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多聚体C9存在于鼠伤寒沙门氏菌细胞壁的独特位置的C5b-9沉积物中。

Multimeric C9 within C5b-9 deposits in unique locations in the cell wall of Salmonella typhimurium.

作者信息

Joiner K A, Tartanian A B, Hammer C H, Schweinle J E

机构信息

Laboratory of Parasitic Disease, National Institute of Allergy and Infectious Diseases, Bethesda, MD 20892.

出版信息

J Immunol. 1989 Jun 15;142(12):4450-7.

PMID:2656866
Abstract

We have shown previously that multimeric C9 within C5b-9 (C9:C5b-8 greater than 3:1) is needed for killing of a rough strain of Escherichia coli. We now extend these studies using serum sensitive, rough (R) and serum resistant, wild type (WT) strains of Salmonella typhimurium as well as a mutant S. typhimurium strain (TS) with a temperature sensitive mutation in synthesis of keto-deoxy-octulosonate, a constituent within the deep core structure of Salmonella LPS. Both R and TS required multimeric C9 within C5b-9 to be killed. Addition at 37 degrees C of increasing inputs of C9 to TS or R bearing C5b-9 led to a dose-related increase in C9 binding and killing. In contrast, addition of high inputs of C9 to the same strains at 4 degrees C, a procedure that limits the C9:C5b-8 ratio to 1:1, resulted in low C9 binding and minimal killing. Bactericidal C5b-9 formed at 37 degrees C on R and TS with high inputs of C9 co-sedimented with the bacterial outer membrane on sucrose density gradient analysis. Non-bactericidal C5b-9 on R, WT, and TS co-sedimented near the inner membrane, despite the presumed lack of association between these constituents. Whereas 125I C9 within the non-bactericidal pools immunoprecipitate with anti-C5, 125I C9 within bactericidal pools did not immunoprecipitate with anti-C5, anti-C7, or anti-C9. These findings suggest that bactericidal C5b-9 may be deposited in a unique location or configuration within the bacterial cell wall.

摘要

我们之前已经表明,C5b-9中的多聚体C9(C9:C5b-8大于3:1)是杀死大肠杆菌粗糙菌株所必需的。我们现在扩展这些研究,使用血清敏感的鼠伤寒沙门氏菌粗糙(R)菌株和血清抗性的野生型(WT)菌株,以及在酮脱氧辛糖酸合成中具有温度敏感突变的鼠伤寒沙门氏菌突变株(TS),酮脱氧辛糖酸是沙门氏菌脂多糖深核心结构中的一种成分。R和TS菌株都需要C5b-9中的多聚体C9才能被杀死。在37℃下向带有C5b-9的TS或R菌株中添加越来越多的C9,导致C9结合和杀伤呈剂量相关增加。相比之下,在4℃下向相同菌株中添加高剂量的C9,这一过程将C9:C5b-8比例限制为1:1,导致C9结合率低且杀伤最小。在37℃下,用高剂量C9在R和TS菌株上形成的杀菌性C5b-9在蔗糖密度梯度分析中与细菌外膜共沉降。R、WT和TS菌株上的非杀菌性C5b-9在内膜附近共沉降,尽管这些成分之间可能缺乏关联。虽然非杀菌池中125I标记的C9能与抗C5免疫沉淀,但杀菌池中125I标记的C9不能与抗C5、抗C7或抗C9免疫沉淀。这些发现表明,杀菌性C5b-9可能沉积在细菌细胞壁内的一个独特位置或构型中。

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