Literature DB >> 27450117

Fluorometric enzymatic assay of l-arginine.

Nataliya Stasyuk1, Galina Gayda2, Hasmik Yepremyan3, Agnieszka Stepien4, Mykhailo Gonchar1.   

Abstract

The enzymes of l-arginine (further - Arg) metabolism are promising tools for elaboration of selective methods for quantitative Arg analysis. In our study we propose an enzymatic method for Arg assay based on fluorometric monitoring of ammonia, a final product of Arg splitting by human liver arginase I (further - arginase), isolated from the recombinant yeast strain, and commercial urease. The selective analysis of ammonia (at 415nm under excitation at 360nm) is based on reaction with o-phthalaldehyde (OPA) in the presence of sulfite in alkali medium: these conditions permit to avoid the reaction of OPA with any amino acid. A linearity range of the fluorometric arginase-urease-OPA method is from 100nM to 6μМ with a limit of detection of 34nM Arg. The method was used for the quantitative determination of Arg in the pooled sample of blood serum. The obtained results proved to be in a good correlation with the reference enzymatic method and literature data. The proposed arginase-urease-OPA method being sensitive, economical, selective and suitable for both routine and micro-volume formats, can be used in clinical diagnostics for the simultaneous determination of Arg as well as urea and ammonia in serum samples.
Copyright © 2016 Elsevier B.V. All rights reserved.

Entities:  

Keywords:  Enzymatic assay; Recombinant arginase I; Sulfite; Urease; l-arginine; o-Phthalaldehyde

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Year:  2016        PMID: 27450117     DOI: 10.1016/j.saa.2016.07.019

Source DB:  PubMed          Journal:  Spectrochim Acta A Mol Biomol Spectrosc        ISSN: 1386-1425            Impact factor:   4.098


  1 in total

Review 1.  Human arginase 1, a Jack of all trades?

Authors:  J Anakha; Priyanka S Kawathe; Sayantap Datta; Snehal Sainath Jawalekar; Uttam Chand Banerjee; Abhay H Pande
Journal:  3 Biotech       Date:  2022-09-07       Impact factor: 2.893

  1 in total

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