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在线磁珠动态蛋白质亲和选择结合液相色谱-质谱联用技术用于筛选药理活性化合物。

Online magnetic bead dynamic protein-affinity selection coupled to LC-MS for the screening of pharmacologically active compounds.

作者信息

Jonker N, Kretschmer A, Kool J, Fernandez A, Kloos D, Krabbe J G, Lingeman H, Irth H

机构信息

BioMolecular Analysis Group, Department of Chemistry, Faculty of Sciences, VU University Amsterdam, De Boelelaan 1083, 1081 HV Amsterdam, The Netherlands.

出版信息

Anal Chem. 2009 Jun 1;81(11):4263-70. doi: 10.1021/ac9000755.

DOI:10.1021/ac9000755
PMID:19476387
Abstract

The online, selective isolation of protein-ligand complexes using cobalt(II)-coated paramagnetic affinity beads (PABs) and subsequent liquid chromatography-mass spectrometry (LC-MS) determination of specifically bound ligands is described. After in-solution incubation of an analyte mixture with His-tagged target proteins, protein-analyte complexes are mixed with the Co(II)-PABs and subsequently injected into an in-house built magnetic trapping device. Bioactive ligands bound to the protein-Co(II)-PABs are retained in the magnetic field of the trapping device while inactive compounds are removed by washing with a pH 7.4 buffer. Active ligands are online eluted toward the LC-MS system using a pH shift. In the final step of the procedure, the protein-Co(II)-PABs are flushed to waste by temporarily lowering the magnetic field. The proof-of-principle is demonstrated by using commercially available Co(II)-PABs in combination with the His-tagged human estrogen-receptor ligand-binding domain. The system is characterized with a number of estrogenic ligands and nonbinding pharmaceutical compounds. The affinities of the test compounds varied from the high micromolar to the subnanomolar range. Typical detection limits are in the range from 20 to 80 nmol/L. The system is able to identify binders in mixtures of compounds, with an analysis time of 9.5 min per mixture. The standard deviation over 24 h is 9%.

摘要

描述了使用钴(II)包被的顺磁性亲和珠(PABs)在线选择性分离蛋白质-配体复合物,以及随后通过液相色谱-质谱(LC-MS)测定特异性结合配体的方法。将分析物混合物与带有His标签的靶蛋白在溶液中孵育后,将蛋白质-分析物复合物与Co(II)-PABs混合,随后注入内部构建的磁捕获装置。与蛋白质-Co(II)-PABs结合的生物活性配体保留在捕获装置的磁场中,而无活性的化合物则通过用pH 7.4缓冲液洗涤去除。活性配体通过pH值变化在线洗脱至LC-MS系统。在该方法的最后一步,通过暂时降低磁场将蛋白质-Co(II)-PABs冲洗至废液中。使用市售的Co(II)-PABs与带有His标签的人雌激素受体配体结合结构域相结合,证明了该原理的可行性。该系统用多种雌激素配体和非结合药物化合物进行了表征。测试化合物的亲和力范围从高微摩尔到亚纳摩尔。典型的检测限在20至80 nmol/L范围内。该系统能够在化合物混合物中识别结合剂,每个混合物的分析时间为9.5分钟。24小时内的标准偏差为9%。

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