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首页> 外文期刊>Journal of Clinical Microbiology >Humoral immune response to Q fever: enzyme-linked immunosorbent assay antibody response to Coxiella burnetii in experimentally infected guinea pigs.
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Humoral immune response to Q fever: enzyme-linked immunosorbent assay antibody response to Coxiella burnetii in experimentally infected guinea pigs.

机译:对Q发热的体液免疫反应:在实验感染的豚鼠中,酶联免疫吸附法对伯氏杆菌的抗体反应。

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The response of guinea pigs experimentally infected with Coxiella burnetii organisms, the etiologic agents of Q fever, was obtained by the measurement of fever, circulating infectious C. burnetii cells, and anti-C. burnetii antibodies. The detection of antibodies by the enzyme-linked immunosorbent assay (ELISA) and traditional methods against phase I whole cells, phase II whole cells, and phase I lipopolysaccharide (LPS-I) (a virulence marker for phase I cells) antigens in the serum samples of infected animals revealed marked differences between intrastrain phase variants. Animals infected with the phase I Nine Mile strain produced a concomitant increase in temperature, circulating infectious C. burnetii cells, and antibodies against phase II cells, phase I cells, and LPS-I. At 15 weeks, a challenge of phase I-infected animals with viable phase I cells resulted in anamnestic antibody responses to phase I cells and LPS-I but not to phase II cells. Infection of animals with the phase II Nine Mile strain produced antibodies against only phase II cells. The challenge of phase II-infected animals at 15 weeks with viable phase II cells resulted in anamnestic antibody responses to phase I and phase II cells but not to LPS-I. Suppression of anti-phase II responses by the phase I challenge was apparent with only the ELISA, because the immunofluorescence, microagglutination, and complement fixation assays were insensitive to these changes. The sensitivity and specificity of the ELISA with whole-cell and the LPS-I antigens in the detection of phase-specific antibody revealed that avirulent phase II cells induced an immune response to phase I antigenic epitopes. Although the avirulent phase II cells were rapidly cleared by the host immune responses, they were sufficiently infective to induce antibody responses to both phase variants. Thus, in the occurrence of Q fever, any conventional serological technique that uses only phase II antigens may not provide a true incidence of naturally acquired infection with both phase I and II C. burnetii organisms.
机译:通过测量发烧,循环传染性伯氏梭状芽胞杆菌细胞和抗C,获得了实验上感染了柯氏杆菌科氏菌(Q病的病原体)的豚鼠的反应。 Burnetii抗体。通过酶联免疫吸附测定(ELISA)和传统方法检测血清中I期全细胞,II期全细胞和I期脂多糖(LPS-1)(I期细胞的毒性标记)抗原的抗体被感染动物的样本显示出菌株内相变体之间的显着差异。感染I期九英里英里株的动物会伴随温度升高,循环感染伯氏梭状芽胞杆菌细胞以及针对II期细胞,I期细胞和LPS-1的抗体而升高。在第15周时,用存活的I期细胞攻击I期感染的动物会导致对I期细胞和LPS-I的记忆消除抗体反应,而对II期细胞无反应。用II Nine Mile株感染动物只会产生针对II期细胞的抗体。用存活的II期细胞在15周时攻击II期感染的动物会导致对I期和II期细胞的记忆消除抗体反应,但对LPS-1没有反应。由于免疫荧光,微凝集和补体固定测定法对这些变化不敏感,因此仅用ELISA即可抑制I期攻击对II期反应的抑制。用全细胞和LPS-1抗原进行ELISA的特异性和特异性检测表明,无毒的II期细胞诱导了对I期抗原表位的免疫反应。尽管无毒的II期细胞可通过宿主免疫反应迅速清除,但它们具有足够的感染力,可诱导对两种相变体的抗体反应。因此,在Q热的发生中,任何仅使用II期抗原的常规血清学技术都可能无法提供I期和II期伯氏梭菌生物体自然获得性感染的真实发生率。

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