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病毒原头部扩张和DNA包装的门户控制。

Portal control of viral prohead expansion and DNA packaging.

作者信息

Ray Krishanu, Oram Mark, Ma Jinxia, Black Lindsay W

机构信息

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

出版信息

Virology. 2009 Aug 15;391(1):44-50. doi: 10.1016/j.virol.2009.05.029. Epub 2009 Jun 21.

Abstract

Bacteriophage T4 terminase packages DNA in vitro into empty small or large proheads (esps or elps). In vivo maturation of esps yields the more stable and voluminous elps required to contain the 170 kb T4 genome. Functional proheads can be assembled containing portal-GFP fusion proteins. In the absence of terminase activity these accumulated in esps in vivo, whereas wild-type portals were found in elps. By nuclease protection assay dsDNAs of lengths 0.1, 0.2, 0.5, 5, 11, 20, 40 or 170 kb were efficiently packaged into wild-type elps in vitro, but less so into esps and gp20-GFP elps; particularly with DNAs shorter than 11 kb. However, 0.1 kb substrates were equally efficiently packaged into all types of proheads as judged by fluorescence correlation spectroscopy. These data suggest the portal controls the expansion of the major capsid protein lattice during prohead maturation, and that this expansion is necessary for DNA protection but not for packaging.

摘要

噬菌体T4端粒酶可在体外将DNA包装到空的小或大前头部(esps或elps)中。esps在体内成熟可产生容纳170 kb T4基因组所需的更稳定、体积更大的elps。可以组装包含门户-GFP融合蛋白的功能性前头部。在没有端粒酶活性的情况下,这些在体内积累在esps中,而野生型门户则存在于elps中。通过核酸酶保护试验,长度为0.1、0.2、0.5、5、11、20、40或170 kb的双链DNA在体外可有效包装到野生型elps中,但在esps和gp20-GFP elps中效率较低;特别是对于短于11 kb的DNA。然而,通过荧光相关光谱法判断,0.1 kb的底物可同样有效地包装到所有类型的前头部中。这些数据表明,门户在原头部成熟过程中控制主要衣壳蛋白晶格的扩展,并且这种扩展对于DNA保护是必要的,但对于包装不是必需的。

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