CN100340255C - 丹皮有效组分及制备方法 - Google Patents
丹皮有效组分及制备方法 Download PDFInfo
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- CN100340255C CN100340255C CNB2005100604375A CN200510060437A CN100340255C CN 100340255 C CN100340255 C CN 100340255C CN B2005100604375 A CNB2005100604375 A CN B2005100604375A CN 200510060437 A CN200510060437 A CN 200510060437A CN 100340255 C CN100340255 C CN 100340255C
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Abstract
本发明提供一种丹皮有效组分,其活性成分的百分含量为芍药苷10~25%,没食子酰芍药苷40~55%,牡丹皮苷h30~45%;制备方法是将丹皮药材粉碎后加热提取,将提取液浓缩成浸膏,与硅胶进行拌样,用正相硅胶柱对其进行分离,将洗脱液浓缩干燥后得样品,用制备液相色谱继续分离得到的有效组分。本发明的丹皮有效组分加入药用添加剂按照药剂学允许的制备方法制成药用制剂并在制备治疗、预防心血管疾病药物中的应用。本发明方法使用了正相硅胶柱,能有效地除去糖、蛋白质、氨基酸等杂质,提高有效成分的含量,能快速准确的得到有效成分,在生产中更易于药物的质量控制。
Description
技术领域
本发明涉及中药提取物,具体地说涉及从丹皮中提取的有效组分及其制备方法,该有效组分主要含有芍药苷、没食子酰芍药苷、牡丹皮皂甙h(Mudanpioside h)三种化合物。
背景技术
冠心病和心绞痛是危害人类健康的“第一杀手”,近年来,随着我国人口老年化以及人们工作、生活、饮食结构及环境等的变化,冠心病等心脑血管疾病的发生率也逐年增多,严重威胁着人民的身心健康。天然产物中许多活性物质具有抗心肌缺血、缺氧作用,其中一些已开发成治疗冠心病和心绞痛的新药,如治疗冠心病的药物地奥心血康,它是由从中药中提取的8种甾体皂甙制成的纯中药制剂;心达康是以沙棘为原料提取加工而成的纯天然药物,其有效成分为沙棘总黄酮。因而从天然产物中寻找具有抗心肌缺血、缺氧生理活性的有效物质,是发现、开发新药的有效途径之一。我国药用生物资源十分丰富,其生理活性物质是研究和发现新药先导化学物,开发新药的天然宝库。目前,我国从天然产物中提取活性物质,用于开发成治疗冠心病、安全性好、毒性低的新药还很少,从天然产物中提取活性物质,开发成具有抗心肌缺血,用于治疗冠心病和心绞痛的新药,具有重要应用价值和广阔发展前景。
丹皮又名牡丹皮,系双子叶植物药毛茛科植物牡丹(Paeoniasuffruticosa Andr.)的根皮。分布河北、河南、山东、四川、陕西、甘肃等地。全国各地均有栽培,药材主产安徽、四川、甘肃、陕西、湖北、湖南、山东、贵州等地,此外,云南、浙江亦产。其性微寒,味辛苦,凉,入心、肝、肾经,具有清热,凉血,和血,消瘀的功效。丹皮炮制最早见于我国梁代陶宏景所撰《集注》中,认为: “皆促破,去心。”《本草纲目》等医书中记载“丹皮木心不入药,需去之。”研究表明:丹皮含丹皮酚(Paeonol)、芍药甙(Paeoniflorin)、羟基芍药甙、苯甲酰芍药甙(Benzoylpaeonifforin)、苯甲酰羟基芍药甙、芍药苷元(Paeoniflorigenone)、6-羟基香豆素(6-hydroxycoumarin)和没食子酸(GallicAcid),以及苯甲酸、植物甾醇、蔗糖、葡萄糖、阿拉伯糖等。挥发油中含有苯甲酸(Benzoic Acid)、十四烷烃(Tetradecane)、2-羟基-4-甲氧基-苯乙酮(2-hydroxy-4-methoxy acetophenone)、2,6-双特丁基对苯醌(2,6-ditert-butyl-p-Benzoquinone)、邻苯二甲酸二乙酯(Diethyl Phthalate)、十四酸异丙酯(Isopropyl Myristate)等化合物(陈悦娇等,广州食品工业科技,2002,1 8(4):36-37)。