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枢纽蛋白 DYNLL1 和 bZIP 转录因子 CREB3L1 的二聚化增强了 CREB3L1 靶基因如精氨酸加压素的转录激活。

Dimerization of hub protein DYNLL1 and bZIP transcription factor CREB3L1 enhances transcriptional activation of CREB3L1 target genes like arginine vasopressin.

机构信息

Molecular Neuroendocrinology Research Group, Bristol Medical School: Translational Health Sciences, University of Bristol, Dorothy Hodgkin Building, Bristol, United Kingdom.

Molecular Neuroendocrinology Research Group, Bristol Medical School: Translational Health Sciences, University of Bristol, Dorothy Hodgkin Building, Bristol, United Kingdom.

出版信息

Peptides. 2024 Sep;179:171269. doi: 10.1016/j.peptides.2024.171269. Epub 2024 Jul 2.

DOI:10.1016/j.peptides.2024.171269
PMID:38960286
Abstract

bZIP transcription factors can function as homodimers or heterodimers through interactions with their disordered coiled-coil domain. Such dimer assemblies are known to influence DNA-binding specificity and/or the recruitment of binding partners, which can cause a functional switch of a transcription factor from being an activator to a repressor. We recently identified the genomic targets of a bZIP transcription factor called CREB3L1 in rat hypothalamic supraoptic nucleus by ChIP-seq. The objective of this study was to investigate the CREB3L1 protein-to-protein interactome of which little is known. For this approach, we created and screened a rat supraoptic nucleus yeast two-hybrid prey library with the bZIP region of rat CREB3L1 as the bait. Our yeast two-hybrid approach captured five putative CREB3L1 interacting prey proteins in the supraoptic nucleus. One interactor was selected by bioinformatic analyses for more detailed investigation by co-immunoprecipitation, immunofluorescent cellular localisation, and reporter assays in vitro. Here we identify dimerisation hub protein Dynein Light Chain LC8-Type 1 as a CREB3L1 interacting protein that in vitro enhances CREB3L1 activation of target genes.

摘要

bZIP 转录因子可以通过与它们的无序卷曲螺旋域相互作用形成同源二聚体或异源二聚体。这种二聚体组装已知会影响 DNA 结合特异性和/或结合伙伴的募集,从而导致转录因子从激活剂到抑制剂的功能转换。我们最近通过 ChIP-seq 鉴定了大鼠下丘脑视上核中一种称为 CREB3L1 的 bZIP 转录因子的基因组靶标。本研究的目的是研究 CREB3L1 蛋白-蛋白相互作用组,对此知之甚少。为此,我们使用大鼠 CREB3L1 的 bZIP 区域作为诱饵,创建并筛选了大鼠视上核酵母双杂交诱饵文库。我们的酵母双杂交方法在视上核中捕获了五个推定的 CREB3L1 相互作用的猎物蛋白。通过生物信息学分析选择了一个相互作用体,通过共免疫沉淀、免疫荧光细胞定位和体外报告基因测定进行更详细的研究。在这里,我们确定了动力蛋白轻链 LC8 型 1 作为 CREB3L1 相互作用蛋白的二聚化中心,该蛋白在体外增强了 CREB3L1 对靶基因的激活。

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