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Rab13 在破骨细胞分化过程中上调,并与小泡相关联,在吸收细胞中呈现出极化分布。

Rab13 is upregulated during osteoclast differentiation and associates with small vesicles revealing polarized distribution in resorbing cells.

机构信息

Department of Cell Biology and Anatomy, Institute of Biomedicine, University of Turku, Turku, Finland.

出版信息

J Histochem Cytochem. 2012 Jul;60(7):537-49. doi: 10.1369/0022155412448069. Epub 2012 May 4.

Abstract

Osteoclasts are bone-resorbing multinucleated cells that undergo drastic changes in their polarization due to heavy vesicular trafficking during the resorption cycle. These events require the precise orchestration of membrane traffic in order to maintain the unique characteristics of the different membrane domains in osteoclasts. Rab proteins are small GTPases involved in regulation of most, if not all, steps of vesicle trafficking. The investigators studied RAB genes in human osteoclasts and found that at least 26 RABs were expressed in osteoclasts. Out of these, RAB13 gene expression was highly upregulated during differentiation of human peripheral blood monocytic cells into osteoclasts. To study its possible function in osteoclasts, the investigators performed immunolocalization studies for Rab13 and various known markers of osteoclast vesicular trafficking. Rab13 localized to small vesicular structures at the superior parts of the osteoclast between the trans-Golgi network and basolateral membrane domain. Rab13 localization suggests that it is not involved in endocytosis or transcytosis of bone degradation products. In addition, Rab13 did not associate with early endosomes or recycling endosomes labeled with EEA1 or TRITC-conjugated transferrin, respectively. Its involvement in glucose transporter traffic was excluded as well. It is suggested that Rab13 is associated with a putative secretory function in osteoclasts.

摘要

破骨细胞是具有多核的骨吸收细胞,由于在吸收周期中囊泡运输非常活跃,破骨细胞的极化会发生剧烈变化。这些事件需要膜运输的精确协调,以维持破骨细胞中不同膜结构域的独特特征。Rab 蛋白是参与调节囊泡运输的大多数(如果不是全部)步骤的小 GTP 酶。研究人员研究了人类破骨细胞中的 Rab 基因,发现至少有 26 种 Rab 在破骨细胞中表达。在这些基因中,Rab13 基因在人外周血单核细胞分化为破骨细胞的过程中表达高度上调。为了研究其在破骨细胞中的可能功能,研究人员对 Rab13 和各种已知的破骨细胞囊泡运输标志物进行了免疫定位研究。Rab13 定位于破骨细胞上半部分的小囊泡结构,位于高尔基网络和基底外侧膜之间。Rab13 的定位表明它不参与内吞作用或骨降解产物的胞吐作用。此外,Rab13 也不与早期内体或用 EEA1 或 TRITC 缀合转铁蛋白标记的再循环内体结合。它也不参与葡萄糖转运蛋白的运输。这表明 Rab13 与破骨细胞中的一种假定分泌功能有关。

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