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优化后的方法(SDS/PAGE 和 LC-MS)揭示了所有检测到的转谷氨酰胺酶介导的反应中的脱酰胺作用。

Optimised methods (SDS/PAGE and LC-MS) reveal deamidation in all examined transglutaminase-mediated reactions.

机构信息

Research Department Covalab S.A.S Lyon France.

Department of Biochemistry and Molecular Biology Faculty of Medicine University of Debrecen Hungary.

出版信息

FEBS Open Bio. 2019 Jan 18;9(2):396-404. doi: 10.1002/2211-5463.12575. eCollection 2019 Feb.

Abstract

Transglutaminases (TGs) are a family of structurally and functionally related enzymes that catalyse calcium-dependent post-translational modifications of proteins through protein-protein crosslinking, amine incorporation, or deamidation. For many years deamidation mediated by TGs was considered to be a side reaction, but recently substrate-specific deamidations have been reported. Here we describe an optimised SDS/PAGE assay for the easy and rapid monitoring of the TG reaction with small peptides. The relative proportion of deamidation to transamidation was evaluated by densitometric analysis and confirmed by nano-liquid chromatography-nano-electrospray ionisation MS. We further investigated the effect of reaction conditions on transamidation and deamidation of TG1, TG2 and blood coagulation factor XIII A-subunit (FXIII-A) enzymes using a panel of glutamine-containing peptide substrates. The ratio of transamidation to deamidation was enhanced at high excess of the acyl-acceptor substrate and increasing pH. In addition, it was influenced by peptide substrates as well. Whereas deamidation was favoured at low cadaverine concentrations and acidic pH, no significant effect of calcium was observed on the ratio of transamidation/deamidation. Under our experimental conditions, deamidation always occurred even at high excess of the acyl-acceptor substrate, and the reaction outcome was shifted to deamidation at neutral pH. Our results provide clear evidence of the deamidation in the TG reaction, and may serve as an important approach for analysis of deamidation to better understand the role of TGs in biological events.

摘要

转谷氨酰胺酶(TGs)是一组结构和功能相关的酶,通过蛋白质-蛋白质交联、胺掺入或脱酰胺作用,催化钙依赖性的蛋白质翻译后修饰。多年来,TG 介导的脱酰胺作用被认为是一种副反应,但最近报道了底物特异性的脱酰胺作用。在这里,我们描述了一种优化的 SDS/PAGE 测定法,用于轻松快速地监测小肽与 TG 的反应。通过密度计分析评估脱酰胺作用与转酰胺作用的相对比例,并通过纳流液相色谱-纳流电喷雾电离 MS 进行确认。我们进一步研究了反应条件对 TG1、TG2 和血液凝固因子 XIII A 亚基(FXIII-A)酶的转酰胺作用和脱酰胺作用的影响,使用了一系列含有谷氨酰胺的肽底物。在高酰基受体底物过量和增加 pH 值的情况下,转酰胺作用与脱酰胺作用的比例增加。此外,肽底物也会影响该比例。虽然在低尸胺浓度和酸性 pH 值下有利于脱酰胺作用,但在转酰胺作用/脱酰胺作用的比例上,钙离子没有显著影响。在我们的实验条件下,即使在高酰基受体底物过量的情况下,也会发生脱酰胺作用,并且在中性 pH 值下,反应结果会向脱酰胺作用转移。我们的结果提供了 TG 反应中脱酰胺作用的确凿证据,并可能成为分析脱酰胺作用以更好地理解 TGs 在生物事件中的作用的重要方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c091/6356169/48e3821696ed/FEB4-9-396-g001.jpg

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