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首页> 外文期刊>Journal of Clinical Microbiology >Double immunofluorescence microscopic technique for accurate differentiation of extracellularly and intracellularly located bacteria in cell culture.
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Double immunofluorescence microscopic technique for accurate differentiation of extracellularly and intracellularly located bacteria in cell culture.

机译:双重免疫荧光显微镜技术可准确区分细胞培养中位于细胞外和细胞内的细菌。

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摘要

A double immunofluorescence staining technique is described for differentiation between cell-attached (extracellular) and ingested (intracellular) bacteria by HEp-2 cells in cell culture monolayers. This method is based upon the observation that membranes of viable mammalian cells are impermeable for antibodies but are rendered permeable by treatment with fixatives. Consequently, extracellular bacteria can be stained by specific rhodamine-labeled antibodies before fixation, and intracellular bacteria can be visualized by treatment with specific fluorescein-labeled antibodies after fixation. The accuracy and simplicity of this method is demonstrated with HEp-2 cell culture monolayers as target cells and an isogenic pair of Yersinia enterocolitica, one of which is phagocytosis resistant and the other of which is phagocytosis sensitive. Furthermore, it is shown that this staining technique is also applicable for studying the interaction of bacteria with macrophages and fibroblasts.
机译:描述了一种双重免疫荧光染色技术,用于通过细胞培养单层中的HEp-2细胞区分细胞附着的细菌(细胞外)和摄入的细菌(细胞内)。该方法基于以下观察:活的哺乳动物细胞的膜对抗体是不可渗透的,但是通过用固定剂处理使其可渗透。因此,在固定之前,细胞外细菌可以用特异性罗丹明标记的抗体染色,而在固定之后,可以通过用特定的荧光素标记的抗体处理来观察细胞内细菌。以HEp-2细胞培养单层作为靶细胞和一个同基因对小肠结肠炎耶尔森菌,证明了该方法的准确性和简便性,其中一个对吞噬作用具有抵抗力,而另一个对吞噬作用敏感。此外,表明该染色技术也可用于研究细菌与巨噬细胞和成纤维细胞的相互作用。

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