SASH1 is a novel binding partner to disassemble Caskin1 tandem SAM homopolymer through heterogeneous SAM-SAM interaction.

The FEBS journal Pub Date : 2024-12-17 DOI:10.1111/febs.17354

Yanhui Wang, Qiangou Chen, Cang Wu, Yuzhen Ding, Lin Yuan, Ziyi Wang, Yu Chen, Jianchao Li, Zhongmin Liu, Kang Xiao, Wei Liu

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Abstract

Calcium/calmodulin-dependent serine protein kinase (CASK) interaction protein 1/2 (Caskin1/2) is essential neuronal synaptic scaffold protein in nervous system development. Knockouts of Caskin1/2 display severe deficits in novelty recognition and spatial memory. The tandem sterile alpha motif (SAM) domains of Caskin1/2, also conserved in their Drosophila homolog Ckn, are known to form homopolymers, yet their dynamic regulation mechanism remains unclear. In this study, SAM and SH3 domain-containing protein 1 (SASH1) was first identified as a novel binding partner of Caskin1/2 through yeast two-hybrid (Y2H) screening. The SAM-SAM interaction between SASH1 and Caskin1 was biochemically characterized by size-exclusion chromatography (SEC), isothermal titration calorimetry (ITC), and glutathione-S-transferase (GST) pull-down and co-immunoprecipitation (co-IP) assays. Structural insights from AlphaFold2-predicted models of the Caskin1-SAMs/SASH1-SAM1 complex, along with mutagenesis validations, revealed key residues at the end-helix (EH)/mid-loop (ML) interface for this interaction. More interestingly, the Caskin1-SAMs homopolymer can be disrupted by the SAM-SAM interaction, which was consistently verified by using sedimentation, transmission electron microscopy (TEM), and immunofluorescence (IF) staining in heterologous cell lines. In summary, our findings provide a solid biochemical basis for the Caskin1/SASH1 interaction and propose a potential mechanism for regulating Caskin1/2 homopolymerization via SAM-SAM interactions. More importantly, the principle governing SAM homopolymer depolymerization is generalized via suggesting two distinct types of heterogeneous SAM-SAM interactions, offering fresh insights into SAM domain-mediated homopolymerization and depolymerization.

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钙/钙调蛋白依赖性丝氨酸蛋白激酶（CASK）相互作用蛋白1/2（Caskin1/2）是神经系统发育过程中必不可少的神经元突触支架蛋白。Caskin1/2基因敲除后会出现严重的新奇事物识别和空间记忆缺陷。众所周知，Caskin1/2的串联不育α基序（SAM）结构域可形成同源多聚物，果蝇同源物Ckn也保留了这一结构域，但它们的动态调控机制仍不清楚。在这项研究中，通过酵母双杂交（Y2H）筛选，SAM 和含 SH3 结构域蛋白 1（SASH1）首次被确定为 Caskin1/2 的新型结合伙伴。通过尺寸排阻色谱法（SEC）、等温滴定量热法（ITC）、谷胱甘肽-S-转移酶（GST）下拉和共免疫沉淀（co-IP）测定，对 SASH1 和 Caskin1 之间的 SAM-SAM 相互作用进行了生化鉴定。从 AlphaFold2 预测的 Caskin1-SAMs/SASH1-SAM1 复合物模型中获得的结构洞察力以及诱变验证揭示了这种相互作用的末端螺旋（EH）/中环（ML）界面上的关键残基。更有趣的是，SAM-SAM 相互作用可破坏 Caskin1-SAMs 的同源聚合体，这一点已在异源细胞系中通过沉积、透射电子显微镜（TEM）和免疫荧光（IF）染色得到了一致验证。总之，我们的研究结果为 Caskin1/SASH1 相互作用提供了坚实的生化基础，并提出了通过 SAM-SAM 相互作用调节 Caskin1/2 均聚的潜在机制。更重要的是，通过提出两种不同类型的异质 SAM-SAM 相互作用，概括了 SAM 均聚物解聚的原理，为 SAM 结构域介导的均聚物和解聚提供了新的见解。

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The FEBS journal

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