吴少华等人首次从丹皮中分离得到了以下五种化合物:白桦脂酸(Betulinic Acid)、白桦脂醇(Betulin),齐墩果酸(Oleanolic Acid)、3β,23-dihydroxy-30-norolean-12,20(29)-dien-28-oic acid、3-O-methylpaeonisuffral(吴少华等,中草药,2002,33(8):679-680)。
丹皮对实验性心肌缺血有减轻损伤程度作用,并能够降低心肌耗氧量,增加冠脉流量,认为丹皮有调节血行,疏通血脉之作用,因而对心肌缺血有保护作用(马玉玲等,山西医药杂志,1984,13(4):212-214)。芍药苷有抗血小板聚集作用,抗血栓形成的作用,对肝脏的保护作用和抗肿瘤作用。芍药苷对心肌细胞Ica、L有阻断作用(张广欣等,中国药理学通报,2003,19(8):863-866)。芍药苷可增加神经细胞存活数量,降低死亡率,对抗KA所致的兴奋性神经损伤(吴玉梅等,中国药理学与毒理学杂志,2002,16(3):172-175)。芍药苷对钙超载所致PC12细胞损伤有显著的保护作用(杨军等,中国新药杂志,2001,10(6):426-428)。芍药苷增强血虚证小鼠骨髓造血干祖细胞的集落形成能力;芍药苷可促进骨髓基质细胞分泌造血因子(G-CSF,GM-CSF,PDGF-α)等,抑制造血抑制因子(M-CIP)的分泌(高月,天津中医药,2003,20(6):47-51)。
发明内容
本发明的目的是提供一种丹皮有效组分,活性成分有芍药苷、没食子酰芍药苷、牡丹皮皂甙h(Mudanpioside h)三种化合物。
本发明方法提供的丹皮有效组分中,芍药苷的含量为10~25%,没食子酰芍药苷的含量为40~55%,牡丹皮苷h(Mudanpioside h)的含量为30~45%。
优选的丹皮有效组分中,芍药苷的含量为12~21%没食子酰芍药苷的含量为42~51%,牡丹皮苷h(Mudanpioside h)的含量为32~4 1%。
最佳的丹皮有效组分中,芍药苷的含量为14~18%,没食子酰芍药苷的含量为44~48%,牡丹皮苷h(Mudanpioside h)的含量为34~38%。
本发明的另一个目的是提供丹皮有效组分的制备方法,通过以下技术方案实现:
将丹皮药材粉碎后加入乙酸乙酯和乙醇,加热提取得提取液,将提取液浓缩成浸膏,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品;用制备液相色谱继续分离得到的有效组分;制备色谱的分离条件:色谱柱为半制备柱,流动相为水和乙腈,梯度洗脱,收集溶液,溶液经浓缩干燥后得到有效组分。
优选的丹皮有效组分制备方法通过以下步骤实现:将丹皮药材粉碎后加入乙酸乙酯和乙醇(1∶0.8~1.2),加热回流0.8~1.2小时,提取1~3次,合并滤液得提取液,将提取液浓缩成浸膏,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯(47~53∶1)作为流动相,得洗脱液I,弃之然后改换氯仿和甲醇(8~13∶1)作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品;用制备液相色谱继续分离得到的有效组分;制备色谱的分离条件:色谱柱为半制备柱,流动相为水和乙腈,梯度洗脱,流速为2.8~3.2ml/min,柱温为室温。收集溶液,溶液经浓缩干燥后得到有效组分。
