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Identification of rab20 as a Potential Regulator of Connexin43 Trafficking

机译:鉴定rab20作为Connexin43贩运的潜在调节剂

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Connexin oligomerization and trafficking are regulated processes. To identify proteins that control connexin43 (Cx43), a screen was designed using HeLa cells expressing a Cx43 construct with di-lysine endoplasmic reticulum (ER)-retention/retrieval motif, Cx43-HKKSL. At moderate levels of expression, Cx43-HKKSL is retained in the ER as monomers; however, Cx43-HKKSL stably overexpressed by HeLa cells localizes to the perinuclear region and oligomerizes. HeLa/Cx43-HKKSL overexpressors were transiently transfected with pooled clones from a human kidney cDNA library and used immunofluorescence microscopy to identify cDNAs that enabled overexpressed Cx43-HKKSL to convert from a perinuclear to ER localization pattern. Using this approach, a small molecular weight GTPase, rab20, was identified as a candidate protein with the ability to regulate Cx43 trafficking. Enhanced green florescent protein (EGFP)-tagged rab20 showed a predominantly perinuclear and ER localization pattern and caused wild-type Cx43 to be retained inside the cell. By contrast, mutant EGFP-rab20T19N, which lacks the ability to bind GTP, had no effect on Cx43. These results suggest Cx43 is transported through an intracellular compartment regulated by rab20 along the secretory pathway.
机译:连接蛋白的低聚和运输是受调控的过程。为了鉴定控制连接蛋白43(Cx43)的蛋白质,设计了使用表达具有双赖氨酸内质网(ER)保留/检索基序Cx43-HKKSL的Cx43构建体的HeLa细胞进行筛选的方法。在中等表达水平下,Cx43-HKKSL作为单体保留在ER中。但是,HeLa细胞稳定过度表达的Cx43-HKKSL定位于核周区域并寡聚。用来自人肾脏cDNA文库的合并克隆瞬时转染HeLa / Cx43-HKKSL过表达子,并使用免疫荧光显微镜鉴定能够使过表达的Cx43-HKKSL从核周定位模式转变为ER定位模式的cDNA。使用这种方法,小分子量的GTP酶rab20被鉴定为具有调节Cx43转运能力的候选蛋白。增强型绿色荧光蛋白(EGFP)标签的rab20显示主要为核周和ER定位模式,并导致野生型Cx43保留在细胞内。相比之下,缺乏结合GTP能力的突变EGFP-rab20T19N对Cx43没有影响。这些结果表明,Cx43沿分泌途径通过rab20调节的细胞内区室转运。

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