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N-连接糖基化对于膜结合转录因子 CREB-H 的最佳蛋白水解激活是必需的。

N-linked glycosylation is required for optimal proteolytic activation of membrane-bound transcription factor CREB-H.

机构信息

Department of Biochemistry, The University of Hong Kong, Faculty of Medicine Building, 21 Sassoon Road, Pokfulam, Hong Kong.

出版信息

J Cell Sci. 2010 May 1;123(Pt 9):1438-48. doi: 10.1242/jcs.067819. Epub 2010 Mar 31.

Abstract

CREB-H is a liver-enriched bZIP transcription factor of the CREB3 subfamily. CREB-H is activated by intramembrane proteolysis that removes a C-terminal transmembrane domain. Aberrant expression of CREB-H is implicated in liver cancer. In this study we characterized N-linked glycosylation of CREB-H in the luminal domain at the C-terminus. We found that CREB-H is modified at three N-linked glycosylation sites in this region. Disruption of all three sites by site-directed mutagenesis completely abrogated N-linked glycosylation of CREB-H. The unglycosylated mutant of CREB-H was not unstable, unfolded or aggregated. Upon stimulation with an activator of intramembrane proteolysis such as brefeldin A and KDEL-tailed site 1 protease, unglycosylated or deglycosylated CREB-H was largely uncleaved, retained in an inactive form in the endoplasmic reticulum, and less capable of activating transcription driven by unfolded protein response element or C-reactive protein promoter. Taken together, our findings suggest that N-linked glycosylation is required for full activation of CREB-H through intramembrane proteolysis. Our work also reveals a novel mechanism for the regulation of CREB-H-dependent transcription.

摘要

CREB-H 是 CREB3 亚家族中一种富含亮氨酸的 bZIP 转录因子。CREB-H 通过跨膜结构域的内切割被激活。异常表达的 CREB-H 与肝癌有关。在本研究中,我们对 CREB-H 在 C 末端的胞浆区的 N 连接糖基化进行了特征描述。我们发现 CREB-H 在该区域的三个 N 连接糖基化位点发生了修饰。通过定点突变破坏这三个位点完全阻断了 CREB-H 的 N 连接糖基化。CREB-H 的未糖基化突变体是稳定的,没有发生错误折叠或聚集。用跨膜蛋白酶的激活剂(如布雷菲德菌素 A 和 KDEL 尾蛋白酶 1)刺激后,未糖基化或去糖基化的 CREB-H 大部分未被切割,以无活性形式保留在内质网中,激活由未折叠蛋白反应元件或 C 反应蛋白启动子驱动的转录的能力降低。总之,我们的研究结果表明,N 连接糖基化是 CREB-H 通过跨膜蛋白酶解充分激活所必需的。我们的工作还揭示了 CREB-H 依赖性转录调控的新机制。

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