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聚焦于罗非鱼天冬氨酸氨肽酶的功能特征研究。

Focusing on the functional characterization of the anserinase from Oreochromis niloticus.

机构信息

Institute of Biostructure and Bioimaging, CNR, Napoli, Italy.

Institute of Biostructure and Bioimaging, CNR, Catania, Italy; Department of Chemical Sciences, University of Catania, Catania, Italy.

出版信息

Int J Biol Macromol. 2019 Jun 1;130:158-165. doi: 10.1016/j.ijbiomac.2019.02.118. Epub 2019 Feb 22.

Abstract

Carnosine, anserine and homocarnosine are the three most representative compounds of the histidine dipeptides family, widely distributed in mammals in different amounts depending on the species and the tissue considered. Histidine dipeptides are mainly degraded by two different carnosinase homologues: a highly specific metal-ion dependent carnosinase (CN1) located in serum and brain and a non-specific cytosolic form (CN2). The hydrolysis of such dipeptides in prokaryotes and eukaryotes is also catalyzed by the anserinase (ANSN). Such naturally occurring dipeptides represent an interesting topic because they seem to have numerous biological roles such as potential neuroprotective and neurotransmitter functions in the brain and therefore ANSN results to be a very interesting target of study. We here report, for the first time, cloning, expression of ANSN from the fish Oreochromis niloticus both in a mammalian and in a prokaryotic system, in order to perform deep functional studies by enzymatic assays in the presence of different metals and substrates. Furthermore, by means of a mass spectrometry-based proteomic approach, we analysed protein sequence and the potential presence of post-translational modifications in the mammalian recombinant protein. Finally, a preliminary structural characterization was carried out on ANSN produced in Escherichia coli.

摘要

肌肽、鹅肌肽和同型肌肽是组氨酸二肽家族中最具代表性的三种化合物,广泛分布于哺乳动物中,其含量因物种和组织而异。组氨酸二肽主要通过两种不同的肌肽酶同工酶降解:一种高度特异性的金属离子依赖型肌肽酶(CN1),位于血清和大脑中,另一种是非特异性的胞质形式(CN2)。原核生物和真核生物中二肽的水解也由鹅肌肽酶(ANSN)催化。这些天然存在的二肽是一个有趣的研究课题,因为它们似乎具有许多生物学功能,如在大脑中具有潜在的神经保护和神经递质功能,因此 ANSN 是一个非常有趣的研究目标。我们首次从鱼类奥利亚罗非鱼中克隆和表达了 ANSN,分别在哺乳动物和原核系统中表达,以便在存在不同金属和底物的情况下通过酶促分析进行深入的功能研究。此外,我们还通过基于质谱的蛋白质组学方法分析了哺乳动物重组蛋白的序列和潜在的翻译后修饰。最后,对大肠杆菌中产生的 ANSN 进行了初步的结构特征分析。

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