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Optimized bacterial expression and purification of the c-Src catalytic domain for solution NMR studies

机译:用于溶液NMR研究的优化细菌表达和c-Src催化域的纯化

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摘要

Progression of a host of human cancers is associated with elevated levels of expression and catalytic activity of the Src family of tyrosine kinases (SFKs), making them key therapeutic targets. Even with the availability of multiple crystal structures of active and inactive forms of the SFK catalytic domain (CD), a complete understanding of its catalytic regulation is unavailable. Also unavailable are atomic or near-atomic resolution information about their interactions, often weak or transient, with regulating phosphatases and downstream targets. Solution NMR, the biophysical method best suited to tackle this problem, was previously hindered by difficulties in bacterial expression and purification of sufficient quantities of soluble, properly folded protein for economically viable labeling with NMR-active isotopes. Through a choice of optimal constructs, co-expression with chaperones and optimization of the purification protocol, we have achieved the ability to bacterially produce large quantities of the isotopically-labeled CD of c-Src, the prototypical SFK, and of its activating Tyr-phosphorylated form. All constructs produce excellent spectra allowing solution NMR studies of this family in an efficient manner.
机译:许多人类癌症的进展与酪氨酸激酶(SFK)的Src家族的表达水平和催化活性升高有关,使其成为关键的治疗靶标。即使可以使用SFK催化域(CD)的活性和非活性形式的多个晶体结构,也无法完全了解其催化调节。同样缺少关于它们与调节磷酸酶和下游靶标相互作用的原子或近原子分辨率信息,这些信息通常是弱的或短暂的。溶液NMR是最适合解决此问题的生物物理方法,以前曾因细菌表达困难以及难以纯化足够数量的可溶性,正确折叠的蛋白质以进行NMR活性同位素经济可行的标记而受到阻碍。通过选择最佳构建体,与分子伴侣共表达以及优化纯化方案,我们已经实现了细菌生产大量c-Src同位素标记CD,原型SFK及其活化Tyr-的能力。磷酸化形式。所有构建体均产生出色的光谱,从而可以有效地进行该家族的溶液NMR研究。

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