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EDEM1 reveals a quality control vesicular transport pathway out of the endoplasmic reticulum not involving the COPII exit sites

机译:EDEM1揭示了不涉及COPII出口位点的从内质网流出的质量控制囊泡运输途径

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Immature and normative proteins are retained in the endoplasmic reticulum (ER) by the quality control machinery. Folding-incompetent glycoproteins are eventually targeted for ER-associated protein degradation (ERAD). EDEM1 (ER degradation-enhancing α-mannosidase-like protein 1), a putative mannose-binding protein, targets misfolded glycoproteins for ERAD. We report that endogenous EDEM1 exists mainly as a soluble glycoprotein. By high-resolution immunolabeling and serial section analysis, we find that endogenous EDEM1 is sequestered in buds that form along cisternae of the rough ER at regions outside of the transitional ER. They give rise to ≈150-nm vesicles scattered throughout the cytoplasm that are lacking a recognizable COPII coat. About 87% of the immunogold labeling was over the vesicles and ≈11% over the ER lumen. Some of the EDEM1 vesicles also contain Derlin-2 and the misfolded Hong Kong variant of α-1-antitrypsin, a substrate for EDEM1 and ERAD. Our results demonstrate the existence of a vesicle budding transport pathway out of the rough ER that does not involve the canonical transitional ER exit sites and therefore represents a previously unrecognized passageway to remove potentially harmful misfolded luminal glycoproteins from the ER.
机译:未成熟的和正常的蛋白质通过质量控制机制保留在内质网(ER)中。折叠功能不全的糖蛋白最终靶向ER相关蛋白降解(ERAD)。 EDEM1(增强ER降解的α-甘露糖苷酶样蛋白1)是一种推定的甘露糖结合蛋白,可靶向ERAD折叠错误的糖蛋白。我们报告内源性EDEM1主要存在为可溶性糖蛋白。通过高分辨率的免疫标记和连续切片分析,我们发现内源性EDEM1被隔离在沿过渡ER外部区域沿粗糙ER的水箱形成的芽中。它们会产生大约150 nm的囊泡,这些囊泡散布在整个细胞质中,缺少可识别的COPII涂层。约87%的免疫金标记位于囊泡上方,约ER内腔约占11%。某些EDEM1囊泡还含有Derlin-2和错误折叠的α-1-抗胰蛋白酶的香港变体,α-1-抗胰蛋白酶是EDEM1和ERAD的底物。我们的结果表明存在从粗糙的ER囊泡出芽的运输途径,不涉及规范的过渡性ER出口位点,因此代表了以前无法识别的从ER去除潜在有害的折叠错误的腔糖蛋白的通道。

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