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LKB1 调控乳腺癌中 PRMT5 的活性。

LKB1 regulates PRMT5 activity in breast cancer.

机构信息

INSERM U1052, Centre de Recherche en Cancérologie de Lyon, Lyon, France.

CNRS UMR5286, Centre de Recherche en Cancérologie de Lyon, Lyon, France.

出版信息

Int J Cancer. 2019 Feb 1;144(3):595-606. doi: 10.1002/ijc.31909. Epub 2018 Oct 31.

Abstract

Protein arginine methyltransferase 5 (PRMT5) is the main enzyme responsible for the symmetrical dimethylation of arginine residues on target proteins in both the cytoplasm and the nucleus. Though its activity has been associated with tumor progression in various cancers, the expression pattern of this oncoprotein has been scarcely studied in breast cancer. In the current work, we analyzed its expression in a large cohort of breast cancer patients, revealing higher nuclear PRMT5 levels in ERα-positive tumors and an association with prolonged disease free and overall survival. Interestingly, high PRMT5 nuclear expression was also associated with higher nuclear liver kinase B1 (LKB1), suggesting that a functional relationship may occur. Consistently, several approaches provided evidence that PRMT5 and LKB1 interact directly in the cytoplasm of mammary epithelial cells. Moreover, although PRMT5 is not able to methylate LKB1, we found that PRMT5 is a bona fade substrate for LKB1. We identified T132, 139 and 144 residues, located in the TIM-Barrel domain of PRMT5, as target sites for LKB1 phosphorylation. The point mutation of PRMT5 T139/144 to A139/144 drastically decreased its methyltransferase activity, due probably to the loss of its interaction with regulatory proteins such as MEP50, pICln and RiOK1. In addition, modulation of LKB1 expression modified PRMT5 activity, highlighting a new regulatory mechanism that could have clinical implications.

摘要

蛋白质精氨酸甲基转移酶 5(PRMT5)是主要的酶,负责细胞质和细胞核中靶蛋白精氨酸残基的对称二甲基化。虽然它的活性与各种癌症的肿瘤进展有关,但这种癌蛋白在乳腺癌中的表达模式研究甚少。在目前的工作中,我们分析了它在一大群乳腺癌患者中的表达情况,揭示了 ERα 阳性肿瘤中核 PRMT5 水平较高,并与无病生存和总生存时间延长有关。有趣的是,高核 PRMT5 表达也与核肝激酶 B1(LKB1)较高有关,表明可能存在功能关系。一致的是,几种方法提供了证据表明 PRMT5 和 LKB1 直接在乳腺上皮细胞的细胞质中相互作用。此外,虽然 PRMT5 不能甲基化 LKB1,但我们发现 PRMT5 是 LKB1 的真正底物。我们确定了位于 PRMT5 TIM-Barrel 结构域中的 T132、139 和 144 位残基是 LKB1 磷酸化的靶位。PRMT5 T139/144 突变为 A139/144 会大大降低其甲基转移酶活性,这可能是由于其与调节蛋白(如 MEP50、pICln 和 RiOK1)的相互作用丧失。此外,调节 LKB1 表达修饰了 PRMT5 活性,突出了一种新的调节机制,可能具有临床意义。

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