CN1631895A - Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound - Google Patents

Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound Download PDF

Info

Publication number
CN1631895A
CN1631895A CN 200310119389 CN200310119389A CN1631895A CN 1631895 A CN1631895 A CN 1631895A CN 200310119389 CN200310119389 CN 200310119389 CN 200310119389 A CN200310119389 A CN 200310119389A CN 1631895 A CN1631895 A CN 1631895A
Authority
CN
China
Prior art keywords
amygdaloside
preparation
group
heart
blood
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
CN 200310119389
Other languages
Chinese (zh)
Other versions
CN1318439C (en
Inventor
吴咸中
伍孝先
赵连根
王兴民
刘俊红
陈玉玲
刘大全
李棣华
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
TIANJIN NANKAI HOSPITAL
Original Assignee
TIANJIN NANKAI HOSPITAL
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by TIANJIN NANKAI HOSPITAL filed Critical TIANJIN NANKAI HOSPITAL
Priority to CNB2003101193893A priority Critical patent/CN1318439C/en
Publication of CN1631895A publication Critical patent/CN1631895A/en
Application granted granted Critical
Publication of CN1318439C publication Critical patent/CN1318439C/en
Anticipated expiration legal-status Critical
Expired - Fee Related legal-status Critical Current

Links

Images

Landscapes

  • Medicines Containing Material From Animals Or Micro-Organisms (AREA)
  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)

Abstract

Disclosed are a method for preparing amygdalin and its application in promoting blood circulation of brain and pancreas and hurt, which belong to medical application of medicine containing organic effective components. The invention has supplied a medical application of prevention, which can prevention and cure cerebral ischemia caused by increase of blood consistency, has protective effect to heart breakdown, cure acute pancreatitis, increases microcirculation of blood in skin issue and promote wound healing. Besides, a method to prepare amygdalin is disclosed, in which apricot is processed through squeezing of oil and hydrophilic degreasing by diethyl ether and other techniques, finally acquiring pure amygdalin with high productivity, purity, simple abstraction and separation.

Description

The application in preparation promotion heart brain pancreas and the sanguimotor amygdaloside preparation of wound of the preparation method of amygdaloside and amygdaloside
Technical field
The present invention relates to contain the medicinal use of the pharmaceutical product of organic effective constituent, specifically being a kind of preparation method of amygdaloside and amygdaloside promotes application in heart brain pancreas and the sanguimotor amygdaloside preparation of wound in preparation.
Background technology
Peach kernel, Semen Armeniacae Amarum are the kind that Chinese Pharmacopoeia is included, aboundresources.
Semen Armeniacae Amarum belongs to the Rosaceae (Rosaceae) bitter, and tepor is slightly poisonous.Have relieving cough and asthma, the function that relaxes bowel.After this product oral administration of therapeutic dose, its effective constituent amygdaloside is slowly hydrolysis in vivo, generates micro-prussic acid gradually, and the latter is sedative effect to respiratory centre, makes respiratory movement be tending towards quiet and effect that present antibechic and relieving asthma.Be cough-relieving, the Chinese medicine of relievining asthma commonly used.Its chemical ingredients: contain amygdaloside (amygdalin), fatty oil, synaptase (emulsin), amygdalase (amygdalase), prunase (prunase), oestrone, alpha-estradiol, desmosterol etc.
Often Semen Armeniacae Amarum being made formulations such as pill, tablet, syrup clinically uses.
Peach kernel belongs to the Rosaceae (Rosaceae), and bitter but sweet flavor is flat.Function cures mainly: the broken capable stasis of blood of blood, moisturize laxation.Control through closing, pyreticosis is held blood, wandering arthritis, malaria, wound, swelling and pain due to blood stasis, the dry constipation of blood.Its chemical ingredients: contain amygdaloside (amygdalin), synaptase (emulsin), fatty wet goods.
Peach kernel also is one of raw material of using always in Chinese patent medicine preparation.
Chinese patent 1319431 discloses a kind of " the enhancement method unit and thing and the evaluation method that contain amygdaloside material anti-tumor activity ", be by infraredly bake, distillers yeast fermentation and dope promote anticancer functions such as containing amygdaloside loquat seed.Under the concentration conditions of the product that adds and increase the treated mistake that contains amygdaloside, in system, increase the formation of lipid peroxide by uviolizing two carbon acids.Lipid peroxide forms manyly more, and the anticancer function in evaluation and the prediction oral route is strong more.The effect that contains the amygdaloside material with this method evaluation.
Chinese patent 1365979 discloses a kind of " extraction separation of effective constituent amygdaloside and process for purification " is that Semen Armeniacae Amarum squeezing is deoiled, and adds the extraction using alcohol 3 times that 3-6 doubly measures, filtration under diminished pressure, merging filtrate, amygdaloside is placed, separated out to decompression recycling ethanol, filter crude product; The amygdaloside crude product through dissolve with ethanol, filtration, refrigeration, place, separate out white bunch shape crystallization, filtration under diminished pressure with a small amount of ether and washing with alcohol, must purity be the quantitative reference substance of amygdaloside more than 99%.This invention has solved for a long time amygdaloside and has made the difficult problem that effective constituent is destroyed, curative effect reduces with synaptase enzymolysis or hydrolysis.Reference substance gets the purity height, has widespread use and is worth.
Summary of the invention
The present invention is in order to solve the medical effect that effective constituent had in the Chinese medicine peach kernel, and provide a kind of medicine source more widely amygdaloside promote application in heart brain pancreas and the sanguimotor amygdaloside preparation of wound in preparation; A kind of preparation method of amygdaloside also is provided simultaneously.
