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参与突触复合体形成的tn5转座酶残基的定点诱变研究。

Site-directed mutagenesis studies of tn5 transposase residues involved in synaptic complex formation.

作者信息

Vaezeslami Soheila, Sterling Rachel, Reznikoff William S

机构信息

Bay Paul Center, Marine Biological Laboratory, Woods Hole, MA 02543, USA.

出版信息

J Bacteriol. 2007 Oct;189(20):7436-41. doi: 10.1128/JB.00524-07. Epub 2007 Aug 10.

Abstract

Transposition (the movement of discrete segments of DNA, resulting in rearrangement of genomic DNA) initiates when transposase forms a dimeric DNA-protein synaptic complex with transposon DNA end sequences. The synaptic complex is a prerequisite for catalytic reactions that occur during the transposition process. The transposase-DNA interactions involved in the synaptic complex have been of great interest. Here we undertook a study to verify the protein-DNA interactions that lead to synapsis in the Tn5 system. Specifically, we studied (i) Arg342, Glu344, and Asn348 and (ii) Ser438, Lys439, and Ser445, which, based on the previously published cocrystal structure of Tn5 transposase bound to a precleaved transposon end sequence, make cis and trans contacts with transposon end sequence DNA, respectively. By using genetic and biochemical assays, we showed that in all cases except one, each of these residues plays an important role in synaptic complex formation, as predicted by the cocrystal structure.

摘要

转座(DNA离散片段的移动,导致基因组DNA重排)在转座酶与转座子DNA末端序列形成二聚体DNA-蛋白质突触复合体时启动。突触复合体是转座过程中发生催化反应的前提条件。参与突触复合体的转座酶-DNA相互作用一直备受关注。在此,我们开展了一项研究,以验证导致Tn5系统中突触形成的蛋白质-DNA相互作用。具体而言,我们研究了(i)精氨酸342、谷氨酸344和天冬酰胺348,以及(ii)丝氨酸438、赖氨酸439和丝氨酸445,根据先前发表的与预切割转座子末端序列结合的Tn5转座酶共晶体结构,它们分别与转座子末端序列DNA形成顺式和反式接触。通过遗传和生化分析,我们表明,除了一种情况外,在所有情况下,这些残基中的每一个在突触复合体形成中都起着重要作用,这与共晶体结构预测的一致。

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