The present patent application is for dividing an application, and original bill application number is 201210203325.0, and the original bill applying date is on June 19th, 2012, and original bill denomination of invention is: the new purposes of Radix Aconiti Coreani total alkaloids and Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems.
Summary of the invention
One of the object of the invention is to provide the preparation method of Radix Aconiti Coreani total alkaloids.
Two of the object of the invention is to provide the application of Radix Aconiti Coreani total alkaloids in the slow Na-ion channel blocker of preparation.
Three of the object of the invention is to provide the application of Guan-fubase A in the slow Na-ion channel blocker of preparation.
Four of the object of the invention is to provide Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems suppressing the new purposes of medicine metabolic enzyme activity.
The object of the invention is to be achieved through the following technical solutions.
A preparation method for Radix Aconiti Coreani total alkaloids, the method comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, organic solvent extraction, reclaims solvent, obtains extract extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with acid solution, by acid solution deepfreeze, get sour water layer;
Step 3: get the acid liquid that step 2 obtains, with organic solvent extraction, sour water mother solution adds alkali liquor and regulates pH to alkalescence;
Step 4: by the solution organic solvent extraction of alkalization in step 3, get organic solvent layer, reclaim solvent, obtain Radix Aconiti Coreani total alkaloids.
Preferably, in described step 1, organic solvent is any one in n-butyl alcohol, isopropyl alcohol, ethanol, ethyl acetate, acetone, petroleum ether, ether;
Described extracting method is that merceration extracts;
Acid solution in described step 2 is one or more in hydrochloric acid, nitric acid, sulphuric acid, phosphoric acid, formic acid, acetic acid, butanoic acid;
Organic solvent in described step 3 and 4 is any one in n-butyl alcohol, ethyl acetate, Ethyl formate, Ethyl formate, chloroform, acetone, petroleum ether, ether;
Alkali liquor in described step 3 is one or more in ammonia, sodium carbonate, sodium bicarbonate.
Preferably, the preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, extract with 50-95% ethanol merceration at 10-30 ℃, reclaim solvent, obtain extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with aqueous hydrochloric acid solution, by acid solution deepfreeze, remove the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate, sour water mother solution adds ammonia and regulates pH=8-11;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
More there is the parameter of choosing to be: in step 2, aqueous hydrochloric acid solution is 0.5-1.5mol/l; And/or in step 3: sour water mother solution adds ammonia and regulates pH=9.
Preferred, the preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, pulverize, at 10-30 ℃, with 2-8, doubly measure 50-95% ethanol merceration and extract 2-4 time, each 12-36 hour, merge extractive liquid,, reclaims solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, the aqueous hydrochloric acid solution of doubly measuring 0.5-1.5mol/l with 1-3 is pinched molten, by acid solution deepfreeze 12-24 hour, removes the oil-soluble impurities on upper strata, gets acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 2-4 time, sour water mother solution adds ammonia and regulates pH=8-11;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate 2-4 time rapidly, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Further preferred, the preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, be ground into 10-20 order coarse powder, extract 4 times at 25 ℃ with 5 times of amount 85% ethanol mercerations, each 24 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 1 times of amount 1mol/l, acid solution, in 2 ℃ of deepfreeze 12-24 hour, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 2 times, sour water mother solution adds ammonia and regulates pH=9;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 4 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Or, step 1: get Radix Aconiti Coreani medical material, be ground into 10-20 order coarse powder, extract 2 times at 10 ℃ with 3 times of amount 95% ethanol mercerations, each 36 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 3 times of amount 0.5mol/l, acid solution, in 2 ℃ of deepfreeze 12-24 hour, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 4 times, sour water mother solution adds ammonia and regulates pH=8;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 2 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Or, step 1: get Radix Aconiti Coreani medical material, be ground into 10-20 order coarse powder, extract 3 times at 30 ℃ with 8 times of amount 75% ethanol mercerations, each 12 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 2 times of amount 1.5mol/l, acid solution, in 2 ℃ of deepfreeze 12-24 hour, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 2 times, sour water mother solution adds ammonia and regulates pH=11;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 4 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Above-mentioned Radix Aconiti Coreani total alkaloids routinely technique is made the total alkali salt of Radix Aconiti Coreani.
Radix Aconiti Coreani total alkaloids of the present invention and total alkali salt can be made the acceptable any conventional dosage form of pharmaceutics by preparation process routinely, intramuscular dose for example, intravenous injection, injectable powder, capsule, granule or tablet.
The application of Radix Aconiti Coreani total alkaloids of the present invention in the slow Na-ion channel blocker of preparation; Described Radix Aconiti Coreani total alkaloids can be the form of free alkali or inorganic acid salt.
The application of a kind of Guan-fubase A in the slow Na-ion channel blocker of preparation; Described Guan-fubase A can be the form of free alkali or inorganic acid salt.
A kind of Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems suppresses the application in drug metabolism enzyme medicine in preparation.
Described drug metabolism enzyme is preferably one or more in cytochrome P 450 Enzyme; CYP2D6 more preferably.
