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百日咳博德特氏菌保护性外膜蛋白P.69的分子克隆与特性分析

Molecular cloning and characterization of protective outer membrane protein P.69 from Bordetella pertussis.

作者信息

Charles I G, Dougan G, Pickard D, Chatfield S, Smith M, Novotny P, Morrissey P, Fairweather N F

机构信息

Wellcome Research Laboratories, Beckenham, Kent, England.

出版信息

Proc Natl Acad Sci U S A. 1989 May;86(10):3554-8. doi: 10.1073/pnas.86.10.3554.

Abstract

Protein P.69 is localized on the outer membrane of Bordetella pertussis and is one of the virulence factors believed to contribute to the disease state of whooping cough. We demonstrate that protein synthesis of P.69 is under genetic control of the vir locus. Using oligonucleotide probes derived from the protein sequence of a cyanogen bromide fragment, we have cloned the gene for P.69 from B. pertussis CN2992. Analysis of the DNA sequence reveals a G + C-rich gene capable of encoding a protein of 910 amino acids with a Mr of 93,478, suggesting that P.69 is a processed form of a larger precursor. In common with some of the genes in the pertussis toxin operon, the sequence CCTGG was found 5' to the ATG initiation codon. At the 3' end, 29 bases after the TAA stop codon, the sequence GTTTTTCCT was found and may have some function in transcription termination. A full-length clone of the gene for P.69 carried by the cosmid pBPI69 was unable to direct the expression of P.69 protein in an Escherichia coli host. The generation of P.69-fusion products allowed the detection of P.69-specific protein products synthesized in E. coli.

摘要

蛋白质P.69定位于百日咳博德特氏菌的外膜上,是被认为与百日咳疾病状态相关的毒力因子之一。我们证明P.69的蛋白质合成受vir基因座的遗传控制。利用源自溴化氰片段蛋白质序列的寡核苷酸探针,我们从百日咳博德特氏菌CN2992中克隆了P.69基因。DNA序列分析揭示了一个富含G + C的基因,能够编码一个由910个氨基酸组成、分子量为93478的蛋白质,这表明P.69是一种较大前体的加工形式。与百日咳毒素操纵子中的一些基因相同,在ATG起始密码子的5'端发现了序列CCTGG。在3'端,TAA终止密码子后的29个碱基处,发现了序列GTTTTTCCT,它可能在转录终止中具有某种功能。黏粒pBPI69携带的P.69基因全长克隆无法在大肠杆菌宿主中指导P.69蛋白的表达。P.69融合产物的产生使得能够检测在大肠杆菌中合成的P.69特异性蛋白质产物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7b4d/287176/d844ebf7ff98/pnas00250-0122-a.jpg

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