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一种使用八面体多吡啶d⁶金属配合物对蛋白质进行半胱氨酸特异性标记的简便通用方法。

A facile and versatile methodology for cysteine specific labeling of proteins with octahedral polypyridyl d⁶ metal complexes.

作者信息

Dwaraknath Sudharsan, Tran Ngoc-Han, Dao Thanh, Colbert Alexander, Mullen Sarah, Nguyen Angelina, Cortez Alejandro, Cheruzel Lionel

机构信息

San José State University, Department of Chemistry, One Washington Square, San José, CA 95192-0101, United States.

San José State University, Department of Chemistry, One Washington Square, San José, CA 95192-0101, United States.

出版信息

J Inorg Biochem. 2014 Jul;136:154-60. doi: 10.1016/j.jinorgbio.2013.12.013. Epub 2014 Jan 10.

Abstract

We have synthesized and characterized four octahedral polypyridyl d(6) metal complexes bearing the 5,6-epoxy-5,6-dihydro-[1,10]phenanthroline ligand (L1) as cysteine specific labeling reagents. The proposed synthetic pathways allow the preparation of the metal complexes containing Re(I), Ru(II), Os(II) and Ir(III) while preserving the epoxide functionality. The complexes were characterized by (1)H and (13)C NMR, mass spectrometry, UV-visible and luminescence spectroscopies as well as cyclic voltammetry. As proof of concept, a set of non-native single cysteine P450 BM3 heme domain mutants previously developed in our laboratory was used to study the labeling reaction. We demonstrate that the proposed labels can selectively react, often in high yield, with cysteine residues of the protein via the nucleophilic thiol ring opening of the epoxide moiety. In addition, under basic conditions, subsequent loss of a water molecule led to the aromatization of the phenanthroline ring on the protein-bound label compounds, as observed by mass spectrometry and luminescence measurements.

摘要

我们合成并表征了四种带有5,6-环氧-5,6-二氢-[1,10]菲咯啉配体(L1)的八面体多吡啶d(6)金属配合物,作为半胱氨酸特异性标记试剂。所提出的合成途径能够制备含有铼(I)、钌(II)、锇(II)和铱(III)的金属配合物,同时保留环氧化物官能团。通过氢谱(1H)、碳谱(13C)核磁共振、质谱、紫外可见光谱和发光光谱以及循环伏安法对这些配合物进行了表征。作为概念验证,我们使用了一组先前在我们实验室开发的非天然单半胱氨酸P450 BM3血红素结构域突变体来研究标记反应。我们证明,所提出的标记物能够通过环氧化物部分的亲核硫醇开环反应,经常以高产率与蛋白质的半胱氨酸残基选择性反应。此外,在碱性条件下,如通过质谱和发光测量所观察到的,随后水分子的失去导致了与蛋白质结合的标记化合物上菲咯啉环的芳构化。

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