最佳的丹皮有效组分制备方法通过以下步骤实现:将丹皮药材粉碎后加入乙酸乙酯和乙醇(1∶1),加热回流1小时,提取2次,合并滤液得提取液;将提取液浓缩成浸膏,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯(50∶1)作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇(10∶1)作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品;用制备液相色谱继续分离得到的有效组分;制备色谱的分离条件:色谱柱为半制备柱(Lichrospher C18;10.0mm×250mm,5μm),流动相为水(A)和乙腈(B),梯度洗脱程序如下:0分钟时,流动相A为80%的水溶液、流动相B为20%的乙腈溶液;40分钟时,流动相A为20%的水溶液、流动相B为80%的乙腈溶液;50分钟时,流动相A为5%的水溶液、流动相B为95%的乙腈溶液;流速为3ml/min,柱温为室温;样品用100%乙醇溶解,经制备液相色谱分离,在时间段1 4.2~18.4min收集溶液,溶液经浓缩干燥后得到有效组分。
本发明的另一个目的是提供该丹皮有效组分加入药用添加剂按照药剂学允许的制备方法制成药用制剂。
本发明的又一个目的是提供该丹皮有效组分及其制剂在制备治疗、预防心血管疾病药物中的应用。
本发明的有益之处是:从丹皮中提取分离的方法,使用了正相硅胶柱,能有效地除去糖、蛋白质、氨基酸等杂质,提高有效成分的含量,同时在制备方法中采用了制备色谱,能快速准确的得到有效成分。本发明提供的丹皮有效组分,对心肌缺血有保护作用,其化学成分简单明确,在药理研究上更易于阐明其作用机制,在生产中更易于药物的质量控制。
附图说明
图1为本发明丹皮有效组分的HPLC分析图。
具体实施方式
下面将结合本发明的实施例进一步详细说明本发明的实质内容,该实施例仅用于说明本发明而对本发明并没有限制。
实施例一 丹皮有效组分的制备工艺
将200g丹皮药材粉碎后加入乙酸乙酯和乙醇,加热提取得提取液,将提取液浓缩成浸膏16.8g,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离首先用石油醚和乙酸乙酯作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品3.9g;用制备液相色谱继续分离得到的样品;制备色谱的分离条件:色谱柱为半制备柱,流动相为水和乙腈,梯度洗脱。样品用100%乙醇溶解,经制备液相色谱分离,在时间段14.2~18.4min收集溶液,浓缩干燥后得到有效组分0.40g。
实施例二 丹皮有效组分的制备工艺
将500g丹皮药材粉碎后加入乙酸乙酯和乙醇(1∶0.8~1.2),加热回流0.8~1.2小时,提取1~3次,合并滤液得提取液,将提取液浓缩成浸膏42g,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯(47~53∶1)作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇(8~13∶1)作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品11.8g;用制备液相色谱继续分离得到的样品;制备色谱的分离条件:色谱柱为半制备柱,流动相为水和乙腈,梯度洗脱,流速为2.8~3.2ml/min,柱温为室温。样品用100%乙醇溶解,经制备液相色谱分离,在时间段14.2~18.4min收集溶液,浓缩干燥后得到有效组分1.04g。
实施例三 丹皮有效组分的制备工艺
取丹皮药材250g,将其粉碎后加入乙酸乙酯和乙醇(1∶1),加热回流1小时,提取2次,滤液合并得提取液。将提取液浓缩成浸膏得22g,将浸膏和硅胶拌样,用正相硅胶柱进行分离,首先用石油醚和乙酸乙酯(50∶1)作为流动相,得洗脱液I,然后改换氯仿和甲醇(10∶1)作为流动相,得洗脱液II,浓缩干燥后得6.2g样品。用制备液相色谱继续分离得到的样品。制备色谱的分离条件:色谱柱为汉邦半制备柱(Lichrospher C18;10.0mm×250mm,5μm),流动相为水(A)和乙腈(B),洗脱梯度见表2,流速为3ml/min,柱温为室温。样品用100%乙醇溶解,经制备液相色谱分离,在时间段14.2~1 8.4min收集溶液,浓缩干燥后得到有效组分0.58g。
实施例四 丹皮有效组分的分析
(1)上述丹皮提取物中芍药苷、没食子酰芍药苷、牡丹皮苷h(Mudanpioside h)、的含量测定(高效液相色谱法)
