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Clonal polymorphisms of outer membrane protein OspB of Borrelia burgdorferi.

机译:伯氏疏螺旋体外膜蛋白OspB的克隆多态性。

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The outer membrane protein OspB of Borrelia burgdorferi, the Lyme borreliosis agent, differs in relative molecular weight (Mr) among strains. To determine whether antigenic variation occurs in B. burgdorferi, a cell population of the human isolate HB19 was cloned first by being diluted in broth and then by being plated on agar medium. Several clones were obtained and characterized by polyacrylamide gel electrophoresis, in situ protease treatment, and Western (immunoblot), Southern, and Northern (RNA) blot analyses. Variants featuring OspB proteins that differed in Mrs and in reactivities with monoclonal antibodies were found. One variant made increased amounts of a 21,000-molecular-weight protein (21K protein) in addition to normal amounts of a 33K OspB protein. Another variant did not produce an OspB protein at all but did express an 18.5K protein. Both the 18.5K and 21K proteins were susceptible in situ to trypsin and were bound by a monoclonal antibody directed against the OspB of strain HB19. There were no differences in the Southern and Northern blot analyses of the different variants. The results led to the following conclusions. (i) Clonal polymorphisms in the surface protein OspB occurred in B. burgdorferi. (ii) Hitherto uncharacterized 18.5K and 21K proteins were protease susceptible, antigenically related to OspB, and apparently produced in greater amounts when an OspB either was not produced or was altered in structure. (iii) The OspB variations, including its absence from cells, were not accounted for by major DNA rearrangements or failure of transcription of the ospB gene.
机译:伯氏疏螺旋体(Berrelia burgdorferi)的外膜蛋白OspB,莱姆氏疏螺旋体病菌,在菌株之间的相对分子量(Mr)不同。为了确定在B.burgdorferi中是否发生抗原变异,首先通过在肉汤中稀释然后在琼脂培养基上铺板来克隆人分离株HB19的细胞群。获得了几个克隆,并通过聚丙烯酰胺凝胶电泳,原位蛋白酶处理以及Western(免疫印迹),Southern和Northern(RNA)印迹分析对其进行了表征。发现了具有OspB蛋白的变体,这些变体的Mrs和与单克隆抗体的反应性不同。除了正常量的33K OspB蛋白外,一种变体还增加了21,000分子量的蛋白(21K蛋白)的含量。另一个变体根本不产生OspB蛋白,但是表达了18.5K蛋白。 18.5K和21K蛋白都对胰蛋白酶原位敏感,并与针对HB19菌株OspB的单克隆抗体结合。不同变体的Southern和Northern印迹分析没有差异。结果得出以下结论。 (i)表面蛋白OspB的克隆多态性发生在伯氏疏螺旋体中。 (ii)迄今为止,未表征的18.5K和21K蛋白是蛋白酶敏感的,与OspB抗原相关,并且当不产生或改变OspB时显然产生更多。 (iii)OspB变异,包括其在细胞中的缺失,不能通过主要的DNA重排或ospB基因转录失败来解释。

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