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马立克氏病研究中的免疫荧光。I. 细胞培养中抗原的检测及八株分离株的抗原比较。

Immunofluorescence in the study of Marek's disease. I. Detection of antigen in cell culture and an antigenic comparison of eight isolates.

作者信息

Purchase H G

出版信息

J Virol. 1969 Jun;3(6):557-65. doi: 10.1128/JVI.3.6.557-565.1969.

Abstract

The indirect fluorescent-antibody (FA) test was applied to the detection of Marek's disease (MD) antigen in cell culture and antibody in the serum of birds. For the detection of antigen, sera were obtained from birds hyperimmunized with the JM strain of MD. MD antigen could be detected in the nucleus and in the cytoplasm of duck and chick embryo fibroblasts and in those of chick kidney cells infected with material known to contain the MD virus. Uninoculated cultures of chicken cells were always free of MD antigen. When chick kidney cells were infected with a stock cellular preparation of MD virus, infected cells could be detected after 24 hr with the FA test. At this time no cytopathological areas were seen by conventional light microscopy. By 7 days after infection, the same number of infected areas were detected by both methods, and the fluorescent areas coincided with the cytopathological areas. This indicates that the fluorescent areas and the areas with cytopathology are caused by the same agent. A straight-line relationship between the dilution of inoculum and the number of fluorescent or morphological foci obtained indicates that one infectious unit produced one fluorescent or morphological focus. In addition, this time sequence study confirmed the cell association of the virus and demonstrated the cell-to-cell spread of infection. Cell cultures inoculated with eight different isolates of MD were tested in all combinations with sera prepared against the same isolates. The antigens were indistinguishable from one another, indicating that either the strains are antigenically identical or there is a common antigen or contaminant in all of them so that they stained equally well. The FA test can detect MD antigen before cytopathological areas develop in cell culture; however, the small size of the area usually examined precludes its use in initial isolations in which only a small number of infectious units are present in the inoculum. MD-infected cells contain a heat-stable antigen similar to that found in herpes simplex-infected cells.

摘要

间接荧光抗体(FA)试验用于检测细胞培养物中的马立克氏病(MD)抗原以及禽类血清中的抗体。为检测抗原,从用MD的JM株进行过超免疫的禽类中获取血清。在鸭和鸡胚成纤维细胞以及已知含有MD病毒的物质感染的鸡肾细胞的细胞核和细胞质中可检测到MD抗原。未接种的鸡细胞培养物始终不含MD抗原。当鸡肾细胞用MD病毒的细胞制备物原液感染时,24小时后用FA试验可检测到感染细胞。此时,用常规光学显微镜未观察到细胞病变区域。感染后7天,两种方法检测到的感染区域数量相同,且荧光区域与细胞病变区域重合。这表明荧光区域和细胞病变区域是由同一病原体引起的。接种物稀释度与获得的荧光或形态学病灶数量之间呈直线关系,表明一个感染单位产生一个荧光或形态学病灶。此外,这项时间序列研究证实了病毒与细胞的关联,并证明了感染的细胞间传播。用针对八种不同MD分离株制备的血清,对接种了这八种分离株的细胞培养物进行了所有组合的检测。这些抗原彼此无法区分,这表明要么这些毒株在抗原性上相同,要么它们都含有一种共同抗原或污染物,因此染色效果相同。FA试验可在细胞培养物中细胞病变区域出现之前检测到MD抗原;然而,通常检查的区域较小,这使得它无法用于初始分离,因为接种物中仅存在少量感染单位。感染MD的细胞含有一种热稳定抗原,类似于单纯疱疹感染细胞中发现的抗原。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3ba5/375812/02476914ddf5/jvirol00306-0018-a.jpg

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