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单体GTP酶Rab35调节吞噬杯的形成以及吞噬体的成熟。

The Monomeric GTPase Rab35 Regulates Phagocytic Cup Formation and Phagosomal Maturation in .

作者信息

Verma Kuldeep, Datta Sunando

机构信息

From the Department of Biological Science, Indian Institute of Science Education and Research Bhopal, Bhopal Bypass Road, Bhauri 462030, India.

From the Department of Biological Science, Indian Institute of Science Education and Research Bhopal, Bhopal Bypass Road, Bhauri 462030, India

出版信息

J Biol Chem. 2017 Mar 24;292(12):4960-4975. doi: 10.1074/jbc.M117.775007. Epub 2017 Jan 26.

Abstract

One of the hallmarks of amoebic colitis is the detection of (Eh) trophozoites with ingested erythrocytes. Therefore, erythrophagocytosis is traditionally considered as one of the most important criteria to identify the pathogenic behavior of the amoebic trophozoites. Phagocytosis is an essential process for the proliferation and virulence of this parasite. Phagocytic cargo, upon internalization, follows a defined trafficking route to amoebic lysosomal degradation machinery. Here, we demonstrated the role of EhRab35 in the early and late phases of erythrophagocytosis by the amoeba. EhRab35 showed large vacuolar as well as punctate vesicular localization. The spatiotemporal dynamics of vacuolar EhRab35 and its exchange with soluble cytosolic pool were monitored by fluorescence recovery after photobleaching experiments. Using extensive microscopy and biochemical methods, we demonstrated that upon incubation with RBCs EhRab35 is recruited to the site of phagocytic cups as well as to the nascent phagosomes that harbor Gal/GalNAc lectin and actin. Overexpression of a dominant negative mutant of EhRab35 reduced phagocytic cup formation and thereby reduced RBC internalization, suggesting a potential role of the Rab GTPase in the cup formation. Furthermore, we also performed a phagosomal maturation assay and observed that the activated form of EhRab35 significantly increased the rate of RBC degradation. Interestingly, this mutant also significantly enhanced the number of acidic compartments in the trophozoites. Taken together, our results suggest that EhRab35 is involved in the initial stage of phagocytosis as well as in the phagolysosomal biogenesis in and thus contributes to the pathogenicity of the parasite.

摘要

阿米巴结肠炎的一个标志是检测到含有吞噬红细胞的(Eh)滋养体。因此,吞噬红细胞传统上被认为是识别阿米巴滋养体致病行为的最重要标准之一。吞噬作用是这种寄生虫增殖和致病力的一个重要过程。吞噬的物质内化后,会沿着特定的运输途径到达阿米巴溶酶体降解机制。在这里,我们展示了EhRab35在阿米巴吞噬红细胞早期和晚期阶段的作用。EhRab35表现出大泡状以及点状小泡定位。通过光漂白后荧光恢复实验监测泡状EhRab35的时空动态及其与可溶性胞质池的交换。使用广泛的显微镜和生化方法,我们证明与红细胞孵育后,EhRab35被募集到吞噬杯位点以及含有半乳糖/ N - 乙酰半乳糖胺凝集素和肌动蛋白的新生吞噬体。EhRab35显性负突变体的过表达减少了吞噬杯的形成,从而减少了红细胞的内化,表明Rab GTP酶在吞噬杯形成中具有潜在作用。此外,我们还进行了吞噬体成熟分析,观察到激活形式的EhRab35显著提高了红细胞降解率。有趣的是,该突变体还显著增加了滋养体中酸性区室的数量。综上所述,我们的结果表明EhRab35参与吞噬作用的初始阶段以及在Eh中的吞噬溶酶体生物发生,因此有助于寄生虫的致病性。

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