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由与内部支架蛋白融合的衣壳蛋白组装噬菌体P2衣壳。

Assembly of bacteriophage P2 capsids from capsid protein fused to internal scaffolding protein.

作者信息

Chang Jenny R, Spilman Michael S, Dokland Terje

机构信息

Department of Microbiology, University of Alabama at Birmingham, AL 35294, USA

出版信息

Virus Genes. 2010 Apr;40(2):298-306. doi: 10.1007/s11262-009-0442-2.

Abstract

Most tailed bacteriophages with double-stranded DNA genomes code for a scaffolding protein, which is required for capsid assembly, but is removed during capsid maturation and DNA packaging. The gpO scaffolding protein of bacteriophage P2 also doubles as a maturation protease, while the scaffolding activity is confined to a 90 residue C-terminal "scaffolding" domain. Bacteriophage HK97 lacks a separate scaffolding protein; instead, an N-terminal "delta" domain in the capsid protein appears to serve an analogous role. We asked whether the C-terminal scaffolding domain of gpO could work as a delta domain when fused to the gpN capsid protein. Varying lengths of C-terminal sequences from gpO were fused to the N-terminus of gpN and expressed in E. coli. The presence of just the 41 C-terminal residues of gpO increased the fidelity of assembly and promoted the formation of closed shells, but the shells formed were predominantly small, 40 nm shells, compared to the normal, 55 nm P2 procapsid shells. Larger scaffolding domains fused to gpN caused the formation of shells of varying size and shape. The results suggest that while fusing the scaffolding protein to the capsid protein assists in shell closure, it also restricts the conformational variability of the capsid protein.

摘要

大多数具有双链DNA基因组的有尾噬菌体编码一种支架蛋白,它是衣壳组装所必需的,但在衣壳成熟和DNA包装过程中会被去除。噬菌体P2的gpO支架蛋白还兼作成熟蛋白酶,而支架活性局限于一个90个残基的C端“支架”结构域。噬菌体HK97缺乏单独的支架蛋白;相反,衣壳蛋白中的N端“δ”结构域似乎起到了类似的作用。我们询问gpO的C端支架结构域与gpN衣壳蛋白融合时是否可以作为δ结构域发挥作用。将gpO不同长度的C端序列与gpN的N端融合,并在大肠杆菌中表达。仅gpO的41个C端残基的存在就提高了组装的保真度并促进了封闭壳的形成,但与正常的55nm P2前衣壳壳相比,形成的壳主要是小的40nm壳。与gpN融合的更大的支架结构域导致形成大小和形状各异的壳。结果表明,虽然将支架蛋白与衣壳蛋白融合有助于壳的封闭,但它也限制了衣壳蛋白的构象变异性。

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