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脱硫生物素与链霉亲和素、抗生物素蛋白及其他生物素结合蛋白的轻松可逆结合:在蛋白质标记、检测及分离中的应用

Easily reversible desthiobiotin binding to streptavidin, avidin, and other biotin-binding proteins: uses for protein labeling, detection, and isolation.

作者信息

Hirsch James D, Eslamizar Leila, Filanoski Brian J, Malekzadeh Nabi, Haugland Rosaria P, Beechem Joseph M, Haugland Richard P

机构信息

Molecular Probes, Inc., Eugene, OR 97402, USA.

出版信息

Anal Biochem. 2002 Sep 15;308(2):343-57. doi: 10.1016/s0003-2697(02)00201-4.

DOI:10.1016/s0003-2697(02)00201-4
PMID:12419349
Abstract

The high-affinity binding of biotin to avidin, streptavidin, and related proteins has been exploited for decades. However, a disadvantage of the biotin/biotin-binding protein interaction is that it is essentially irreversible under physiological conditions. Desthiobiotin is a biotin analogue that binds less tightly to biotin-binding proteins and is easily displaced by biotin. We synthesized an amine-reactive desthiobiotin derivative for labeling proteins and a desthiobiotin-agarose affinity matrix. Conjugates labeled with desthiobiotin are equivalent to their biotinylated counterparts in cell-staining and antigen-labeling applications. They also bind to streptavidin and other biotin-binding protein-based affinity columns and are recognized by anti-biotin antibodies. Fluorescent streptavidin conjugates saturated with desthiobiotin, but not biotin, bind to a cell-bound biotinylated target without further processing. Streptavidin-based ligands can be gently stripped from desthiobiotin-labeled targets with buffered biotin solutions. Thus, repeated probing with fluorescent streptavidin conjugates followed by enzyme-based detection is possible. In all applications, the desthiobiotin/biotin-binding protein complex is easily dissociated under physiological conditions by either biotin or desthiobiotin. Thus, our desthiobiotin-based reagents and techniques provide some distinct advantages over traditional 2-iminobiotin, monomeric avidin, or other affinity-based techniques.

摘要

生物素与抗生物素蛋白、链霉抗生物素蛋白及相关蛋白质的高亲和力结合已被利用了数十年。然而,生物素/生物素结合蛋白相互作用的一个缺点是,在生理条件下它基本上是不可逆的。脱硫生物素是一种生物素类似物,它与生物素结合蛋白的结合较弱,容易被生物素取代。我们合成了一种用于标记蛋白质的胺反应性脱硫生物素衍生物和一种脱硫生物素-琼脂糖亲和基质。用脱硫生物素标记的共轭物在细胞染色和抗原标记应用中与它们的生物素化对应物相当。它们还能与链霉抗生物素蛋白和其他基于生物素结合蛋白的亲和柱结合,并能被抗生物素抗体识别。用脱硫生物素而非生物素饱和的荧光链霉抗生物素蛋白共轭物无需进一步处理就能与细胞结合的生物素化靶标结合。基于链霉抗生物素蛋白的配体可以用缓冲生物素溶液从脱硫生物素标记的靶标上温和地洗脱下来。因此,可以用荧光链霉抗生物素蛋白共轭物进行重复探测,然后进行基于酶的检测。在所有应用中,脱硫生物素/生物素结合蛋白复合物在生理条件下很容易被生物素或脱硫生物素解离。因此,我们基于脱硫生物素的试剂和技术比传统的2-亚氨基生物素、单体抗生物素蛋白或其他基于亲和的技术具有一些明显的优势。

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