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纸质出版日期:2017
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梁军, 孙黎明, 夏永刚, 等. 亲水作用色谱-质谱法测定麻黄根多糖单糖的组成[J]. 中国实验方剂学杂志, 2017,23(7):73-78.
LIANG Jun, SUN Li-ming, XIA Yong-gang, et al. Analysis of Monosaccharide Compositions of Ephedrae Radix et Rhizoma Polysaccharide Based on UPLC-MS/MS[J]. Chinese journal of experimental traditional medical formulae, 2017, 23(7): 73-78.
梁军, 孙黎明, 夏永刚, 等. 亲水作用色谱-质谱法测定麻黄根多糖单糖的组成[J]. 中国实验方剂学杂志, 2017,23(7):73-78. DOI: 10.13422/j.cnki.syfjx.2017070073.
LIANG Jun, SUN Li-ming, XIA Yong-gang, et al. Analysis of Monosaccharide Compositions of Ephedrae Radix et Rhizoma Polysaccharide Based on UPLC-MS/MS[J]. Chinese journal of experimental traditional medical formulae, 2017, 23(7): 73-78. DOI: 10.13422/j.cnki.syfjx.2017070073.
目的:建立一种亲水相互作用色谱-质谱(HILIC-UPLC-MS/MS)检测分析方法,用于直接检测麻黄根多糖的单糖组成。方法:采用ACQUITY UPLC BEH Amide色谱柱(2.1 mm×100 mm,1.7 μm),流动相A为乙腈-水(95:5),B为乙腈-水(5:95),柱温60℃,梯度洗脱(0~10 min,92%~70% A;10~10.1 min,70%~92% A;10.1~15 min,92% A),进样量2 μL,流速0.2 mL·min-1;质谱采用电喷雾离子源,负离子模式下多反应离子检测。Turbo V离子源参数如下:毛细管电压-4.5 kV,源温度550℃;气帘气和碰撞气压力分别设为30 psi和10 psi;雾化气和气化气压力均为55 psi,碰撞电池入口电位和出口电位均为-10 V。结果:该方法在12 min内实现8种未衍生单糖成分的完全基线分离,精密度、稳定性和重复性的RSD均<2.1%,各成分的回收率在99.3%~102.5%,RSD在1.5%~2.9%,应用上述建立的方法分别对5批麻黄根多糖进行单糖组成分析,结果显示,麻黄根中检测到5种单糖分别为L-鼠类糖,L-阿拉伯糖,D-甘露糖,D-半乳糖,D-半乳糖醛酸。结论: HILIC-UPLC-MS/MS方法灵敏度高、重复性好、快速、准确、样品前处理简单、无需衍生化,可用于植物多糖中单糖及寡糖的快速检测。
Objective: To establish an analysis method for direct detection of monosaccharide compositions of Ephedrae Radix et Rhizoma polysaccharide by HILIC-LC-MS/MS. Method: The separation was performed on ACQUITY UPLC BEH Amide column (2.1 mm×100 mm
1.7 μm) with 95%acetonitrile (A)-95% water (B) as the mobile phase for gradient elution (0-10 min
92%-70% A; 10-10.1 min
70%-92% A; 10.1-15 min
92%A) at a flow rate of 0.2 mL·min-1. The injection volume was 2 μL
and the column temperature was 60℃. In mass spectrometry
electrospray ion source was used:multiple reaction ion monitoring mode (MRM) under the negative ion. Turbo V ion source parameters were common to all analytes
as follows:the capillary voltage was -4.5 kV
and the source temperature was at 550℃. The curtain gas and collision gas setting were 30 psi and 10 psi
respectively. The pressure for nebulization gas and vaporization gas setting were 55 psi. The entrance potential (EP) and collision cell exit (CXP) were all -10 V. Result: Eight monosaccharide components were separated clearly within 12 min. The RSD values of precision
stability and reproducibility were all less than 2.1%. The average recoveries were 99.3%-102.5%
with RSD of 1.5%-2.9%. The developed method has been successfully applied to determine the major saccharides in 5 Ephedra Radixet Rhizoma polysaccharide samples. It was clear that the predominant composition monosaccharide in Ephedra Radixet Rhizoma polysaccharides were Rha
Ara
Man
Gal and GalUA. Conclusion: The established method for determination of the eight monosaccharides is stable
reliable
accurate
and reproducible
its sample pre-treatment is simple
without derivatization
and can be used for rapid detection of monosaccharide compositions in plant polysaccharide.
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