Dynein Light Intermediate Chains Exhibit Different Arginine Methylation Patterns

IF 2.6 4区医学 Q2 MEDICAL LABORATORY TECHNOLOGY Journal of Clinical Laboratory Analysis Pub Date : 2024-03-25 DOI:10.1002/jcla.25030

Weiwen Bu, Jie Di, Junkui Zhao, Ruming Liu, Yue Wu, Jie Ran, Te Li

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Abstract

Background

The motor protein dynein is integral to retrograde transport along microtubules and interacts with numerous cargoes through the recruitment of cargo-specific adaptor proteins. This interaction is mediated by dynein light intermediate chain subunits LIC1 (DYNC1LI1) and LIC2 (DYNC1LI2), which govern the adaptor binding and are present in distinct dynein complexes with overlapping and unique functions.

Methods

Using bioinformatics, we analyzed the C-terminal domains (CTDs) of LIC1 and LIC2, revealing similar structural features but diverse post-translational modifications (PTMs). The methylation status of LIC2 and the proteins involved in this modification were examined through immunoprecipitation and immunoblotting analyses. The specific methylation sites on LIC2 were identified through a site-directed mutagenesis analysis, contributing to a deeper understanding of the regulatory mechanisms of the dynein complex.

Results

We found that LIC2 is specifically methylated at the arginine 397 residue, a reaction that is catalyzed by protein arginine methyltransferase 1 (PRMT1).

Conclusions

The distinct PTMs of the LIC subunits offer a versatile mechanism for dynein to transport diverse cargoes efficiently. Understanding how these PTMs influence the functions of LIC2, and how they differ from LIC1, is crucial for elucidating the role of dynein-related transport pathways in a range of diseases. The discovery of the arginine 397 methylation site on LIC2 enhances our insight into the regulatory PTMs of dynein functions.

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Dynein轻中间链表现出不同的精氨酸甲基化模式

背景：运动蛋白动力蛋白（dynein）是沿微管逆向运输不可或缺的部分，它通过招募货物特异性适配蛋白与许多货物相互作用。这种相互作用由动力蛋白轻中间链亚基 LIC1（DYNC1LI1）和 LIC2（DYNC1LI2）介导，它们控制适配体的结合，存在于不同的动力蛋白复合物中，具有重叠和独特的功能：我们利用生物信息学方法分析了 LIC1 和 LIC2 的 C 端结构域（CTD），发现它们具有相似的结构特征，但翻译后修饰（PTM）却各不相同。通过免疫沉淀和免疫印迹分析研究了LIC2的甲基化状态以及参与这种修饰的蛋白质。通过定点突变分析确定了 LIC2 上的特定甲基化位点，有助于加深对动力蛋白复合体调控机制的理解：结果：我们发现 LIC2 在精氨酸 397 残基上被特异性甲基化，该反应由蛋白精氨酸甲基转移酶 1（PRMT1）催化：结论：LIC 亚基的不同 PTM 为动力蛋白高效运输各种货物提供了一种多功能机制。了解这些 PTM 如何影响 LIC2 的功能，以及它们与 LIC1 的区别，对于阐明与动力蛋白相关的转运途径在一系列疾病中的作用至关重要。LIC2 上精氨酸 397 甲基化位点的发现增强了我们对动力蛋白功能调控 PTM 的洞察力。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Journal of Clinical Laboratory Analysis 医学-医学实验技术

CiteScore

5.60

自引率

7.40%

发文量

584

审稿时长

6-12 weeks

期刊介绍： Journal of Clinical Laboratory Analysis publishes original articles on newly developing modes of technology and laboratory assays, with emphasis on their application in current and future clinical laboratory testing. This includes reports from the following fields: immunochemistry and toxicology, hematology and hematopathology, immunopathology, molecular diagnostics, microbiology, genetic testing, immunohematology, and clinical chemistry.