The medical compounds of drug metabolism enzyme CYP2D6 of the present invention institute metabolism and the molecular characterization of salt thereof are: in molecular structure of compounds, there is a nitrogen-atoms at distance oxidation site 5~7A place.Comprise that antidepressants are as amitriptyline, imipramine, clomipramine, desipramine, nortriptyline, fluoxetine, paroxetine, venlafaxine etc.; Beta-blocker is as carvedilol, Propranolol, metoprolol, alprenolol, bufuralol, timolol, bunitrolol etc.; Psychosis is as chlorpromazine, perphenazine, risperidone, tolperisone etc.; Antihypertensive is as debrisoquin, indoramine, urapidil etc.; Anti-anginal drug is as Parker former times woods, terodiline etc.; Analgesic is as tramadol; Medicine for the treatment of cough and asthma is as codeine, dextromethorphan etc.; Anti-arrhythmic is as encainide, sparteine, flecainide, Propafenone, mexiletine, amidonal.Described Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems can be the form of free alkali or inorganic acid salt; Be preferably hydrochlorate or sulfate.
Guan-fubase A of the present invention and Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems can be bought from market, also can from Radix Aconiti Coreani, extract method separated or by chemosynthesis and obtain, and its structural formula is as follows:
Guan-fubase A (GFA): R1=R3=-Ac; R2=H
Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems (GFI): R1=-Ac; R2=R3=H
The specific embodiment
Experimental example 1: Radix Aconiti Coreani total alkaloid salt antiarrhythmic pharmacological research
1. experiment material: Radix Aconiti Coreani total alkaloid salt, by the embodiment of the present invention 3 preparations; Lidocaine hydrochloride injection, the Shandong Province Xi Erkang pharmaceutical Co. Ltd of swimming; Experiment is provided with rabbit and is provided by animal housing of China Medicine University by Shanghai Si Laike animal center with rat.
2. the ARR protective effect that Radix Aconiti Coreani total alkali salt pair electricity irritation Rabbit Heart brings out
2.1 experimental technique
12 of rabbit, body weight 2.4 ± 0.6kg, is divided into two groups, and 6 every group, half and half, one group of male and female are Radix Aconiti Coreani total alkali group, and another group is lignocaine group.Urethane 1.2g/kg ear edge iv anesthesia is opened breast and is exposed heart, and is connected in pressure transducer with Gu Shi lever aroused in interest under artificial respiration, from JL-3 Xing San road physiograph, traces the easypro contracting curve of heart.Stimulating electrode is placed in to apex (positive pole) with left side, atrioventricular junction place (negative pole) and is connected in DGQ-2 type stimulator, and the method stimulation 10s with the wide 1ms of ripple, frequency 20Hz, stimulates once every 2min, successively increases stimulus intensity (mV).Record the Cor Leporis chamber of the causing value value in contrast of quivering.Then by rabbit ear vein, inject respectively Radix Aconiti Coreani total alkali or lignocaine, the various dose administration 10min of being separated by, after each administration, 5min measures and causes the threshold that quivers, and compares before administration.
2.2 experimental result
Experimental result is in Table 1.
The impact (N=6) (X ± S) of table 1 Radix Aconiti Coreani total alkali salt pair Cor Leporis electricity threshold of ventricular fibrillation current
* P<0.05, * * P<0.01 (with before administration relatively)
Result shows that the total alkali salt 2,4 of iv Radix Aconiti Coreani, 8mg/kg all can improve the Cor Leporis chamber of the causing value of cutting off from of quivering, and increases and act on reinforcement with dosage; The total alkali salt 4 of iv Radix Aconiti Coreani, 8mg/kg can significantly improve the Cor Leporis chamber of the causing value (P<0.05, P<0.01) of quivering.Illustrating to quiver to be significantly improved in chamber that the Radix Aconiti Coreani total alkaloids salt pair Stimulation In Rabbits heart causes causes the threshold effect that quivers.
3. the protective effect of Radix Aconiti Coreani total alkali salt pair Aconitine Induced rat ventricular arrhythmia
3.1 experimental technique
40 of rats, body weight 202 ± 16g, male and female half and half, are divided into 5 groups at random, with after 1.2g/kg urethane ip anesthesia, give the total alkali salt 4,8 of Radix Aconiti Coreani, 16mg/kg and lignocaine 15mg/kg respectively by tail vein.Matched group iv equivalent normal saline.After 2 minutes, with WSQ-A type micro-transfusion system, by external jugular vein constant speed, inject aconitine solution (1 μ g/ml, 0.2ml/min), and monitor the chamber of appearance early by electrocardioscope, chamber is fast, records the consumption of aconitine when quiver in chamber.
3.2 experimental result
The results are shown in Table 2.
The protective effect of table 2iv Radix Aconiti Coreani total alkali to Aconitine Induced rat ventricular arrhythmia
* p<0.05, * * p<0.01 (with matched group comparison)
During result shows, Radix Aconiti Coreani total alkaloid salt can increase Aconitine Induced chamber early, chamber speed, and the dosage quivering in chamber, total its increasing acting on Radix Aconiti Coreani alkali salt dosage increases; Wherein the total alkali salt of Radix Aconiti Coreani of high dose (8,16mg/g) can obviously increase Aconitine Induced chamber early; chamber speed; dosage (the P<0.05 quivering in chamber; P<0.01), the ventricular arrhythmia that iv Radix Aconiti Coreani total alkali salt pair Aconitine Induced is described there is significant protective effect.
