Lahue R S, Su S S, Modrich P
Proc Natl Acad Sci U S A. 1987 Mar;84(6):1482-6. doi: 10.1073/pnas.84.6.1482.
The involvement of d(GATC) sequences in Escherichia coli DNA mismatch correction was ascertained by analyzing in vitro repair efficiencies of a series of related, covalently closed circular DNA heteroduplexes that contained from zero to four d(GATC) sites. A heteroduplex with four d(GATC) sites was repaired with high efficiency by extracts of E. coli, whereas no significant correction occurred on a closely related molecule lacking such sequences. Heteroduplexes containing one or two d(GATC) sites were corrected at rates between 10% and 93% of that observed for the four-site molecule, but repair efficiency did not correlate in a simple way with the number of sites present. The methylation state at a single d(GATC) sequence was sufficient to direct strandedness of repair, and correction of heteroduplexes containing one or more d(GATC) sites required functional mutH, mutL, and mutS gene products. In addition, DNA repair synthesis dependent on mutH and mutS also required the presence of at least one d(GATC) site. Although mismatch correction was not observed on a covalently closed circular heteroduplex lacking a d(GATC) sequence, such molecules were subject to strand-specific repair if they contained a strand-specific single-strand break. However, this correction reaction did not require mutH, mutL, mutS, or uvrD gene products. Consequently, we have concluded that d(GATC) sequences are directly involved in mismatch correction mediated by the mutHLS system.
通过分析一系列相关的、共价闭合环状DNA异源双链体(含有零至四个d(GATC)位点)的体外修复效率,确定了d(GATC)序列在大肠杆菌DNA错配修复中的作用。含有四个d(GATC)位点的异源双链体可被大肠杆菌提取物高效修复,而在缺乏此类序列的密切相关分子上则未发生明显的校正。含有一个或两个d(GATC)位点的异源双链体的校正率为四位点分子的10%至93%,但修复效率与存在的位点数量并无简单的关联。单个d(GATC)序列处的甲基化状态足以指导修复的链特异性,含有一个或多个d(GATC)位点的异源双链体的校正需要功能性的mutH、mutL和mutS基因产物。此外,依赖mutH和mutS的DNA修复合成也需要至少一个d(GATC)位点的存在。虽然在缺乏d(GATC)序列的共价闭合环状异源双链体上未观察到错配校正,但如果此类分子含有链特异性单链断裂,则会进行链特异性修复。然而,这种校正反应不需要mutH、mutL、mutS或uvrD基因产物。因此,我们得出结论,d(GATC)序列直接参与由mutHLS系统介导的错配校正。
