HPCE测定附子活性成分的血浆蛋白结合率

梁勇; 郭鹏; 陈作; 李艳灵; 郝征; 高克俭<sup>*</sup>

引用本文:	梁勇,郭鹏,陈作,李艳灵,郝征,高克俭.HPCE测定附子活性成分的血浆蛋白结合率[J].中国现代应用药学,2018,35(11):1632-1636.
	LIANG Yong,GUO Peng,CHEN Zuo,LI Yanling,HAO Zheng,GAO Kejian.Study on the Plasma Protein Combine Rate of the Active Compounds of Aconiti Lateralis Radix Praeparata by HPCE[J].Chin J Mod Appl Pharm(中国现代应用药学),2018,35(11):1632-1636.

【打印本页】【HTML】【下载PDF全文】【查看/发表评论】【EndNote】【RefMan】【BibTex】

←前一篇|后一篇→

过刊浏览高级检索

本文已被：浏览 2084次下载 1254次	码上扫一扫！
分享到：微信更多字体:加大+\|默认\|缩小-
HPCE测定附子活性成分的血浆蛋白结合率
梁勇¹, 郭鹏², 陈作¹, 李艳灵¹, 郝征³, 高克俭¹
1.天津市北辰区中医医院, 天津 300400;2.天津市儿童医院, 天津 300134;3.天津中医药大学, 天津 300193

摘要:

目的建立适用于附子生物碱类化学成分血浆蛋白结合率的方法。方法通过考察进样方式、电泳缓冲液组成等因素确定色谱条件，并采用该条件测定苯甲酰次乌头原碱、苯甲酰新乌头原碱和苯甲酰乌头原碱的血浆蛋白结合率。结果经考察确定色谱条件为：电压进样，缓冲液为100 mmol·L^-1硼砂-硼酸缓冲溶液（pH=9.0）∶甲醇=7∶3，分离电压为15 kV，检测波长为230 nm。在1，2，5 μg·mL^-1 3个剂量下，附子中苯甲酰次乌头原碱的蛋白结合率分别为（43.81±3.2）%，（42.51±3.6）%，（42.09±2.3）%；苯甲酰新乌头原碱的蛋白结合率分别为（39.59±4.0）%，（34.58±3.7）%，（37.02±3.0）%；苯甲酰乌头原碱的蛋白结合率分别为（48.23±4.6）%，（33.26±3.9）%，（32.60±3.8）%。结论超滤法结合HPCE技术可作为一种新型药物蛋白结合率测定的方法。

关键词: 高效毛细管电泳超滤附子血浆蛋白

DOI：10.13748/j.cnki.issn1007-7693.2018.11.008

分类号:R917

基金项目:天津市北辰科技发展计划重点项目（2016-SHGY-19，2015-SHGY-20）

Study on the Plasma Protein Combine Rate of the Active Compounds of Aconiti Lateralis Radix Praeparata by HPCE

LIANG Yong¹, GUO Peng², CHEN Zuo¹, LI Yanling¹, HAO Zheng³, GAO Kejian¹

1.Tianjin Beichen District Hospital of Traditional Chinese Medicine, Tianjin 300400, China;2.Tianjin Children's Hospital, Tianjin 300134, China;3.Tianjin University of Traditional Chinese Medicine, Tianjin 300193, China

Abstract:

OBJECTIVE To establish a method for evaluating the plasma protein binding rate of alkaloid in Aconiti Lateralis Radix Praeparata. METHODS The chromatography condition such as sample injection condition and the ingredient of electrophoretic buffer solution were evaluated. And the plasma protein binding rate of benzoylhypaconine, benzoylaconine and benzoylmesaconine were analyzed. RESULTS The chromatography condition was as followes:voltage injection, electrophoretic buffer solution[100 mmol·L^-1 borate saline buffer (pH=9.0):menthol=7:3], separation voltage was 15 kV, the detection wavelength was 230 nm. Within the level of 1, 2, 5 μg·mL^-1, the plasma protein binding rates of benzoylhypaconine were (43.81±3.2)%, (42.51±3.6)%, (42.09±2.3)%; the plasma protein binding rates of benzoylaconine were (39.59±4.0)%, (34.58±3.7)%, (37.02±3.0)%; and the plasma protein binding rates of benzoylmesaconine were (48.23±4.6)%, (33.26±3.9)%, (32.60±3.8)%. CONCLUSION Ultrafiltration combined with HPCE technology can be used as a new method for the analysis of plasma protein binding rate.

Key words: high performance capillary electrophoresis (HPCE) ultrafiltration Aconiti Lateralis Radix Praeparata plasma protein