ovary cells deficient in the ERCC1 and ERCC4 gene products also support the reaction.

摘要

在人类细胞核提取物中已证实可修复12、27、62和216个核苷酸的未配对插入/缺失异源双链。当存在于共价闭合环状异源双链或在异源双链3'端含有单链断裂的异源双链中时,这些结构会经历低水平的修复反应,且修复过程中链偏向性很小。然而,在插入/缺失异源双链5'端存在单链断裂会大大提高修复效率,并将修复导向被切割的DNA链。由于修复的切口方向与特定异源双链所在的链无关,所以观察到的链偏向性并非由螺旋外DNA片段对异源双链施加的不对称性导致。该系统的链特异性修复需要ATP和四种dNTP,并受到阿非科林的抑制。修复与错配修复蛋白MSH2、MSH6、MLH1和PMS2无关,其发生机制与传统错配修复系统不同。人类细胞核提取物中的大异源双链修复也与XPF基因产物无关,缺乏ERCC1和ERCC4基因产物的中国仓鼠卵巢细胞提取物也支持该反应。

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