The principle of the invention:
Though peach kernel, almond have difference in function aspect curing mainly, but its contained chemical ingredients has great common point.After determining the clear and definite function of promoting blood circulation to disperse blood clots of peach kernel by the quadrature screening, determine to extract the main component-amygdaloside in the peach kernel, and qualitative analysis amygdaloside and assay have been carried out, because amygdaloside also is present in the Semen Armeniacae Amarum, and Semen Armeniacae Amarum technology of overvoltage oil when medicinal, therefore it is more convenient to extract processing, so in the experimental study of amygdaloside, all use from the Semen Armeniacae Amarum cake and extract amygdaloside.
Amygdalate main effective constituent is amygdaloside, amygdaloside easily is stored in heterocellutate synaptase enzymolysis in the Semen Armeniacae Amarum together, its chemical property is for being soluble in hot ethanol, be insoluble in ethanol, so select for use and squeeze the almond cake of removing overwhelming majority oil, adopt the further degreasing of ether, the method for alcohol reflux is obtained through refining amygdaloside fast, simply.
The preparation method of amygdaloside:
The Semen Armeniacae Amarum 1Kg of squeezing after the deoiling 4000-5000ml that adds diethyl ether divides 2 reflux degreasings, filters standby; Add 95% alcohol reflux three times after the dregs of a decoction are waved most ether, each 3000-5000ml, filtered while hot, merging filtrate, decompression recycling ethanol is doubly measured volume to the 1-2 of crude drug amount, is placed to room temperature, adds the ether of 1/2 amount again, the container bottom chromatography goes out to be stained with the oily precipitation of wall, produce supernatant liquor, place, separate out crystallization, suction filtration gets the amygdaloside crude product; The amygdaloside crude product is added 20-40 times of dissolve with ethanol, filtration, places, separates out the crystallization of amygdaloside white plates, and filtration under diminished pressure with the crystallization of 100-200mL washing with alcohol, promptly gets the pure product of amygdaloside, and yield is more than 4%, and purity reaches more than 90%.
Described preparation method, but its amygdaloside crude product repeated treatments 1-2 time, but each amount of alcohol must reduce by half.
The application of amygdaloside in preparation promotion heart brain pancreas and the sanguimotor amygdaloside preparation of wound:
One. amygdaloside is to the effect of cerebral blood circulation.
1. treatment is because of the cerebral ischemia of blood viscosity due to raising.The circulation blood flow at the input all can increasing of amygdaloside vein rat's pial and brain essence two positions illustrates that the vasodilation reaction at two positions has synchronism; Effect manifests later, and after the intravenous injection 30 minutes, effect is increase progressively, in the time of 60 minutes and before the administration notable difference is arranged.For this reason, before causing the blood flow reduction, give amygdaloside, the pathogenic effects of energy antagonism dextran.
2. to the influence of brain microcirculation disorder.Be used for prevention and treatment as injection suprarenin, Pituitrin and mesencephalic arteries ligation.
Two. the amygdaloside treatment is in heart failure.
Semen Armeniacae Amarum is done and can be kept contract power and contraction frequency of isolated rat heart coronary flow, the heart in a long time and remain unchanged.Use the amygdaloside perfusion and can make isolated heart in the long period, keep the heart normal function, cardiac failure is had provide protection.
Three. amygdaloside treatment acute pancreatitis.
Amygdaloside has influence preferably to pancreatic blood flow and oxygen consumption, and white corpuscle rolls and the increase of adhesion number in the time of reducing heavy acute pancreatitis, can increase velocity of blood flow and wall is cut rate; By suppressing white corpuscle endotheliocyte excessive adhesion, reduce white corpuscle in in-house gathering, thereby the outer internal organs of pancreas are shielded; The transition of rat blood serum NO raises during to acute pancreatitis the reduction effect.
Four. amygdaloside is short through wound healing.
Improve the subcutis oxygen partial pressure, increase the skin histology microcirculation blood flow, the quickening that cicatrizes a wound improves the otch breaking tenacity, is of value to the healing of ischemic skin incision.
Zhi Bei amygdaloside productive rate height, purity height, preparation method is easy like this.
As above Zhi Bei amygdaloside shows to have prevention and treatment because of the cerebral ischemia of blood viscosity due to raising through experimentation on animals, and cardiac failure is had provide protection, to treatment of acute pancreatitis with promote the effect of wound healing, and has significant effect.Therefore, the present invention provides a kind of new pharmaceutical preparation for clinical medicine, and provides new medicinal use for said preparation.
Description of drawings
Fig. 1 is sample chromatogram figure of the present invention
Fig. 2 is the reference substance color atlas
Fig. 3 be physiological saline to rat's pial (on) and the microcirculatory influence of brain essence (descending).
Fig. 4 be amygdaloside to rat's pial (on) and the microcirculatory influence of brain essence (descending).
The rat's pial that Fig. 5 causes for the polymer dextran (on) and brain essence (descending) microcirculation variation.
The rat's pial that Fig. 6 causes the polymer dextran for amygdaloside (on) and the prophylactic effect of brain essence (descending) microcirculation disturbance.
Fig. 7 a is that the YHI+ amygdaloside organizes microcirculation to change to pancreas.
Fig. 7 b is that physiological saline organizes microcirculation to change to pancreas.
