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GDI对小GTP酶Rab5的捕获:由p38丝裂原活化蛋白激酶调控

Capture of the small GTPase Rab5 by GDI: regulation by p38 MAP kinase.

作者信息

Felberbaum-Corti Michela, Cavalli Valeria, Gruenberg Jean

出版信息

Methods Enzymol. 2005;403:367-81. doi: 10.1016/S0076-6879(05)03032-6.

Abstract

The small GTPase Rab5 is one of the key regulators of early endocytic traffic and, like other GTPases, cycles between GTP- and GDP-bound states as well as between membrane and cytosol. The latter cycle is controlled by a guanine nucleotide dissociation inhibitor (GDI), which functions as a Rab vehicle in the cytosol. GDI extracts from membranes the inactive GDP-bound form of the Rab. Then, the cytosolic GDI:Rab complex is delivered to the appropriate target membrane, where the Rab protein is reloaded, presumably via a GDI displacement factor (Pfeffer and Aivazian, 2004). We previously reported that the formation of the GDI:Rab5 complex is stimulated by the mitogen-activated protein kinase p38 (Cavalli et al., 2001). Mol. Cell7, 421-432.]. Selective activation of p38 MAPK increases endocytic rates in vivo, presumably allowing more efficient internalization of cell surface components for repair, storage, or degradation. These observations emphasize the possibility that external stimuli contribute to the regulation of membrane traffic. Here, we describe how to monitor the ability of GDI to extract Rab5 from early endosomal membranes in vitro and the role of p38 MAPK in this process. In addition, we detail how to investigate the possible role of p38 MAPK in the regulation of endocytosis in vivo.

摘要

小GTP酶Rab5是早期内吞运输的关键调节因子之一,与其他GTP酶一样,在结合GTP和GDP的状态之间循环,同时也在膜和细胞质之间循环。后一个循环由鸟嘌呤核苷酸解离抑制剂(GDI)控制,GDI在细胞质中作为Rab的载体发挥作用。GDI从膜上提取无活性的结合GDP形式的Rab。然后,细胞质中的GDI:Rab复合物被递送到合适的靶膜,在那里Rab蛋白可能通过GDI置换因子重新装载(Pfeffer和Aivazian,2004年)。我们之前报道过,丝裂原活化蛋白激酶p38可刺激GDI:Rab5复合物的形成(Cavalli等人,2001年)。[《分子细胞》7卷,421 - 432页。]p38 MAPK的选择性激活会在体内提高内吞速率,可能使细胞表面成分能更有效地进行内化以用于修复、储存或降解。这些观察结果强调了外部刺激有助于调节膜运输的可能性。在这里,我们描述如何在体外监测GDI从早期内体膜中提取Rab5的能力以及p38 MAPK在此过程中的作用。此外,我们详细介绍如何研究p38 MAPK在体内调节内吞作用中可能发挥的作用。

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