Chemically Induced Nuclear Pore Complex Protein Degradation via TRIM21

核孔 降级(电信) 化学 核蛋白 细胞生物学 生物物理学 泛素 生物化学 计算机科学 生物 转录因子 细胞质 电信 基因
作者
Xiaomei Li,Qingyang Wang,Anping Guo,Yaping Qiu,Qiuxia Chen,You Li,Lanjun Zhang,Yaxin Guo,Xiaoyun Meng,Shiqian Li,Guizhi Liu,Liyun Zhang,J. Liu,Xin Li,Longying Cai,Xuemin Cheng,Chuan Liu,Xiaotao Wang,Andrew Wood,James B. Murray
出处
期刊:ACS Chemical Biology [American Chemical Society]
标识
DOI:10.1021/acschembio.4c00833
摘要

Despite the exciting progress of bifunctional degrader molecules, also known as proteolysis-targeting chimeras (PROTACs), the rapidly expanding field is still significantly hampered by the lack of available E3 ligase ligands. Our research bridges this gap by uncovering a series of small-molecule ligands to the E3 ligase TRIM21 through DNA-Encoded Library (DEL) technology. We confirmed their interaction with TRIM21 using crystallography and demonstrated their antiproliferative effects across various cancer cell types. Furthermore, proteomic studies identified that the mRNA Export Factor GLE1 and the Nuclear Pore Complex Protein NUP155 were significantly downregulated on TRIM21 ligand treatment. This degradation required TRIM21 and was ubiquitin-proteasome-dependent. More specifically, NUP155 was the primary target for the TRIM21 ligands, while GLE1 was considered a passenger target on initial degradation of NUP155. Using immunofluorescence techniques, we further demonstrated that the degradation of GLE1 and NUP155 proteins impaired the integrity of the nuclear envelope, leading to cell death. Highlighted by this research, a novel mode of action has been discovered for the TRIM21 E3 ligase ligand, acting as a monovalent degrader that triggers de novo interaction with functional complex proteins and induces their degradation.
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