Embodiment
Directly get almond cake 1Kg, suitably pulverize the back and cross 20 mesh sieves, the 4000mL that adds diethyl ether divides 2 reflux degreasings, filter, add 95% alcohol reflux three times, each 5000mL after the dregs of a decoction are waved most ether, filtered while hot, merging filtrate, decompression recycling ethanol is to 1500mL, be placed to room temperature slightly, add the ether of 1/2 amount again, place, the container bottom chromatography goes out to be stained with the oily mater of wall, and supernatant liquor is produced, and continues to place, separate out crystallization, suction filtration gets amygdaloside crude product 61g.The amygdaloside crude product is added 1200mL ethanol heating for dissolving, filtration, places, separates out the crystallization of amygdaloside white plates, and filtration under diminished pressure is used the small amount of ethanol wash crystallization, uses 200mL washing with alcohol 2 times, gets the pure product 41g of amygdaloside, and purity reaches more than 90%.
Pharmaceutical dosage form: injection powder preparation.
The clinical using dosage of recommendation of injection amygdaloside powder preparation is 2ml/kg/h, and the conversion method of a transfusion dosage and an implantation dosage is undetermined.
One. the qualitative and detection by quantitative of amygdaloside:
1. thin-layer chromatography:
Get amygdaloside standard substance (Chinese biological goods calibrating institute, lot number 820-9401), be mixed with the solution that 1mL contains 2mg with methyl alcohol, in contrast product solution.Get the amygdaloside that the present invention obtains through refining, be mixed with the solution that 1mL contains 2mg with methyl alcohol equally, as need testing solution.Draw above-mentioned two kinds of solution 10uL respectively, point is on same silica GF254 thin layer plate (Yantai Chemical Industry Research Inst.), developping agent is the water saturation chloroform: methyl alcohol (2: 1), launch, take out, dry, put under the ultraviolet lamp (UV254) and inspect, in the trial-product chromatogram, with the corresponding position of reference substance chromatogram on show the blackening point of same color.
2.HPLC method is measured amygdaloside content:
Chromatographic condition: with octadecylsilane chemically bonded silica is weighting agent; Moving phase is the water that contains 0.1% phosphoric acid: methyl alcohol (80: 20); The detection wavelength is 210nm, and flow velocity is 0.9mL/min, and theoretical plate number is calculated by amygdaloside should be not less than 5000.
Get amygdaloside standard substance (lot number 820-9401), be mixed with the solution that 1mL contains about 0.2mg with methyl alcohol, in contrast product solution.Get the present invention again and make amygdaloside and be mixed with the solution that 1mL contains about 0.2mg, as need testing solution with methyl alcohol.
The drafting of typical curve: by above-mentioned chromatographic condition, sample introduction 4ul, 8ul, 10ul, 12ul, 16ul draw the area integral value respectively, with ug is X-coordinate, and area is an ordinate zou, the drawing standard graphic representation, be a straight line, linear equation is Y=8.893e-007X+1.686e-002, R=0.9999
Press the external standard method trial-product, sample introduction 10ul, reference substance is consistent with the liquid chromatogram retention time of trial-product.Amygdaloside content is 98.4%.
Adopt the normalization method of high-efficient liquid phase technique to carry out purity test, with the above-mentioned content basically identical of surveying.Standard substance content is 97.70%, and the amygdaloside content that the present invention obtains through refining is 99.18%.
Two. the pharmacological action of amygdaloside:
(1) promote cerebral blood circulation, treatment is because of the cerebral ischemia of blood viscosity due to raising.
1. to the influence of brain microcirculation
Purpose: for measuring the input of amygdaloside vein to rat's pial and the microcirculatory influence of brain essence.
Method: 40 of healthy II level Wistar rats are divided into 4 groups, 10 every group.During experiment with rat with 10% urethane intraperitoneal injection of anesthesia (1ml/100g body weight), endocranium is worn out after vowing strong seam both sides sphenotresia by crown portion, inserts laser-Doppler microcirculation electrode respectively, measures pia mater and brain essence blood flow.The stable back of blood flow in each group respectively vein input physiological saline (control group) and basic, normal, high dosage amygdaloside (1.5%, 3% and 6%, 2ml/h).Observing two position microcirculation blood flows changed 1 hour.
The result: physiological saline does not have influence, and three dosage amygdalosides all can increase by two position blood flows, and are the most obvious with effect of high dosage.
Conclusion: the input of amygdaloside vein can increase rat's pial and brain essence microcirculation blood flow.(table 1,2)
Table 1 amygdalosides etc. are to the influence of rat's pial microcirculation blood flow (PU) (x ± s)
After the administration (branch)
Group administration preceding 5 15 30 60
Control group (7) 216.62 ± 131.73 208.51 ± 139.19 198.05 ± 137.99 197.25 ± 136.12 207.28 ± 140.61
Administration I group (7) 143.69 ± 104.28 132.68 ± 69.27 138.38 ± 69.30 151.76 ± 89.00 182.93 ± 125.93 *
Administration II group (10) 180.57 ± 43.25 175.70 ± 44.26 179.98 ± 46.34 210.40 ± 62.69 222.40 ± 75.60 *
Administration III group (9) 151.87 ± 74.24 162.11 ± 90.96 168.23 ± 87.85 174.15 ± 100.96 188.84 ± 102.41 *
With before the administration relatively: *P<0.05 () number of animals
Table 2 amygdalosides etc. are to the influence of rat brain essence microcirculation blood flow (PU) (x ± s)
After the administration (branch)
Group administration preceding 5 15 30 60
Control group (7) 130.79 ± 40.11 130.35 ± 32.77 141.30 ± 6.30 134.99 ± 44.55 122.94 ± 62.55
Low dose group (7) 145.19 ± 104.82 144.36 ± 109.55 146.18 ± 110.16 154.53 ± 133.75 161.79 ± 145.62 *
Middle dosage group (10) 103.21 ± 26.40 101.88 ± 29.76 103.53 ± 32.90 108.14 ± 33.06 112.20 ± 29.76 *
High dosage I group (9) 110.13 ± 30.46 108.68 ± 31.77 110.41 ± 34.36 115.10 ± 41.04 128.09 ± 53.55 *
With before the administration relatively: *P<0.05 () number of animals
2. to the influence of brain microcirculation disorder
Purpose: the provide protection of the rat brain microcirculation disturbance that the research amygdaloside causes the polymer dextran.
