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幽门螺杆菌细胞及其表面成分与宫颈癌细胞膜的黏附。

Adherence of Helicobacter pylori cells and their surface components to HeLa cell membranes.

作者信息

Fauchère J L, Blaser M J

机构信息

Research Service, Veterans Administration Medical Center, Denver, Colorado.

出版信息

Microb Pathog. 1990 Dec;9(6):427-39. doi: 10.1016/0882-4010(90)90061-t.

Abstract

Four Helicobacter pylori strains were used to develop in vitro methods to assess adherence to HeLa cells. Using direct detection by microscopy, adhesion scores increased with the initial bacteria-to-cell ratio. The urease method assessed H. pylori bound to HeLa cells by their urease activity. The percentage of the original inoculum adhering to HeLa cells remained constant for initial ratios from 10(2) to 10(5) bacteria per cell. An ELISA using anti-H. pylori serum assessed whole bacteria or components bound to HeLa cell fractions. By all three methods, the four H. pylori strains were adherent to HeLa cells or membranes whereas Campylobacter fetus and Providencia control strains were not. The adherence of H. pylori whole cells decreased following extraction with saline, water, or glycine buffer and most of the superficial adhering material (SAM) was present in the saline or water extracts. SAM bound better to HeLa membranes than to calf fetuin or bovine serum albumin (BSA); binding was inhibited by preincubation of SAM with HeLa membranes but not with fetuin or BSA or by pretreatment of HeLa membranes with neuraminidase. These data indicate that SAM has a specific receptor on the HeLa cell membranes. By gel exclusion chromatography of bacterial extracts, the most adherent components were found in the fractions which also contained the highest urease activity; these fractions included urease subunit antigens. We conclude that adherence of H. pylori can be assessed by microtiter assays and involves bacterial surface material which co-purifies with urease and is different from the N-acetyl-neuraminyl-lactose binding hemagglutinin.

摘要

使用4株幽门螺杆菌菌株开发体外方法来评估其对HeLa细胞的黏附。通过显微镜直接检测发现,黏附分数随初始细菌与细胞比例的增加而升高。脲酶法通过幽门螺杆菌的脲酶活性来评估其与HeLa细胞的结合情况。对于每细胞10(2)至10(5)个细菌的初始比例,黏附于HeLa细胞的原始接种物百分比保持恒定。使用抗幽门螺杆菌血清的ELISA法评估与HeLa细胞组分结合的完整细菌或成分。通过所有这三种方法,4株幽门螺杆菌菌株均能黏附于HeLa细胞或细胞膜,而胎儿弯曲杆菌和普罗威登斯对照菌株则不能。用盐水、水或甘氨酸缓冲液提取后,幽门螺杆菌全细胞的黏附能力下降,且大部分表面黏附物质(SAM)存在于盐水或水提取物中。SAM与HeLa细胞膜的结合优于与小牛胎球蛋白或牛血清白蛋白(BSA)的结合;SAM与HeLa细胞膜预孵育可抑制结合,但与胎球蛋白或BSA预孵育则不能,用神经氨酸酶预处理HeLa细胞膜也可抑制结合。这些数据表明SAM在HeLa细胞膜上有特异性受体。通过对细菌提取物进行凝胶排阻色谱分析,发现最具黏附性的成分存在于脲酶活性也最高的组分中;这些组分包括脲酶亚基抗原。我们得出结论,幽门螺杆菌的黏附可通过微量滴定法进行评估,且涉及与脲酶共纯化且不同于N - 乙酰神经氨酸乳糖结合血凝素的细菌表面物质。

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