RecA-independent recombination: Dependence on the Escherichia coli RarA protein

被引:20
作者
Jain, Kanika [1 ]
Wood, Elizabeth A. [1 ]
Romero, Zachary J. [1 ]
Cox, Michael M. [1 ]
机构
[1] Univ Wisconsin, Dept Biochem, 433 Babcock Dr, Madison, WI 53706 USA
关键词
in vivo cloning; Mgs1; RarA; RecA; recombination; translesion DNA polymerases; MEDIATED TRANSLESION SYNTHESIS; DNA-POLYMERASE IV; DELETION FORMATION; REPLICATION FORKS; GENETIC-RECOMBINATION; IN-VIVO; SEQUENCE-ANALYSIS; REPAIR; DAMAGE; WRNIP1;
D O I
10.1111/mmi.14655
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Most, but not all, homologous genetic recombination in bacteria is mediated by the RecA recombinase. The mechanistic origin of RecA-independent recombination has remained enigmatic. Here, we demonstrate that the RarA protein makes a major enzymatic contribution to RecA-independent recombination. In particular, RarA makes substantial contributions to intermolecular recombination and to recombination events involving relatively short (<200 bp) homologous sequences, where RecA-mediated recombination is inefficient. The effects are seen here in plasmid-based recombination assays and in vivo cloning processes. Vestigial levels of recombination remain even when both RecA and RarA are absent. Additional pathways for RecA-independent recombination, possibly mediated by helicases, are suppressed by exonucleases ExoI and RecJ. Translesion DNA polymerases may also contribute. Our results provide additional substance to a previous report of a functional overlap between RecA and RarA.
引用
收藏
页码:1122 / 1137
页数:16
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