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Slp4-a 在血脑屏障中囊泡融合前弯曲过程中的作用。

Effect of Slp4-a on Membrane Bending During Prefusion of Vesicles in Blood-Brain Barrier.

机构信息

School of Mechanical and Materials Engineering, Washington State University, Pullman, WA 99164-2920.

出版信息

J Biomech Eng. 2023 Jan 1;145(1). doi: 10.1115/1.4054985.

Abstract

Vesicle exocytosis is a promising pathway for brain drug delivery through the blood-brain barrier to treat neurodegenerative diseases. In vesicle exocytosis, the membrane fusion process is initiated by the calcium sensor protein named synaptotagmin-like protein4-a (Slp4-a). Understanding conformational changes of Slp4-a during the prefusion stage of exocytosis will help to develop vesicle-based drug delivery to the brain. In this work, we use molecular dynamics (MD) simulations with a hybrid force field coupling united-atom protein model with MARTINI coarse-grained (CG) solvent to capture the conformational changes of Slp4-a during the prefusion stage. These hybrid coarse-grained simulations are more efficient than all-atom MD simulations and can capture protein interactions and conformational changes. Our simulation results show that the calcium ions play critical roles during the prefusion stage. Only one calcium ion can remain in each calcium-binding pocket of Slp4-a C2 domains. The C2B domain of calcium-unbound Slp4-a remains parallel to the endothelial membrane, while the C2B domain of calcium-bound Slp4-a rotates perpendicular to the endothelial membrane to approach the vesicular membrane. For the calcium-bound case, three Slp4-a proteins can effectively bend lipid membranes at the prefusion stage, which could later trigger lipid stalk between membranes. This work provides a better understanding how C2 domains of Slp4-a operate during vesicle exocytosis from an endothelial cell.

摘要

囊泡胞吐是一种有前途的脑内递药途径,可以通过血脑屏障来治疗神经退行性疾病。在囊泡胞吐中,膜融合过程由钙传感器蛋白——突触融合蛋白相关蛋白 4-a(Slp4-a)启动。了解 Slp4-a 在胞吐前融合阶段的构象变化,将有助于开发基于囊泡的脑内递药。在这项工作中,我们使用分子动力学(MD)模拟,该模拟采用混合力场,将全原子蛋白模型与 MARTINI 粗粒(CG)溶剂耦合,以捕捉 Slp4-a 在胞吐前融合阶段的构象变化。这些混合粗粒模拟比全原子 MD 模拟更高效,能够捕捉蛋白相互作用和构象变化。我们的模拟结果表明,钙离子在胞吐前融合阶段起着关键作用。每个 Slp4-a C2 结构域的钙结合口袋中只能保留一个钙离子。无钙结合的 Slp4-a 的 C2B 结构域与内皮细胞膜保持平行,而钙结合的 Slp4-a 的 C2B 结构域则垂直于内皮细胞膜旋转,以接近囊泡膜。对于钙结合的情况,三个 Slp4-a 蛋白可以在胞吐前融合阶段有效地弯曲脂质膜,这可能会引发膜间脂质柄。这项工作提供了对 Slp4-a 的 C2 结构域在血管内皮细胞中囊泡胞吐过程中如何发挥作用的更好理解。

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