Simultaneous Determination of Chlorogenic Aicd, Macranthoidin B and Dipsacoside B in Lonicerae Flos by UPLC with PDA and ELSD

ZHAO Liu-cun; YE Shi-yun; YANG Chun; LIN Chang-hu; ZHAO Xun; GUO Yun

doi:10.13422/j.cnki.syfjx.2015070064

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Simultaneous Determination of Chlorogenic Aicd, Macranthoidin B and Dipsacoside B in Lonicerae Flos by UPLC with PDA and ELSD

更新时间：2024-09-23

- Simultaneous Determination of Chlorogenic Aicd, Macranthoidin B and Dipsacoside B in Lonicerae Flos by UPLC with PDA and ELSD
- Chinese Journal of Experimental Traditional Medical Formulae Vol. 21, Issue 7, Pages: 64-67(2015)
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- DOI：10.13422/j.cnki.syfjx.2015070064
  CLC： O657;R284.1
- Published：2015
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ZHAO Liu-cun, YE Shi-yun, YANG Chun, et al. Simultaneous Determination of Chlorogenic Aicd, Macranthoidin B and Dipsacoside B in Lonicerae Flos by UPLC with PDA and ELSD[J]. Chinese journal of experimental traditional medical formulae, 2015, 21(7): 64-67.
DOI：

ZHAO Liu-cun, YE Shi-yun, YANG Chun, et al. Simultaneous Determination of Chlorogenic Aicd, Macranthoidin B and Dipsacoside B in Lonicerae Flos by UPLC with PDA and ELSD[J]. Chinese journal of experimental traditional medical formulae, 2015, 21(7): 64-67. DOI： 10.13422/j.cnki.syfjx.2015070064.

摘要

目的: 建立超高效液相色谱-紫外检测器-蒸发光检测器联用(UPLC-PDA-ELSD)同时测定山银花中绿原酸、灰毡毛忍冬皂苷乙和川续断皂苷乙含量的方法

并考察贵州地区山银花的质量。方法: 采用ACQUITY UPLC BEH C18色谱柱(2.1 mm×100 mm

1.7 μm)

流动相乙腈(A)-0.4%乙酸水(B)

梯度洗脱(0~2 min

7%A;2~2.3 min

7%~28%A;2.3~10 min

28%A;10~10.5 min

28%~7%A)

梯度流速(0~2 min

0.35 mL·min-1;2~2.3 min

0.35~0.25 mL·min-1;2.3~2.6 min

0.25~0.15 mL·min-1;2.6~2.8 min

0.15~0.1 mL·min-1;2.8~4 min

0.1~0.2 mL·min-1;4~4.3 min

0.2~0.3 mL·min-1;4.3~4.5 min

0.3~0.35 mL·min-1;4.5~10.5 min

0.35 mL·min-1)

PDA(紫外检测器)检测绿原酸(330 nm);ELSD(蒸发光散射检测器)检测灰毡毛忍冬皂苷乙和川续断皂苷乙

漂移管温度60 ℃

喷雾器温度48 ℃

气体压力20 psi

色谱柱温度50 ℃。结果: 绿原酸、灰毡毛忍冬皂苷乙和川续断皂苷乙3种成分分别在0.304 5~1.522 5(R2=0.999 4)

0.449~1.436 8(R2=0.999 3)

0.044 6~0.223 μg(R2=0.999 4)呈良好的线性关系。结论: 该方法能方便准确的测定贵州山银花中绿原酸、灰毡毛忍冬皂苷乙和川续断皂苷乙的含量

并能有效缩短测量时间和节省试剂。此方法适用于测定考察贵州地区山银花的质量。

Abstract

Objective: To establish a method for determination of chlorogenic acid

galuteolin and dipsaeoside B in Lonicerae Flos using Ultra Performance Liquid Chromatography

and inspect the quality of the Lonicerae Flos in Guizhou. Method: ACQUITY UPLC BEH C18(2.1 mm× 100 mm

1.7 μm) column was adopted. Two solution were acetonitrile and water containing 0.4% acetic acid

with gradient elution of (0-2 min

7% A;2-2.3 min

7%-28% A;2.3-10 min

28% A;10-10.5 min

28%-7% A)

and velocity gradient(0-2 min

0.35 mL·min-1;2-2.3 min

0.35-0.25 mL·min-1;2.3-2.6 min

0.25-0.15 mL·min-1;2.6-2.8 min

0.15-0.1 mL·min-1;2.8-4 min

0.1-0.2 mL·min-1;4-4.3 min

0.2-0.3 mL·min-1;4.3-4.5 min

0.3-0.35 mL·min-1;4.5-10.5 min

0.35 mL·min-1). The PDA detection wavelength was 330 nm for chlorogenic aicd. The ELSD detection was for macranthoidin B and dipsacoside B. The temperature of drift tube was maintained at 60 ℃

the temperature of nebulizer was 48 ℃

with the nitrogen flow rate of 20 psi

and the column temperature was maintained at 50 ℃. Result: The linear response ranges of chlorogenic acid

galuteolin and dipsaeoside B were 0.304 5-1.522 5(R2=0.999 4)

0.449-1.436 8(R2=0.9993)

0.044 6-0.223 μg (R2=0.999 4)

respectively. Conclusion: The method is convenient and accurate to determine the content of chlorogenic acid

macranthoidin B and dipsacoside B in Lonicerae Flos

and can shorten the measuring time and saves reagent effectively. The established method has used to measure quality of the Lonicerae Flos in Guizhou.

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