色谱条件 色谱柱Agilent Zorbax SB-C18柱(4.6mm×150mm,5μm);采用梯度洗脱,流动相A相为0.2%冰醋酸水溶液,流动相B相为含0.2%冰醋酸的乙腈溶液;梯度洗脱程序如下:0分钟时,流动相A为90%的0.2%冰醋酸水溶液、流动相B为10%的0.2%冰醋酸的乙腈溶液;10分钟时,流动相A为50%的0.2%冰醋酸水溶液、流动相B为50%的0.2%冰醋酸的乙腈溶液;30分钟时流动相A为5%的0.2%冰醋酸水溶液、流动相B为95%的0.2%冰醋酸的乙腈溶液;流速0.5mL·min-1;检测波长全波长;柱温30℃;ELSD条件:漂移管温度100℃;氮气流速1.4L/min
供试品溶液的制备 称取本品,用甲醇溶液溶解在容量瓶中,稀释至刻度,摇匀,即得。
测定方法 精密吸取供试品溶液,注入液相色谱仪,测定,即得。
(2)上述丹皮提取物HPLC-ELSD指纹图谱
测定方法 参见(1)上述丹皮提取物中的芍药苷、没食子酰芍药苷、牡丹皮苷h(Mudanpioside h)含量测定(高效液相色谱法)。记录色谱时间为30分钟。
分析结果 丹皮有效组分的HPLC-ELSD分析谱图见图1,图1中的1、2、3号峰,分别是芍药苷、Mudanpioside h和没食子酰芍药苷。三个峰的相对保留时间依次为9.8(芍药苷),10.67(没食子酰芍药苷),10.97(牡丹皮苷h)。
本发明中,芍药苷的结构式为:
本发明中,没食子酰芍药苷的结构式为:
本发明中,牡丹皮苷h(Mudanpioside h)的结构式为:
实施例五 丹皮有效组分制剂
取实施例三的丹皮有效组分0.5g与10.5g聚乙二醇-6000混合均匀,加热熔融,化料后移至滴丸滴灌中,药液滴至6~8℃液体石蜡中,除油,制得滴丸400粒。
实施例六 丹皮有效组分制剂
取实施例三的丹皮有效组分0.5g、葡萄糖4.5g、硫代硫酸钠0.9g和蒸馏水1ml,上述组分混合均匀后,冷冻干燥,分装500支,即得。
实施例七 丹皮有效组分制剂
取降香油1.5g,加入到13ml饱和的羟丙基β-环糊精中,搅拌溶解,滤过,滤叶低温干燥,的降香油和羟丙基β-环糊精的包合物粉末。除上述降香油合羟丙基β-环糊精的包合物粉末外,再取实施例三的丹皮提取物0.5g、甘露醇5.5g、依地酸钙钠0.9g和蒸馏水2ml,上述组分混匀后,冷冻干燥,分装300支,即得。
实施例八 丹皮有效组分的药理实验
药理模型:乳鼠心肌细胞缺血缺氧模型
原代心肌细胞培养 出生1~3天SD乳鼠处死后,取心脏,经PBS液清洗后减成1mm3左右的碎块。用0.125%胰蛋白酶(Sigma,USA)+0.05%胶原酶II(Gibco,USA)于37度消化3~4次。差速贴壁法分离成纤维细胞1.5小时后,细胞悬液转移至48孔板中(每孔约4×105细胞)。经DMEM(Gibco,USA)加10%胎牛血清(Falcon,USA)培养3-6天的细胞供药效筛选。筛选前1天替换为无血清培养液。培养3~6天的心肌细胞,PBS洗涤后加入含药培养液。置于95%N2和5%CO2培养箱中缺氧6小时。然后在CO2培养箱中复氧3小时。取细胞上清液测定LDH含量。
给药方案 提取得到的丹皮有效组分用无糖Hanks液配成10-4g/mL供试液,脂溶性成分可加入少量DMSO助溶(DMSO终浓度控制在0.2%以下)。各组分在培养液中的终浓度控制在10-5g/mL。
乳酸脱氢酶含量测定 细胞培养液中乳酸脱氢酶含量能够表示细胞损伤程度。漏入上清液中的乳酸脱氢酶含量越高,表明细胞损伤也显著。乳酸脱氢酶测定试剂盒购自南京建成生物工程研究所。测定方法为:取30微升细胞上清液,加入50微升基质缓冲液及10微升乳酸脱氢酶辅酶,37度振荡15分钟,再加入50微升2,4-二硝基苯肼,37度振荡15分钟。平行空白。取反应液50微升加入200微升0.4mol/L氢氧化钠溶液,静置3~4分钟后,用酶标仪于450nm测定光度值。
药效结果
所有数据用均值±方差表示。采用单边方差分析和T检验进行统计学分析。与模型组相比,P<0.05认为显著有效。药效结果见表1。根据心肌细胞乳酸脱氢酶(LDH)检测结果,丹皮有效组分对降低LDH释放有非常显著效果。
表1
| Mean | Std | P | |