Experimental example 2 Radix Aconiti Coreani total alkaloidss and the research of Guan-fu base A hydrochloride to the slow sodium-ion channel blocking effect of cardiac muscle
1 experimental technique
1.1 myocardial cell are separated
Normal guinea pig (male and female are not limit, 250 ± 20g) is hit dizzy, opens rapidly breast and takes out heart, put into 4 ℃ without calcium tyrode's solution, after pruning, by aorta, heart is hung on Langendorff device, with 37 ℃ without calcium tyrode's solution constant temperature perfusion, flow velocity 6~8mL/min.The about 5min of perfusion, clean and to change after congestion containing enzyme without the about 10~15min of calcium Zinciodati Comp solution perfusion, until cardiac muscle, present and expand when loose and translucent, cut left ventricle, in KB liquid, with glass dropper, blow and beat gently, filter, can obtain band clear, the bar-shaped Ventricular Myocytes of any surface finish, is kept in KB liquid.All experiments are all used 95%O with solution
2+ 5%CO
2saturated.
1.2 full cell patch pincers recording methods
At room temperature draw cell-preservation liquid number and drip in 2mL Tissue Culture Dish, be placed on inverted microscope (Nikon) object stage, treat that cell is standing adherent, with extracellular fluid perfusion, clean cell.Electrode is selected hard glass to draw the drawing of instrument (HEKA) secondary through microelectrode and is formed, after overheated polishing, electrode fills take interior liquid to enter resistance value after water is 4-6M Ω, choose that band is clear, neat in edge, surface be without granule, shrinkage-free cell, regulate Three dimensional steerable device to make eletrode tip shift to cell surface, gently execute negative pressure, form after high resistance seals, compensate fast electric capacity and form full cell record pattern to larger negative pressure suction broken cell film.Compensate slow electric capacity and series resistance, make electric capacity wink mark reduce to minimum.Maintain current potential-90mV, arrive+20mV of depolarization keeps 50ms, draws fast sodium current, and the electric current after fast sodium current complete deactivation is slow sodium current.Use the administration of regional perfusion drug-supplying system, record blank extracellular fluid, containing Radix Aconiti Coreani total alkali (by the embodiment of the present invention 1 preparation) or Guan-fu base A hydrochloride 0.1mmol/L, electric current when 0.3mmol/L and 1mmol/L, using blank electric current and the difference of administration electric current and the ratio of blank electric current as suppression ratio, relation with Hill equation y=Vmax*x^n/ (k^n+x^n) matching concentration and suppression ratio, draws half-inhibition concentration IC
50.
1.3 experimental solutions preparations
Without calcium tyrode's solution: weigh appropriate various solutes, be mixed with containing NaCl, KCl, MgCl with ultra-pure water
2, glucose, HEPES, taurine be respectively the solution of 137mmol/L, 5.4mmol/L, 1.2mmol/L, 10mmol/L, 10mmol/L, 10mmol/L, with NaOH, regulating pH is 7.40.
Containing enzyme without calcium tyrode's solution: in without calcium tyrode's solution, add bovine serum albumin and collagenase II type, make its concentration be respectively 1mg/mL, 0.3mg/mL, with NaOH, regulating pH is 7.40.
KB liquid: weigh appropriate various solutes, be mixed with containing KOH, KCl, KH with ultra-pure water
2pO
4, glutamic acid, MgCl
2, taurine, EGTA, HEPES, glucose be respectively the solution of 70mmol/L, KCl40mmol/L, 20mmol/L, 50mmol/L, 3mmol/L, 20mmol/L, 0.5mmol/L, 10mmol/L, 10mmol/L, with KOH, regulating pH is 7.40.
Liquid in electrode: weigh appropriate various solutes, be mixed with containing CsF, CsCl, MgCl with ultra-pure water
2, NaCl, Na
2-ATP, EGTA, HEPSE are respectively the solution of 110mmol/L, 20mmol/L, 3mmol/L, 10mmol/L, 5mmol/L, 10mmol/L, 5mmol/L, with CsOH, regulate pH to 7.2.
Extracellular fluid: add CsCl, CoCl without calcium tyrode's solution
2, CaCl
2make its concentration be respectively 5mmol/L, 3mmol/L, 1mmol/L.
2 experimental results
The results are shown in Figure 1-4.
Result demonstration, Radix Aconiti Coreani total alkaloids and Guan-fu base A hydrochloride are respectively IC to the slow sodium current inhibition strength of guinea pig ventricular myocardium
50=0.439mmol/L (relative molecular mass is with 465 calculating), IC50=0.580mmol/L.
Experimental example 3 Radix Aconiti Coreani total alkaloids Study on Preparation
1 Radix Aconiti Coreani ethanol merceration extracts and the comparison of alcohol heating reflux extracting method
1.1 experimental technique
Cold-maceration: will be ground into 500 grams of 10~20 object Radix Aconiti Coreani granules, with 25 ℃ of 1000ml95% ethanol, soak 24 hours, leach, adding for the second time 25 ℃ of 1000ml95% ethanol soaks 12 hours again, leach, adding for the third time 25 ℃ of 1000ml95% ethanol soaks 4 hours, leach, merge leachate, filter, decompression filtrate recycling ethanol obtains thick alcohol extractum, add a small amount of distilled water, place refrigerator, cold filtration, remove the impurity such as pigment, with petroleum ether extraction for several times, to remove wherein liposoluble constituent, use again chloroform extraction, chloroform extraction liquid is with reclaiming chloroform after natrium carbonicum calcinatum dewatering and filtering to dry, 95% ethanol turns molten, add hydrochloric acid to pH=3, then add crystal seed, place crystallize, with 95% ethyl alcohol recrystallization, obtain Radix Aconiti Coreani total alkaloid salt 0.098g, solution after chloroform extraction, n-butanol extraction, after reclaim under reduced pressure n-butyl alcohol, 95% ethanol turns molten, place refrigerator crystallize, through Molisch, react, TLC contrast, be accredited as glucide and obtain 0.83g.
