CN1748735A

CN1748735A - Chinese herbal medicine composition and preparing method

Info

Publication number: CN1748735A
Application number: CN 200510072287
Authority: CN
Inventors: 肖伟
Original assignee: Jiangsu Kanion Pharmaceutical Co Ltd
Current assignee: Jiangsu Kanion Pharmaceutical Co Ltd
Priority date: 2001-09-13
Filing date: 2001-09-13
Publication date: 2006-03-22
Anticipated expiration: 2021-09-13
Also published as: CN100409866C

Abstract

The present invention relates to a kind of Chinese herbal medicine composition for treating women's blood stasis. The Chinese herbal medicine composition is prepared with cassia twig, white peony root, tuckahoe and tree peony bark in certain weight proportion, and through water vapor distillation, alcohol extraction, concentration, palletizing, drying and other steps to form capsule. The Chinese herbal medicine composition of the present invention has the features of determined curative effect, no toxic side effect, controllable quality and easy absorption.

Description

A kind of Chinese herbal medicine compositions and preparation method

Technical field

The present invention relates to a kind of pharmaceutical composition for the treatment of gynecological's Blood stasis, cardiovascular and cerebrovascular disease and respiratory system disease etc. and preparation method thereof, specifically relating to the Chinese herbal medicine is feedstock composition and preparation method thereof.Patent application of the present invention is for dividing an application, and the original bill application number is 01815449.2, and the applying date is a calendar year 2001 JIUYUE 13 days, and denomination of invention is a kind of Chinese herbal medicine compositions and preparation method.

Background technology

In Han dynasty Zhang Zhongjing " Medical Treasures of the Golden Chamber ", point out that cassia twig tuckahoe has the function of blood circulation promoting and blood stasis dispelling, slow elininating inflammation.But Chinese medicine is not studied its effect as yet comprehensively at present.

Modern medicine study shows: the generation of the anovulatory dysfunctional uterine hemorrhage of hysteromyoma, chronic pelvic inflammatory enclosed mass, endometrium irregular shedding is all gone down with the interior endocrine disturbance of body, immunologic function, metabolism disorder is relevant.This understanding with motherland's traditional medicine is consistent.Motherland's medical science is thought: the women is to after the middle age, physiological function is tending towards decline, and a large amount of wasting QI-bloods when menstruation, motherhood, middle-aged women is under family life and social life dual-pressure in addition, easily because of factors such as emotion cause qi depression to blood stasis, passages through which vital energy circulates obstructed, dash and appoint stasis of blood resistance, stay disease in uterus Cheng Jicheng, be referred to as gynecological's syndrome of blood stasis.Gynecological's Blood stasis, motherland's medical science think, under physiological status, and blood in arteries and veins, circulate " pulse felt like the flowing of water without return "." blood vessels circulation, disease must not be given birth to ", and when blood stasis disease occurring, then " capable the mistakes degree of blood " produces pathological states such as " blood clotting and do not flow ", " blood weep and obstructed ".To this, motherland's medical science element is means to invigorate blood circulation, and obstructed blood vessels is circulated again, thereby reach blood stasis dispelling, the purpose that eliminates a disease.Its Therapeutic Principle is a blood circulation promoting and blood stasis dispelling, slow elininating inflammation.

At present above-mentioned gynaecopathia is had hormonotherapy, operative therapy and tcm therapy, but therapeutic effect is unsatisfactory.

The inventor has not only carried out compatibility research to components such as Ramulus Cinnamomi, Poria on the basis of motherland's theory of medicine, and has carried out the research of multifunctional medical efficacious prescriptions faces.Result of study is found, form and through the medicament of technologies such as extraction preparations by Ramulus Cinnamomi, Poria, the Radix Paeoniae Alba, Semen Persicae and Cortex Moutan, it has the function of blood circulation promoting and blood stasis dispelling, slow elininating inflammation preferably, not only diseases such as the treatment Blood stasis of gynecological such as hysteromyoma, pelvic inflammatory disease, dysmenorrhea, menoxenia, gynecological bleeding disease there is tangible curative effect, and find that respiratory system disease, diseases of urinary system etc. also has curative effect significantly for treatment cardiovascular and cerebrovascular disease such as hypertension, heart disease etc.

Summary of the invention

Primary and foremost purpose of the present invention provides a kind of pharmaceutical composition that is used for the treatment of gynecological's Blood stasis, cardiovascular and cerebrovascular disease, respiratory system and diseases of urinary system;

Another object of the present invention provides the purposes of described pharmaceutical composition as the medicine of preparation treatment gynecological's Blood stasis such as pelvic inflammatory disease, dysmenorrhea, menoxenia and women's hemorrhage;

A further object of the present invention provides the purposes of described pharmaceutical composition as preparation treatment cardiovascular and cerebrovascular disease such as hypertension and cardiopathic medicine;

A further object of the present invention provides the purposes of described pharmaceutical composition as the medicine of preparation treatment respiratory system disease or diseases of urinary system;

A further object of the present invention provides described preparation of drug combination method;

A further object of the present invention provides the finger printing of described pharmaceutical composition.

The present invention relates to a kind of pharmaceutical composition that is used for the treatment of gynecological's Blood stasis, cardiovascular and cerebrovascular disease, respiratory system and diseases of urinary system, this pharmaceutical composition is by following materials of weight proportions and the medicament made with following method.

Ramulus Cinnamomi 1-2 part Radix Paeoniae Alba 1-2 part

Poria 1-2 part Semen Persicae 1-2 part

Cortex Moutan 1-2 part.

The preparation method of described medicine comprises:

At first get the Cortex Moutan of aequum, it is carried out steam distillation, so that from wherein extracting paeonol.With the extracting solution cold preservation after the aqueous solution distillation, filter to get filtrate, it is the paeonol crude product; Above-mentioned filtration gained medicinal residues are mixed with the Poria of Ramulus Cinnamomi, the Radix Paeoniae Alba, Semen Persicae and half amount of aequum, extract to wherein adding adequate amount of ethanol, get ethanol extract after each the filtration, to add suitable quantity of water with the medicinal residues behind the ethanol extraction again decocts, after each the filtration aqueous extract, the aqueous solution merging after ethanol extract and aqueous extract and the above-mentioned Cortex Moutan distillation is condensed into extractum; The Poria powder of remaining half amount is broken into fine powder, with described concentrated extract mixing, granulation, drying, adds the paeonol crude product more again, make capsule behind the mixing.

According to pharmaceutical composition of the present invention, it is characterized in that, in described preparation, wherein saidly add an amount of ethanol and be extracted as 90% ethanol that adds 3 times of amounts and extract, and extract secondary; The described suitable quantity of water that adds decocts to adding 4 times of water and decocts, and decocts three times; The described ethanol that adds extracts each extraction 2 hours, and the described water that adds decocts each decoction 2 hours.

