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艰难梭菌毒素A与培养的L细胞之间的相互作用。

Interaction of Clostridium difficile toxin A with L cells in culture.

作者信息

Shahrabadi M S, Bryan L E, Lee P W

出版信息

Can J Microbiol. 1984 Jul;30(7):874-83. doi: 10.1139/m84-137.

Abstract

Toxin A of Clostridium difficile was purified by column chromatography and acetic acid precipitation. Cells exposed to toxin A showed polarization of nuclei towards one pole of the cells. Toxin A was conjugated to ferritin and applied to L cells to localize binding sites of this toxin to the cell surface. It was found that toxin A conjugate attached to the cell membrane in aggregated form. Antibody specific to toxin A was prepared and used for localization of intracellular toxins in intoxicated cells. Toxin A was found inside the cytoplasm 6 h after cell treatment, mainly in the form of aggregates inside the cytoplasmic vacuoles. At 24 h after exposure, toxin A could be detected within the cytoplasm. Tunicamycin treatment of cells reduced the cell-binding efficiency of toxin A to 50%, but neuraminidase did not effect toxin binding significantly.

摘要

艰难梭菌毒素A通过柱色谱法和醋酸沉淀法进行纯化。暴露于毒素A的细胞显示细胞核向细胞的一极极化。毒素A与铁蛋白结合,并应用于L细胞以定位该毒素在细胞表面的结合位点。结果发现,毒素A结合物以聚集形式附着在细胞膜上。制备了毒素A特异性抗体,并用于定位中毒细胞内的毒素。细胞处理6小时后,在细胞质中发现了毒素A,主要以细胞质空泡内的聚集体形式存在。暴露24小时后,可在细胞质中检测到毒素A。衣霉素处理细胞可将毒素A的细胞结合效率降低至50%,但神经氨酸酶对毒素结合没有显著影响。

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