Circumfluence method: will be ground into 500 grams of 10~20 order Radix Aconiti Coreani granules, use respectively 95% ethanol 1000ml, 800ml, 600ml hot dipping in 60 ℃ ± 2 ℃ water-baths is extracted 2 hours, 1 hour, 0.5 hour, merge extractive liquid, reclaim ethanol and obtain thick alcohol extractum, add a small amount of distilled water, place refrigerator, cold filtration, remove the impurity such as resin-like pigment, with petroleum ether extraction for several times, to remove wherein liposoluble constituent, use again chloroform extraction, chloroform extraction liquid dewaters with natrium carbonicum calcinatum, after filtering, reclaim chloroform to dry, 95% ethanol turn molten after, add hydrochloric acid to pH=3, add crystal seed, place crystallize, use 95% ethyl alcohol recrystallization, obtain 0.10g Radix Aconiti Coreani total alkaloid salt.Solution after chloroform extraction, n-butanol extraction, turns molten with 95% ethanol after reclaim under reduced pressure n-butyl alcohol, places refrigerator crystallize, and through Molisch reaction, TLC contrast, is accredited as glucide, obtains 1.50g.
1.2 experimental result
The results are shown in Table 3.
The comparison of two kinds of process for extracting of table 3
Extracting method |
Radix Aconiti Coreani total alkaloid salt yield % |
Saccharide yield % |
Cold-maceration |
0.0196 |
0.166 |
Circumfluence method |
0.0200 |
0.500 |
Result shows: merceration and reflux, extract, are carried, and Guan-fu base A hydrochloride yield is more approaching; But reflux, extract,, glucide yield, up to 0.5%, also has other water-solubility impurity, has not only affected Alkaloid separation, returns post processing and makes troubles, and therefore extracts Radix Aconiti Coreani total alkaloid salt and should adopt cold-maceration to be advisable.
2 ethanol merceration Study on extraction
2.1 instruments and medicine:
An Jielun Agilent ll00 high performance liquid chromatograph (quaternary gradient pump, DAD detector); Prunus mume (sieb.) sieb.et zucc. Teller-Tuo benefit (METTLER) AE-240 double-range electronic analytical balance; B ü chi RotavaporR-114 type Rotary Evaporators.
Guan-fubase A reference substance is bought from Nat'l Pharmaceutical & Biological Products Control Institute, and Radix Aconiti Coreani medical material is bought by Liaoning, Jilin.
Methanol, acetonitrile, sodium heptanesulfonate is chromatographically pure.
Water is pure water.
Other reagent are analytical pure.
The foundation of 2.2 Guan-fubase A content assaying methods
(1) chromatographic condition:
Take octadecylsilane chemically bonded silica as filler; With 1.5mg/mL heptanesulfonic acid sodium water solution (containing 0.2% triethylamine, adjusting pH=5.0 with phosphoric acid), for mobile phase A, take acetonitrile as Mobile phase B; Elution program is in Table 4; Flow velocity 1ml/min; Detect wavelength: 205nm; Column temperature: 25 ℃; Analysis time 40min; Theoretical cam curve is calculated and should be not less than 20000 by Guan-fubase A peak.
Table 4 elution program
Time (minute) |
Mobile phase A (%) |
Mobile phase B (%) |
0~16min |
80→76 |
20→24 |
16~22min |
76→70 |
24→30 |
22~38min |
70→66 |
30→34 |
38~40min |
66 |
34 |
Gradient elution completes back balance 10min |
80 |
20 |
(2) range of linearity:
It is appropriate that precision takes Guan-fu base A hydrochloride reference substance, and the mobile phase (A:B=3:1) of take is dissolved and is mixed with the solution that concentration is 1mg/ml; By above-mentioned chromatographic condition analysis, take reference substance peak area as vertical coordinate (y), reference substance concentration is abscissa (x), obtains regression equation y=6.38 * 103x+1.29 * 102, r=0.9998, linear range is 0.5-2.5mg/ml.
(3) preparation of reference substance solution:
It is appropriate that precision takes Guan-fu base A hydrochloride reference substance, and the mobile phase (A:B=3:1) of take is dissolved and is mixed with the solution that concentration is 1mg/ml, obtains.
2.2 experimental technique
Choose concentration of alcohol (%, A), merceration number of times (B), merceration time (my god, C), four factors of ethanol consumption (V/W, D) investigate, each factor is chosen three levels, adopts L9 (3
4) orthogonal table tests, quadrature gauge outfit designs in Table 5.The extractum obtaining dissolves with 400ml0.1mol/lHCl solution, is extracted with ethyl acetate 3 times, and water intaking layer, adjusts pH=9 with ammonia, is extracted with ethyl acetate 3 times, gets ethyl acetate layer, and reclaim under reduced pressure is drained to foaming without ethyl ester.Vacuum drying oven is dry, obtains total biological alkali extract of korean aconite roof, measures the content of Guan-fubase A.
