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Quality Control Autophagy Degrades Soluble ERAD-Resistant Conformers of the Misfolded Membrane Protein GnRHR

机译:质量控制自噬降解膜折叠蛋白GnRHR的可溶性抗ERAD构象异构体。

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Molecular chaperones triage misfolded proteins via action as substrate selectors for quality control (QC) machines that fold or degrade clients. Herein, the endoplasmic reticulum (ER)-associated Hsp40 JB12 is reported to participate in partitioning mutant conformers of gonadotropin-releasing hormone receptor (GnRHR), a G protein-coupled receptor, between ER-associated degradation (ERAD) and an ERQC autophagy pathway. ERQC autophagy degrades E90K-GnRHR because pools of its partially folded and detergent-soluble degradation intermediates are resistant to ERAD. S168R-GnRHR is globally misfolded and disposed of via ERAD, but inhibition of p97, the protein retrotranslocation motor, shunts S168R-GnRHR from ERAD to ERQC autophagy. Partially folded and grossly misfolded forms of GnRHR associate with JB12 and Hsp70. Elevation of JB12 promotes ERAD of S168R-GnRHR, with E90K-GnRHR being resistant. E90K-GnRHR elicits association of the Vps34 autophagy initiation complex with JB12. Interaction between ER-associated Hsp40s and the Vps34 complex permits the selective degradation of ERAD-resistant membrane proteins via ERQC autophagy.
机译:分子伴侣分子通过作为折叠或降解客户的质量控制(QC)机器的底物选择剂,对错误折叠的蛋白质进行分类。在此,据报道内质网(ER)相关的Hsp40 JB12参与ER相关降解(ERAD)和ERQC自噬途径之间的促性腺激素释放激素受体(GnRHR)(一种G蛋白偶联受体)的突变构象体的分配。 。 ERQC自噬可降解E90K-GnRHR,因为其部分折叠且可溶于洗涤剂的降解中间产物池对ERAD具有抗性。 S168R-GnRHR在全球被错误折叠并通过ERAD进行处理,但是对蛋白逆转马达p97的抑制将S168R-GnRHR从ERAD分流到ERQC自噬。 GnRHR的部分折叠和严重错误折叠形式与JB12和Hsp70相关。 JB12的升高可促进S168R-GnRHR的ERAD,而E90K-GnRHR具有抗性。 E90K-GnRHR引发Vps34自噬起始复合物与JB12的关联。 ER相关的Hsp40与Vps34复合物之间的相互作用允许通过ERQC自噬选择性降解ERAD抗性膜蛋白。

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