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增强型农杆菌介导的转化揭示了外源性质粒 DNA 在受体细菌中的安装被核酸外切酶 VII 和 SbcCD 减弱。

Enhanced Agrobacterium-mediated transformation revealed attenuation of exogenous plasmid DNA installation in recipient bacteria by exonuclease VII and SbcCD.

机构信息

Program of Basic Biology, Graduate School of Integrated Sciences for Life, Hiroshima University, Hiroshima, Japan.

Department of Biological Science, Graduate School of Science, Hiroshima University, Hiroshima, Japan.

出版信息

Genes Cells. 2020 Oct;25(10):663-674. doi: 10.1111/gtc.12802. Epub 2020 Sep 30.

DOI:10.1111/gtc.12802
PMID:32799424
Abstract

In DNA transfer via type IV secretion system (T4SS), relaxase enzyme releases linear ssDNA in donor cells and recircularizes in recipient cells. Using VirB/D4 T4SS, Agrobacterium cells can transfer an IncQ-type plasmid depending on Mob relaxase and a model T-DNA plasmid depending on VirD2 relaxase. Mobilization to Escherichia coli of the former plasmid is much more efficient than that of the latter, whereas an entirely reverse relationship is observed in transfer to yeast. These data suggest that either plasmid recircularization or conversion of ssDNA to dsDNA in the recipient bacterial cells is a rate-limiting step of the transfer. In this study, we examined involvement of exonuclease genes in the plasmid acceptability. By the VirD2-dependent T-DNA plasmid, E. coli sbcDΔ and sbcCΔ mutant strains produced threefold more exconjugants, and a sbcDΔ xseAΔ mutant strain yielded eightfold more exconjugants than their wild-type strain. In contrast to the enhancing effect on the VirD2-mediated transfer, the mutations exhibited a subtle effect on the Mob-mediated transfer. These results support our working hypothesis that VirD2 can transport its substrate ssDNA efficiently to recipient cells and that recipient nucleases degrade the ssDNA because VirD2 has some defect(s) in the circularization and completion of complementary DNA synthesis.

摘要

在通过 IV 型分泌系统(T4SS)进行 DNA 转移的过程中,松弛酶在供体细胞中释放线性 ssDNA,并在受体细胞中重新环化。利用 VirB/D4 T4SS,根瘤农杆菌细胞可以转移一种 IncQ 型质粒,这取决于 Mob 松弛酶,还可以转移一种依赖于 VirD2 松弛酶的模型 T-DNA 质粒。前一种质粒在大肠杆菌中的转移效率比后者高得多,而在向酵母的转移中则观察到完全相反的关系。这些数据表明,无论是质粒的重新环化还是 ssDNA 向 dsDNA 的转化,都是转移的限速步骤。在这项研究中,我们研究了外切核酸酶基因在质粒可接受性中的作用。通过依赖 VirD2 的 T-DNA 质粒,E. coli sbcDΔ 和 sbcCΔ 突变株产生的外接合子数量增加了三倍,而 sbcDΔ xseAΔ 突变株产生的外接合子数量比其野生型菌株增加了八倍。与对 VirD2 介导的转移的增强作用相反,这些突变对 Mob 介导的转移只有细微的影响。这些结果支持了我们的工作假设,即 VirD2 可以有效地将其底物 ssDNA 运送到受体细胞,并且由于 VirD2 在环状和互补 DNA 合成的完成方面存在一些缺陷,受体核酸酶会降解 ssDNA。

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