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肺炎支原体抗原在大肠杆菌中的表达。

Expression of Mycoplasma pneumoniae antigens in Escherichia coli.

作者信息

Trevino L B, Haldenwang W G, Baseman J B

出版信息

Infect Immun. 1986 Jul;53(1):129-34. doi: 10.1128/iai.53.1.129-134.1986.

Abstract

A genomic library of Mycoplasma pneumoniae was generated by using bacteriophage lambda EMBL3 as the vector. Screening of the library for the expression of M. pneumoniae protein antigens with adsorbed anti-M. pneumoniae serum revealed strong reactivity from a third of those clones which contained mycoplasma DNA inserts. Three of the most highly reactive clones were analyzed in detail and found to synthesize discrete mycoplasma proteins. Two carried overlapping fragments of mycoplasma DNA which encoded a protein that was readily detected in Escherichia coli after infection with recombinant bacteriophage. The third clone contained a novel mycoplasma DNA fragment which directed the synthesis of two additional mycoplasma proteins. Further screening of the library with antiserum raised against the major M. pneumoniae adhesin protein P1 (165 kilodaltons [kDa]) yielded one clone which produced an immunologically reactive protein of 140 kDa. Adsorption of anti-P1 serum by this clone selected a population of antibodies that were reactive with M. pneumoniae adhesin P1 (165 kDa). These results demonstrate that immunologically active M. pneumoniae proteins are synthesized in E. coli.

摘要

以噬菌体λEMBL3为载体构建了肺炎支原体基因组文库。用吸附的抗肺炎支原体血清筛选该文库中肺炎支原体蛋白抗原的表达情况,发现三分之一含有支原体DNA插入片段的克隆呈现强反应性。对三个反应性最强的克隆进行了详细分析,发现它们能合成离散的支原体蛋白。其中两个克隆携带支原体DNA的重叠片段,该片段编码的一种蛋白在用重组噬菌体感染大肠杆菌后很容易被检测到。第三个克隆包含一个新的支原体DNA片段,它指导合成另外两种支原体蛋白。用针对肺炎支原体主要黏附蛋白P1(165千道尔顿[kDa])产生的抗血清进一步筛选文库,得到一个产生140 kDa免疫反应性蛋白的克隆。该克隆对抗P1血清的吸附作用筛选出了一群与肺炎支原体黏附蛋白P1(165 kDa)反应的抗体。这些结果表明,具有免疫活性的肺炎支原体蛋白可在大肠杆菌中合成。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7a9b/260086/6f03f7f55a09/iai00100-0139-a.jpg

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