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货物介导的内吞衔接蛋白 Sla1 在.中的募集

Cargo-mediated recruitment of the endocytic adaptor protein Sla1 in .

机构信息

Department of Biochemistry and Molecular Biology, Colorado State University, Fort Collins, CO 80523-1870, USA.

Department of Biochemistry and Molecular Biology, Colorado State University, Fort Collins, CO 80523-1870, USA

出版信息

J Cell Sci. 2020 Oct 12;133(19):jcs247684. doi: 10.1242/jcs.247684.

Abstract

Endocytosis of plasma membrane proteins is mediated by their interaction with adaptor proteins. Conversely, emerging evidence suggests that adaptor protein recruitment to the plasma membrane may depend on binding to endocytic cargo. To test this idea, we analyzed the yeast adaptor protein Sla1, which binds membrane proteins harboring the endocytic signal NPFxD via the Sla1 SHD1 domain. Consistently, SHD1 domain point mutations that disrupted NPFxD binding caused a proportional reduction in Sla1-GFP recruitment to endocytic sites. Furthermore, simultaneous SHD1 domain point mutation and deletion of the C-terminal LxxQxTG repeat (SR) region linking Sla1 to coat proteins Pan1 and End3 resulted in total loss of Sla1-GFP recruitment to the plasma membrane. These data suggest that multiple interactions are needed for recruitment of Sla1 to the membrane. Interestingly, a Sla1 fragment containing just the third SH3 domain, which binds ubiquitin, and the SHD1 domain displayed broad surface localization, suggesting plasma membrane recruitment is mediated by interaction with both NPFxD-containing and ubiquitylated plasma membrane proteins. Our results also imply that a Sla1 NPF motif adjacent to the SR region might regulate the Sla1-cargo interaction, mechanistically linking Sla1 cargo binding to endocytic site recruitment.

摘要

内吞细胞膜蛋白是由其与衔接蛋白的相互作用介导的。相反,新出现的证据表明,衔接蛋白向质膜的募集可能依赖于与内吞货物的结合。为了验证这一观点,我们分析了酵母衔接蛋白 Sla1,它通过 Sla1 SHD1 结构域与含有内吞信号 NPFxD 的膜蛋白结合。一致地,破坏 NPFxD 结合的 SHD1 结构域点突变导致 Sla1-GFP 向内吞部位的募集比例减少。此外,同时进行 SHD1 结构域点突变和删除连接 Sla1 到外衣蛋白 Pan1 和 End3 的 C 端 LxxQxTG 重复(SR)区,导致 Sla1-GFP 完全丧失向质膜的募集。这些数据表明,Sla1 向膜的募集需要多种相互作用。有趣的是,仅包含第三个 SH3 结构域(与泛素结合)和 SHD1 结构域的 Sla1 片段显示出广泛的表面定位,表明 Sla1 的质膜募集是通过与含有 NPFxD 和泛素化质膜蛋白的相互作用介导的。我们的结果还表明,位于 SR 区域附近的 Sla1 NPF 基序可能调节 Sla1-货物相互作用,在机制上连接 Sla1 货物结合与内吞部位的募集。

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