| 丹皮有效组分 | 0.1355 | 0.031522 | 0.003716 |
| 模型组 | 0.22575 | 0.032887 |
实施例九 丹皮有效组分的又一个药理实验
药理模型:脐静脉内皮细胞缺氧复氧模型
原代脐静脉内皮细胞培养 取健康新生儿脐带,用30~50mlHanks液洗净静脉血管内的残留血迹。视脐带长度加入相应量的0.1%胶原酶I,转入培养箱消化15~20分钟。随后将脐带内消化液小心收集到烧杯中,并用Hanks液将烧杯润洗两次,一并收集到烧杯中分装于离心管,900rpm离心10分钟。吸去上清液,用M199培养液(含10%胎牛血清,100U/ml双抗,0.15mg/ml Heparin,10uMVC)充分溶解沉淀。将所得细胞悬液分装于5cm2培养瓶,置于培养箱内培养。第二天换成采用含30ug/ml ECGS的M199培养液,之后每三天换一次培养液直至细胞铺满底面。所用细胞均为原代内皮细胞。造模前将培养瓶内细胞接种至96孔板并培养一天,所用细胞量为3.5~4万/孔。造模时,吸弃旧的M199培养液,加入含药无酚红M199培养液,每孔总量为100ul。置于95%N2和5%CO2培养箱中缺氧12小时,然后在CO2培养箱中复氧2小时。取细胞上清液测定LDH含量和NO含量。
给药方案 提取得到的丹皮有效组分用无糖Hanks液配成10-4g/mL供试液,脂溶性成分可加入少量DMSO助溶(DMSO终浓度控制在0.2%以下)。各组分在无酚红M199培养液中的终浓度控制在10-5g/mL。
乳酸脱氢酶含量测定 细胞培养液中乳酸脱氢酶含量能够表示细胞损伤程度。漏入上清液中的乳酸脱氢酶含量越高,表明细胞损伤也显著。乳酸脱氢酶测定试剂盒购自南京建成生物工程研究所。测定方法为:取30微升细胞上清液,加入50微升基质缓冲液及10微升乳酸脱氢酶辅酶,37度振荡15分钟,再加入50微升2,4-二硝基苯肼,37度振荡15分钟。平行空白。取反应液50微升加入200微升0.4mol/L氢氧化钠溶液,静置3~4分钟后,用酶标仪于450nm测定光度值。
药效结果 所有数据用均值±方差表示。采用单边方差分析和T检验进行统计学分析。与模型组相比,P<0.05认为显著有效。药效结果见表2。根据内皮细胞乳酸脱氢酶检测结果,丹皮有效组分对降低LDH释放有非常显著效果。
表2
| 组分 | Mean | Std | P |
| 丹皮有效组分模型组 | 0.1040.122 | 0.0160.006 | 0.049 |
无需进一步详细阐述,相信采用前面所公开的内容,本领域技术人员可最大限度地应用。因此,前面的优选具体实施方案应被理解为仅是举例说明,而非以任何方式限制本发明的范围。
Claims (10)
1.一种丹皮有效组分,活性成分有芍药苷、没食子酰芍药苷、牡丹皮皂甙h,其特征是:芍药苷的含量为10~25%,没食子酰芍药苷的含量为40~55%,牡丹皮苷h的含量为30~45%。
2.根据权利要求1所述的的丹皮有效组分,其特征是:芍药苷的含量为12~21%,没食子酰芍药苷的含量为42~51%,牡丹皮苷h的含量为32~41%。
3.根据权利要求1所述的的丹皮有效组分,其特征是:芍药苷的含量为14~18%,没食子酰芍药苷的含量为44~48%,牡丹皮苷h的含量为34~38%。
4.根据权利要求1-3任一所述的丹皮有效组分的制备方法,其特征是:通过以下技术方案实现:将丹皮药材粉碎后加入乙酸乙酯和乙醇,加热提取得提取液,将提取液浓缩成浸膏,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品,用制备液相色谱继续分离得到的有效组分,制备色谱的分离条件为色谱柱采用半制备柱,流动相为水和乙腈,梯度洗脱。
5.根据权利要求1-3任一所述的丹皮有效组分的制备方法,其特征是:通过以下技术方案实现:将丹皮药材粉碎后加入乙酸乙酯和乙醇=1∶0.8~1.2,加热回流0.8~1.2小时,提取1~3次,合并滤液得提取液,将提取液浓缩成浸膏,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯=47~53∶1作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇=8~13∶1作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得有效组分,用制备液相色谱继续分离得到的有效组分。
