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2
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In vivo and in vitro examination of stability of primary hyperoxaluria-associated human alanine:glyoxylate aminotransferase.原发性高草酸尿症相关的人丙氨酸:乙醛酸转氨酶稳定性的体内和体外检测
J Biol Chem. 2008 Nov 7;283(45):30493-502. doi: 10.1074/jbc.M803525200. Epub 2008 Sep 9.
2
Throughput and efficiency of a mass spectrometry-based screening assay for protein-ligand binding detection.基于质谱的蛋白质-配体结合检测筛选分析方法的通量与效率
J Am Soc Mass Spectrom. 2008 Sep;19(9):1303-11. doi: 10.1016/j.jasms.2008.06.007. Epub 2008 Jun 27.
3
Ga3+ as a mechanistic probe in Fe3+ transport: characterization of Ga3+ interaction with FbpA.镓离子(Ga³⁺)作为铁离子(Fe³⁺)转运机制的探针:镓离子与铁结合蛋白A(FbpA)相互作用的表征
J Biol Inorg Chem. 2008 Aug;13(6):887-98. doi: 10.1007/s00775-008-0376-5. Epub 2008 May 7.
4
Ex vivo analysis of synergistic anion binding to FbpA in Gram-negative bacteria.革兰氏阴性菌中协同阴离子与FbpA结合的体外分析。
Biochemistry. 2008 Apr 8;47(14):4298-305. doi: 10.1021/bi701188x. Epub 2008 Mar 14.
5
H/D exchange and mass spectrometry-based method for biophysical analysis of multidomain proteins at the domain level.基于氢/氘交换和质谱的多结构域蛋白质结构域水平生物物理分析方法。
Anal Chem. 2007 Nov 15;79(22):8728-39. doi: 10.1021/ac071380a. Epub 2007 Oct 19.
6
A two-stage differential hydrogen deuterium exchange method for the rapid characterization of protein/ligand interactions.一种用于快速表征蛋白质/配体相互作用的两阶段差分氢氘交换方法。
J Biomol Tech. 2007 Sep;18(4):194-204.
7
H/D exchange- and mass spectrometry-based strategy for the thermodynamic analysis of protein-ligand binding.基于氢/氘交换和质谱的蛋白质-配体结合热力学分析策略。
Anal Chem. 2007 Aug 1;79(15):5869-77. doi: 10.1021/ac0700777. Epub 2007 Jun 21.
8
Structural and thermodynamic characterization of a cytoplasmic dynein light chain-intermediate chain complex.细胞质动力蛋白轻链-中间链复合物的结构与热力学特征
Proc Natl Acad Sci U S A. 2007 Jun 12;104(24):10028-33. doi: 10.1073/pnas.0703614104. Epub 2007 Jun 5.
9
Stable RNA interference-mediated suppression of cyclophilin A diminishes non-small-cell lung tumor growth in vivo.稳定的RNA干扰介导的亲环素A抑制作用可减少体内非小细胞肺癌肿瘤的生长。
Cancer Res. 2005 Oct 1;65(19):8853-60. doi: 10.1158/0008-5472.CAN-05-1219.
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基于氢/氘交换和蛋白酶消化的蛋白质-配体结合检测筛选分析方法。

Hydrogen/deuterium exchange- and protease digestion-based screening assay for protein-ligand binding detection.

机构信息

Department of Chemistry, Duke University, Durham, North Carolina 27708, USA.

出版信息

Anal Chem. 2009 Aug 15;81(16):6860-7. doi: 10.1021/ac900854t.

DOI:10.1021/ac900854t
PMID:20337380
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2858457/
Abstract

A protease digestion strategy was incorporated into single-point stability of unpurified proteins from rates of H/D exchange (SUPREX), which is a hydrogen/deuterium (H/D) exchange- and mass spectrometry-based assay for the detection of protein-ligand binding. Single-point SUPREX is an abbreviated form of SUPREX in which protein-ligand binding interactions are detected by measuring the increase in a protein's thermodynamic stability upon ligand binding. The new protease digestion protocol provides a noteworthy increase in the efficiency of single-point SUPREX because peptide masses can be determined with greater precision than intact protein masses in the matrix-assisted laser desorption ionization (MALDI) readout of single-point SUPREX. The protocol was evaluated in test screens on two model protein systems, including cyclophilin A (CypA) and the minor allele variant of human alanine:glyoxylate aminotransferase (AGTmi). The test screening results obtained on both proteins revealed that the peptide readout of the single-point SUPREX-protease digestion protocol was more efficient than the intact protein readout of the original single-point SUPREX protocol at discriminating hits and nonhits. In addition to this improvement in screening efficiency, the protease digestion strategy described here is expected to significantly increase the generality of the single-point SUPREX assay.

摘要

采用蛋白酶消化策略,结合未纯化蛋白质的氢/氘(H/D)交换单点稳定性(SUPREX),这是一种基于 H/D 交换和质谱的测定方法,用于检测蛋白质-配体结合。单点 SUPREX 是 SUPREX 的缩写形式,通过测量配体结合后蛋白质热力学稳定性的增加来检测蛋白质-配体结合相互作用。新的蛋白酶消化方案显著提高了单点 SUPREX 的效率,因为在单点 SUPREX 的基质辅助激光解吸电离(MALDI)读出中,与完整蛋白质质量相比,肽质量可以更精确地确定。该方案在两个模型蛋白系统(包括亲环素 A(CypA)和人类丙氨酸:乙醛酸转氨酶(AGTmi)的次要等位基因变体)的测试筛选中进行了评估。在这两种蛋白质上进行的测试筛选结果表明,与原始单点 SUPREX 方案的完整蛋白质读数相比,单点 SUPREX-蛋白酶消化方案的肽读数在区分命中和未命中方面更有效。除了提高筛选效率外,这里描述的蛋白酶消化策略预计还将显著提高单点 SUPREX 测定的通用性。