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Protein higher-order-structure determination by fast photochemical oxidation of proteins and mass spectrometry analysis.通过快速光化学氧化蛋白质和质谱分析来确定蛋白质的高级结构。
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Covalent Labeling with an α,β-Unsaturated Carbonyl Scaffold for Studying Protein Structure and Interactions by Mass Spectrometry.通过质谱法研究蛋白质结构和相互作用的 α,β-不饱和羰基支架的共价标记。
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Assembly of a GPCR-G Protein Complex.G 蛋白偶联受体- G 蛋白复合物的组装。
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可溶性蛋白和跨膜蛋白的碳正离子足迹分析

Carbocation Footprinting of Soluble and Transmembrane Proteins.

机构信息

Department of Chemistry, Washington University in St. Louis, St. Louis, Missouri 63130, United States.

Department of Biochemistry and Molecular Biophysics, Washington University School of Medicine, St. Louis, Missouri 63110, United States.

出版信息

Anal Chem. 2021 Oct 5;93(39):13101-13105. doi: 10.1021/acs.analchem.1c03274. Epub 2021 Sep 24.

DOI:10.1021/acs.analchem.1c03274
PMID:34558889
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8900486/
Abstract

Here, we introduce carbocations (RC) as laser-initiated footprinting reagents for proteins. We screened seven candidates and selected trifluomethoxy benzyl bromide (TFBB) as an effective precursor for the electrophilic trifluomethoxy benzyl carbocation (TFB) under laser (248 nm) irradiation on the fast photochemical oxidation of proteins (FPOP) platform. Initial results demonstrate that this electrophilic cation reagent affords residue coverage of nucleophilic amino acids including H, W, M, and S. Further, the addition of TFB increases the hydrophobicity of the peptides so that separation of isomeric peptide products by reversed-phase LC is improved, suggesting opportunities for subresidue footprinting. Comparison of apo- and holo-myoglobin footprints shows that the TFB footprinting is sensitive to protein conformational change and solvent accessibility. Interestingly, because the TFB is amphiphilic, the reagent can potentially footprint membrane proteins as demonstrated for vitamin K epoxide reductase (VKOR) stabilized in a micelle. Not only does footprinting of the extra-membrane domain occur, but also some footprinting of the hydrophobic transmembrane domain is achieved owing to the interaction of TFB with the micelle. Carbocation precursors are stable and amenable for tailoring their properties and those of the incipient carbocation, enabling targeting their soluble or membrane-associated or embedded regions and distinguishing between the extra- and trans-membrane domains of membrane proteins.

摘要

在这里,我们介绍碳阳离子(RC)作为蛋白质的激光引发足迹试剂。我们筛选了七种候选物,并选择三氟甲氧基苄基溴(TFBB)作为在快速光化学蛋白质氧化(FPOP)平台上激光(248nm)照射下有效亲电三氟甲氧基苄基碳阳离子(TFB)的前体。初步结果表明,这种亲电阳离子试剂可提供包括 H、W、M 和 S 在内的亲核氨基酸的残基覆盖率。此外,TFB 的加入增加了肽的疏水性,从而改善了反相 LC 分离异构肽产物的能力,这表明有可能进行亚残基足迹分析。apo-和 holo-肌红蛋白足迹的比较表明,TFB 足迹分析对蛋白质构象变化和溶剂可及性敏感。有趣的是,由于 TFB 具有两亲性,因此该试剂可以对膜蛋白进行足迹分析,如在胶束中稳定的维生素 K 环氧化物还原酶(VKOR)中所示。不仅发生了额外膜域的足迹分析,而且由于 TFB 与胶束的相互作用,还实现了疏水跨膜域的一些足迹分析。碳阳离子前体稳定,并且可以定制其性质和初始碳阳离子的性质,从而能够靶向其可溶性或膜相关或嵌入式区域,并区分膜蛋白的外跨膜域。