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一种新型的蛋白精氨酸甲基转移酶 1(PRMT1)剪接异构体,缺乏二聚化臂,并与细胞恶性相关。

A novel splicing isoform of protein arginine methyltransferase 1 (PRMT1) that lacks the dimerization arm and correlates with cellular malignancy.

机构信息

Institute of Molecular Biology and Biotechnology (IMBB-FORTH), Laboratory for Epigenetics and Chromosome Biology, Ioannina, Greece.

Cardiothoracic Pharmacology, National Heart and Lung Institute, Imperial College, London, UK.

出版信息

J Cell Biochem. 2018 Feb;119(2):2110-2123. doi: 10.1002/jcb.26373. Epub 2017 Oct 18.

DOI:10.1002/jcb.26373
PMID:28857308
Abstract

Methylation of arginine residues is an important modulator of protein function that is involved in epigenetic gene regulation, DNA damage response and RNA maturation, as well as in cellular signaling. The enzymes that catalyze this post-translational modification are called protein arginine methyltransferases (PRMTs), of which PRMT1 is the predominant enzyme. Human PRMT1 has previously been shown to occur in seven splicing isoforms, which are differentially abundant in different tissues, and have distinct substrate specificity and intracellular localization. Here we characterize a novel splicing isoform which does not affect the amino-terminus of the protein like the seven known isoforms, but rather lacks exons 8 and 9 which encode the dimerization arm of the enzyme that is essential for enzymatic activity. Consequently, the isoform does not form catalytically active oligomers with the other endogenous PRMT1 isoforms. Photobleaching experiments reveal an immobile fraction of the enzyme in the nucleus, in accordance with earlier results from our laboratory that had shown a tight association of inhibited or inactivated PRMT1 with chromatin and the nuclear scaffold. Thus, it apparently is able to bind to the same substrates as catalytically active PRMT1. This isoform is found in a variety of cell lines, but is increased in those of cancer origin or after expression of the EMT-inducing transcriptional repressor Snail1. We discuss that the novel isoform could act as a modulator of PRMT1 activity in cancer cells by acting as a competitive inhibitor that shields substrates from access to active PRMT1 oligomers.

摘要

精氨酸残基的甲基化是蛋白质功能的一个重要调节因子,涉及表观遗传基因调控、DNA 损伤反应和 RNA 成熟,以及细胞信号转导。催化这种翻译后修饰的酶称为蛋白质精氨酸甲基转移酶(PRMTs),其中 PRMT1 是主要的酶。先前已经表明,人类 PRMT1 存在七种剪接异构体,它们在不同组织中的丰度不同,并且具有不同的底物特异性和细胞内定位。在这里,我们描述了一种新的剪接异构体,它不像已知的七种异构体那样影响蛋白质的氨基末端,而是缺乏编码酶二聚化臂的外显子 8 和 9,而酶二聚化臂对于酶活性是必需的。因此,该异构体不会与其他内源性 PRMT1 异构体形成催化活性的寡聚体。光漂白实验揭示了核内酶的不可移动部分,与我们实验室的早期结果一致,该结果表明抑制或失活的 PRMT1 与染色质和核支架紧密结合。因此,它显然能够与催化活性的 PRMT1 结合相同的底物。这种异构体存在于多种细胞系中,但在源自癌症的细胞系或表达 EMT 诱导转录抑制因子 Snail1 后增加。我们讨论了新型异构体可以通过作为竞争性抑制剂来调节癌细胞中 PRMT1 的活性,该抑制剂可以保护底物免受与活性 PRMT1 寡聚体的接触。

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