The design of table 5 orthogonal experiment gauge outfit
2.3 experimental result
The results are shown in Table 6
Table 6 Orthogonal experiment results
Each factor R value size relatively, can find out which factor in extraction process in the highest flight.Press R value size, each factor primary and secondary is sequentially: A>C>D>B.In conjunction with the results of analysis of variance, factor A is the most remarkable, and factor C slightly takes second place, and factor B, D are not significantly factor.From the viewpoint of orthogonal test, only choose the best level collocation of significance factor, determine optimised process, significantly factor can not take the circumstances into consideration to determine one according to experiment condition (as saved medical material, solvent, time, the energy etc.) in principle.Therefore, best combination scheme is in this experiment: A2B1C3D1, the optimum extraction process of Radix Aconiti Coreani medical material be use compared with the medicinal powder of coarsegrain at the temperature of 25 ℃ with 5 times of amount ethanol extractions of 85% 4 times, each merceration 24h.
3 impurity-removing method researchs
3.1 experimental techniques: Radix Aconiti Coreani, after ethanol merceration extracts, except containing alkaloid, also has a large amount of fat-soluble pigments, resin, oils and fats etc., 2% aqueous hydrochloric acid solution is pinched molten rear acid liquid, is toughness caramel.In order to remove oil-soluble impurities, carried out following test:
Method one: acid liquid is directly filtered, remove pigment, resin, oils and fats etc.
Method two: adopt 2 ℃ of deepfreezes of acid liquid to make the floating layering of liposoluble constituent, the time is about 12~24 hours.
3.2 experimental result
The results are shown in Table 7.Result shows to adopt the method for 2 ℃ of deepfreezes of acid liquid better.
Table 7 sour water position alkaloid is removed pigment, the comparison of resin and oil and fat method
4 alkalization process researchs
4.1 experimental technique
Medicinal powder ethanol merceration by 5 times of amounts 85% at the temperature of 25 ℃ extracts 4 times, each merceration 24h, decompression recycling ethanol, to without alcohol taste, obtains alcohol extractum, pinches molten with hydrochloric acid solution, ethyl acetate extraction 3 times, sour water layer is adjusted to pH=9 with ammonia respectively, and NaOH solution is adjusted to pH=10, pH=11, is extracted with ethyl acetate rapidly respectively 3 times, reclaim under reduced pressure ethyl acetate, to foaming, is measured respectively Guan-fubase A content.
4.2 experimental result
The results are shown in Table 8.
Table 8 alkalization process result of study
? |
PH=9 (ammonia) |
pH=10(NaOH) |
pH=11(NaOH) |
Content (mg/g) |
17.38 |
16.78 |
16.53 |
Result shows, with ammonia, regulates pH=9, and Guan-fubase A content is the highest, and has good stability, and finally alkalization condition is defined as regulating pH=9 with ammonia.
5 Radix Aconiti Coreani total alkaloids process for refining researchs
5.1 experimental technique
Choose sour water consumption (V/W, A), acid number (mol/L, B), sour water layer extraction times is (inferior, C), aqueous alkali layer extraction times is (inferior, D) four factors are investigated, each factor is chosen three levels, adopts L9 (34) orthogonal table to test, and the rate of transform is tested as quantitative target.Orthogonal design gauge outfit is in Table 9.
The design of table 9 orthogonal design gauge outfit
5.2 experimental result
The results are shown in Table 10.
Table 10 orthogonal experiments
Result shows, factor D is the most remarkable, and factor B slightly takes second place, and factor A, C are significantly factor.Therefore, best combination scheme is in this experiment: A
1b
1c
1d
3be that the best process for refining of total biological alkali extract of korean aconite roof is for pinching molten with medical material alcohol leaching cream with the hydrochloric acid solution of 1 times of amount 1mol/L, be extracted with ethyl acetate 2 times, sour water layer is adjusted to pH=9 with ammonia, be extracted with ethyl acetate rapidly 4 times, ethyl acetate layer reclaim under reduced pressure ethyl acetate, to foaming, drying under reduced pressure had both obtained total biological alkali extract of korean aconite roof.
6 pulverizing medicinal materials granularity researchs
6.1 experimental technique
Radix Aconiti Coreani is ground into 10~20 orders, and 60~80 two kinds, order granularities, adopt merceration and timing agitation merceration, and extraction time is 48 hours, repeats 3 times, and extracting solution content is measured through HPLC.
6.2 experimental result
The results are shown in Table 11.
The content of the Guan-fubase A in table 1195% ethanol extraction different grain size Radix Aconiti Coreani
Experimental result shows, it is 10~20 orders that Radix Aconiti Coreani extracts optimal granularity, and optimum extraction mode is merceration timing agitation.
Embodiment 4 impacts of people's hepatomicrosome the effects hydrochloric acid Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems on the mono-substrate utilization ability of CYP2D6
1 experiment material and instrument:
1.1 experiment material
Mix people's hepatomicrosome (HLM) purchased from Ruide Liver Disease Inst. (Shanghai) Co., Ltd., liver by 10 donors makes, its CYP1A2, CYP2C9, CYP2C19, CYP2D6, CYP3A4, CYP2E1 activity are identified by auspicious moral, containing protein concentration 10mg/500 μ l.
Dextromethorphan hydrobromide (dextromethorphan hydrobromide) levofloxacin (levofloxacin) is purchased from Nat'l Pharmaceutical & Biological Products Control Institute.Radix Aconiti Coreani element in ninth of the ten Heavenly Stems standard substance are purchased from Nat'l Pharmaceutical & Biological Products Control Institute.
