首页> 外文期刊>Analytica chimica acta >Analysis of steroids in yeast-mediated cell culture by on-line solid-phase extraction coupled high-performance liquid chromatography electrospray-ionization/mass spectrometry and novel continuous postcolumn infusion of internal standard technique
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Analysis of steroids in yeast-mediated cell culture by on-line solid-phase extraction coupled high-performance liquid chromatography electrospray-ionization/mass spectrometry and novel continuous postcolumn infusion of internal standard technique

机译:在线固相萃取-高效液相色谱电喷雾电离/质谱联用以及内标技术连续后注入新技术分析酵母介导的细胞培养物中的类固醇

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摘要

The reduction of 17-ketosteroid estrone or androstenedione to corresponding 17a- and 17β-estradiol or testosterone and epitestosterone has been performed with Saccharomyces cereuisiae. In the analysis of the cell culture, the solid-phase extraction (SPE) method was on-line coupled to high-performance liquid chromatography electrospray-ionization/mass spectrometry (HPLC-ESI/MS) for sample pretreatment to eliminate the complicated matrix interference and preconcentrate of the analytes before chromatographic separation. A novel quantification method with the continuous postcolumn infusion of internal standard was developed for the determination of substrate and products. This novel quantitative method can stabilize and enhance the ionization of all analytes during analysis. The HPLC-ESI/MS analysis of estrone, 17α-, and 17β-estradiol was operated with a negative ion mode and the analysis of androstenedione, testosterone, and epitestosterone was operated with a positive ion mode. The optimal concentration of the internal standard progesterone with the continuous postcolumn infusion technique was 3 μgmL~(-1) for estrogen analysis and 1 ng mL~(-1) for androgen analysis and both were at a constant infusion rate of 0.5 μL min~(-1). All of the linear correlation coefficients of the standard calibration curves were over 0.99 and had a linear range from 0 to 50 ngmL~(-1). The limit of detections (LODs) and the limit of quantitations (LOQs) for steroids analyzed were from 0.12 to 0.36 ngmL~(-1) and from 0.4 to 1.2 ngmL~(-1), respectively. The analysis accuracies and precisions were better than 94% and lower than 8.8% R.S.D., respectively. The developed method for the analysis of steroids in the cell culture was successful.
机译:用酿酒酵母已将17-酮类固醇雌酮或雄烯二酮还原为相应的17a-和17β-雌二醇或睾丸激素和表睾酮。在细胞培养分析中,固相萃取(SPE)方法与高效液相色谱电喷雾电离/质谱(HPLC-ESI / MS)在线耦合以进行样品预处理,从而消除了复杂的基质干扰在色谱分离之前对分析物进行预浓缩。开发了一种新的定量方法,采用柱后连续内标法测定底物和产物。这种新颖的定量方法可以稳定和增强分析过程中所有分析物的电离。雌酮,17α-和17β-雌二醇的HPLC-ESI / MS分析采用负离子模式,而雄烯二酮,睾丸激素和表睾酮的分析采用正离子模式。连续柱后输注技术测定内标孕酮的最佳浓度,雌激素分析的最佳浓度为3μgmL〜(-1),雄激素分析的最佳浓度为1 ng mL〜(-1),两者的恒定输注速率均为0.5μLmin〜。 (-1)。标准校正曲线的所有线性相关系数均超过0.99,线性范围为0至50 ngmL〜(-1)。分析类固醇的检出限(LOD)和定量限(LOQ)分别为0.12至0.36 ngmL〜(-1)和0.4至1.2 ngmL〜(-1)。分析精度和精密度分别优于R.S.D.的94%和8.8%。成功开发出的用于分析细胞培养物中类固醇的方法。

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