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噬菌体 T4 终止酶的 C 末端结构域在 DNA 包装过程中与头部门控夹区域结合。

The C-terminal domain of the bacteriophage T4 terminase docks on the prohead portal clip region during DNA packaging.

机构信息

Department of Biochemistry and Molecular Biology, University of Maryland School of Medicine, 108N. Greene St., Baltimore, MD 21201, USA.

出版信息

Virology. 2013 Nov;446(1-2):293-302. doi: 10.1016/j.virol.2013.07.011. Epub 2013 Sep 7.

Abstract

Bacteriophage ATP-based packaging motors translocate DNA into a pre-formed prohead through a dodecameric portal ring channel to high density. We investigated portal-terminase docking interactions at specifically localized residues within a terminase-interaction region (aa279-316) in the phage T4 portal protein gp20 equated to the clip domain of the SPP1 portal crystal structure by 3D modeling. Within this region, three residues allowed A to C mutations whereas three others did not, consistent with informatics analyses showing the tolerated residues are not strongly conserved evolutionarily. About 7.5nm was calculated by FCS-FRET studies employing maleimide Alexa488 dye labeled A316C proheads and gp17 CT-ReAsH supporting previous work docking the C-terminal end of the T4 terminase (gp17) closer to the N-terminal GFP-labeled portal (gp20) than the N-terminal end of the terminase. Such a terminase-portal orientation fits better to a proposed "DNA crunching" compression packaging motor and to portal determined DNA headful cutting.

摘要

噬菌体 ATP 基包装马达通过十二聚体门户环通道将 DNA 转运到预先形成的头部中,以达到高密度。我们通过 3D 建模研究了特定定位于噬菌体 T4 门户蛋白 gp20 中的终止酶相互作用区域 (aa279-316) 内的门户末端酶对接相互作用,该区域与 SPP1 门户晶体结构的剪辑结构域相当。在该区域内,三个残基允许 A 到 C 的突变,而其他三个残基则不允许,这与信息学分析一致,表明允许的残基在进化上没有得到强烈保守。通过使用马来酰亚胺 Alexa488 染料标记 A316C 头部和 gp17 CT-ReAsH 的 FCS-FRET 研究,计算出约 7.5nm,这支持了先前的工作,即将 T4 终止酶 (gp17) 的 C 末端更接近 N 末端 GFP 标记的门户 (gp20) 而不是终止酶的 N 末端。这种终止酶-门户的取向更适合于提出的“DNA 压碎”压缩包装马达和由门户决定的 DNA 满载切割。

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