Na
2hPO
412H
2o, NaH
2pO
42H
2o, KCl, MgCl
26H
2o is purchased from Nanjing chemical reagent factory; Methanol (chromatographically pure), acetonitrile (chromatographically pure), nicotinamide-adenine dinucleotide phosphate (NADP+), G6P (G-6-P), glucose-6-phosphate dehydrogenase (G6PDH) are purchased from Sigma company.All the other reagent are commercially available analytical pure.
Microsome buffer (PBS): 0.1M KCl-phosphate buffer, contains: 0.1M KCl, 0.1M Na
2hPO
4, 0.1M NaH
2pO
4; PH=7.4.
NADPH energy-regenerating system: face with newly joining, contain: 10mM G-6-P, 0.5mM NADP+, 10mM MgCl
2, 1U/mL G6PDH.
1.2 instrument
The Finnigan of U.S. power & light company high performance liquid chromatography-quadrupole rod tandem mass spectrum combined instrument (containing Finnigan Surveyor highly effective liquid phase chromatographic system, Finnigan TSQ Quantum Discovery max mass spectrometer system, electric spray ion source, Xcalibur1.2 work station and LCQuan data processing software).
GENIE VORTEX-2 vortex mixed device; EPPENDORF High speed refrigerated centrifuge; Milli-Q Gradient A1 ultrapure water machine (Millipore Inc, USA).
2 experimental techniques:
Choose 0,0.2,0.8,2, hydrochloric acid Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems and people's hepatomicrosome of 10,50, a 100 μ mol/L concentration, and dextromethorphan/5 μ mol/L is in 37 ℃ and people's hepatomicrosome (final concentration is 0.2mg/mL) preheating 5min in 37 ℃ of waters bath with thermostatic control, then adds NADPH energy-regenerating system to start reaction.Optimization incubation time is 20min.In whole reaction system the content of organic solvent be controlled at≤1%.After 0 ℃ of ice bath cessation reaction, with containing interior mark (levofloxacin, methanol solution (1:1, v/v) Direct precipitation albumen 200ng/mL), the 3min that fully vibrates, quantitative transferase 45 0 μ L supernatant after the centrifugal 10min of 20000rpm, with 5 μ L sample introductions.Set up the blank that does not add hydrochloric acid Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems (replacing with solvent dimethyl sulfoxide) simultaneously.
3 experimental results
Experimental result is shown in Fig. 5.Result demonstration, the IC50 of hydrochloric acid Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems is 22 μ M, shows that hydrochloric acid Radix Aconiti Coreani element in the ninth of the ten Heavenly Stems can suppress the vigor of CYP2D6 enzyme effectively.
The total alkali salt of experimental example 5 Radix Aconiti Coreani Chinese People's Anti-Japanese Military and Political College Mus atrial fibrillation Functional observation
1 experiment purpose
Adopt ACh-CaCl
2cause rat atrial fibrillation model, the anti-atrial fibrillation effect of the total alkali salt of research Radix Aconiti Coreani, experimental result demonstration, preventative the giving of the total alkali salt of Radix Aconiti Coreani, can obviously reduce the atrial fibrillation persistent period, effectively suppresses the broadening of QRS wave group.Experiment is usingd dronedarone as positive control.The total alkali salt of Radix Aconiti Coreani is at ACh-CaCl
2cause on rat atrial fibrillation model anti-atrial fibrillation effect definite.
2 experiment materials
2.1 laboratory animal
Adult SD rats, male, clean level, by Shanghai, western pul-Bi Kai laboratory animal company limited provides.The quality certification number: SCXK (Shanghai) 2008-0016.Temperature 20-24 ℃, raises under the environment of humidity 50%, throws light on 12 hours.Freely drink water, feed.
2.2 reagent and instrument
Dronedarone, sterling;
The total alkali salt of Radix Aconiti Coreani, by embodiment 3 preparations;
Acetylcholine, sterling, Sigma;
All the other reagent: domestic, analytical pure, commercially available;
BL-420F biological function experimental system: Chengdu TME Technology Co., Ltd..
3 experiment grouping and operations
Normal group and modeling, treatment group are established in experiment.10 of normal rats, ip normal saline 7 days.All the other rat 10% chloral hydrate anesthesia rats (0.3ml/100g), tail vein injection ACh-CaCl
2mixed liquor (0.1g CaCl2+6.6ugACh/10mlH2O, 0.1ml/100g), once a day, the 4th day, 1. rat is divided into model group, the 2. total alkali salt low dose group of Radix Aconiti Coreani (2mg/kg), 3. dosage group (6mg/kg) in the total alkali salt of Radix Aconiti Coreani, the 4. total alkali salt high dose group of Radix Aconiti Coreani (18mg/kg) and dronedarone group (30mg/kg) at random.Drug effect matched group is established 6mg/kg dosage.The equal po administration of all medicines 3 days, observes drug effect.
