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齿垢密螺旋体重组主要外鞘蛋白(Msp)的序列分析、表达及结合活性

Sequence analysis, expression, and binding activity of recombinant major outer sheath protein (Msp) of Treponema denticola.

作者信息

Fenno J C, Müller K H, McBride B C

机构信息

Department of Microbiology and Immunology, University of British Columbia, Vancouver, Canada.

出版信息

J Bacteriol. 1996 May;178(9):2489-97. doi: 10.1128/jb.178.9.2489-2497.1996.

Abstract

The gene encoding the major outer sheath protein (Msp) of the oral spirochete Treponema denticola ATCC 35405 was cloned, sequenced, and expressed in Escherichia coli. Preliminary sequence analysis showed that the 5' end of the msp gene was not present on the 5.5-kb cloned fragment described in a recent study (M. Haapasalo, K. H. Müller, V. J. Uitto, W. K. Leung, and B. C. McBride, Infect. Immun. 60:2058-2065,1992). The 5' end of msp was obtained by PCR amplification from a T. denticola genomic library, and an open reading frame of 1,629 bp was identified as the coding region for Msp by combining overlapping sequences. The deduced peptide consisted of 543 amino acids and had a molecular mass of 58,233 Da. The peptide had a typical prokaryotic signal sequence with a potential cleavage site for signal peptidase 1. Northern (RNA) blot analysis showing the msp transcript to be approximately 1.7 kb was consistent with the identification of a promoter consensus sequence located optimally upstream of msp and a transcription termination signal found downstream of the stop codon. The entire msp sequence was amplified from T. denticola genomic DNA and cloned in E. coli by using a tightly regulated T7 RNA polymerase vector system. Expression of Msp was toxic to E. coli when the entire msp gene was present. High levels of Msp were produced as inclusion bodies when the putative signal peptide sequence was deleted and replaced by a vector-encoded T7 peptide sequence. Recombinant Msp purified to homogeneity from a clone containing the full-length msp gene adhered to immobilized laminin and fibronectin but not to bovine serum albumin. Attachment of recombinant Msp was decreased in the presence of soluble substrate. Attachment of T. denticola to immobilized laminin and fibronectin was increased by pretreatment of the substrate with recombinant Msp. These studies lend further support to the hypothesis that Msp mediates the extracellular matrix binding activity of T. denticola.

摘要

编码口腔螺旋体齿垢密螺旋体ATCC 35405主要外鞘蛋白(Msp)的基因被克隆、测序并在大肠杆菌中表达。初步序列分析表明,msp基因的5′端不存在于最近一项研究(M. Haapasalo、K. H. Müller、V. J. Uitto、W. K. Leung和B. C. McBride,《感染与免疫》60:2058 - 2065,1992)中描述的5.5 kb克隆片段上。通过从齿垢密螺旋体基因组文库进行PCR扩增获得msp的5′端,并通过组合重叠序列鉴定出一个1629 bp的开放阅读框作为Msp的编码区。推导的肽由543个氨基酸组成,分子量为58233 Da。该肽具有典型的原核信号序列,带有信号肽酶1的潜在切割位点。Northern(RNA)印迹分析显示msp转录本约为1.7 kb,这与在msp上游最佳位置发现的启动子共有序列以及在终止密码子下游发现的转录终止信号一致。整个msp序列从齿垢密螺旋体基因组DNA中扩增出来,并使用严格调控的T7 RNA聚合酶载体系统克隆到大肠杆菌中。当存在完整的msp基因时,Msp的表达对大肠杆菌有毒性。当假定的信号肽序列被删除并用载体编码的T7肽序列取代时,会产生高水平的Msp包涵体。从含有全长msp基因的克隆中纯化至同质的重组Msp可黏附于固定化的层粘连蛋白和纤连蛋白,但不黏附于牛血清白蛋白。在可溶性底物存在的情况下,重组Msp的黏附减少。用重组Msp预处理底物可增加齿垢密螺旋体对固定化层粘连蛋白和纤连蛋白的黏附。这些研究进一步支持了Msp介导齿垢密螺旋体细胞外基质结合活性这一假说。

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本文引用的文献

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Compilation of E. coli mRNA promoter sequences.大肠杆菌信使核糖核酸启动子序列的汇编。
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Effect of outer membrane of Treponema denticola on bone resorption.齿垢密螺旋体外膜对骨吸收的影响。
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