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Substrate-Induced Conformational Changes of the Tyrocidine Synthetase 1 Adenylation Domain Probed by Intrinsic Trp Fluorescence

机译:通过本征TRP荧光探测酪氨酸合成酶1腺苷酸化结构域的基材诱导的构象变化

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Nonribosomal peptide synthetases (NRPS) are multifunctional proteins that catalyze the synthesis of the peptide products with enormous biological potential. The process of biosynthesis starts with the adenylation (A) domain, which during the catalytic cycle undergoes extensive structural rearrangements. In this paper, we present the first study of the tyrocidine synthetase 1 A-domain (TycA-A) fluorescence properties. The TycA-A protein contains five potentially fluorescent Trp residues at positions 227, 301, 323, 376 and 406. The contribution of each Trp to the TycA-A emission was determined using protein variants bearing single Trp to Phe substitutions. The accessibility of the Trp side chains during adenylation showed that only W227 is affected by substrate binding. The protein variant containing solely fluorescent W227 residue was constructed and further used as a probe to explore the binding effect of different non-cognate amino acid substrates. The results indicate a different accessibility of W227 residue in the presence of non-cognate amino acids, which might offer an explanation for the higher aminoacyl-adenenylate leakage. Overall, our results suggest that intrinsic tryptophan fluorescence could be used as a method to probe the effect of substrate binding on the local structure in NRPS adenylation domains.
机译:非纤维素肽合成酶(NRP)是多功能蛋白质,其催化具有巨大的生物潜力的肽产物的合成。生物合成的方法从腺苷酸化(A)结构域开始,在催化循环期间经历广泛的结构重排。在本文中,我们介绍了酪甲合成酶1A-结构域(TYCA-A)荧光性质的第一次研究。 TYCA-A蛋白质在227,301,323,376和406处含有五个可能的荧光TRP残基。使用携带单TRP的蛋白质变体对PHE取代的蛋白质变体确定每个TRP对TYCA的贡献。腺苷期间TRP侧链的可访问性显示,仅W227受基质结合的影响。构建含有荧光W227残基的蛋白质变体并进一步用作探针以探讨不同非同源氨基酸基材的结合效果。结果表明,在非同源氨基酸存在下,W227残基的不同可达性,这可能对较高的氨基酰基 - 亚苯基化物渗漏提供解释。总体而言,我们的结果表明,固有色氨酸荧光可以用作探测底物结合对NRPS腺苷酸域中的局部结构的效果的方法。

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