Method: use 10% dextran tail vein injection (9ml/kg) and cause rat brain microcirculation disturbance, the amygdaloside of (treatment group) or preceding 30min (prevention group) tail vein input is meanwhile observed its treatment and prophylactic effect to brain microcirculation disorder.Cerebral blood flow change application laser Doppler flowmetry (LDF, Sweden, 5001 series) is measured.
The result: the polymer dextran obviously reduces the rat brain microcirculation, and amygdaloside does not show obvious therapeutic action, but significant prophylactic effect is arranged.
Conclusion: amygdaloside has tangible prophylactic effect to the rat brain microcirculation disturbance that the polymer dextran causes.(table 3,4; Fig. 5,6)
Table 3 amygdaloside changes (x ± s) to brain microcirculation disorder rat's pial microcirculation blood flow (PU)
After the administration (branch)
Before the group administration
5 15 30 60
Control group (7) 216.62 ± 131.73 208.51 ± 139.19 198.05 ± 137.99 197.25 ± 136.12 207.28 ± 140.61
Model group (8) 150.77 ± 63.49 122.11 ± 48.77 115.23 ± 64.38 107.60 ± 66.04 *90.60 ± 46.79 *
Treatment group (11) 141.37 ± 68.52 109.17 ± 74.04 102.78 ± 49.66 *87.03 ± 45.86 *90.13 ± 55.67 *
Prevention group (9) 142.36 ± 28.22 144.02 ± 32.85 136.99 ± 33.85 133.44 ± 35.82 142.14 ± 43.81
With before the administration relatively: *P<0.05; *P<0.01 () number of animals
Table 4 amygdaloside changes (x ± s) to brain microcirculation disorder rat brain essence microcirculation blood flow (PU)
After the administration (branch)
Before the group administration
5 15 30 60
Control group (7) 130.79 ± 40.11 130.35 ± 32.77 141.30 ± 6.30 134.99 ± 44.55 122.94 ± 62.55
Model group (8) 132.37 ± 36.07 106.59 ± 36.36 *91.33 ± 30.67 *84.60 ± 22.05 * *84.46 ± 24.63 * *
Treatment group (11) 143.87 ± 34.58 128.92 ± 41.14 98.75 ± 33.46 *89.63 ± 31.52 *90.51 ± 36.52 *
Prevention group (9) 143.87 ± 19.64 151.55 ± 41.59 149.07 ± 63.30 143.64 ± 83.21 159.33 ± 124.44
With before the administration relatively: *P<0.05; *P<0.01 () number of animals
(2). treatment is in heart failure
Purpose: observed amygdaloside to the contract influence of power, coronary flow and contraction frequency of the isolated rat heart heart.
Method: using modified Langendorff isolated heart perfusion method.After stationary phase, carry out perfusion, observe desired indicator and change with the perfusate that contains amygdaloside.
The result: control group (isolated heart perfusate) is because the condition restriction control group of isolated perfusion sample is promptly seen coronary flow decline after 10 minutes, and amygdaloside administration group (application contains the perfusate perfusion of amygdaloside) just begins to descend to testing latter stage (50,60 minutes) coronary flow.Then can to keep coronary flow in 60 minute observation period constant if share with radix paeoniae rubrathe extracting solution; Amygdaloside does not have influence substantially to heart contraction frequency and convergent force.
Conclusion: with the continuity of perfusion time, the heart coronary flow reduces gradually, gives amygdaloside and can keep contract power and contraction frequency of isolated rat heart coronary flow, the heart in a long time and remain unchanged.(table 5)
Table 5 amygdalosides etc. are to the influence of isolated rat perfusion heart coronary flow
Group is moving gives After the administration
The thing medicine
Not
Before the number
5 10 15 20 25 30 40 50 60
Control group 8 4.54 4.88 4.26 4.19 4.00 ± 4.06 ± 3.93 ± 3.95 ± 3.96 ± 4.09 ±
± ± ± ± 1.13 ** 1.02 * 1.08 ** 1.08 * 1.24 * 1.22
1.17 1.32 1.10 * 1.10 *
Compound Salviae Miltiorrhizae 8 4.46 4.84 4.46 4.24 4.15 ± 4.08 ± 4.16 ± 4.04 ± 3.90 ± 3.71 ±
Injection liquid ± ± ± ± 1.17 1.14 1.21 1.08 1.02 1.00 *
1.51 1.47 1.22 1.17
Peach kernel extracts 9 4.78 4.98 4.87 4.76 4.71 ± 4.66 ± 4.60 ± 4.37 ± 4.14 ± 4.12 ±
Liquid ± ± ± ± 0.88 0.98 0.93 0.93 0.90 *0.69 *
1.05 1.07 0.83 0.79
The radix paeoniae rubrathe extracts 11 5.77 5.70 5.66 5.75 5.91 ± 5.81 ± 5.74 ± 5.44 ± 5.05 ± 4.73 ±
Liquid ± ± ± ± 2.42 2.50 2.58 2.28 2.24 *2.25 *
2.35 2.07 2.20 2.27
Peach kernel+red 9 5.41 5.67 5.39 5.34 5.37 ± 5.46 ± 5.40 ± 5.23 ± 5.23 ± 4.77 ±
Chinese herbaceous peony ± ± ± ± 3.13 3.20 3.08 2.94 3.91 2.41
Extracting solution 3.31 3.20 2.98 3.05
Annotate: *With comparison P<0.05 before the administration *With comparison P<0.01 before the administration
(3). the treatment acute pancreatitis
1. to the pancreatitic provide protection of the impatient property of rabbit experiment
Using heavy acute pancreatitis (SAP) model of rabbit proves, press down enzyme injection liquid (YHI) and amygdaloside and merge intravenous injection (1g/kg, be dissolved in the 10mL physiological saline and give), the trend (control group 33.3% that increases rabbit survival time and five days survival rates is arranged; Treatment group 83.3%).Medicine makes animal serum amylase obviously descend (table 6).Pancreas organizes microcirculation obviously to improve (Fig. 7), and makes SAP seriousness index IL-6 be starkly lower than control group (table 7).Pathological examination results shows that also leukocyte infiltration, steatonecrosis, index such as hemorrhage all are light (table 8) than control group.The experiment prompting, YHI and amygdaloside combined utilization have provide protection to rabbit SAP.
