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用于酪氨酸蛋白硫酸转移酶活性的荧光肽传感器。

Fluorescent peptide sensors for tyrosylprotein sulfotransferase activity.

作者信息

Zhou Wenbo, Duckworth Benjamin P, Geraghty Robert J

机构信息

Center for Drug Design, Academic Health Center, University of Minnesota, Minneapolis, MN 55455, USA.

Center for Drug Design, Academic Health Center, University of Minnesota, Minneapolis, MN 55455, USA.

出版信息

Anal Biochem. 2014 Sep 15;461:1-6. doi: 10.1016/j.ab.2014.05.025. Epub 2014 Jun 5.

DOI:10.1016/j.ab.2014.05.025
PMID:24909447
Abstract

Tyrosine sulfurylation is a post-translational modification important for protein-protein interactions in the extracellular space that are instrumental in cell adhesion, cell signaling, immune responses, and pathogen recognition of host cells. Tyrosine sulfurylation is catalyzed by the tyrosylprotein sulfotransferases (TPSTs), and in humans there are two isoforms: hTPST1 and hTPST2. The study of hTPST function and the development of small molecule probes to examine the role of hTPSTs in cell biology have been delayed by the absence of a continuous direct assay for hTPST activity. We have developed a fluorescent peptide-based assay to directly monitor tyrosine sulfurylation in real time. TPST-mediated tyrosine sulfurylation of the peptides disrupts fluorophore quenching and results in increased fluorescence emission. The assay can be used to study TPST enzymatic activity, and we show that recombinant hTPSTs are active in the absence of divalent metal ions and that optimal activity is at pH 6.0. We further show that the assay can also be used to identify inhibitors of tyrosine sulfurylation. A clear understanding of hTPST function in normal cell biology and in disease states will require the identification of small molecule inhibitors or probes to modulate enzymatic activity, and our results will facilitate that process.

摘要

酪氨酸硫酸化是一种翻译后修饰,对细胞外空间中的蛋白质-蛋白质相互作用很重要,这些相互作用在细胞黏附、细胞信号传导、免疫反应和宿主细胞的病原体识别中发挥作用。酪氨酸硫酸化由酪氨酰蛋白磺基转移酶(TPSTs)催化,在人类中有两种同工型:hTPST1和hTPST2。由于缺乏用于hTPST活性的连续直接测定方法,hTPST功能的研究以及用于研究hTPST在细胞生物学中作用的小分子探针的开发一直被推迟。我们开发了一种基于荧光肽的测定方法,以实时直接监测酪氨酸硫酸化。TPST介导的肽的酪氨酸硫酸化破坏了荧光团猝灭并导致荧光发射增加。该测定方法可用于研究TPST的酶活性,并且我们表明重组hTPST在没有二价金属离子的情况下具有活性,最佳活性在pH 6.0。我们进一步表明该测定方法还可用于鉴定酪氨酸硫酸化的抑制剂。要清楚了解hTPST在正常细胞生物学和疾病状态中的功能,需要鉴定小分子抑制剂或探针来调节酶活性,我们的结果将促进这一过程。

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