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RAB26 和 RAB3D 是 MIST1 的直接转录靶标,可调节外分泌颗粒成熟。

RAB26 and RAB3D are direct transcriptional targets of MIST1 that regulate exocrine granule maturation.

机构信息

Department of Pathology and Immunology, Washington University School of Medicine, Box 8118, 660 S. Euclid Ave., St. Louis, MO 63110, USA.

出版信息

Mol Cell Biol. 2010 Mar;30(5):1269-84. doi: 10.1128/MCB.01328-09. Epub 2009 Dec 28.

DOI:10.1128/MCB.01328-09
PMID:20038531
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2820885/
Abstract

Little is known about how differentiating cells reorganize their cellular structure to perform specialized physiological functions. MIST1, an evolutionarily conserved transcription factor, is required for the formation of large, specialized secretory vesicles in gastric zymogenic (chief) cells (ZCs) as they differentiate from their mucous neck cell progenitors. Here, we show that MIST1 binds to highly conserved CATATG E-boxes to directly activate transcription of 6 genes, including those encoding the small GTPases RAB26 and RAB3D. We next show that RAB26 and RAB3D expression is significantly downregulated in Mist1(-)(/)(-) ZCs, suggesting that MIST1 establishes large secretory granules by inducing RAB transcription. To test this hypothesis, we transfected human gastric cancer cell lines stably expressing MIST1 with red fluorescent protein (RFP)-tagged pepsinogen C, a key secretory product of ZCs. Those cells upregulate expression of RAB26 and RAB3D to form large secretory granules, whereas control, non-MIST1-expressing cells do not. Moreover, granule formation in MIST1-expressing cells requires RAB activity because treatment with a RAB prenylation inhibitor and transfection of dominant negative RAB26 abrogate granule formation. Together, our data establish the molecular process by which a transcription factor can directly induce fundamental cellular architecture changes by increasing transcription of specific cellular effectors that act to organize a unique subcellular compartment.

摘要

关于分化细胞如何重组其细胞结构以执行专门的生理功能,人们知之甚少。MIST1 是一种进化上保守的转录因子,它是胃酶原(主)细胞(ZCs)从其粘液颈细胞前体分化时形成大型专门分泌小泡所必需的。在这里,我们表明 MIST1 结合高度保守的 CATATG E 盒,直接激活包括编码小 GTPase RAB26 和 RAB3D 的 6 个基因的转录。接下来,我们表明 Mist1(-)(/)(-) ZCs 中 RAB26 和 RAB3D 的表达显著下调,这表明 MIST1 通过诱导 RAB 转录来建立大型分泌颗粒。为了验证这一假说,我们用红色荧光蛋白(RFP)标记的胃蛋白酶原 C 转染稳定表达 MIST1 的人胃癌细胞系。这些细胞上调 RAB26 和 RAB3D 的表达,形成大型分泌颗粒,而对照的非 MIST1 表达细胞则没有。此外,MIST1 表达细胞中的颗粒形成需要 RAB 活性,因为 RAB prenylation 抑制剂处理和显性负 RAB26 转染会破坏颗粒形成。总之,我们的数据确立了一种分子过程,即转录因子可以通过增加特定细胞效应物的转录,直接诱导基本的细胞结构变化,这些细胞效应物作用于组织独特的亚细胞隔室。

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