Table 6 presses down enzyme injection liquid (YHI) and amygdaloside to the influence of Severe Acute Pancreatitis SAP rabbit anteserum amylase (U/L) (x ± s)
Behind the AP (my god)
Group AP preceding 135
Treatment group 867.67 ± 374.62 (6) 6320.83 ± 2614.12 (6) 4774.0 ± 1859.36 (5) *1596.6 ± 760.50 (5)
Control group 838.17 ± 189.12 (6) 7856.67 ± 3745.03 (5) *7038.0 ± 3687.41 (4) *2095.0 ± 1081.87 (2) *
*With comparison P<0.01 before the SAP; *With comparison P<0.02 before the AP; () number of animals () survival number
Table 7YHI and amygdaloside are to the influence of SAP rabbit anteserum IL-6 level (x ± s)
Behind the AP (my god)
Group AP preceding 135
Treatment group 32.37 ± 9.11 (6) 69.75 ± 19.18 (5) 72.25 ± 10.14 (4) 70.25 ± 10.34 (2)
Control group 34.0 ± 16.40 (6) 59.50 ± 17.59 (6) 50.33 ± 16.57 (5) *46.50 ± 14.94 (5) *
Interleukin-6 unit: U/mL () number of animals *Compare P<0.05 with control group
Table 8 presses down the influence to the pathological change of Severe Acute Pancreatitis SAP rabbit of enzyme injection liquid (YHI) and amygdaloside
The treatment of control group group
1 leaflet structure completely destroy has more complete leaflet
2 acinuses destroy atrophy
3 pancreatic ducts: there is expansion in havoc in the leaflet
Remaining existence between leaflet
4 fatty tissue completely destroys are light-moderate damage
It is few that 5 inflammatory cell abscess form abscess, and leukocyte infiltration is in a small amount arranged in the remaining leaflet
The large stretch of kitchen range of 6 hemorrhagic focuss is little and lack
7 interstitial fibers hamartoplasiaes amount around abscess and necrotic tissue few around abscess and necrotic tissue hyperplasia more
8 pancreas islet do not have existence
Amygdaloside is to intestines blood flow and the strongest medicine of oxygen consumption effect, after experiment confirm also has influence preferably to pancreatic blood flow and oxygen consumption through the orthogonal experiment proof.This experiment is share the acute heavy pancreatitis of treatment rabbit with pressing down enzyme injection liquid and amygdaloside, obtains satisfied result, and this suppresses pancreatin with them, and it is relevant to improve the pancreas blood circulation.(table 8)
2. mechanism analysis
(1) to the influence of leukocyte adhesion
1. amygdaloside is to the microcirculatory influence of living rats
Purpose: observe amygdaloside to the microcirculatory influence of rat mesentery live body.
Method: open abdomen behind the rat anesthesia, find out nearly colon portion mesojejunum and be laid on the special insulation mouse version, carry out microscopic examination.The microcirculation of observed capillary vessel posterior vein is recorded in video-tape gives over to analysis.Amygdaloside tail vein injection (2ml/kg), heavy acute pancreatitis (SAP) are used ductus pancreaticus injection Sodium taurine salt method and are caused.
Result: SAP obviously worsens the every index of microcirculation (white corpuscle rolling number, adhesion number, mean blood flow velocity, He Bi cut rate), gives amygdaloside and can prevent microcirculation disturbance when the AP modeling
Conclusion: white corpuscle when amygdaloside can reduce rat SAP rolls and adheres to number to be increased, and can increase velocity of blood flow and wall is cut rate.(table 9)
Table 9 amygdaloside is to the microcirculatory influence of SAP rat mesentery live body (x ± s)
Behind the AP+ amygdaloside (min)
AP preceding 20 40 60 80 100 120
Adhere to (8) 0.13 ± 0.35 0.50 ± 0.76 0.25 ± 0.46 0.25 ± 0.46 0.25 ± 0.46 0.13 ± 0.15 0.13 ± 0.35
Roll (8) 6.88 ± 5.17 8.00 ± 7.62 9.50 ± 11.77 12.50 ± 13.34 13.13 ± 13.96 14.88 ± 16.27 15.25 ± 16.48
Bore (8) 25.98 ± 3.18 26.23 ± 2.80 25.95 ± 2.66 26.07 ± 2.80 26.08 ± 2.80 26.08 ± 2.80 26.08 ± 2.80
Flow velocity (8) 193.79 ± 15.18 191.24 ± 24.95 197.42 ± 19.33 194.42 ± 23.54 194.02 ± 23.54 196.95 ± 20.90 196.95 ± 20.90
Wall cuts (8) 38.07 ± 4.21 35.87 ± 4.82 37.08 ± 4.75 36.70 ± 5.01 36.70 ± 5.01 37.15 ± 4.70 37.15 ± 4.70
Annotate: only behind the AP 0min and 10min wall cut with AP before relatively, P<0.05, () number of animals
2. amygdaloside is to the influence of acute heavy pancreatitis (SAP) pancreas in rat, lung leukocyte recruitment
Purpose: the leukocyte recruitment to experimental SAP pancreas in rat, lung carries out quantitative examination.
