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Antigens in culture supernatant of Mycobacterium tuberculosis: epitopes defined by monoclonal and human antibodies

机译:结核分枝杆菌培养上清液中的抗原:单克隆抗体和人类抗体定义的表位

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摘要

Antigens of Mycobacterium tuberculosis found in the supernatant of heat-treated cultures were characterized in order to explore whether antigens from this source could be used for the development of a serological test. Culture supernatants and sonicates of 12, 25 and 39 d cultures were analysed by SDS-PAGE. In culture supernatant, major protein bands of 65, 24, and 12 kDa were visible after Coomassie brilliant blue staining. Using murine monoclonal antibodies in Western blots, a pattern of protein bands distinct from that of the corresponding M. tuberculosis sonicates was found in all the culture supernatants. Gel permeation chromatography, in the presence of SDS, was used to separate the major protein bands in the culture supernatant. In ELISA, sera from 20 of 26 patients with tuberculosis reacted with fractions containing mainly 24 kDa or 12 kDa proteins, whereas none of the control sera reacted. In Western blots, each patient serum had its own characteristic banding pattern with culture supernatant, but all the sera from tuberculosis patients and control subjects reacted with protein bands of 65, 61, 58, 30 and 24 kDa. The 12 kDa protein was recognized only by sera from patients with tuberculosis in both Western blots and ELISA. This suggests that different kinds of epitopes on proteins of M. tuberculosis are detected by human antibodies in Western blots and ELISA. We assume that epitopes recognized in Western blots by patients with tuberculosis and control subjects are ubiquitous and are also present on normal commensal bacteria. Epitopes recognized by only some patients with tuberculosis in Western blots may be linear and M. tuberculosis specific. Epitopes recognized by tuberculosis patients but by none of the control subjects in ELISA may be conformation related and M. tuberculosis specific. The major protein bands found in supernatants of heat-treated cultures, 24 and 12 kDa, possess epitopes that may be M. tuberculosis specific and are potentially valuable for the development of a serological test
机译:表征经过热处理的培养物上清液中发现的结核分枝杆菌抗原,以探讨该来源的抗原是否可用于血清学检测。通过SDS-PAGE分析12、25和39 d培养物的培养物上清液和超声处理。在培养上清液中,考马斯亮蓝染色后可见65、24和12 kDa的主要蛋白带。在Western印迹中使用鼠类单克隆抗体,在所有培养上清液中均发现了与相应结核分枝杆菌超声产物不同的蛋白条带模式。在SDS存在下,使用凝胶渗透色谱法分离培养上清液中的主要蛋白条带。在ELISA中,来自26名结核病患者中的20名血清与主要含有24 kDa或12 kDa蛋白的级分反应,而对照血清均无反应。在蛋白质印迹法中,每种患者血清与培养物上清液都有其自身的特征性条带模式,但是来自结核病患者和对照受试者的所有血清均与65、61、58、30和24 kDa的蛋白条带反应。在蛋白质印迹和ELISA中,只有结核病患者的血清才能识别12 kDa蛋白。这表明通过人抗体在蛋白质印迹和ELISA中检测到结核分枝杆菌蛋白上不同类型的表位。我们假设结核病患者和对照对象在Western印迹中识别的表位是普遍存在的,并且在正常的共生细菌中也存在。仅某些结核病患者在Western印迹中识别的表位可能是线性的,并且是结核分枝杆菌特异性的。结核病患者识别的抗原决定簇,但ELISA中没有一个对照对象识别的抗原决定簇,可能与构象相关且与结核分枝杆菌有关。在热处理培养物上清液中发现的主要蛋白条带(24和12 kDa)具有可能是结核分枝杆菌特异的表位,对于血清学检测的发展具有潜在的价值

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