The preferred following method of preparation of drug combination method of the present invention:

Medical material is removed impurity, and Ramulus Cinnamomi, Cortex Moutan, the Radix Paeoniae Alba, Semen Persicae are clean with wash quickly, drying, and epoxyethane fumigation sterilization back is standby; The independent microwave sterilizating of Poria; Peach kernel powder is broken into coarse powder, recovery rate 96-98%; The Radix Paeoniae Alba is cut into the 2-3mm sheet; Cortex Moutan is ground into coarse powder, recovery rate 95～98%; Ramulus Cinnamomi is ground into coarse powder, recovery rate 96～97%; The Poria powder of getting formula ratio 50% is broken into fine powder, and is standby, and fine powder is crossed 100 eye mesh screens, recovery rate 92%～98%;

Cortex Moutan was soaked 4-8 hour, and steam distillation extracts paeonol, and the collection distillate is that the 100-200 of medical material doubly measures, and medicinal liquid and residue are deposited in addition, distillate 0-4 ℃ cold preservation, and the leaching paeonol dries, and gets the paeonol crude product; Ramulus Cinnamomi was soaked 4-8 hour, and vapor distillation extracted volatile oil 2-6 hour, got volatile oil, and medicinal liquid and residue are deposited in addition; Cortex Moutan and Ramulus Cinnamomi residue and the Radix Paeoniae Alba, Semen Persicae and remaining Poria add 2-4 and doubly measure the 70-95% alcohol reflux 2 times, each 2 hours, medicinal residues add 4-8 times of water gaging and decoct 2 times, each 2 hours, filter, alcohol extract reclaims ethanol, merges with water extract and Cortex Moutan, Ramulus Cinnamomi medicinal liquid, be concentrated into 75 ℃-80 ℃ following relative density 1.27 above extractum, recovery rate is 5%～18%;

With the paeonol crude product according to 1: the ratio of 5-1: 7g/g joins in the ethanol of 85-95%, stirs to make dissolving, makes the paeonol alcoholic solution, and is standby;

With Ramulus Cinnamomi Volatile oil according to 1: the ratio of 5-1: 7L/kg joins in the ethanol of 85-95%, stir to make dissolving, the Ramulus Cinnamomi Volatile oil alcoholic solution, standby;

Ratio according to beta-schardinger dextrin-and paeonol 4-8: 1g/g takes by weighing beta-schardinger dextrin-, make 80 ℃ of aqueous solutions, under continuous stirring, add the paeonol alcoholic solution, 40-80 ℃ is stirred after 1-3 hour down, refrigerator cold-storage 24h is put in taking-up, and sucking filtration precipitates with absolute ethanol washing according to a conventional method, drying at room temperature promptly gets the white powder clathrate;

Take by weighing beta-schardinger dextrin-according to the ratio of beta-schardinger dextrin-and Ramulus Cinnamomi Volatile oil 4-6: 1g/ml and be mixed with 45 ℃ of saturated aqueous solutions, under continuous stirring, add the Ramulus Cinnamomi Volatile oil alcoholic solution, after under the 35-45 ℃ of temperature insulated and stirred 1-3 hour, refrigerator cold-storage 24h is put in taking-up, and sucking filtration precipitates with petroleum ether according to a conventional method, drying at room temperature promptly gets the white powder clathrate;

Extractum and Poria powder mixing behind the vacuum drying, are ground into fine powder;

According to soft material powder and dextrin is that 20: 1 ratio adds dextrin in the soft material powder, adds 40-60% ethanol again by well-established law, and 30 mesh sieves are granulated, vacuum drying, granulate, granule I; Paeonol beta-schardinger dextrin-wrappage, Ramulus Cinnamomi Volatile oil beta-schardinger dextrin-wrappage and be equivalent to the silicon dioxide of soft material powder amount 2 ‰, with high efficient mixed machine mix homogeneously, mixtures II, with granule I and mixtures II stirring, mix homogeneously, granulate; Get particles filled capsule, every loading amount is 0.31g;

According to medicament capsule disintegration of present composition and preparation method thereof preparation less than 25 minutes, content of paeoniflorin is the 3.90-5.90mg/ grain, paeonol content is the 2.20-3.30mg/ grain.

Finger printing standard according to the medicament capsule of present composition and preparation method thereof preparation is as follows:

1, the preparation of capsule test solution of the present invention

1.1 the preparation of volatile ingredient: get 10 of finished products, remove capsule shell and add water 50ml, ether 30ml, 90min refluxes in 75 ℃ of water-baths, put coldly, divide and to get ether layer, water layer reuse extracted with diethyl ether three times, inferior 20ml, merge ether solution, in 35 ℃ of water-baths, volatilize, add diethyl ether to 5ml.

1.2 the preparation of water soluble ingredient: get 3 of finished products, remove capsule shell, add water 200ml, backflow 30min (boiling picks up counting), put cold, centrifugal 10min, supernatant filters through the 0.45um filter membrane, gets subsequent filtrate promptly.

1.3 the preparation of liposoluble constituent: with the precipitation after centrifugal in 1.2 with the water flushing to colourless, add methanol 20m backflow 30min (boiling picks up counting), put cold, centrifugal 10min, methanol solution volatilizes in 75 ℃ of water-baths and adds methanol to 2ml, and the 0.45um filter membrane filters, and gets subsequent filtrate promptly.

2, the preparation of object of reference solution

2.1 the preparation of cinnamic aldehyde (cinnamaldehyde) solution: the solution of making about 0.5mg/mL with ether promptly.

2.2 the preparation of paeoniflorin (paeoniflorin) solution: the solution of making 0.5mg/mL with methanol promptly.

2.3 the preparation of Poria control medicinal material solution: get Indian Bread 1g, add methanol 10ml, backflow 30min (boiling picks up counting) is put coldly, centrifugal, and supernatant filters through the 0.45um filter membrane, gets subsequent filtrate promptly.

3, assay method

3.1 instrument: gas chromatograph, tool temperature programming function and fid detector.Chromatograph of liquid, tool gradient elution function and variable wavelength UV-detector, gradient hysteresis volume is 1.4mL, Alltima guard column+chromatographic column volume is 3mL.The collection of chromatographic data is finished by chromatographic work station with processing.

3.2 reagent: cinnamic aldehyde, paeoniflorin reference substance and Poria control medicinal material.Ether, methanol, phosphoric acid are chromatographically pure for the analytical pure acetonitrile, and water is ultra-pure water.

3.3 condition determination

3.3.1 gas chromatogram: HP-55% phenyl methyl siloxanes (phenyl methylsiloxane) capillary column (30.0m * 0.32mm * 0.25um).Column temperature Carrier gas N2, flow velocity 1.5ml/min.Fid detector, H2 40ml/min, air 350ml/min.Make-up gas N2 (30ml/min).250 ℃ of injector temperatures.Split sampling, split ratio are 50: 1, sample size 2ul.280 ℃ of detector temperatures.Writing time 72min.

3.3.2 high performance liquid chromatography

3.3.2.1 the liquid chromatograph of water soluble ingredient: chromatographic column: Alltima C18 5um, 7.5mm * 4.6mm (guard column)+250mm * 4.6mm (chromatographic column).30 ℃ of column temperatures.Flow velocity 1ml/min detects wavelength 230nm.Sample introduction 5ul, writing time 70min.

Mobile phase CH3CN-H2O-H3PO4

A 50 ∶ 950∶ 1

B 400∶ 600∶ 1

3.3.2.2 the liquid chromatograph at fat-soluble position: chromatographic column: with the 3.3.2.1 item.50 ℃ of column temperatures.Flow velocity 1ml/min detects wavelength 210 and 242nm.Sample introduction 5ul, writing time 76min.

Mobile phase: CH3CN-H2O-H3PO4

A 600∶ 400∶ 1

B 950∶ 50∶ 1

4, system suitability test

4.1 gas chromatogram

4.1.1 number of theoretical plate: get cinnamic aldehyde solution 2 μ l, injecting chromatograph is pressed condition determination record chromatogram.Press the cinnamic aldehyde peak and calculate, number of theoretical plate should be not less than 800000.

4.1.2 replica test: get cinnamic aldehyde solution, continuous sample introduction 5 times, each 2 μ l, the relative standard deviation of its peak area measured value (RSD) should be not more than 3.0%.

4.2 liquid chromatograph

4.2.1 number of theoretical plate: get paeoniflorin solution 1 μ l, injecting chromatograph is pressed condition determination record chromatogram.Press the paeoniflorin peak and calculate, number of theoretical plate should be not less than 250000.

4.2.2 replica test: get paeoniflorin solution, continuous sample introduction 5 times, each 1 μ l, the relative standard deviation of its peak area measured value (RSD) should be not more than 3.0%.

