首页> 外文期刊>Journal of Pharmaceutical and Biomedical Analysis: An International Journal on All Drug-Related Topics in Pharmaceutical, Biomedical and Clinical Analysis >Simultaneous determination of bilirabin and its giucuronides ie liver microsomes aed recombieant UGT1A1 enzyme incubation systems by HPLC method and its application to bilirabin glucuroeidation studies
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Simultaneous determination of bilirabin and its giucuronides ie liver microsomes aed recombieant UGT1A1 enzyme incubation systems by HPLC method and its application to bilirabin glucuroeidation studies

机译:高效液相色谱法同时测定胆红素及其菊酯类化合物,即肝微粒体和UGT1A1重组酶温育系统,并将其应用于胆红素葡萄糖苷酸化研究

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摘要

Bilirubin, an important endogenous substances and liver function index in humans, is primarily eliminated via UGT1A1 -catalyzed glucuronidation. Instability of bilirubin and its giucuronides brings substantial technical challenges to conduct in vitro bilirubin glucuronidation assay. In the present study, we developed a simple and robust HPLC method for simultaneous determination of unconjugated bilirubin (UCB) and its multiple giucuronides, i.e. bilirubin monoglucuronides (BMGs, including BMG1 and BMG2 isomers) and diglucuronide (BDG) in rat liver microsomes (RLM), human liver microsomes (HLM) and recombinant human UGT1A1 enzyme (UGT1A1) incubation systems, and applied it to study in vitro bilirubin glucuronidation. UCB, BMG1, BMG2, BDG and their isomers in the incubation mixtures were successfully separated using a C18 column with UV detection at 450 nm and mobile phase consisted of 0.1% formic acid in water and acetonitrile by a linear gradient elution program. Assay linearities of bilirubin were confirmed in the range 0.01-2 muM. Precision of UCB, BMG1, BMG2 and BDG (n = 5) at low, medium and high concentration was within the range of RSD 0.4-3.7%, accuracy expressed in the mean assay recoveries of them (n = 5) ranged from 92.8 ± 1.5% to 104.3 ± 2.2% for intra- and inter-day assays and the mean extraction recoveries of them (n = 5) were above 91.5 ± 1.0%. Stability of bilirubin and its giucuronides was satisfactory at 37 °C in the incubation solutions during the reaction (30 min), 25degC for 24 h and -70 °C for 7 d in the processed incubation samples with methanol. Furthermore, we established stable, reliable in vitro incubation systems and optimized the incubation conditions to characterize the kinetics of bilirubin glucuronidation by RLM, HLM and UGT1A1, respectively. The kinetic parameters of formation of total bilirubin giucuronides (TBG, the sum of BMG1, BMG2 and BDG) were as follows: K_m of 0.45 ± 0.016,0.40 ± 0.022,0.44 ± 0.018 muM, V_(max) of 2.65 ± 0.057,1.86 ± 0.029,2.95 ± 0.036 nmoi/mg/min, CL_(int) of 5.92 ±0.22,4.70 ±0.079,6.72 ±0.27 mL/mg/min by RLM, HLM and UGT1A1, respectively. Bilirubin glucuronidation obeyed the Hill equation by RLM and the Michaelis-Menten equation by HLM and UGT1A1 in the range of substrate concentration selected, respectively. In addition, the relative proportions between BDG and BMGs were in connection with enzyme sources (e.g. RLM, HLM and UGT1A1) and bilirubin concentration.
机译:胆红素是人类重要的内源性物质和肝功能指标,主要通过UGT1A1催化的葡萄糖醛酸化作用消除。胆红素及其菊酯的不稳定性给进行体外胆红素葡萄糖醛酸化测定带来了巨大的技术挑战。在本研究中,我们开发了一种简单而强大的HPLC方法,用于同时测定大鼠肝微粒体(RLM)中未结合的胆红素(UCB)及其多种giucuronides,即胆红素单葡糖醛酸内酯(BMG,包括BMG1和BMG2异构体)和diglucuronide(BDG) ),人肝微粒体(HLM)和重组人UGT1A1酶(UGT1A1)培养系统,并将其用于体外胆红素葡萄糖醛酸化研究。使用C18色谱柱,在450 nm处进行UV检测,成功分离了孵育混合物中的UCB,BMG1,BMG2,BDG及其异构体,通过线性梯度洗脱程序,流动相由0.1%甲酸的水溶液和乙腈组成。胆红素的测定线性被证实在0.01-2μM的范围内。低,中和高浓度下UCB,BMG1,BMG2和BDG(n = 5)的精密度在RSD 0.4-3.7%的范围内,以它们的平均测定回收率(n = 5)表示的准确度为92.8±日间和日间测定的1.5%至104.3±2.2%,它们的平均提取回收率(n = 5)高于91.5±1.0%。在反应过程中(30分钟),在孵育溶液中37℃,在25℃下处理24小时和-70℃下在处理过的含有甲醇的孵育样品中,胆红素及其giucuronides的稳定性令人满意。此外,我们建立了稳定,可靠的体外培养系统,并优化了培养条件以表征分别通过RLM,HLM和UGT1A1进行的胆红素葡萄糖醛酸化动力学。形成总胆红素giucuronides(TBG,BMG1,BMG2和BDG之和)的动力学参数如下:K_m为0.45±0.016,0.40±0.022,0.44±0.018μM,V_(max)为2.65±0.057,1.86通过RLM,HLM和UGT1A1分别获得的±0.029,2.95±0.036 nmoi / mg / min,CL_(int)为5.92±0.22,4.70±0.079,6.72±0.27 mL / mg / min。在所选底物浓度范围内,胆红素葡萄糖醛酸化分别遵循RLM的Hill方程和HLM和UGT1A1的Michaelis-Menten方程。此外,BDG和BMG之间的相对比例与酶源(例如RLM,HLM和UGT1A1)和胆红素浓度有关。

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