首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Use of a hybrid protein consisting of the variable region of the Borrelia burgdorferi flagellin and part of the 83-kDa protein as antigen for serodiagnosis of Lyme disease.
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Use of a hybrid protein consisting of the variable region of the Borrelia burgdorferi flagellin and part of the 83-kDa protein as antigen for serodiagnosis of Lyme disease.

机译:由伯氏疏螺旋体鞭毛蛋白可变区和部分83-kDa蛋白组成的杂合蛋白作为抗原用于莱姆病的血清诊断。

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摘要

A hybrid protein consisting of the variable region of the Borrelia burgdorferi flagellin (an 18-kDa fragment) and a 59-kDa fragment (lacking the N-terminal part) of the 83-kDa protein has been constructed by genetic engineering. It was expressed as a nonfusion protein of an apparent molecular weight of 77,000 in Escherichia coli. The suitability of this new antigen for the diagnosis of Lyme disease was tested by immunoblotting; for comparison, the recombinant variable region of the flagellin, the 18-kDa fragment (p18), and the whole recombinant 83-kDa protein (p83), both expressed in E. coli, were used. A total of 120 serum samples from various stages of Lyme disease, which were positive in two serological assays, a passive hemagglutination assay and an indirect immunofluorescence assay, were tested. By indirect immunofluorescence, 74 samples were positive for immunoglobulin G (IgG) antibodies and 72 were positive for IgM antibodies. Of these serum samples, 69 of 74 (93%) contained IgG antibodies against p18 and/or p83, and IgG antibodies were detected by the hybrid protein in 67 (90%) samples. IgM antibodies against p18 and/or p83 were detected in 60 of 72 (83%) serum samples, and 57 (79%) serum samples were reactive with the hybrid protein. Twenty serum samples of patients with a history of syphilis and 40 serum samples, negative in routine B. burgdorferi serology, were tested as controls. The hybrid protein, made up of specific epitopes of an early (p18) and late (p83) antigen, is recognized by almost the same number of patient serum samples as the individual antigens.
机译:通过基因工程已经构建了由博氏疏螺旋体鞭毛蛋白的可变区(18-kDa片段)和83-kDa蛋白的59-kDa片段(缺少N末端部分)组成的杂合蛋白。它在大肠杆菌中表达为表观分子量为77,000的非融合蛋白。通过免疫印迹测试了这种新抗原对莱姆病诊断的适用性。为了进行比较,使用了均在大肠杆菌中表达的鞭毛蛋白的重组可变区,18 kDa片段(p18)和整个重组83 kDa蛋白(p83)。总共测试了来自莱姆病各个阶段的120份血清样品,这些样品在两种血清学检测(被动血凝检测和间接免疫荧光检测)中均为阳性。通过间接免疫荧光,74个样品的免疫球蛋白G(IgG)抗体呈阳性,72个样品的IgM抗体呈阳性。在这些血清样本中,74个样本中有69个(93%)包含针对p18和/或p83的IgG抗体,杂交蛋白在67个样本中(90%)检测到IgG抗体。在72个血清样品中,有60个(83%)检测到针对p18和/或p83的IgM抗体,而57个样品(79%)与杂交蛋白反应。将具有梅毒史的患者的20份血清样品和常规B. burgdorferi血清学阴性的40份血清样品作为对照。由早期(p18)和晚期(p83)抗原的特定表位组成的杂合蛋白可被与个体抗原几乎相同数量的患者血清样品识别。

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