5, finger printing and characteristic peak

5.1 the gas chromatogram finger printing of capsule volatile ingredient of the present invention

5.5.1 the gas chromatogram finger printing of capsule volatile ingredient of the present invention (comprising the object of reference cinnamic aldehyde): see Fig. 1.Wherein the 4h peak is paeonol (paeonol).

5.5.2 the characteristic peak and the relative peak area limit thereof of the gas chromatogram finger printing of capsule volatile ingredient of the present invention are:

Characteristic peak sequence number 1h, relative retention time/relative peak area is 0.757/1.183, fluctuation range is 0.770-0.745/1.740-0.690;

Characteristic peak sequence number s, relative retention time/relative peak area is 1/1;

Characteristic peak sequence number 2h, relative retention time/relative peak area is 1.275, fluctuation range is 1.280-1.270;

Characteristic peak sequence number 3h, relative retention time/relative peak area is 1.290/0.696, fluctuation range is 1.295-1.285/1.110-0.350;

Characteristic peak sequence number 4h, relative retention time/relative peak area is 1.449/5.565, fluctuation range is 1.455-1.440/8.080-3.460;

Characteristic peak sequence number 5h, relative retention time/relative peak area is 1.704/0.093, fluctuation range is 1.710-1.700/0.140-0.060;

Characteristic peak sequence number 6h, relative retention time/relative peak area is 2.146/0.164, fluctuation range is 2.150-2.140/0.255-0.080;

Characteristic peak sequence number 7h, relative retention time/relative peak area is 3.061/0.115, fluctuation range is 3.070-3.055/0.160-0.070;

5.2 the capsular HPLC finger printing of the present invention

5.2.1 the HPLC finger printing of water soluble ingredient

5.2.1.1 capsule water soluble ingredient liquid-phase chromatograph finger print atlas of the present invention (comprising the object of reference paeoniflorin): see Fig. 2.Wherein the 1s peak is gallic acid (gallic acid), and the 4s peak is that peony lactone glycoside 10s peak is 1,2,3; 4,6-five-O-galloyl-beta-D-glucose (1,2,3; 4,6-penta-O-galloyl-β-D-glucose), the 13s peak mainly contains paeonol.

5.2.1.2 the characteristic peak and the relative peak area limit thereof of capsule water soluble ingredient HPLC finger printing of the present invention are:

Characteristic peak sequence number 1s, relative retention time/relative peak area is 0.261/0.645, fluctuation range is 0.275-0.250/0.750-0.460;

Characteristic peak sequence number 2s, relative retention time/relative peak area is 0.349/0.103, fluctuation range is 0.360-0.340/0.160-0.070;

Characteristic peak sequence number 3s, relative retention time/relative peak area is 0.584/0.128, fluctuation range is 0.600-0.560-/0.230-0.065;

Characteristic peak sequence number 4s, relative retention time/relative peak area is 0.915/0.212, fluctuation range is 0.920-0.910/0.250-0.170;

Characteristic peak sequence number 5s, relative retention time/relative peak area is 1.076/0.089, fluctuation range is 1.085-1.070/0.130-0.065;

Characteristic peak sequence number 6s, relative retention time/relative peak area is 1.118/0.046, fluctuation range is 1.125-1.110/0.060-0.035;

Characteristic peak sequence number 7s, relative retention time/relative peak area is 1.162/0.052, fluctuation range is 1.175-1.155/0.080-0.030;

Characteristic peak sequence number 8s, relative retention time/relative peak area is 1.196/0.083, fluctuation range is 1.210-1.180/0.105-0.055;

Characteristic peak sequence number 9s, relative retention time/relative peak area is 1.268/0.076, fluctuation range is 1.285-1.250/0.090-0.065;

Characteristic peak sequence number 10s, relative retention time/relative peak area is 1.312/0.211, fluctuation range is 1.330-1.295/0.255-0.140;

Characteristic peak sequence number 11s, relative retention time/relative peak area is 1.420/0.404, fluctuation range is 1.450-1.400/0.470-0.310;

Characteristic peak sequence number 12s, relative retention time/relative peak area is 2.107/0.149, fluctuation range is 2.170-2.060/0.195-0.130;

Characteristic peak sequence number 13s, relative retention time/relative peak area is 2.389/0.981, fluctuation range is 2.465-2.340/1.475-0.680;

5.2.2 capsule liposoluble constituent of the present invention is at the HPLC at 210nm place finger printing

5.2.2.1 capsule liposoluble constituent liquid chromatograph of the present invention (210nm) finger printing (comprising object of reference acetyl pachymic acid pachymic acid): see Fig. 3.Wherein the 1z peak contains dehydrogenation pachymic acid (dehydrotumulosic acid), and 6z contains at the peak 3 beta-hydroxy Pilus Caprae seu Ovis steroid trienic acids [3 β-hydroxylanosta-7,9 (11), 24-trien-21-oic acid].

5.2.2.2 capsule liposoluble constituent of the present invention in the characteristic peak and the relative peak area limit thereof of the HPLC of 210nm place finger printing is:

Characteristic peak sequence number 1z, relative retention time/relative peak area is 0.367/0.322, fluctuation range is 0.375-0.355/0.540-0.180;

Characteristic peak sequence number 2z, relative retention time/relative peak area is 0.408/0.580, fluctuation range is 0.420-0.395/0.900-0.410;

Characteristic peak sequence number 3z, relative retention time/relative peak area is 0.897/0.280, fluctuation range is 0.905-0.890/0.350-0.220;

Characteristic peak sequence number 4z, relative retention time/relative peak area is 0.980/0.752, fluctuation range is 0.985-0.975/0.940-0.600;

Characteristic peak sequence number 5z, relative retention time/relative peak area is 1.019/0.286, fluctuation range is 1.025-1.015/0.410-0.210;

Characteristic peak sequence number 6z, relative retention time/relative peak area is 1.143/4.650, fluctuation range is 1.150-1.135/5.950-2.900;

Characteristic peak sequence number 7z, relative retention time/relative peak area is 1.305/0.959, fluctuation range is 1.315-1.295/1.450-0.575;

5.2.3 capsule liposoluble constituent of the present invention is at the HPLC at 242nm place finger printing

5.2.3.1 capsule liposoluble constituent liquid chromatograph of the present invention (242nm) finger printing (comprising object of reference Polyporus acid C polyporenic acid C): see Fig. 4.Wherein 3z ' number peak contains dehydrogenation pachymic acid (dehydrotumulosic acid), 4z ' number the peak contains 3-table dehydrogenation pachymic acid (3-epi-dehydrotumulosicacid), 6z ' number peak is dehydrogenation acetyl pachymic acid (dehydropachymic acid), 7z ' number the peak contains 3 β hydroxyl Pilus Caprae seu Ovis steroid trienic acid [3 β-hydroxylanosta-7,9 (11), 24-trien-21-oicacid].

5.2.3.2 capsule liposoluble constituent of the present invention in the characteristic peak and the relative peak area limit thereof of the HPLC of 242nm place finger printing is:

Characteristic peak sequence number 1z ', relative retention time/relative peak area is 0.520/0.155, fluctuation range is 0.530-0.510/0.185-0.120;

Characteristic peak sequence number 2z ', relative retention time/relative peak area is 0.566/0.184, fluctuation range is 0.570-0.560/0.230-0.140;

Characteristic peak sequence number 3z ', relative retention time/relative peak area is 0.686/1.385, fluctuation range is 0.690-0.680/1.950-0.900;

Characteristic peak sequence number 4z ', relative retention time/relative peak area is 1.128/0.481, fluctuation range is 1.135-1.125/0.530-0.430;

Characteristic peak sequence number 5z ', relative retention time/relative peak area is 1.557/0.181, fluctuation range is 1.585-1.525/0.240-0.150;

Characteristic peak sequence number 6z ', relative retention time/relative peak area is 1.763/1.414, fluctuation range is 1.800-1.720/1.700-1.250;

Characteristic peak sequence number 7z ', relative retention time/relative peak area is 2.133/0.630, fluctuation range is 2.190-2.070/0.840-0.480;

Characteristic peak sequence number 8z ', relative retention time/relative peak area is 3.033/0.463, fluctuation range is 3.105-2.950/0.680-0.160;

Medicine of the present invention has the effect for the treatment of multiple disease through animal experiment study and clinical research proof, and evident in efficacy.