4 experimental techniques
10% chloral hydrate anesthesia rat (0.3ml/100g), records II lead electrocardiogram after anesthesia.In the II lower tail vein injection ACh-CaCl that leads
2mixed liquor (0.1g CaCl
2+ 6.6ugACh/10mlH
2o, 0.1ml/100g), record the atrial fibrillation persistent period.Second and third day repeats above operation.The 4th day, each treatment group is 3h before starting modeling, and gavage gives the medicine of corresponding dosage, tail vein injection ACh-CaCl
2mixed liquor, dosage and volume, with first three day, record the atrial fibrillation time.More than repeating, be operated to the 7th day.Each organizes rat modeling, after having treated, puts to death rat, and speed is cored and dirtyly in freezing K-H liquid, cleaned, and separated left atrium, gets right ventricle muscle, uses the measurement of biological function experimental system to bring out the threshold value of atrium action potential and the effective refractory period in atrium.
5 experimental results
Experimental data adopts means standard deviation (x ± s) to represent (n=6),
5.1 Radix Aconiti Coreani total alkali salt antagonism atrial fibrillation effects
Experimental result is in Table 12, Fig. 6.Result shows: rat tail vein injection ACH-Cacl2 mixed liquor, with modeling time lengthening, the rat atrial fibrillation time obviously extends, and gives after the total alkali salt of Radix Aconiti Coreani, according to concentration, shortens the rat atrial fibrillation time.
The impact (x ± s, n=6) of table 12. Radix Aconiti Coreani total alkali salt pair rat atrial fibrillation time (s)
The impact of 5.2 Radix Aconiti Coreani total alkali salt pair atrial fibrillation rat ERP
Experiment has been measured respectively and has respectively been organized rat left atrium ERP numerical value, and as the preliminary index of weighing rat electrocardio reconstruct after atrial fibrillation, experimental result is as table 13, Fig. 7.Result shows: rat model atrium and ventricular muscles ERP obviously shorten, and after pointing out repeatedly atrial fibrillation to stimulate, the reconstruct of rat myocardial cell electricity, forms atrial fibrillation substrate, and the total alkali salt of Radix Aconiti Coreani can effectively suppress the electric reconstruct of myocardial cell, maintains electrocardio stable.
The impact (x ± s, n=6) of table 13 Radix Aconiti Coreani total alkali salt pair rat ERP
To sum up, (2,6,18mg/kg) po (oral) administration, can resist rat atrial fibrillation to three dosage of the total alkali salt of Radix Aconiti Coreani, shortens the atrial fibrillation persistent period, improves the atrial electrical remodeling that atrial fibrillation causes, three dosage give, and result shows obvious dose-effect relationship.Anti-atrial fibrillation effect is definite.
The therapeutical effect (acetylcholine merging) of the dog atrial fibrillation that experimental example 6 Radix Aconiti Coreani total alkali salt pair rapid atrial pacings cause
1 experimental technique
Adult beagle dog, male and female are not limit, body weight 10-20kg.The anesthesia of intravenous injection pentobarbital sodium solution (3% solution, 10ml/kg).According to circumstances append in right amount anesthetis.After anesthesia, lie on the back fixing.Cut off cervical region and front by hair.Medisection cervical region, does tracheal intubation and connects Ventilators (16 beats/min of respiratory frequencys, tidal volume 12ml/kg, respiratory quotient 3:5).Separated right vagus nerve, cuts off, and inserts pair of electrodes connect electrostimulator at proximal part.Medisection breastbone top tissue, breaks the 3rd before subsides left border of sternum, and 4 ribs, expose pericardium.Cut off pericardium and make pericardium hanging basket, expose heart.On right atrium surface, hook the electrode that a pair of use 4 * 6 sewing needles are made, connect electrostimulator.Every half an hour, use 0.1ms, the continued stimulus of 20Hz, the intensity that 0.05V increases progressively stimulates right atrium to measure pacing threshold.Pacing threshold refers under normal condition and uses 20Hz, the voltage that 50 trains of 1ms can pace-making atrium.Jugular vein instillation acetylcholine 200 μ g/mL, 0.2ml/min, then with 2 times of pacing thresholds, stimulate and cause atrial fibrillation, measure the atrial fibrillation persistent period. at pacing threshold and cause the threshold that quivers stable after respectively gavage to the total alkali salt of Radix Aconiti Coreani (preparing by embodiment 3) (4mg/kg, 8mg/kg) He Jue naphthalene Dalong (20mg/kg).Within after administration every 0.5 hour, measure pacing threshold and cause quiver threshold and atrial fibrillation persistent period.
2 experimental results
The results are shown in Figure 8-9.
Experimental result shows, the total alkali salt 4 of Radix Aconiti Coreani, and 8mg/kg is preventative to be given, and electrocardio dystopy pacing threshold increases, and prompting atrium electrical stability increases, and the atrial fibrillation persistent period obviously shortens, and shows the anti-atrial fibrillation effect of medicine.
