鉴定包含介导肺炎支原体细胞黏附的表位的P1基因结构域。
Identification of P1 gene domain containing epitope(s) mediating Mycoplasma pneumoniae cytoadherence.
作者信息
Dallo S F, Su C J, Horton J R, Baseman J B
机构信息
Department of Microbiology, University of Texas Health Science Center, San Antonio 78284.
出版信息
J Exp Med. 1988 Feb 1;167(2):718-23. doi: 10.1084/jem.167.2.718.
Abstract
A genomic library of Mycoplasma pneumoniae was constructed by cloning sheared genomic DNA into the expression vector lambda gt11. Recombinant clones were screened using anti-M. pneumoniae mAbs reactive with adhesin P1 epitopes that mediate cytadherence. 10 clones with different size inserts were isolated. These clones possessed P1 sequences localized to the COOH terminus of the P1 gene. All clones produced fusion proteins that reacted with acute and convalescent sera of patients infected with M. pneumoniae. Interestingly, one clone, P1-7, contained an epitope that was confined to a region of 13 amino acids present in the M. pneumoniae genome as a single copy. The identification of this cytadherence-related epitope permits the production of a synthetic peptide that can be used as a rational vaccine candidate and serodiagnostic probe.
摘要
通过将经剪切的基因组DNA克隆到表达载体λgt11中,构建了肺炎支原体的基因组文库。使用与介导细胞粘附的粘附素P1表位反应的抗肺炎支原体单克隆抗体筛选重组克隆。分离出10个具有不同大小插入片段的克隆。这些克隆具有定位于P1基因COOH末端的P1序列。所有克隆均产生与感染肺炎支原体患者的急性期和恢复期血清反应的融合蛋白。有趣的是,一个名为P1-7的克隆含有一个表位,该表位局限于肺炎支原体基因组中以单拷贝形式存在的13个氨基酸区域。该细胞粘附相关表位的鉴定使得能够生产一种合成肽,其可用作合理的疫苗候选物和血清学诊断探针。
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