Experimental example 1: reduce the rat whole blood viscosity

Extracting male Wistar rat, body weight 250-300g is divided into 5 groups at random, and the capsule of the present invention that gavages various dose respectively reaches with the volume normal saline, once a day, continuous 5 days.1.5 hours slight etherizations after the last administration, abdomen initiatively brain are got blood, anticoagulant heparin.Measure whole blood contrast viscosity with XN-5 type blood viscometer.The results are shown in Table 1.

Table 1 capsule of the present invention is to the influence of rat whole blood viscosity

Medicine	Dosage (g/kg)	Number of animals	Whole blood contrast viscosity is low to be cut	The whole blood contrast viscosity height is cut
Medicine	Dosage (g/kg)	Number of animals	Whole blood contrast viscosity is low to be cut	The whole blood contrast viscosity height is cut	Normal saline capsule of the present invention capsule of the present invention capsule persantin of the present invention	- 5.0 10.0 20.0 0.2	8 8 8 8 8	29.85±9.33 17.98±4.78 ^** 16.69±4.86 ^* 15.36±4.38 ^** 16.12±6.92 ^*	12.10±1.90 9.66±1.47 ^* 8.49±1.81 ^ 6.68±2.15 ^ 12.10±1.90

Annotate: compare with matched group ^*P＜0.05, ^*P＜0.01, ^{* *}P＜0.001 (as follows), numeral is X ± SD in the table

The result shows, gavages capsule of the present invention, can obviously reduce the rat whole blood contrast viscosity (low cutting. height is cut).Remarkable with the matched group comparing difference.

Experimental example 2: anticoagulant

1. the rabbit platelet aggregation test that exsomatizes

Get the about 2.5kg rabbit of body weight, common carotid artery intubate blood-letting under the waking state.3.13% sodium citrate anticoagulant.Whole blood is 9: 1 with the ratio of anticoagulant.1000rpm preparation in centrifugal 7 minutes PRP (platelet rich plasma) again with 3000rpm preparation in centrifugal 10 minutes PPP (platelet poor plasma), tests with SPA-III type PPP platelet aggregation instrument by the Born method behind the absorption PRP.Incubated 10 minutes 37 ℃ of following temperature with the capsule of the present invention of variable concentrations and deployed PRP.Matched group gives the normal saline with volume.The ADP final concentration is 1um.Experimental result sees Table 2.

Table 2 capsule of the present invention is to the influence of the stripped platelet aggregation of rabbit

Medicine	Concentration (mq/ml)	Number of samples	Aggregation rate (%)	Suppression ratio (%)
Medicine	Concentration (mq/ml)	Number of samples	Aggregation rate (%)	Suppression ratio (%)	Physiological saline capsule of the present invention capsule of the present invention capsule of the present invention capsule of the present invention capsule aspirin of the present invention physiological saline	- 12.5 25.0 37.5 50.0 75.0 0.3 -	5 5 5 5 5 5 5 5	67.95±19.32 51.32±11.78 ^ 39.60±12.23 ^ 25.56±9.95 ^* 13.74±5.32 ^* 3.18±2.21 ^* 57.28±1.68 ^ 66.17±1.07	24.47±7.76 41.72±7.96 62.38±6.54 79.78±3.50 95.33±1.46

Experimental result shows that capsule of the present invention can suppress the inductive rabbit platelet aggregation of ADP (adenosine diphosphate (ADP)), and its inhibitory action and being proportionate property of dosage.Positive drug aspirin inhibitory action is obvious.Capsule IC of the present invention as calculated ₅₀=25.12mg/ml.

2. rat is at the body platelet aggregation test

Get male Witar rat, body weight 250-300g is divided into 5 groups at random.Gavage the capsule of the present invention of various dose respectively.Matched group gives with the volume normal saline.Once a day, continuous 5 days.After the last administration 1.5 hours with slight etherization, abdominal aortic blood, 3.13% sodium citrate anticoagulant.Positive drug gives aspirin once, and the same legal system is equipped with rat platelet blood plasma and carries out focusing experiment.The results are shown in Table 3.

Experimental result shows, can obviously suppress the inductive platelet aggregation of ADP behind the oral capsule of the present invention of rat, and dosage increases effect and strengthens.

Table 3 capsule of the present invention is to the influence of rat platelet aggregation

Medicine	Dosage (g/kg)	Number of animals	Aggregation rate (%)
Medicine	Dosage (g/kg)	Number of animals	Aggregation rate (%)	Normal saline capsule of the present invention capsule of the present invention capsule aspirin of the present invention	- 5.0 10.0 20.0 0.1	7 7 7 7 6	65.33±11.05 56.19±7.70 51.78±9.68 ^* 44.86±7.99 ^ 26.58±10.58 ^

Experimental example 3: diastole rat uterine smooth muscle

Get the female rat of body weight 200 ± 10g, in experiment intramuscular injection the previous day 1mg/Kg benzene two methylestradiol, the dislocation of rat cervical vertebra is put to death during experiment, cut open the belly and take out the uterus rapidly, place the vessel that fill Rockwell liquid immediately, separate and remove Uterus wall fat and connective tissue on every side, get the about 15mm of both sides cornua uteri, hang in the bath that fills 10ml Rockwell liquid 32 ± 0.5 ℃ of temperature.Feeding contains 5%CO ₂Oxygen, resting tension is 1g.The contracting agent concentration of oxytocin is 10 ^-3U/ml.Ask for an interview following table 4:

The inhibitory action that table 4 capsule of the present invention shrinks rat uterus due to the oxytocin

Concentration (mg/ml)	Inhibition percent (X ± SD)
Concentration (mg/ml)	Inhibition percent (X ± SD)	3	9.06±5.78
5.6	32.39±9.15	3	9.06±5.78
5.6	32.39±9.15	10	53.63±20.78
17.78	85.63±5.91	10	53.63±20.78
17.78	85.63±5.91	30	96.01±2.8

Above-mentioned table 4 explanation capsule of the present invention is to 10 ^-3The uterotonic inhibitory action of isolated rat due to the u/ml oxytocin.

The result shows that capsule of the present invention can suppress the uterine contraction that oxytocin causes, its half-inhibition concentration is 7.92 ± 0.49 (mg/ml).

Experimental example 4: analgesic activity

1. acetic acid twisting method

Select Kunming mouse for use, body weight 18-22g is divided into 5 groups at random, 10 every group, gavages capsule 2.5,5.0 of the present invention, 10.0g/kg respectively.The normal saline contrast, positive drug aminophenazone, 1 hour difference lumbar injection 0.8% acetic acid 0.1ml/10g after the administration.Observed and recorded 0-10 minute, mice produces in 10-20 minute turned round the body number of times.The results are shown in Table 5.

