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首页> 外文期刊>Journal of Chromatography, Biomedical Applications >Extractionless method for the simultaneous high-performance liquid chromatographic determination of urinary caffeine metabolites for N-acetyltransferase 2, cytochrome P450 1A2 and xanthine oxidase activity assessment
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Extractionless method for the simultaneous high-performance liquid chromatographic determination of urinary caffeine metabolites for N-acetyltransferase 2, cytochrome P450 1A2 and xanthine oxidase activity assessment

机译:同时萃取高效液相色谱法测定尿咖啡因代谢产物的N-乙酰转移酶2,细胞色素P450 1A2和黄嘌呤氧化酶活性的无萃取方法

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摘要

Urinary metabolic ratios of caffeine are used in humans to assess the enzymatic activities of cytochrome P450 isoenzyme lA2 (CYPIA2), xanthine oxidase (XO) and for phenotyping individuals for the bimodal N-acetyltransferase 2 (NAT2), all of them involved in the activation or detoxification of various xenobiotic compounds. Most reported analytical procedures for the measurement of the urinary metabolites of caffeine include a liquid-liquid extraction of urine samples prior to their analysis by reversed-phase HPLC. At neutral to basic pH however, 5-acetylarnino-6-formylarnino-3-methyluracil (AFMU), a ~ metabolite of caffeine, spontaneously decomposes to 5-acetylamino-6-arnino-3-methyluracil (AAMU). Since AAMU is not l extracted in most organic solvents, the extent of AFMU decomposition cannot be precisely assessed. Although the : decomposition reaction can be minimized by immediate acidification of the urine, accurate results can only be obtained whenboth AAMU and AFMU are monitored, or alternatively, if AAMU is measured after complete transformation of AFMU into J AAMU in basic conditions. We report a liquid chromatographic method for the simultaneous quantitative analysis of the five , urinary metabolites of caffeine used for the CYPIA2, XO and NAT2 phenotyping studies: AAMU, AFMU, I-methylx- anthine, I-methyluric acid and 1,7:.dimethyluric acid. These metabolites are satisfactory separated from all other known caffeine metabolites as well as endogenous urinary constituents. Sample treatment does not require any liquid-liquid fex~ction procedure. Urine samples are diluted and centrifuged before being injected (10 I-Ll) onto a YMC-Pack Polyamine n (250x4.6 mm) column. A step-wise gradient elution program is applied using acetonitrile-0.75% (v/v) formic acid: i (91:9) at 0 min-+(75:25) at 25 min-+(65:35) at 35 min-+(65:35) at 45 min, followed by a re-equilibration step to the initial i solvent composition. The flow-rate is 1.0 ml/min and the separations are monitored by UV absorbance at 260 and 280 nm. The procedure described here represents a substantial improvement over previous methods: a single analysis and a minimal I' urine sample treatment enables the simultaneous quantitation of five caffeine metabolites, notably AFMU and AAMU, used f for the determination of CYP450 lA2, XO and NAT2 enzyme activity. Importantly enough, phenotyping individuals for the bimodal NAT2 is made possible without the uncertainty associated with the defonnylation of AFMU, which is likely to ~ happen at all steps prior to the analysis, during sample storage and even in the bladder of the subjects.
机译:咖啡因的尿代谢比在人类中用于评估细胞色素P450同工酶lA2(CYPIA2),黄嘌呤氧化酶(XO)的酶活以及用于双峰N-乙酰基转移酶2(NAT2)的表型分析,所有这些都涉及激活或各种异生物素化合物的解毒。大多数报道的用于测量咖啡因尿液代谢物的分析程序包括尿液样品的液-液萃取,然后通过反相HPLC分析。然而,在中性至碱性pH值下,咖啡因的一种代谢物5-乙酰氨基-6-甲酰基氨基-3-甲基尿嘧啶(AFMU)自发分解为5-乙酰氨基-6-氨基3-3-甲基尿嘧啶(AAMU)。由于AAMU不能在大多数有机溶剂中提取,因此无法精确评估AFMU的分解程度。尽管可以通过立即尿液酸化来最大程度地降低分解反应,但只有在同时监测AAMU和AFMU的情况下,或者在碱性条件下将AFMU完全转化为J AAMU后再测量AAMU时,才能获得准确的结果。我们报告了一种液相色谱方法,用于同时定量分析用于CYPIA2,XO和NAT2表型研究的咖啡因的五种尿液代谢物:AAMU,AFMU,I-甲基x-蒽基,I-甲基尿酸和1,7:。二甲基尿酸。这些代谢物与所有其他已知的咖啡因代谢物以及内源性尿液成分分离令人满意。样品处理不需要任何液液交换程序。将尿液样品稀释并离心,然后将其注射(10 I-L1)到YMC-Pack多胺n(250x4.6 mm)色谱柱上。使用乙腈-0.75%(v / v)甲酸:0分钟下的i(91:9)-+(75:25)下25分钟-+(65:35)于35分钟应用逐步梯度洗脱程序在45分钟时达到+-(65:35),然后重新平衡至初始溶剂组成。流速为1.0 ml / min,并通过260和280 nm处的UV吸光度监控分离。这里描述的程序代表了对先前方法的实质性改进:一次分析和最少的I'尿液样品处理就可以同时定量五种咖啡因代谢物,特别是AFMU和AAMU,用于测定CYP450 IA2,XO和NAT2酶活动。足够重要的是,在没有与AFMU脱甲酰化相关的不确定性的情况下,使双峰型NAT2的表型化成为可能,这可能在分析之前的所有步骤,样品存储期间甚至受试者的膀胱中发生。

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