Method: the SAP modeling method injects through jugular vein before the modeling with 1. 99mThe white corpuscle of Tc mark, the radioactivity of pancreas, lung is measured each internal organs myeloperoxidase (MPO) activity behind the record SAP, and it is quantitative to carry out leukocyte recruitment, and the tissues observed pathological change.
The result: the SAP rat in the time of 3 hours pancreas, lung leukocyte recruitment obviously increase, and increase gradually.Amygdaloside can obviously resist the gathering of white corpuscle at pancreas, lung.
Conclusion: amygdaloside adheres to by suppressing the white corpuscle endotheliocyte, reduces the gathering of white corpuscle at tissue, thereby the outer internal organs of pancreas are shielded.(table 10)
Table 10 SAP lung tissue of rats exit dose changes (%ID/G)
Group 3h 6h 12h 24h
Sham operated rats 0.164 ± 0.011 *
SAP group 0.545 ± 0.010 0.532 ± 0.014 0.529 ± 0.010 0.540 ± 0.011
The SAP+ red sage root 0.512 ± 0.014 0.528 ± 0.018 0.537 ± 0.011 0.540 ± 0.024
SAP+ amygdaloside 0.232 ± 0.018 *0.240 ± 0.016 *0.240 ± 0.015 *0.0241 ± 0.020 *
Compare with SAP group, SAP+ red sage root group *P<0.05, *P<0.01,
3. amygdaloside is to the influence of SAP rat CD11b/CD18 expression
Purpose: the influence that the research amygdaloside is expressed SAP rat CD11b/CD18.To inquire into the mechanism that it regulates leukocyte recruitment.
Method: rat is divided into model group, treatment group at random.The treatment group is got lung and pancreatic tissue sample causing SAP after jugular vein input amygdaloside 0.1ml/100g put to death animal in 1,3,6 and 24 hour after the treatment, and the immunohistochemical methods method is measured CD118/CD18 and expressed.
The result: each is organized and is not all measured activity in the pancreatic tissue, and 3 hours lungs are expressed and increased after the model group animal sees SAP, and the treatment treated animal is treated and seen that lung CD11b expressed obvious decline in back 1 hour, further reduces in 3,6,12 hours.
Conclusion: the lung CD11b/CD18 that amygdaloside can make the SAP rat raise expresses obviously and reduces.Inference thinks that it is regulated white corpuscle raising at least in tissue and expresses relevant (table 11,12) with adhesion molecule CD11b/CD18.
Each treated animal lung tissue CD11b of table 11 expresses (positive cell/visual field)
Group 1h 3h 6h 12h 24h
Sham operated rats 3.3 ± 2.5 *
SAP group 14.2 ± 6.8 26.7 ± 8.1 ★ 45.7 ± 11.8 ★ ★ 73.7 ± 13.8 ★ ★ 79.8 ± 14.9
The SAP+ red sage root 12.8 ± 6.4 24.7 ± 8.6 43.5 ± 12.9 70.2 ± 13.7 71.9 ± 16.5
SAP+ amygdaloside 4.5 ± 2.3 ※ 6.9 ± 4.5 ※ ※ 8.3 ± 4.9 ※ ※ 11.5 ± 5.8 ※ ※ 9.0 ± 5.6 ※ ※
*Compare P<0.01 with SAP group, SAP+ red sage root group;
★ compares P<0.05 with previous time period; ★ ★ compares P<0.01 with previous time period;
※ compares P<0.05 with SAP group, SAP+ red sage root group; ※ ※ compares P<0.01 with SAP group, SAP+ red sage root group.
Each treated animal lung tissue CD18 of table 12 expresses (positive cell/visual field)
Group 1h 3h 6h 12h 24h
Sham operated rats 4.8 ± 2.8 *
SAP group 17.1 ± 7.3 30.8 ± 8.6 ★ 47.1 ± 14.7 ★ ★ 75.7 ± 16.1 ★ ★ 82.2 ± 19.4
The SAP+ red sage root 16.5 ± 5.5 25.8 ± 7.3 47.4 ± 12.6 71.8 ± 13.7 69.5 ± 20.8
SAP+ amygdaloside 4.7 ± 3.0 ※ ※ 7.0 ± 3.9 ※ ※ 8.2 ± 5.5 ※ ※ 11.9 ± 5.2 ※ ※ 9.3 ± 5.2 ※ ※
The same
4. amygdaloside is to the influence of induced lung microvascular endothelial and leukocyte adhesion rate
Purpose: the vitro culture induced lung microvascular endothelial that the observation amygdaloside pair cell factor is brought out and the influence of leukocyte adhesion.
After the result shows PMEC (Pulmonary Microvascular Endothelial Cells) and contains the tumour factor and IL-1 β substratum and hatch jointly, the remarkable mutual adhesive attraction of leukocyte increasing and endotheliocyte.Add amygdaloside or amygdaloside pastille serum in substratum after, adhesion rate obviously descends.