Table 5 capsule of the present invention is to the influence of 0.8% acetic acid induced mice writhing response

Medicine	Dosage (g/kg)	Number of animals	Route of administration	Turned round the body number of times 0-10 minute	Turned round the body number of times 10-20 minute	Turned round the body number of times 0-20 minute
Medicine	Dosage (g/kg)	Number of animals	Route of administration	Turned round the body number of times 0-10 minute	Turned round the body number of times 10-20 minute	Turned round the body number of times 0-20 minute	Edition with parallel text invention capsule capsule aminophenazone of the present invention aminophenazone	- 2.5 5.0 10.0 0.1	10 10 10 10 10	P.O P.O P.O P.O P.O	22.7±4.4 19.3±2.5 ^* 14.0±6.0 ^* 10.8±6.6 ^***	23.6±6.6 19.1±6.6 12.9±6.6 ^ 9.6±7.3 ^*	46.3±7.3 38.4±5.4 ^* 26.9±11.7 ^* 20.4±13.6 ^* 2.8±4.1 ^*

Experimental result shows, oral capsule 2.5g/Kg of the present invention can make the mouse writhing number of times reduce, and 0-20 minute suppression ratio is respectively 17%, 41.9%, 55.9% (2.5,5.0,10.0g/Kg), and be remarkable with the matched group comparing difference.The effect of positive drug aminophenazone is obvious.

1, mice tail-flick method

Kunming mouse, body weight 18-22g immerses its afterbody 1/3 place in 55 ± 0.5 ℃ of waters bath with thermostatic control before administration, remembers that it gets rid of the time, is divided into 8 groups by the threshold of pain and body weight, 10 every group, gavages medicine, normal saline, the positive drug indometacin of various dose respectively.1,2, the 4 hour whipping time after the record administration.The results are shown in Table 6.

That the result shows is oral 10,20g/Kg osmanthus Fu extract all can prolong the mice whipping time.

Table 6 capsule of the present invention is to the whipping time that influences (second) of mice whipping time

Rank	Dosage (g/kg)	Number of animals	Before the administration	After the administration 60 (minute)	After the administration 120 (minute)	After the administration 240 (minute)
Rank	Dosage (g/kg)	Number of animals	Before the administration	After the administration 60 (minute)	After the administration 120 (minute)	After the administration 240 (minute)	Matched group capsule of the present invention capsule of the present invention capsule indometacin of the present invention	- 5 10 20 0.01	10 10 10 10 10	1.58±0.43 1.56±0.40 1.55±0.46 1.50±0.47 1.58±0.79	1.49±0.4 1.71±0.37 2.21±0.93 ^* 2.57±0.95 ^** 2.23±0.53 ^*	1.57±0.38 1.91±0.58 2.42±0.95 ^** 2.61±1.27 2.56±0.40	1.54±0.41 1.89±0.66 2.70±0.92 ^* 2.50±0.43 ^* 1.52±0.56

Annotate: compare P＜0.05 before and after self ^*P＜0.01 ^{* *}P＜0.001 (as follows)

Experimental example 5: antiinflammatory action (mice ear method)

Select Kunming mouse for use, body weight 20-25g, by the body weight random packet, the medicine of oral various dose three days.Be coated with proinflammatory agent (including 2% Oleum Tiglii, 20% dehydrated alcohol, 5% distilled water and 73% ether) to mouse ear simultaneously in the last administration, be applied to two sides, left ear front and back, the about 0.5ml of every Mus coating, 2 hours execution animals behind coating, lay the auricle at the same position of ears weighs with the 9mm card punch, left side auricle deducts the auris dextra sheet and heavily is the swelling degree, and matched group and administration swelling degree are carried out statistical procedures.Experimental result sees Table 7.

That the result shows is oral 10 to mice, 20g/Kg osmanthus Fu extract all has tangible antiinflammatory action, and dosage raising effect strengthens.

Table 7 capsule of the present invention is to the bullate influence of mouse ear

Group	Dosage (g/Kg)	Number of animals	Average swelling degree (mg)
Group	Dosage (g/Kg)	Number of animals	Average swelling degree (mg)	Matched group capsule of the present invention capsule of the present invention capsule hydrocortisone of the present invention	- 5 10 20 0.025	10 10 10 10 10	18.36±7.09 17.75±4.81 9.05±5.92 ^ 5.92±3.11 ^* 4.68±3.43 ^***

The clinical observation of experimental example 6:50 example

1, diagnostic criteria:

Western medicine diagnose standard: work out with reference to two editions state-compiled textbooks of national institution of higher learning " obstetrics and gynecology " and " disease clinical diagnosis and criterion of therapeutical effect " (Jiangsu Province Department of Public Health compiles 1990); The tcm diagnosis standard: diagnostic criteria and five editions state-compiled textbooks of national high universities and colleges " traditional Chinese obstetrics and gynecology " with reference to second national blood circulation promoting and blood stasis dispelling research academic conference November in 1986 are worked out about the diagnosis of gynecological's Blood stasis.

2, criterion of therapeutical effect:

Formulate according to " new drug (Chinese medicine) clinical research guideline " and " clinical disease diagnosis and criterion of therapeutical effect ".

3, observational technique:

Medication: give clothes capsule of the present invention, every day 3 times, each 3.All take medicine after meal.The hysteromyoma person, withdraw menstrual period, and the chronic pelvic inflammatory disease inflammatory mass person take medicine continuously, and anovulatory dysfunctional uterine hemorrhage person blood is only withdrawn, and 3 months is a course of treatment.

The lab testing method: all do hemorheology and platelet aggregation inspection before and after observing the case treatment.Hemorheology index comprises six of whole blood contrast viscosities, plasma viscosity, erythrocyte sedimentation rate, hematocrit, whole blood reduced viscosity, ESR equation K value.The platelet aggregation index comprises one minute aggregation rate, five minutes aggregation rate.

4, curative effect is summed up:

Capsule cure rate 28% of the present invention, cure-remarkable-effectiveness rate 60%, total effective rate 96%.Observe as can be known by clinical verification, capsule of the present invention to improve menorrhagia, leak down, through more than dim, primary symptom such as lower abdomen pain and double diseases such as the waist sacrum is miserable, rectal tenesmus have significant curative effect, its improvement rate is all more than 80%.Before the treatment through woman inspection and the ultrasound diagnosis person's (comprising hysteromyoma and chronic pelvic inflammatory disease inflammatory mass) that confirms there is the abdominal mass, the check of treatment back, the woman examines enclosed mass has 28% to disappear, 36% dwindles, 32% control development, 2% increases.This experimental example has confirmed that medicine of the present invention has the effect of gynecological's Blood stasis diseases such as treatment hysteromyoma, chronic pelvic inflammatory disease, dysmenorrhea, functional bleeding.

Conclusion:

Above-mentioned experimental example shows that medicine of the present invention has blood viscosity lowering, anticoagulant, and the effect of anti-inflammatory and antalgic, and the circulation that increases blood vessels is the important method of treatment blood stasis disease, and patients' such as hysteromyoma, dysmenorrhea, pelvic inflammatory disease blood viscosity is than normal person height, therefore, this experimental example has confirmed that medicine of the present invention has the function of blood circulation promoting and blood stasis dispelling, to gynaecopathia due to the blood stasis, gynaecopathia

As hysteromyoma, chronic pelvic inflammatory disease, anovulatory dysfunctional uterine hemorrhage etc. definite curative effect is arranged.

Description of drawings:

Fig. 1 becomes meeting GC-FP for capsule volatility of the present invention;

Fig. 2 is capsule water soluble ingredient HPLC-FP of the present invention;

Fig. 3 is that capsule liposoluble constituent of the present invention is at the HPLC-FP of 210nm place;

Fig. 4 is that capsule liposoluble constituent of the present invention is at the HPLC-FP of 242nm place.

