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首页> 外文期刊>Infection and immunity >Stable expression of lipooligosaccharide antigens during attachment, internalization, and intracellular processing of Neisseria gonorrhoeae in infected epithelial cells.
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Stable expression of lipooligosaccharide antigens during attachment, internalization, and intracellular processing of Neisseria gonorrhoeae in infected epithelial cells.

机译:淋病奈瑟氏菌在感染的上皮细胞的附着,内化和细胞内加工过程中稳定表达脂寡糖抗原。

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Immunoelectron microscopy enables the detection and localization of bacterial antigens during in vitro infection (J.F.L. Weel and J.P.M. van Putten, Microb. Pathog. 4:213-222, 1988). In this study, we have used this method to get information on the role of lipooligosaccharides (LOS) in the pathogenesis of neisserial infections at the mucosal level. Ultrathin cryosections of Chang conjunctive epithelial cells infected with Neisseria gonorrhoeae (3 to 18 h) were incubated with LOS-specific monoclonal antibodies and gold-labeled protein A and viewed in the electron microscope. Our results demonstrate that the probed LOS determinants are stably expressed during the adherence, internalization, and intracellular processing of the bacteria. There was no indication of an adaptation of the gonococcal LOS expression to the host cell environment or of a degradation of the probed epitopes. The gold particles, representing LOS molecules, were predominantly located at the bacterial membranes, but sometimes the host cell plasma membrane was labeled as well, suggesting that LOS or LOS-containing membrane fragments interacted with the eucaryotic cells. This was confirmed when purified LOS was added to the cells. Two hours after LOS exposure, gold particles were observed at the plasma membrane of a subpopulation of the cells. After 18 h of LOS exposure, gold particles were also found in large vacuoles inside the cells, suggesting that LOS molecules were internalized by the cells. The function of observed LOS binding and endocytosis in the pathogenesis of neisserial infections remains to be defined.
机译:免疫电子显微镜术能够在体外感染期间检测和定位细菌抗原(J.F.L. Weel和J.P.M. van Putten,Microb.Pathog。4:213-222,1988)。在这项研究中,我们已经使用这种方法来获得脂膜寡糖(LOS)在黏膜水平的奈瑟菌感染的发病机理中的作用的信息。将淋病奈瑟氏菌感染的张氏结膜上皮细胞的超薄冷冻切片(3至18小时)与LOS特异性单克隆抗体和金标记的蛋白A孵育,并在电子显微镜下观察。我们的结果表明,所探测的LOS决定簇在细菌的粘附,内化和细胞内加工过程中稳定表达。没有迹象表明淋球菌LOS表达适应宿主细胞环境或所探测的表位的降解。代表LOS分子的金颗粒主要位于细菌膜上,但有时也对宿主细胞的质膜进行标记,表明LOS或含LOS的膜片段与真核细胞相互作用。当将纯化的LOS添加到细胞中时,可以确认这一点。 LOS暴露两小时后,在细胞亚群的质膜上观察到金颗粒。 LOS暴露18小时后,在细胞内部的大液泡中也发现了金颗粒,这表明LOS分子已被细胞内化。观察到的LOS结合和内吞作用在奈瑟菌感染的发病机理中的功能仍有待确定。

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