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溶组织内阿米巴:功能性Gs和Gi蛋白作为滋养体与纤连蛋白相互作用中可能的信号转导元件的鉴定

Entamoeba histolytica: identification of functional Gs and Gi proteins as possible signal transduction elements in the interaction of trophozoites with fibronectin.

作者信息

Soid-Raggi L G, Torres-Márquez M E, Meza I

机构信息

Departamento de Biología Celular, CINVESTAV del IPN, México, D.F., México.

出版信息

Exp Parasitol. 1998 Nov;90(3):262-9. doi: 10.1006/expr.1998.4333.

DOI:10.1006/expr.1998.4333
PMID:9806871
Abstract

Trophozoites of Entamoeba histolytica adhere to several components of the extracellular matrix. Binding is mediated by specific receptors identified in the parasite surface. Interaction of trophozoites with FN induces the formation of special adhesion structures that are dynamic cytoskeleton membrane complexes and facilitate both adhesion and substrate degradation. The process requires activation of signaling pathways in which PLC, IP3, Ca2-, and PKC participate. These observations, and recent experiments showing increments in cAMP in the trophozoites during the interaction with FN, suggest that FN receptors in the amebic surface could be coupled to G-proteins. We report here that trophozoite plasma membrane peptides of 92, 49, 42, 37, and 21 kDa are ADP-ribosylated by Vibrio cholerae and Bordetella pertussis toxins. Three of them are also recognized by antibodies prepared against the alpha-subunit of Gs-and Gi-proteins. Adenylyl cyclase activity detected in isolated membranes was strongly stimulated by treatment with the toxins. Forskolin (an agonist of the enzyme) and FN also induced increments in the enzymatic activity. Live amebas incubated with the toxins showed enhanced adhesion to FN substrates and a striking reorganization of polymerized actin. The actin rearrangement is reminiscent of the one induced by either forskolin or dibutyril cyclic AMP treatment. Our present data show the presence and the functionality of Gs- and Gi-like proteins and their apparent activation during in vitro interaction of amebas with FN and complement previous observations indicating the operation of signal transduction mechanisms in E. histolytica.

摘要

溶组织内阿米巴滋养体可黏附于细胞外基质的多种成分。这种黏附由寄生虫表面鉴定出的特定受体介导。滋养体与纤连蛋白(FN)的相互作用会诱导形成特殊的黏附结构,这些结构是动态的细胞骨架膜复合物,有助于黏附和底物降解。该过程需要磷脂酶C(PLC)、肌醇三磷酸(IP3)、钙离子(Ca2+)和蛋白激酶C(PKC)参与的信号通路激活。这些观察结果,以及最近显示在与FN相互作用期间滋养体中环磷酸腺苷(cAMP)增加的实验,表明阿米巴表面的FN受体可能与G蛋白偶联。我们在此报告,92 kDa、49 kDa、42 kDa、37 kDa和21 kDa的滋养体质膜肽可被霍乱弧菌和百日咳博德特氏菌毒素进行ADP核糖基化。其中三种还可被针对Gs和Gi蛋白α亚基制备的抗体识别。用毒素处理后,在分离的膜中检测到的腺苷酸环化酶活性受到强烈刺激。福斯可林(该酶的激动剂)和FN也会诱导酶活性增加。用毒素孵育的活阿米巴显示出对FN底物的黏附增强以及聚合肌动蛋白的显著重组。肌动蛋白的重组让人联想到福斯可林或二丁酰环磷腺苷处理所诱导的重组。我们目前的数据显示了Gs和Gi样蛋白的存在及其功能,以及它们在阿米巴与FN体外相互作用期间的明显激活,补充了之前表明溶组织内阿米巴存在信号转导机制的观察结果。

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