Conclusion: the excessive adhesion that suppresses the white corpuscle endotheliocyte is one of important mechanism of action of amygdaloside.(table 13)
Table 13. induced lung microvascular endothelial and leukocyte adhesion rate
Group n adhesion rate (%)
Normal control group 6 12.72 ± 1.91
TNF-α organizes 6 32.53 ± 3.22 *
TNF-α+amygdaloside (1) group 6 16.27 ± 1.80 *△ △
TNF-α+amygdaloside (2) group 6 17.23 ± 2.48 *△ △
TNF-α+red sage root group 6 24.81 ± 2.02 *△ △ ▲ ▲
IL-1 organizes 6 31.89 ± 4.35 *
IL-1+ amygdaloside (1) group 6 17.27 ± 2.05 *△ △
IL-1+ amygdaloside (2) group 6 18.22 ± 2.66 *△ △
IL-1+ red sage root group 6 24.4 ± 2.63
*Compare P<0.05 with the normal control group
*Compare P<0.01 with the normal control group
△ △ compares P<0.01 with the corresponding model group
▲ ▲ compare P<0.01 with the amygdaloside group
(2) to the influence of serum levels of nitric oxide
Purpose: NO is the important vessel active factor, but its excessive rising is also unfavorable to blood fortune.This is tested in acute pancreatitis in rats and has observed the influence of amygdaloside to serum levels of nitric oxide (NO) concentration.
Method: the method for using retrograde injection Sodium taurine salt in the bile duct causes rat acute pancreatitis, collects blood specimen and measures kit measurement treatment front and back Serum concentration of NO with NO.
The result: amygdaloside can make it obvious reduction.
Conclusion: the excessive rising of rat blood serum NO has the reduction effect during amygdaloside acute pancreatitis.(table 14)
Table 14 amygdaloside is to the influence (x ± s, μ mol/L) of acute pancreatitis in rats Serum concentration of NO
After treating before the n treatment
Control group 6 1.28 ± 0.55 3.22 ± 0.79 *
Red sage root group 4 1.30 ± 0.67 3.09 ± 1.28 *
Radix paeoniae rubrathe group 4 1.00 ± 0.30 1.80 ± 1.40
Amygdaloside group 6 1.18 ± 0.81 0.41 ± 0.29 *
Amygdaloside complex group 6 2.68 ± 0.55 1.16 ± 0.33 *
Annotate: with comparison before the pancreatitis, *P<0.05, *P<0.01
(4) promote wound healing
Ischemic is the important disadvantageous effect factor in the wound healing process, and this experimental applications rabbit ear ischemic skin incision model is studied the effect of wound healing amygdaloside.
Model and method: 12 of rabbit, with side rabbit ear depilation, make the portion's ischemia model of picking up the ears after the anesthesia by the WUShi method.Make a 5cm, vertical, the surgery breach that is deep to cartilage again in this ear side, use the 5# silk suture.Postoperative was measured the skin microcirculation (laser doppler flowmetry method) and the subcutis oxygen partial pressure (tissue oxygen meter method) of next-door neighbour's notching edge in 3,5,7,10,14 and 28 days respectively, got otch skin in the 28th day, carefully cut fat, use three sections wide skin grafts of 8mm and measure tissue segments big powers degree with simplified method.
Result: experimental results show that amygdaloside can improve the subcutis oxygen partial pressure, increase the skin histology microcirculation blood flow, wound healing is accelerated, improve the disconnected big powers of otch degree.
1. generalized case, ischemic rabbit ear control group to 12 day are recovered the skin normal color not yet, and the amygdaloside group is changeed blush in the 10th day skin by purple.
2. subcutis oxygen partial pressure (PO 2) cause ischemic after control group obviously reduce, recovery is arranged in the time of 10 days slightly.14-28
Before it still was lower than operation, treatment was organized in the 7th day and is begun to recover, and recovers normal substantially during to 10 days.(table 15)
3. microcirculation inspection: see that all skin microcirculation obviously reduces after causing ischemia model for two groups, control group recovered to postoperative in 10 days yet, and the treatment group was then obviously recovered in postoperative in 10 days, recovered normal substantially during to 14 days.(table 16)
4. otch breaking tenacity: treatment group otch breaking tenacity is apparently higher than control group in the time of the 28th day.(table 17)
Conclusion: amygdaloside is of value to the healing of ischemic skin incision.
Table 15 skin histology oxygen partial pressure (PO 2) change (x ± s)
Behind the ischemic (my god)
Group ischemic preceding 357 10 14 28
Control group 51.6 ± 2.4 25.0 ± 2.8 *24.7 ± 2.7 *26.0 ± 3.1 *27.2 ± 2.3 *34.5 ± 5.1 *35.5 ± 5.1 *
(mmHg)
Treatment group 52.0 ± 2.1 25.2 ± 2.8 *24.0 ± 2.9 *43.0 ± 4.2 *40.5 ± 3.6 49.0 ± 3.0 49.3 ± 2.8 *
(mmHg)
*With preceding relatively P<0.05 of treatment
The variation of table 16 rabbit ear skin microcirculation blood flow (x ± s)
Before the group ischemic Behind the ischemic (my god)
3 5 7 10 14 28
Control group 22.5 ± 1.9 12.5 ± 1.9 *13.6 ± 2.8 *15.0 ± 2.6 *15.2 ± 2.4 *14.8 ± 2.9 *16.6 ± 2.2 *
(mmHg)
Treatment group 22.6 ± 1.0 13.5 ± 1.9 *15.3 ± 2.9 *19.8 ± 1.2 *21.3 ± 1.4 21.0 ± 1.6 21.6 ± 1.2
(mmHg)
*With preceding relatively P<0.05 of treatment
Table 17 skin incision breaking tenacity (x ± s)
Control group (gram) treatment group (gram)
10.66±2.50 16.0±2.76 *
*Compare P<0.05 with control group
The amygdaloside of the present invention preparation is through combination of Chinese tradiational and Western medicine acute abdomen institute pathologic, physiologic research department, Tianjin, the toxicity test done of Tianjin combination of Chinese tradiational and Western medicine acute abdomen institute drug research chamber is reported as follows.