Embodiment 1:

Get the Cortex Moutan of 144Kg, it is carried out steam distillation, so that from wherein extracting paeonol.With the extracting solution cold preservation after the aqueous solution distillation, filter to get filtrate, it is the paeonol crude product; Above-mentioned filtration gained medicinal residues are mixed with 144Kg Ramulus Cinnamomi, the 144Kg Radix Paeoniae Alba, 144Kg Semen Persicae and 72kg Poria, to the 90% alcohol reflux secondary that wherein adds 3 times of amounts, each reflux, extract, 2 hours, get ethanol extract after each the filtration, to add 4 times of water gagings again with the medicinal residues behind the ethanol extraction decocts 3 times, each 3 hours, get extracting solution after each the filtration.Aqueous solution after ethanol extract and aqueous extract and the above-mentioned Cortex Moutan distillation is merged and be condensed into extractum, it is concentrated into relative density more than 1.27 in 75～80 ℃, must about 120kg extractum; The Poria powder of remaining half amount 72kg is broken into fine powder,,, adds above-mentioned paeonol crude product again, make capsule behind the mixing through granulation, drying again with described concentrated extract mixing.The above-mentioned medicament that makes can be made into 10,000 boxes, every box 60 capsules.

Embodiment 2:

Take by weighing: Ramulus Cinnamomi 144kg Poria 144kg Cortex Moutan 144kg

Radix Paeoniae Alba 144kg Semen Persicae 144kg

Medical material is removed impurity, and Ramulus Cinnamomi, Cortex Moutan, the Radix Paeoniae Alba, Semen Persicae are clean with wash quickly, drying, and epoxyethane fumigation sterilization back is standby; The independent microwave sterilizating of Poria.Peach kernel powder is broken into coarse powder, recovery rate 96-98%; The Radix Paeoniae Alba is cut into the 2-3mm sheet; Cortex Moutan is ground into coarse powder, recovery rate 95～98%; Ramulus Cinnamomi is ground into coarse powder, recovery rate 96～97%; The Poria powder of getting formula ratio 50% is broken into fine powder, gets fine powder 70-72kg, and standby, fine powder is crossed 100 eye mesh screens, recovery rate 92%～98%;

Cortex Moutan was soaked 4 hours, and steam distillation extracts paeonol, and collecting distillate is 200 times of amounts of medical material, and medicinal liquid and residue are deposited in addition, distillate 0-4 ℃ cold preservation, and the leaching paeonol dries, and gets paeonol crude product 1.6-1.8kg; Ramulus Cinnamomi was soaked 6 hours, and vapor distillation extracted volatile oil 4 hours, got volatile oil 0.82-0.93L, and medicinal liquid and residue are deposited in addition; Cortex Moutan and Ramulus Cinnamomi residue and the Radix Paeoniae Alba, Semen Persicae and remaining Poria add 3 times of amount 90% alcohol reflux 2 times, each 2 hours, medicinal residues add 4 times of water gagings and decoct 2 times, each 2 hours, filter, alcohol extract reclaims ethanol, merge with water extract and Cortex Moutan, Ramulus Cinnamomi medicinal liquid, be concentrated at 75-80 ℃ of following relative density 1.27 above extractum, get extractum 110～130kg, recovery rate 5%～18%;

Paeonol crude product 1.6～1.8kg is joined in the ethanol of 9.0kg95%, stir and make dissolving, make the paeonol alcoholic solution; Ramulus Cinnamomi Volatile oil 0.82～0.93L is joined in the ethanol of 5kg95%, stir and make dissolving, make the Ramulus Cinnamomi Volatile oil alcoholic solution;

Take by weighing beta-schardinger dextrin-10.2g and make 80 ℃ of aqueous solutions, under continuous stirring, add the paeonol alcoholic solution, 80 ℃ were stirred after 3 hours, refrigerator cold-storage 24h is put in taking-up, sucking filtration is with a small amount of absolute ethanol washing precipitation, drying at room temperature, promptly get the white powder clathrate, heavy altogether 9.86kg, paeonol inclusion rate 70%～72%, bag and thing recovery rate 82%～86%;

Take by weighing beta-schardinger dextrin-3.72kg and be mixed with 45 ℃ of saturated aqueous solutions, under continuous stirring, add the Ramulus Cinnamomi Volatile oil alcoholic solution, 45 ℃ are stirred after 3 hours, take out and put refrigerator cold-storage 24h, sucking filtration, with a small amount of petroleum ether precipitation, drying at room temperature promptly gets the white powder clathrate, heavy altogether 3.70kg, Ramulus Cinnamomi Volatile oil inclusion rate 61%～64%, bag and thing recovery rate 83%～85%;

Extractum and Poria powder mixing behind the vacuum drying, are ground into fine powder, about 164kg, yield 94%～98%; Add in the soft material powder and account for dextrin into 8.2kg, add an amount of 60% ethanol again, 30 mesh sieves are granulated, vacuum drying, granulate, get the granule worker: paeonol-cyclodextrin wrappage, Ramulus Cinnamomi Volatile oil-cyclodextrin wrappage and 0.33kg silicon dioxide with high efficient mixed machine mix homogeneously, get the about 13.8kg of mixtures II, with granule I and mixtures II stir, mix homogeneously, granulate gets 186kg, recovery rate 96%～98% approximately;

Get particles filled capsule, every loading amount is 0.31g, and is promptly aluminum-plastic packaged.

Embodiment 3:

Take by weighing: Ramulus Cinnamomi 170kg Poria 120kg Cortex Moutan 170kg

Radix Paeoniae Alba 130kg Semen Persicae 130kg

Claims

1, a kind of pharmaceutical composition for the treatment of gynaecopathia is characterized in that this pharmaceutical composition is the capsule of being made as follows by following proportion raw material medicine:

Get Ramulus Cinnamomi 1-2 weight portion, Radix Paeoniae Alba 1-2 weight portion, Poria 1-2 weight portion, Semen Persicae 1-2 weight portion, Cortex Moutan 1-2 weight portion;

According to soft material powder and dextrin is that 20: 1 ratio adds dextrin in the soft material powder, adds 40-60% ethanol again by well-established law, and 30 mesh sieves are granulated, vacuum drying, granulate, granule I; Paeonol Benexate Hydrochloride, Ramulus Cinnamomi Volatile oil Benexate Hydrochloride and be equivalent to the silicon dioxide of soft material powder amount 2 ‰, with high efficient mixed machine mix homogeneously, mixtures II, with granule I and mixtures II stirring, mix homogeneously, granulate; Get particles filled capsule, every loading amount is 0.31g.

2, a kind of pharmaceutical composition for the treatment of gynaecopathia is characterized in that this pharmaceutical composition is the capsule of being made as follows by following proportion raw material medicine:

Get Ramulus Cinnamomi 170kg, Poria 120kg, Cortex Moutan 170kg, Radix Paeoniae Alba 130kg, Semen Persicae 130kg;

Medical material is removed impurity, and Ramulus Cinnamomi, Cortex Moutan, the Radix Paeoniae Alba, Semen Persicae are clean with wash quickly, drying, and epoxyethane fumigation sterilization back is standby; The independent microwave sterilizating of Poria; Peach kernel powder is broken into coarse powder, recovery rate 96-98%; The Radix Paeoniae Alba is cut into the 2-3mm sheet; Cortex Moutan is ground into coarse powder, recovery rate 95～98%; Ramulus Cinnamomi is ground into coarse powder, recovery rate 96～97%; The Poria powder of getting formula ratio 50% is broken into fine powder, gets fine powder 70-72kg, and standby, fine powder is crossed 100 eye mesh screens, recovery rate 92%～98%;

Take by weighing beta-schardinger dextrin-3.72kg and be mixed with 45 ℃ of saturated aqueous solutions, under continuous stirring, add the Ramulus Cinnamomi Volatile oil alcoholic solution, 45 ℃ are stirred after 3 hours, take out and put refrigerator cold-storage 24h, sucking filtration, with a small amount of petroleum ether precipitation, drying at room temperature promptly gets the white powder clathrate, heavy altogether 3.70kg, Ramulus Cinnamomi Volatile oil inclusion rate 61%～64%, clathrate recovery rate 83%～85%;

