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首页> 外文期刊>Journal of enzyme inhibition and medicinal chemistry. >Cyclopropane-1,2-dicarboxylic acids as new tools for the biophysical investigation of O -acetylserine sulfhydrylases by fluorimetric methods and saturation transfer difference (STD) NMR
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Cyclopropane-1,2-dicarboxylic acids as new tools for the biophysical investigation of O -acetylserine sulfhydrylases by fluorimetric methods and saturation transfer difference (STD) NMR

机译:环丙烷-1,2-二羧酸是通过荧光法和饱和转移差异(STD)NMR进行O-乙酰丝氨酸巯基化酶生物物理研究的新工具

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Abstract Cysteine is a building block for many biomolecules that are crucial for living organisms. O-Acetylserine sulfhydrylase (OASS), present in bacteria and plants but absent in mammals, catalyzes the last step of cysteine biosynthesis. This enzyme has been deeply investigated because, beside the biosynthesis of cysteine, it exerts a series of “moonlighting” activities in bacteria. We have previously reported a series of molecules capable of inhibiting Salmonella typhimurium (S. typhymurium) OASS isoforms at nanomolar concentrations, using a combination of computational and spectroscopic approaches. The cyclopropane-1,2-dicarboxylic acids presented herein provide further insights into the binding mode of small molecules to OASS enzymes. Saturation transfer difference NMR (STD-NMR) was used to characterize the molecule/enzyme interactions for both OASS-A and B. Most of the compounds induce a several fold increase in fluorescence emission of the pyridoxal 5′-phosphate (PLP) coenzyme upon binding to either OASS-A or OASS-B, making these compounds excellent tools for the development of competition-binding experiments.
机译:摘要半胱氨酸是许多对生物至关重要的生物分子的构建基。 O-乙酰丝氨酸巯基化酶(OASS)存在于细菌和植物中,而在哺乳动物中却不存在,它催化半胱氨酸生物合成的最后一步。该酶已被深入研究,因为除了半胱氨酸的生物合成外,它还在细菌中发挥了一系列“月光下”的活动。我们先前已经报道了一系列能够结合计算和光谱方法在纳摩尔浓度下抑制鼠伤寒沙门氏菌(鼠伤寒沙门氏菌)OASS亚型的分子。本文提供的环丙烷-1,2-二羧酸为小分子与OASS酶的结合方式提供了进一步的见解。饱和转移差异NMR(STD-NMR)用于表征OASS-A和B的分子/酶相互作用。大多数化合物诱导吡upon醛5'-磷酸(PLP)辅酶的荧光发射增加几倍。与OASS-A或OASS-B结合,使这些化合物成为开展竞争结合实验的极佳工具。

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