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使用靶向半胱氨酸的乙烯基砜-环辛炔标签对蛋白质进行荧光探针标记的系统研究。

A systematic study of protein labeling by fluorogenic probes using cysteine targeting vinyl sulfone-cyclooctyne tags.

作者信息

Söveges B, Imre T, Szende T, Póti Á L, Cserép G B, Hegedűs T, Kele P, Németh K

机构信息

Research Centre for Natural Sciences of Hungarian Academy of Sciences, Institute of Organic Chemistry, Chemical Biology Research Group, H-1117 Budapest, Magyar tudósok krt. 2, Hungary.

出版信息

Org Biomol Chem. 2016 Jul 7;14(25):6071-8. doi: 10.1039/c6ob00810k. Epub 2016 May 31.

Abstract

Fluorescent tagging of proteins via accessible cysteine residues is of paramount importance. In this study, model proteins of interest (mitogen-activated protein kinases) were labeled successfully in native state on their free thiols by direct fluorescence derivatization, or in a sequential manner where conjugation of the site specific linker and the fluorophore is carried out in two steps. To this end we designed and prepared two novel chemical reporters carrying vinyl sulfone as Cys targeting function and cyclooctyne motifs, suitable for subsequent conjugation with fluorogenic azides via copper free strain-promoted azide-alkyne click chemistry. Direct and sequential labeling reaction steps were analyzed by native PAGE, capillary zone electrophoresis and tandem mass spectrometry. The efficiency of tagging was correlated with solvent accessibility of the Cys residues. Our results indicated that conjugation of native proteins by vinyl sulfone linkers was fast and thiol-selective. Subsequent click reaction with fluorogenic dyes generates intensive fluorescence signals and fulfills all requirements of bioorthogonality.

摘要

通过可及的半胱氨酸残基对蛋白质进行荧光标记至关重要。在本研究中,目标模型蛋白(丝裂原活化蛋白激酶)通过直接荧光衍生化在其游离硫醇上以天然状态成功标记,或者以一种顺序方式进行标记,其中位点特异性连接子和荧光团的缀合分两步进行。为此,我们设计并制备了两种新型化学报告分子,它们带有乙烯砜作为半胱氨酸靶向功能基团和环辛炔基序,适用于随后通过无铜应变促进的叠氮化物-炔烃点击化学与荧光叠氮化物缀合。通过非变性聚丙烯酰胺凝胶电泳、毛细管区带电泳和串联质谱分析直接和顺序标记反应步骤。标记效率与半胱氨酸残基的溶剂可及性相关。我们的结果表明,通过乙烯砜连接子对天然蛋白质进行缀合快速且具有硫醇选择性。随后与荧光染料的点击反应产生强烈的荧光信号,并满足生物正交性的所有要求。

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