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跨膜蛋白通过糖基化序列的胞浆内向胞腔逆行转位的拓扑调节。

Topological regulation of a transmembrane protein by luminal-to-cytosolic retrotranslocation of glycosylated sequence.

机构信息

Department of Molecular Genetics, University of Texas Southwestern Medical Center, Dallas, TX 75390, USA.

Department of Molecular Genetics, University of Texas Southwestern Medical Center, Dallas, TX 75390, USA.

出版信息

Cell Rep. 2023 Apr 25;42(4):112311. doi: 10.1016/j.celrep.2023.112311. Epub 2023 Mar 26.

Abstract

Transmembrane proteins must adopt proper topology to perform their functions. We previously demonstrated that ceramide regulates TM4SF20 (transmembrane 4 L6 family 20) by altering the topology of the transmembrane protein, but the underlying mechanism remains obscure. Here we report that TM4SF20 is synthesized in the endoplasmic reticulum (ER) with a cytosolic C terminus and a luminal loop before the last transmembrane helix where N132, N148, and N163 are glycosylated. In the absence of ceramide, the sequence surrounding glycosylated N163 but not N132 is retrotranslocated from lumen to cytosol independent of ER-associated degradation. Accompanying this retrotranslocation, the C terminus of the protein is relocated from cytosol to lumen. Ceramide delays the retrotranslocation process, causing accumulation of the protein that is originally synthesized. Our findings suggest that N-linked glycans, although synthesized in the lumens, may be exposed to cytosol through retrotranslocation, a reaction that may play a crucial role in topological regulation of transmembrane proteins.

摘要

跨膜蛋白必须采用适当的拓扑结构来发挥其功能。我们之前证明,神经酰胺通过改变跨膜蛋白的拓扑结构来调节 TM4SF20(跨膜 4 L6 家族 20),但其潜在机制尚不清楚。在这里,我们报告 TM4SF20 在合成时,内质网(ER)中的细胞质 C 末端和跨膜螺旋 13 之前的腔环,在该位置 N132、N148 和 N163 发生糖基化。在没有神经酰胺的情况下,围绕糖基化 N163 但不是 N132 的序列会独立于 ER 相关降解从腔到细胞质反向转位。伴随着这种反向转位,蛋白质的 C 末端从细胞质重新定位到腔中。神经酰胺会延迟反向转位过程,导致原本合成的蛋白质积累。我们的发现表明,尽管 N 连接的糖基化在腔中合成,但可能通过反向转位暴露于细胞质中,这种反应可能在跨膜蛋白拓扑调节中发挥关键作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0d88/10520219/c0629356e30d/nihms-1895575-f0002.jpg

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