The therapeutical effect (vagus nerve stimulation merging) of the dog atrial fibrillation that experimental example 7 Radix Aconiti Coreani total alkali salt pair rapid atrial pacings cause
1 experimental technique
Adult beagle dog, male and female are not limit, body weight 10-20kg.The anesthesia of intravenous injection pentobarbital sodium solution (3% solution, 10ml/kg).According to circumstances append in right amount anesthetis.After anesthesia, lie on the back fixing.Cut off cervical region and front by hair.Medisection cervical region, does tracheal intubation and connects Ventilators (16 beats/min of respiratory frequencys, tidal volume 12ml/kg, respiratory quotient 3:5).Separated right vagus nerve, cuts off, and inserts pair of electrodes connect electrostimulator at proximal part.Medisection breastbone top tissue, breaks the 3rd before subsides left border of sternum, and 4 ribs, expose pericardium.Cut off pericardium and make pericardium hanging basket, expose heart.On right atrium surface, hook the electrode that a pair of use 4 * 6 sewing needles are made, connect electrostimulator.Every half an hour, use 0.1ms, the continued stimulus of 20Hz, the intensity that 0.05V increases progressively stimulates right atrium to measure pacing threshold.Use 0.1ms, 5V, the impulse stimulation vagus nerve of 5-20Hz, makes R-R interval surpass 1s, uses 0.1ms simultaneously, 20Hz, the train of 50 times causes atrial fibrillation, and intensity increases progressively with 0.05V, and the voltage while having lasting atrial fibrillation to stimulate for 50 times after finishing is for causing the threshold that quivers.Pacing threshold and causing quiver threshold stable after respectively gavage to (4mg/kg) He Jue naphthalene Dalong (20mg/kg) of the total alkali salt of Radix Aconiti Coreani (preparing by the embodiment of the present invention 3).Mensuration pacing threshold per hour and cause the threshold that quivers after administration.
2 experimental results
The results are shown in Table 14.
Table 14 Radix Aconiti Coreani total alkali is on pacing threshold and the impact that causes the threshold that quivers
Experimental result shows, preventative the giving of the total alkali salt 4mg/kg of Radix Aconiti Coreani, and electrocardio dystopy pacing threshold increases 69.3%, and prompting atrium electrical stability increases, and effect is with certainly how close.Due to electric Stabilization, cause that the stimulus intensity of atrial fibrillation need increase more than 86%, show the anti-atrial fibrillation effect of medicine.From the drug effect time, the total alkali salt of Radix Aconiti Coreani onset time needs 2 hours-3 hours, than certainly how slightly slow, but the persistent period is longer.
Embodiment
Embodiment 1
The preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, be ground into 20 order coarse powder, extract 4 times at 25 ℃ with 5 times of amount 85% ethanol mercerations, each 24 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 1 times of amount 1mol/l, acid solution, in 2 ℃ of deepfreezes 24 hours, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 2 times, sour water mother solution adds ammonia and regulates pH=9;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 4 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Embodiment 2
The preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, be ground into 20 order coarse powder, extract 2 times at 10 ℃ with 3 times of amount 95% ethanol mercerations, each 36 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 3 times of amount 0.5mol/l, acid solution, in 2 ℃ of deepfreezes 24 hours, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 4 times, sour water mother solution adds ammonia and regulates pH=8;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 2 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Embodiment 3
The preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, be ground into 20 order coarse powder, extract 4 times at 25 ℃ with 5 times of amount 85% ethanol mercerations, each 24 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 1 times of amount 1mol/l, acid solution, in 2 ℃ of deepfreezes 24 hours, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 2 times, sour water mother solution adds ammonia and regulates pH=9;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 4 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.
Step 5: the total alkaloids dissolve with ethanol that step 4 is obtained, salt adding acid for adjusting pH=3, standing, sucking filtration, crystallize, obtains Radix Aconiti Coreani total alkaloid salt.
Embodiment 4
The preparation method of Radix Aconiti Coreani total alkaloid salt comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, be ground into 20 order coarse powder, extract 3 times at 30 ℃ with 8 times of amount 75% ethanol mercerations, each 12 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous hydrochloric acid solution of 2 times of amount 1.5mol/l, acid solution, in 2 ℃ of deepfreezes 12 hours, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, be extracted with ethyl acetate 2 times, sour water mother solution adds ammonia and regulates pH=11;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 4 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids;
Step 5: the total alkaloids dissolve with ethanol that step 4 is obtained, salt adding acid for adjusting pH=3, standing, sucking filtration, crystallize, obtains Radix Aconiti Coreani total alkaloid salt.
Embodiment 5
The preparation of Radix Aconiti Coreani total alkaloids salt tablets:
By the total alkali salt of Radix Aconiti Coreani of embodiment 5 preparations, SMCC90 (MCC102 containing 98% and 2% micropowder silica gel), dicalcium phosphate dihydrate, colloidal silica, magnesium stearate, be the ratio of 50:72:25:3:0.75 by weight, first by crude drug and colloidal silica premix, then add diluent SMCC90 and dicalcium phosphate dihydrate, finally add magnesium stearate lubricant, mix, tabletting, obtains Korean monkshood root total alkali salt tablet.
Described tablet day, taking dose was 90-150mg/65kg.
Embodiment 6
The preparation method of Radix Aconiti Coreani total alkaloids comprises the steps:
Step 1: get Radix Aconiti Coreani medical material, be ground into 20 order coarse powder, extract 2 times at 10 ℃ with 3 times of amount ethyl acetate mercerations, each 36 hours, merge extractive liquid,, reclaimed solvent, obtains extractum;
Step 2: get the extractum that step 1 obtains, pinch moltenly with the aqueous acetic acid of 3 times of amount 0.5mol/l, acid solution, in 2 ℃ of deepfreezes 12 hours, is removed to the oil-soluble impurities on upper strata, get acid liquid;
Step 3: get the acid liquid that step 2 obtains, use acetone extract 4 times, sour water mother solution adds ammonia and regulates pH=8;
Step 4: the solution through liquid ammonia alkalinization in step 3 is extracted with ethyl acetate rapidly 2 times, gets ethyl acetate layer, reclaim solvent, vacuum drying, obtains Radix Aconiti Coreani total alkaloids.