解码多泛素对 KV7.1 功能表达的调控1 的功能性表达

bioRxiv - Molecular Biology Pub Date : 2024-09-17 DOI:10.1101/2024.09.17.613539

Sri Karthika Shanmugam, Scott A Kanner, Xinle M Zou, Enoch Amarh, Papiya Choudhury, Rajesh SONI, Robert S Kass, Henry M Colecraft

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引用次数: 0

摘要

蛋白质通过不同的多泛素连接链进行翻译后修饰是泛素密码的重要组成部分，泛素密码普遍调节蛋白质的表达和功能，从而控制生物学。由于缺乏在活细胞中特异性调节单个蛋白质上多泛素连接的方法，研究进展受阻。在这里，我们利用对水解不同多泛素连接具有偏好的去泛素酶（DUBs）来弥补这一差距：OTUD1--K63；OTUD4--K48；Cezanne--K11；TRABID--K29/K33；USP21--非特异性。我们开发了一套由 DUB 催化结构域与 GFP 靶向纳米抗体融合而成的工程化去泛素化酶（enDUBs），并用它们来研究离子通道 YFP-KCNQ1 的多泛素连接调控。在 HEK293 细胞中表达的 YFP-KCNQ1 的质谱分析表明，通道多泛素化以 K48（72%）和 K63（24%）连接为主。NEDD4-2 和 ITCH 都会降低 KCNQ1 的功能表达，但具有独特的多泛素化特征。所有 enDUBs 都减少了 KCNQ1 泛素化，但对通道表达、表面密度、离子电流和亚细胞定位产生了独特的影响。结果表明，K11、K29/K33 和 K63 链介导了 KCNQ1-YFP 在细胞内的净保留，但实现的方式不同：K11 促进 ER 保留/降解，增强内吞，减少再循环；K29/K33 促进 ER 保留/降解；K63 增强内吞，减少再循环。enDUB对KCNQ1-YFP的影响模式在心肌细胞中有所不同，这强调了泛素编码的可变性。令人惊讶的是，enDUB-O4降低了KCNQ1-YFP的表面密度，这表明K48在前向转运中的作用。最后，连接选择性 enDUB 在挽救不同的转运缺陷长 QT 综合征 1 型突变方面表现出不同的能力。这些结果揭示了不同的多泛素链控制着 KCNQ1 功能表达的不同方面，证明了泛素密码的可塑性，并将连接选择性 enDUBs 作为一种有效的工具来帮助揭开多泛素密码的神秘面纱。

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Decoding polyubiquitin regulation of KV7. 1 functional expression with engineered linkage-selective deubiquitinases

Protein posttranslational modification with distinct polyubiquitin linkage chains is a critical component of the ubiquitin code that universally regulates protein expression and function to control biology. Functional consequences of diverse polyubiquitin linkages on proteins are mostly unknown, with progress hindered by a lack of methods to specifically tune polyubiquitin linkages on individual proteins in live cells. Here, we bridge this gap by exploiting deubiquitinases (DUBs) with preferences for hydrolyzing different polyubiquitin linkages: OTUD1 - K63; OTUD4 - K48; Cezanne - K11; TRABID - K29/K33; and USP21 - non-specific. We developed a suite of engineered deubiquitinases (enDUBs) comprised of DUB catalytic domains fused to a GFP-targeted nanobody and used them to investigate polyubiquitin linkage regulation of an ion channel, YFP-KCNQ1. Mass spectrometry of YFP-KCNQ1 expressed in HEK293 cells indicated channel polyubiquitination with K48 (72%) and K63 (24%) linkages being dominant. NEDD4-2 and ITCH both decreased KCNQ1 functional expression but with distinctive polyubiquitination signatures. All enDUBs reduced KCNQ1 ubiquitination but yielded unique effects on channel expression, surface density, ionic currents, and subcellular localization. The pattern of outcomes indicates K11, K29/K33, and K63 chains mediate net KCNQ1-YFP intracellular retention, but achieved in different ways: K11 promotes ER retention/degradation, enhances endocytosis, and reduces recycling; K29/K33 promotes ER retention/degradation; K63 enhances endocytosis and reduces recycling. The pattern of enDUB effects on KCNQ1-YFP differed in cardiomyocytes, emphasizing ubiquitin code mutability. Surprisingly, enDUB-O4 decreased KCNQ1-YFP surface density suggesting a role for K48 in forward trafficking. Lastly, linkage-selective enDUBs displayed varying capabilities to rescue distinct trafficking-deficient long QT syndrome type 1 mutations. The results reveal distinct polyubiquitin chains control different aspects of KCNQ1 functional expression, demonstrate ubiquitin code plasticity, and introduce linkage-selective enDUBs as a potent tool to help demystify the polyubiquitin code.

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bioRxiv - Molecular Biology

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