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噬菌体λ重组双链断裂修复模型的证据。

Evidence for the double-strand break repair model of bacteriophage lambda recombination.

作者信息

Takahashi N, Kobayashi I

机构信息

Department of Infectious Diseases Research, National Children's Medical Research Center, Tokyo, Japan.

出版信息

Proc Natl Acad Sci U S A. 1990 Apr;87(7):2790-4. doi: 10.1073/pnas.87.7.2790.

Abstract

We have obtained evidence for the repair of double-strand gaps promoted by the Red function of bacteriophage lambda. A double-strand gap was made in one of the two regions of homology in an inverted orientation on a plasmid DNA molecule. The gapped plasmid was introduced into Escherichia coli cells expressing the red alpha (exo) and red beta (bet) genes of lambda. The gap was repaired by DNA synthesis copying an intact duplex. This gap repair was sometimes accompanied by reciprocal recombination (crossing over). The gap stimulated recombination about 100-fold. Our results are compatible with previous proposals that lambda homologous recombination involves the following early steps: (i) generation of double-stranded ends by the packaging machinery or by the replication machinery; (ii) production of a single-stranded tail with a 3'-hydroxyl end by 5'----3' degradation by lambda exonuclease (red alpha gene product); (iii) pairing of the single-stranded tail with a complementary strand from a homologous duplex with the help of beta protein (red beta gene product); (iv) priming of DNA synthesis at this 3'-hydroxyl end to copy the second DNA molecule.

摘要

我们已经获得了噬菌体λ的Red功能促进双链缺口修复的证据。在质粒DNA分子上一个反向的两个同源区域之一中制造了一个双链缺口。将有缺口的质粒导入表达λ的redα(exo)和redβ(bet)基因的大肠杆菌细胞中。通过复制完整双链体的DNA合成来修复缺口。这种缺口修复有时伴随着相互重组(交叉)。缺口刺激重组约100倍。我们的结果与先前的提议一致,即λ同源重组涉及以下早期步骤:(i)通过包装机制或复制机制产生双链末端;(ii)通过λ核酸外切酶(redα基因产物)的5'→3'降解产生具有3'-羟基末端的单链尾巴;(iii)在β蛋白(redβ基因产物)的帮助下,单链尾巴与来自同源双链体的互补链配对;(iv)在此3'-羟基末端引发DNA合成以复制第二个DNA分子。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b9f2/53776/9799e3544477/pnas01032-0417-a.jpg

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