Extractum and Poria powder mixing behind the vacuum drying, are ground into fine powder, about 164kg, yield 94%～98%; Add the 8.2kg dextrin in the soft material powder, add an amount of 60% ethanol again, 30 mesh sieves are granulated, vacuum drying, and granulate gets granule I; Paeonol-cyclodextrin clathrate, Ramulus Cinnamomi Volatile oil-cyclodextrin clathrate and 0.33kg silicon dioxide with high efficient mixed machine mix homogeneously, get the about 13.8kg of mixtures II, with granule I and mixtures II stir, mix homogeneously, granulate gets 186kg, recovery rate 96%～98% approximately;

3, a kind of pharmaceutical composition for the treatment of gynaecopathia is characterized in that this pharmaceutical composition is the capsule of being made as follows by following proportion raw material medicine:

Get Ramulus Cinnamomi 144kg, Poria 144kg, Cortex Moutan 144kg, Radix Paeoniae Alba 144kg, Semen Persicae 144kg;

Take by weighing beta-schardinger dextrin-10.2g and make 80 ℃ of aqueous solutions, under continuous stirring, add the paeonol alcoholic solution, 80 ℃ were stirred after 3 hours, refrigerator cold-storage 24h is put in taking-up, sucking filtration is with a small amount of absolute ethanol washing precipitation, drying at room temperature, promptly get the white powder clathrate, heavy altogether 9.86kg, paeonol inclusion rate 70%～72%, clathrate recovery rate 82%～86%;

Extractum and Poria powder mixing behind the vacuum drying, are ground into fine powder, about 164kg, yield 94%～98%; Add in the soft material powder and account for the dextrin into 8.2kg, add an amount of 60% ethanol again, 30 mesh sieves are granulated, vacuum drying, granulate, granule I; Paeonol-cyclodextrin wrappage, Ramulus Cinnamomi Volatile oil-cyclodextrin clathrate and 0.33kg silicon dioxide with high efficient mixed machine mix homogeneously, get the about 13.8kg of mixtures II, with granule I and mixtures II stir, mix homogeneously, granulate gets 186kg, recovery rate 96%～98% approximately;

4, preparation of drug combination method as claimed in claim 1 is characterized in that this method is:

According to soft material powder and dextrin is that 20: 1 ratio adds dextrin in the soft material powder, adds 40-60% ethanol again by well-established law, and 30 mesh sieves are granulated, vacuum drying, granulate, granule I; Paeonol beta-schardinger dextrin-wrappage, Ramulus Cinnamomi Volatile oil beta-schardinger dextrin-wrappage and be equivalent to the silicon dioxide of soft material powder amount 2 ‰, with high efficient mixed machine mix homogeneously, mixtures II, with granule I and mixtures II stirring, mix homogeneously, granulate; Get particles filled capsule, every loading amount is 0.31g.

5, preparation of drug combination method as claimed in claim 2 is characterized in that this method is:

Extractum and Poria powder mixing behind the vacuum drying, are ground into fine powder, about 164kg, yield 94%～98%; Add in the soft material powder and account for the dextrin into 8.2kg, add an amount of 60% ethanol again, 30 mesh sieves are granulated, vacuum drying, granulate, granule I; Paeonol-cyclodextrin clathrate, Ramulus Cinnamomi Volatile oil-cyclodextrin clathrate and 0.33kg silicon dioxide with high efficient mixed machine mix homogeneously, get the about 13.8kg of mixtures II, with granule I and mixtures II stir, mix homogeneously, granulate gets 186kg, recovery rate 96%～98% approximately;

6, preparation of drug combination method as claimed in claim 3 is characterized in that this method is:

Extractum and Poria powder mixing behind the vacuum drying, are ground into fine powder, about 164kg, yield 94%～98%; Add the 8.2kg dextrin in the soft material powder, add an amount of 60% ethanol again, 30 mesh sieves are granulated, vacuum drying, and granulate gets granule I; Paeonol-cyclodextrin wrappage, Ramulus Cinnamomi Volatile oil-cyclodextrin clathrate and 0.33kg silicon dioxide with high efficient mixed machine mix homogeneously, get the about 13.8kg of mixtures II, with granule I and mixtures II stir, mix homogeneously, granulate gets 186kg, recovery rate 96%～98% approximately;

7,, it is characterized in that content of paeoniflorin is that 3.90-5.90mg/ grain, paeonol content are the 2.20-3.30mg/ grain in this medicament capsule as the pharmaceutical composition of claim 1,2 or 3 described treatment gynaecopathias.

8, as the method for quality control of the pharmaceutical composition of claim 1,2 or 3 described treatment gynaecopathias, it is characterized in that the finger printing of each composition in this medicament capsule is as follows:

The characteristic peak and the relative peak area limit thereof of the gas chromatogram finger printing of volatile ingredient are: characteristic peak sequence number 1h, and relative retention time/relative peak area is 0.757/1.183, fluctuation range is 0.770-0.745/1.740-0.690; Characteristic peak sequence number s, relative retention time/relative peak area is 1/1; Characteristic peak sequence number 2h, relative retention time/relative peak area is 1.275, fluctuation range is 1.280-1.270; Characteristic peak sequence number 3h, relative retention time/relative peak area is 1.290/0.696, fluctuation range is 1.295-1.285/1.110-0.350; Characteristic peak sequence number 4h, relative retention time/relative peak area is 1.449/5.565, fluctuation range is 1.455-1.440/8.080-3.460; Characteristic peak sequence number 5h, relative retention time/relative peak area is 1.704/0.093, fluctuation range is 1.710-1.700/0.140-0.060; Characteristic peak sequence number 6h, relative retention time/relative peak area is 2.146/0.164, fluctuation range is 2.150-2.140/0.255-0.080; Characteristic peak sequence number 7h, relative retention time/relative peak area is 3.061/0.115, fluctuation range is 3.070-3.055/0.160-0.070;

The characteristic peak and the relative peak area limit thereof of water soluble ingredient HPLC finger printing are: characteristic peak sequence number 1s, and relative retention time/relative peak area is 0.261/0.645, fluctuation range is 0.275-0.250/0.750-0.460; Characteristic peak sequence number 2s, relative retention time/relative peak area is 0.349/0.103, fluctuation range is 0.360-0.340/0.160-0.070; Characteristic peak sequence number 3s, relative retention time/relative peak area is 0.584/0.128, fluctuation range is 0.600-0.560-/0.230-0.065; Characteristic peak sequence number 4s, relative retention time/relative peak area is 0.915/0.212, fluctuation range is 0.920-0.910/0.250-0.170; Characteristic peak sequence number s, relative retention time/relative peak area is 1/1; Characteristic peak sequence number 5s, relative retention time/relative peak area is 1.076/0.089, fluctuation range is 1.085-1.070/0.130-0.065; Characteristic peak sequence number 6s, relative retention time/relative peak area is 1.118/0.046, fluctuation range is 1.125-1.110/0.060-0.035; Characteristic peak sequence number 7s, relative retention time/relative peak area is 1.162/0.052, fluctuation range is 1.175-1.155/0.080-0.030; Characteristic peak sequence number 8s, relative retention time/relative peak area is 1.196/0.083, fluctuation range is 1.210-1.180/0.105-0.055; Characteristic peak sequence number 9s, relative retention time/relative peak area is 1.268/0.076, fluctuation range is 1.285-1.250/0.090-0.065; Characteristic peak sequence number 10s, relative retention time/relative peak area is 1.312/0.211, fluctuation range is 1.330-1.295/0.255-0.140; Characteristic peak sequence number 11s, relative retention time/relative peak area is 1.420/0.404, fluctuation range is 1.450-1.400/0.470-0.310; Characteristic peak sequence number 12s, relative retention time/relative peak area is 2.107/0.149, fluctuation range is 2.170-2.060/0.195-0.130; Characteristic peak sequence number 13s, relative retention time/relative peak area is 2.389/0.981, fluctuation range is 2.465-2.340/1.475-0.680;

