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开发一种无需衍生化的荧光检测高效液相色谱新方法,用于测定人血浆中的嘌呤核苷磷酸化酶活性。

Development of a new HPLC method using fluorescence detection without derivatization for determining purine nucleoside phosphorylase activity in human plasma.

作者信息

Giuliani Patricia, Zuccarini Mariachiara, Buccella Silvana, Rossini Margherita, D'Alimonte Iolanda, Ciccarelli Renata, Marzo Matteo, Marzo Antonio, Di Iorio Patrizia, Caciagli Francesco

机构信息

Department of Medical, Oral and Biotechnological Sciences, Laboratory of Pharmacology and Toxicology, University of Chieti-Pescara, Via dei Vestini 29, 66013 Chieti, Italy.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2016 Jan 15;1009-1010:114-21. doi: 10.1016/j.jchromb.2015.12.012. Epub 2015 Dec 10.

DOI:10.1016/j.jchromb.2015.12.012
PMID:26720700
Abstract

Purine nucleoside phosphorylase (PNP) activity is involved in cell survival and function, since PNP is a key enzyme in the purine metabolic pathway where it catalyzes the phosphorolysis of the nucleosides to the corresponding nucleobases. Its dysfunction has been found in relevant pathological conditions (such as inflammation and cancer), so the detection of PNP activity in plasma could represent an attractive marker for early diagnosis or assessment of disease progression. Thus the aim of this study was to develop a simple, fast and sensitive HPLC method for the determination of PNP activity in plasma. The separation was achieved on a Phenomenex Kinetex PFP column using 0.1% formic acid in water and methanol as mobile phases in gradient elution mode at a flow rate of 1ml/min and purine compounds were detected using UV absorption and fluorescence. The analysis was fast since the run was achieved within 13min. This method improved the separation of the different purines, allowing the UV-based quantification of the natural PNP substrates (inosine and guanosine) or products (hypoxanthine and guanine) and its subsequent metabolic products (xanthine and uric acid) with a good precision and accuracy. The most interesting innovation is the simultaneous use of a fluorescence detector (excitation/emission wavelength of 260/375nm) that allowed the quantification of guanosine and guanine without derivatization. Compared with UV, the fluorescence detection improved the sensitivity for guanine detection by about 10-fold and abolished almost completely the baseline noise due to the presence of plasma in the enzymatic reaction mixture. Thus, the validated method allowed an excellent evaluation of PNP activity in plasma which could be useful as an indicator of several pathological conditions.

摘要

嘌呤核苷磷酸化酶(PNP)活性与细胞存活和功能相关,因为PNP是嘌呤代谢途径中的关键酶,它催化核苷磷酸解为相应的碱基。在相关病理状况(如炎症和癌症)中已发现其功能异常,因此检测血浆中的PNP活性可能是早期诊断或评估疾病进展的一个有吸引力的标志物。因此,本研究的目的是开发一种简单、快速且灵敏的HPLC方法来测定血浆中的PNP活性。分离在Phenomenex Kinetex PFP柱上进行,以0.1%甲酸水溶液和甲醇为流动相,采用梯度洗脱模式,流速为1ml/min,使用紫外吸收和荧光检测嘌呤化合物。分析速度很快,因为整个运行在13分钟内完成。该方法改善了不同嘌呤的分离效果,能够对天然PNP底物(肌苷和鸟苷)或产物(次黄嘌呤和鸟嘌呤)及其后续代谢产物(黄嘌呤和尿酸)进行基于紫外的定量,具有良好的精密度和准确性。最有趣的创新是同时使用了荧光检测器(激发/发射波长为260/375nm),无需衍生化即可对鸟苷和鸟嘌呤进行定量。与紫外检测相比,荧光检测将鸟嘌呤检测的灵敏度提高了约10倍,并且几乎完全消除了由于酶促反应混合物中存在血浆而产生的基线噪声。因此,经过验证的该方法能够很好地评估血浆中的PNP活性,这可能作为几种病理状况的一个指标。

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