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Sculpting ion channel functional expression with engineered ubiquitin ligases

机译:用工程遍在蛋白连接酶雕刻离子通道功能性表达

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摘要

The functional repertoire of surface ion channels is sustained by dynamic processes of trafficking, sorting, and degradation. Dysregulation of these processes underlies diverse ion channelopathies including cardiac arrhythmias and cystic fibrosis. Ubiquitination powerfully regulates multiple steps in the channel lifecycle, yet basic mechanistic understanding is confounded by promiscuity among E3 ligase/substrate interactions and ubiquitin code complexity. Here we targeted the catalytic domain of E3 ligase, CHIP, to YFP-tagged KCNQ1 ± KCNE1 subunits with a GFP-nanobody to selectively manipulate this channel complex in heterologous cells and adult rat cardiomyocytes. Engineered CHIP enhanced KCNQ1 ubiquitination, eliminated KCNQ1 surface-density, and abolished reconstituted K+ currents without affecting protein expression. A chemo-genetic variation enabling chemical control of ubiquitination revealed KCNQ1 surface-density declined with a ~ 3.5 hr t1/2 by impaired forward trafficking. The results illustrate utility of engineered E3 ligases to elucidate mechanisms underlying ubiquitin regulation of membrane proteins, and to achieve effective post-translational functional knockdown of ion channels.
机译:表面离子通道的功能库通过运输,分选和降解的动态过程来维持。这些过程的失调是多种离子通道病变的基础,包括心律不齐和囊性纤维化。泛素化可有效调节通道生命周期中的多个步骤,但基本的机理理解却被E3连接酶/底物相互作用的混杂以及泛素代码的复杂性所困扰。在这里,我们将E3连接酶CHIP的催化结构域靶向带有GFP纳米抗体的YFP标签的KCNQ1±KCNE1亚基,以选择性地操纵异源细胞和成年大鼠心肌细胞中的这种通道复合物。工程化的CHIP增强了KCNQ1的泛素化,消除了KCNQ1的表面密度,并取消了重构的K + 电流,而没有影响蛋白质的表达。化学上的变化使得能够化学控制泛素化,这表明前向贩运受损使KCNQ1表面密度下降了约3.5小时t1 / 2。结果表明,工程化的E3连接酶可用于阐明膜蛋白的泛素调节基础,并实现离子通道的有效翻译后功能抑制。

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