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B2LiVe,一种无需标记的 1D-NMR 方法,用于定量两亲性肽或蛋白质与膜泡的结合。

B2LiVe, a label-free 1D-NMR method to quantify the binding of amphitropic peptides or proteins to membrane vesicles.

机构信息

Institut Pasteur, Université de Paris Cité, CNRS UMR3528, Biochemistry of Macromolecular Interactions Unit, 75015 Paris, France; Université de Paris Cité, 75005 Paris, France.

Institut Pasteur, Université de Paris Cité, CNRS UMR3528, Biochemistry of Macromolecular Interactions Unit, 75015 Paris, France.

出版信息

Cell Rep Methods. 2023 Nov 20;3(11):100624. doi: 10.1016/j.crmeth.2023.100624. Epub 2023 Oct 30.

Abstract

Amphitropic proteins and peptides reversibly partition from solution to membrane, a key process that regulates their functions. Experimental approaches classically used to measure protein partitioning into lipid bilayers, such as fluorescence and circular dichroism, are hardly usable when the peptides or proteins do not exhibit significant polarity and/or conformational changes upon membrane binding. Here, we describe binding to lipid vesicles (B2LiVe), a simple, robust, and widely applicable nuclear magnetic resonance (NMR) method to determine the solution-to-membrane partitioning of unlabeled proteins or peptides. B2LiVe relies on previously described proton 1D-NMR fast-pulsing techniques. Membrane partitioning induces a large line broadening, leading to a loss of protein signals; therefore, the decrease of the NMR signal directly measures the fraction of membrane-bound protein. The method uses low polypeptide concentrations and has been validated on several membrane-interacting polypeptides, ranging from 3 to 54 kDa, with membrane vesicles of different sizes and various lipid compositions.

摘要

两亲性蛋白和肽可逆地从溶液分配到膜中,这是调节它们功能的关键过程。当肽或蛋白质在与膜结合时没有表现出显著的极性和/或构象变化时,经典上用于测量蛋白质分配到脂质双层中的实验方法,如荧光和圆二色性,几乎无法使用。在这里,我们描述了结合脂质体(B2LiVe),一种简单、强大且广泛适用的核磁共振(NMR)方法,用于确定未标记的蛋白质或肽的溶液到膜的分配。B2LiVe 依赖于先前描述的质子 1D-NMR 快速脉冲技术。膜分配会引起大的线宽增加,导致蛋白质信号丢失;因此,NMR 信号的减少直接测量膜结合蛋白质的分数。该方法使用低多肽浓度,并已在几种膜相互作用的多肽上得到验证,范围从 3 到 54 kDa,使用不同大小和各种脂质组成的膜囊泡。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1adb/10694493/1809ba7f4649/fx1.jpg

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