6.根据权利要求5所述的丹皮有效组分的制备方法,其特征是:制备色谱的分离条件为色谱柱采用半制备柱,流动相为水和乙腈,梯度洗脱,流速为2.8~3.2ml/min,柱温为室温。
7.根据权利要求1-3任一所述的丹皮有效组分的制备方法,其特征是:通过以下技术方案实现:将丹皮药材粉碎后加入乙酸乙酯和乙醇=1∶1,加热回流1小时,提取2次,合并滤液得提取液;将提取液浓缩成浸膏,并将其与硅胶进行拌样,用正相硅胶柱对其进行分离,首先用石油醚和乙酸乙酯=50∶1作为流动相,得洗脱液I,弃之,然后改换氯仿和甲醇=10∶1作为流动相,得洗脱液II,将洗脱液II浓缩干燥后得样品,用制备液相色谱继续分离得到的有效组分。
8.根据权利要求6所述的丹皮有效组分的制备方法,其特征是:制备色谱的分离条件为色谱柱为半制备柱,流动相为水A和乙腈B,梯度洗脱程序如下为0分钟时,流动相A为80%的水溶液、流动相B为20%的乙腈溶液;40分钟时,流动相A为20%的水溶液、流动相B为80%的乙腈溶液;50分钟时,流动相A为5%的水溶液、流动相B为95%的乙腈溶液;流速为3ml/min,柱温为室温;样品用100%乙醇溶解,经制备液相色谱分离,在时间段14.2~18.4min收集溶液,溶液经浓缩干燥后得到有效组分。
9.根据权利要求1-3任一所述的丹皮有效组分,其特征是:丹皮有效组分加入药用添加剂按照药剂学允许的制备方法制成药用制剂。
10.根据权利要求1-3任一所述的丹皮有效组分在制备治疗、预防心血管疾病药物中的应用。
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Effective date of registration: 20070817 Address after: 310027 No. 38, Zhejiang Road, Hangzhou, Zhejiang, Xihu District Co-patentee after: Tianjin Tianshili Pharmaceutical Co., Ltd. Patentee after: Zhejiang University Address before: 310027 No. 38, Zhejiang Road, Hangzhou, Zhejiang, Xihu District Co-patentee before: Tianshili Modern Traditional Chinese Medicine Research & Devleopment Co., Ltd., Patentee before: Zhejiang University |
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Address after: 310027 Hangzhou, Zhejiang Province, Xihu District, Zhejiang Road, No. 38, No. Patentee after: Zhejiang University Patentee after: Tasly Pharmaceutical Group Co., Ltd. Address before: 310027 Hangzhou, Zhejiang Province, Xihu District, Zhejiang Road, No. 38, No. Patentee before: Zhejiang University Patentee before: Tianjin Tianshili Pharmaceutical Co., Ltd. |
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Granted publication date: 20071003 Termination date: 20180819 |