Liposoluble constituent in the characteristic peak and the relative peak area limit thereof of the HPLC of 210nm place finger printing is: characteristic peak sequence number 1z, and relative retention time/relative peak area is 0.367/0.322, fluctuation range is 0.375-0.355/0.540-0.180; Characteristic peak sequence number 2z, relative retention time/relative peak area is 0.408/0.580, fluctuation range is 0.420-0.395/0.900-0.410; Characteristic peak sequence number 3z, relative retention time/relative peak area is 0.897/0.280, fluctuation range is 0.905-0.890/0.350-0.220; Characteristic peak sequence number 4z, relative retention time/relative peak area is 0.980/0.752, fluctuation range is 0.985-0.975/0.940-0.600; Characteristic peak sequence number s, relative retention time/relative peak area is 1/1; Characteristic peak sequence number 5z, relative retention time/relative peak area is 1.019/0.286, fluctuation range is 1.025-1.015/0.410-0.210; Characteristic peak sequence number 6z, relative retention time/relative peak area is 1.143/4.650, fluctuation range is 1.150-1.135/5.950-2.900; Characteristic peak sequence number 7z, relative retention time/relative peak area is 1.305/0.959, fluctuation range is 1.315-1.295/1.450-0.575;

Liposoluble constituent in the characteristic peak and the relative peak area limit thereof of the HPLC of 242nm place finger printing is: characteristic peak sequence number 1z ', and relative retention time/relative peak area is 0.520/0.155, fluctuation range is 0.530-0.510/0.185-0.120; Characteristic peak sequence number 2z ', relative retention time/relative peak area is 0.566/0.184, fluctuation range is 0.570-0.560/0.230-0.140; Characteristic peak sequence number 3z ', relative retention time/relative peak area is 0.686/1.385, fluctuation range is 0.690-0.680/1.950-0.900; Characteristic peak sequence number s, relative retention time/relative peak area is 1/1; Characteristic peak sequence number 4z ', relative retention time/relative peak area is 1.128/0.481, fluctuation range is 1.135-1.125/0.530-0.430; Characteristic peak sequence number 5z ', relative retention time/relative peak area is 1.557/0.181, fluctuation range is 1.585-1.525/0.240-0.150; Characteristic peak sequence number 6z ', relative retention time/relative peak area is 1.763/1.414, fluctuation range is 1.800-1.720/1.700-1.250; Characteristic peak sequence number 7z ', relative retention time/relative peak area is 2.133/0.630, fluctuation range is 2.190-2.070/0.840-0.480; Characteristic peak sequence number 8z ', relative retention time/relative peak area is 3.033/0.463, fluctuation range is 3.105-2.950/0.680-0.160;

Above-mentioned finger printing is realized in following condition:

The preparation of need testing solution volatile ingredient: get 10 of finished products, remove capsule shell and add water 50ml, ether 30ml, 90min refluxes in 75 ℃ of water-baths, put coldly, divide and to get ether layer, water layer reuse extracted with diethyl ether three times, each 20ml, merge ether solution, in 35 ℃ of water-baths, volatilize, add diethyl ether to 5ml;

The preparation of need testing solution water soluble ingredient: get 3 of finished products, remove capsule shell, add water 200ml, backflow 30min, put cold, centrifugal 10min, supernatant filters through the 0.45um filter membrane, gets subsequent filtrate promptly;

The preparation of need testing solution liposoluble constituent: the precipitation in the preparation with above-mentioned need testing solution water soluble ingredient after centrifugal with the water flushing to colourless, add methanol 20ml backflow 30min, put cold, centrifugal 10min, methanol solution volatilizes in 75 ℃ of water-baths and adds methanol to 2ml, 0.45um filter membrane filters, and gets subsequent filtrate promptly;

The preparation of object of reference solution: cinnamic aldehyde is made the solution of 0.5mg/ml with ether; The solution that paeoniflorin is made 0.5mg/ml with methanol promptly; Poria control medicinal material solution adds methanol 10ml for getting Indian Bread 1g, and backflow 30min is put coldly, centrifugal, and supernatant filters through the 0.45um filter membrane, gets subsequent filtrate promptly;

Determining instrument: gas chromatograph, tool temperature programming function and fid detector; Chromatograph of liquid, tool gradient elution function and variable wavelength UV-detector, gradient hysteresis volume is 1.4ml, Alltima guard column+chromatographic column volume is 3ml; The collection of chromatographic data is finished by chromatographic work station with processing; Reagent adopts cinnamic aldehyde, paeoniflorin reference substance and Poria control medicinal material; Ether, methanol, phosphoric acid are analytical pure, and acetonitrile is a chromatographically pure, and water is ultra-pure water;

The gas Chromatographic Determination condition: adopting the trade mark is the 5% phenyl methyl siloxanes capillary column of HP-5, column length 30.0m, internal diameter 0.32mm, thickness 0.25 μ m; Injector temperature is 250 ℃; Detector temperature is 280 ℃; Carrier gas N ₂, flow velocity 1.5ml/min; Fid detector, H ₂40ml/min, air 350ml/min, make-up gas N ₂30ml/min; Split ratio is 50: 1; Temperature programming: 80 ℃ of initial temperatures, kept 5 minutes, rise to 250 ℃ with 3 ℃ of per minutes, kept 10 minutes, measure, writing time 72min;

The liquid phase condition determination of water soluble ingredient finger printing: chromatographic column is filler with the octadecylsilane chemically bonded silica, model Alltima, column length 250mm, internal diameter 4.6mm, particle diameter 5 μ m; Guard column is filler with the octadecylsilane chemically bonded silica, model Alltima, column length 7.5mm, internal diameter 4.6mm, particle diameter 5 μ m; With the aqueous solution that contains 0.1% phosphoric acid and 5% acetonitrile is mobile phase A, is Mobile phase B with the aqueous solution that contains 0.1% phosphoric acid and 50% acetonitrile; Elution program is, 0 to 70 minute, mobile phase A dropped to 0% by 100% linearity, and Mobile phase B rises to 100% by 0% linearity; 30 ℃ of column temperatures; Flow velocity 1ml/min detects wavelength 230nm; Sample introduction 5ul, writing time 70min;

The liquid phase condition determination of liposoluble constituent finger printing: chromatographic column is filler with the octadecylsilane chemically bonded silica, model Alltima, column length 250mm, internal diameter 4.6mm, particle diameter 5 μ m; Guard column is filler with the octadecylsilane chemically bonded silica, model Alltima, column length 7.5mm, internal diameter 4.6mm, particle diameter 5 μ m; With the aqueous solution that contains 0.1% phosphoric acid and 60% acetonitrile is mobile phase A, is Mobile phase B with the aqueous solution that contains 0.1% phosphoric acid and 95% acetonitrile; Elution program is, 0 to 25 minute, carry out eluting with 100% mobile phase A, and mobile phase A dropped to 0% by 100% linearity in 25 to 65 minutes, and Mobile phase B rises to 100%, 65 to 76 minute by 0% linearity, carries out eluting with 100% Mobile phase B; 50 ℃ of column temperatures, flow velocity 1ml/min; Detect wavelength 210nm and 242nm, sample introduction 5ul, writing time 76min.

9, as the application in the medicine of preparation treatment gynecological Blood stasis of the pharmaceutical composition of claim 1,2 or 3 described treatment gynaecopathias.

10, as the application in the medicine of preparation treatment pelvic inflammatory disease of the pharmaceutical composition of claim 1,2 or 3 described treatment gynaecopathias.

11, as the application in the medicine of preparation treatment dysmenorrhea of the pharmaceutical composition of claim 1,2 or 3 described treatment gynaecopathias.