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大肠杆菌细胞毒性坏死因子1:p21 Rho GTP酶组成性激活诱导肌动蛋白组装的证据。

Escherichia coli cytotoxic necrotizing factor 1: evidence for induction of actin assembly by constitutive activation of the p21 Rho GTPase.

作者信息

Fiorentini C, Donelli G, Matarrese P, Fabbri A, Paradisi S, Boquet P

机构信息

Department of Ultrastructures, Istituto Superiore di Sanità, Rome, Italy.

出版信息

Infect Immun. 1995 Oct;63(10):3936-44. doi: 10.1128/iai.63.10.3936-3944.1995.

DOI:10.1128/iai.63.10.3936-3944.1995
PMID:7558302
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC173553/
Abstract

Cytotoxic necrotizing factor type 1 (CNF1) induces in HEp-2 cells an increase in F-actin structures, which was detectable by fluorescence-activated cell sorter analysis 24 h after addition of this factor to the culture medium. Increase in F-actin was correlated with the augmentation of both the cell volume and the total cell actin content. Actin assembly-disassembly is controlled by small GTP-binding proteins of the Rho family, which have been reported recently to be modified by CNF1 treatment. Clostridium difficile toxin B and Clostridium botulinum exoenzyme C3, both known to act on the Rho GTPase, were used as biological tools to study the effect of CNF1 on this protein. CNF1 incubated before, during, or after exposure to the chimeric toxin C3B (which is the product of a genetic fusion between the DNA coding for C3 and the one coding for the B fragment of diphtheria toxin) protected HEp-2 cells from the disruption of F-actin structures caused by inactivation of the Rho GTPase through its ADP-ribosylation. On the other hand, C. difficile toxin B cytopathic effect was not observed upon preincubation of cells with CNF1. Toxins acting through a Rho-independent mechanism, such as cytochalasin D and Clostridium spiroforme iota-like toxin, could not be modified in their cellular activities by CNF1 treatment. All of our results suggest that CNF1 modifies the Rho molecule, thus probably protecting this GTPase from further bacterial toxin modification.

摘要

1型细胞毒性坏死因子(CNF1)可诱导人喉表皮样癌细胞(HEp-2细胞)中F-肌动蛋白结构增加,在向培养基中添加该因子24小时后,通过荧光激活细胞分选分析可检测到这种增加。F-肌动蛋白的增加与细胞体积和细胞总肌动蛋白含量的增加相关。肌动蛋白的组装-解聚受Rho家族的小GTP结合蛋白控制,最近有报道称这些蛋白会被CNF1处理修饰。已知作用于Rho GTP酶的艰难梭菌毒素B和肉毒梭菌外切酶C3被用作生物学工具来研究CNF1对该蛋白的影响。在接触嵌合毒素C3B(它是编码C3的DNA与编码白喉毒素B片段的DNA基因融合的产物)之前、期间或之后孵育CNF1,可保护HEp-2细胞免受因Rho GTP酶通过其ADP核糖基化失活而导致的F-肌动蛋白结构破坏。另一方面,在用CNF1预孵育细胞后未观察到艰难梭菌毒素B的细胞病变效应。通过不依赖Rho的机制起作用的毒素,如细胞松弛素D和螺旋体梭菌iota样毒素,其细胞活性不会因CNF1处理而改变。我们所有的结果表明,CNF1修饰了Rho分子,因此可能保护这种GTP酶免受进一步的细菌毒素修饰。

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Escherichia coli cytotoxic necrotizing factor 1: evidence for induction of actin assembly by constitutive activation of the p21 Rho GTPase.大肠杆菌细胞毒性坏死因子1:p21 Rho GTP酶组成性激活诱导肌动蛋白组装的证据。
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A chimeric toxin to study the role of the 21 kDa GTP binding protein rho in the control of actin microfilament assembly.一种用于研究21 kDa GTP结合蛋白rho在肌动蛋白微丝组装调控中作用的嵌合毒素。
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