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Quantification of Protein-Induced Membrane Remodeling Kinetics In Vitro with Lipid Multilayer Gratings

机译:脂质多层光栅的蛋白质诱导的膜重塑动力学的体外定量。

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摘要

The dynamic self-organization of lipids in biological systems is a highly regulated process that enables the compartmentalization of living systems at micro- and nanoscopic scales. Consequently, quantitative methods for assaying the kinetics of supramolecular remodeling such as vesicle formation from planar lipid bilayers or multilayers are needed to understand cellular self-organization. Here, a new nanotechnology-based method for quantitative measurements of lipid–protein interactions is presented and its suitability for quantifying the membrane binding, inflation, and budding activity of the membrane-remodeling protein Sar1 is demonstrated. Lipid multilayer gratings are printed onto surfaces using nanointaglio and exposed to Sar1, resulting in the inflation of lipid multilayers into unilamellar structures, which can be observed in a label-free manner by monitoring the diffracted light. Local variations in lipid multilayer volume on the surface is used to vary substrate availability in a microarray format. A quantitative model is developed that allows quantification of binding affinity (KD) and kinetics (kon and koff). Importantly, this assay is uniquely capable of quantifying membrane remodeling. Upon Sar1-induced inflation of single bilayers from surface supported multilayers, the semicylindrical grating lines are observed to remodel into semispherical buds when a critical radius of curvature is reached.
机译:脂质在生物系统中的动态自组织是一个高度受控的过程,可在微观和纳米尺度上对生物系统进行分区。因此,需要定量的方法来分析超分子重塑的动力学,例如由平面脂质双层或多层形成的囊泡,以了解细胞的自组织。在这里,提出了一种新的基于纳米技术的定量测量脂蛋白相互作用的方法,并证明了其对定量膜重塑蛋白Sar1的膜结合,膨胀和萌芽活性的适用性。使用纳米凹版将脂质多层光栅印刷到表面上并暴露于Sar1,导致脂质多层充胀成单层结构,可以通过监测衍射光以无标签的方式观察到。表面脂质多层体积的局部变化用于改变微阵列形式的底物利用率。建立了定量模型,可以量化结合亲和力(KD)和动力学(kon和koff)。重要的是,该测定法独特地能够量化膜重塑。在Sar1诱导的单双层从表面支撑的多层充气后,当达到临界曲率半径时,观察到半圆柱光栅线会重塑为半球形芽。

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