建立了利用固相萃取-液相色谱-串联质谱同时测定水稻中17种细胞分裂素含量的分析方法。水稻样品经冷冻研磨,用甲醇-水(80∶20,v/v)溶液浸提,经聚合物阳离子交换树脂(PCX)纯化,采用 ZORBAX Extend-C18色谱柱,以甲醇和5 mmol/L甲酸铵水溶液为流动相进行梯度洗脱。采用电喷雾正离子模式电离,选择反应监测模式扫描,外标法定量。优化了色谱分离条件,研究了不同提取溶剂对17种细胞分裂素的提取效率,并考察了 PCX 固相萃取柱的纯化效果。结果表明,17种细胞分裂素在线性范围内的相关系数( r)均大于0.9984,方法检出限为0.01~0.05 ng/g。水稻根、茎和叶基质在0.2、1和5 ng/g 3个添加水平的平均回收率为60.2%~125.4%( n=6),相对标准偏差( RSD)为5.4%~29.7%。在水稻样品中检出5种细胞分裂素,其含量为0.02~0.93 ng/g。本方法纯化效果好、灵敏度高,可用于水稻中多种痕量细胞分裂素的同时分析。
A method was developed for the determination of 17 cytokinins in rice by solid phase extraction and liquid chromatography-tandem mass spectrometry. The rice samples were cryo-genically ground under liquid nitrogen and extracted with methanol-water(80∶20,v/v)at 4 ℃for 16 h. The supernatant was purified on a column packed with polymer cation exchange resin ( PCX). The samples were transported and eluted on an analytical column ZORBAX Extend-C18 (100 mm×2. 1 mm,1. 8 μm)by methanol and 5 mmol/L ammonium formate aqueous solution. All the analytes were detected in selected reaction monitoring( SRM)mode under positive elec-trospray ionization( ESI+)and quantified by external standard method. The separation condi-tions were optimized in order to achieve the sufficient separation for the several isomers of cytokinins,such as trans-zeatin-7-glucoside( tZ7G),trans-zeatin-9-glucoside( tZ9G),and trans-zeatin-O-glucoside( tZOG ). Moreover,the extraction efficiency of different extraction solvents and clean-up effects of PCX cartridge for each analyte were further investigated. The results showed that the correlation coefficients were not less than 0. 998 4 in the linear range, and the limits of detection were ranged from 0. 01 to 0. 05 ng/g. The mean recoveries of the 17 cytokinins at three spiked levels of 0. 2,1 and 5 ng/g were from 60. 2% to 125. 4% with the rela-tive standard deviations(RSDs)of 5. 4%-29. 7%(n=6). Finally,five endogenous cytokinins were successfully quantified in real sample,and their contents were between 0. 02 and 0. 93 ng/g. It means that this method is reliable for quantitative analysis of cytokinins in rice.
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