One. the amygdaloside acute toxicity test
1. experimental technique:
The preliminary experiment result shows that the peak concentration amygdaloside does not generally have lethality, so adopt peak concentration, maximum volume dose regimen.And proof amygdaloside maxima solubility is 19%.
Get 20 of healthy Kunming mouses, male and female half and half.Experiment day every mouse was observed seven days continuously through tail vein injection 19% amygdaloside 0.5ml.
Medicine is faced with preceding and is prepared with physiological saline by the drug research chamber preparation of this institute.
2. experimental result:
At once do not see after the administration that animal has acute poisoning symptoms such as expiratory dyspnea, tic, gatism, animal wool is smooth, activity freely, exploratory reflex is arranged.Animal appetite is good in seven days observation processes, can take food naturally, intake, and does not see vomiting, diarrhoea phenomenon, and last the weight of animals increased (average 27.05 ± 1. grams before the administration, average 30.9 ± 1.91 grams after the administration) in seven days.No any animal dead in seven days whole observation processes.
3. conclusion: mouse is 19% to the maximum tolerated dose of amygdaloside, 0.5ml.By the mouse mean body weight is 25 grams/only calculating, and always giving dose is 3.8g/kg, once gives (inject in about 5 seconds and finish).Clinical recommendation consumption is 3%, 2ml/kg/h, promptly 2.7 * 10 -3Ml/kg/5sec, just 8.3 * 10 -5G/kg.Therefore 45783.13 times of the quite clinical recommendation consumption of this experiment gained mouse maximum tolerated dose.(above is rough calculation, will not import the cumulative effect of medicine continuously and estimate interior.
Two. the amygdaloside long term toxicity test
(1) animal and material
1. animal: 80 of healthy wistar rats (cleaning level), available from four of Military Medical Science Institutes, about body weight 250 grams.Test is divided into 4 groups, and 20 every group, male and female half and half.Observe a week record appetite and body weight before the test.
2. trial drug: amygdaloside, white powder, by the drug research chamber preparation of this institute, before the test with the physiological saline wiring solution-forming.
(2) test method
1. test grouping: test is divided into four groups, promptly blank 9 (not adding processing), control group (physiological saline group), high dose group (9% amygdaloside), the low dose group (3% amygdaloside) organized.
2. medication: three treated animal every days of back are respectively through intraperitoneal injection of saline, each 1ml of amygdaloside, continuous two weeks.
3. observation index: observe every day diet, two just, hair and active situation.The next day measure body weight.Test end is the rat sacrificed by decapitation, get blood specimen and measure liver, renal function and blood picture and change, and core, liver, spleen, lung, kidney, testis and ovary tissue sample carry out the pathological tissue inspection, the calculating organ coefficient of weighing.
(3) test-results
1. blood picture: 14 days rat red blood cell count(RBC)s (RBC), white blood cell count(WBC) (WBC), oxyphorase (HGB), cell specific volume (HCT), MCV (MCV), mean corpuscular hemoglobin (MCH) and mean corpuscular hemoglobin concentration (MCHC)s (MCHC) more all do not have significant difference with blank group after the administration, only platelet count (PLT) changes, low dose group (827 ± 89.8 vs 670 ± 174 * 10 that obviously raise 9/ μ l, p=0.01), but the physiological saline group is also than blank group rising (805.4 ± 88.92 vs 670 ± 174 * 10 9/ μ l p=0.038), therefore may be accidental variation.(table 18,19)
2. liver function: intraperitoneal is injected two weeks of amygdaloside continuously to rats'liver function free of toxic effects, and the test end is respectively organized visible glutamate pyruvate transaminase and reduced, and comprises that physiological saline group (p<0.05), total protein and albumin raise.The total bilirubin no change.(table 20)
3. renal function: intraperitoneal is injected two weeks of amygdaloside does not continuously have any toxic action to the kidney of rats function, and blood urea nitrogen and creatinine and blank treated animal relatively do not have significant difference.(table 21)
4. body weight: two week of amygdaloside abdominal injection the back rat body weights obviously increase, physiological saline treated animal body weight also increases, only control group is not obvious, but increase trend is also arranged.(table 22)
5. organ weights and organ coefficient
Each organ coefficient between each group does not have significant difference.(table 23)
Table 21. amygdaloside long term injections is to the influence of kidney of rats function
Urea (mmo/l) Cr (umol/l)
The blank NS high dosage of blank NS high dosage low dosage low dosage
Average 7.5475 6.563 5.9555 6.1409 33.738 28.99 25.911 29.34
Standard deviation 2.865 0.7498 0.6195 1.0482 8.8343 3.743 4.0444 3.4408
P value 0.3049 0.086 0.1399 0.13 0.0138 0.1373
Annotate: Urea urea; The Cr creatinine
Table 22. amygdaloside long term injections is to the influence (gram) of rat body weight
Group NS High dosage Low dosage Contrast
After testing before the preceding test of the test back test back test before test the test back before the test
250.0 271.6 247.45 262.09 245.4 260.17 258.3 263.33
29.51 41.59 33.60 38.19 42.9 39.34 43.98 40.06
P value 0.001 0.0002 0.00036 0.8
P value: compare before and after the test
Table 18 amygdaloside long term injections is to the influence of rat blood picture
RBC (10 9/L) WBC (10 12/L) HGB (g/L) PLT (10 9/uL)
The blank NS high dosage of blank NS high dosage low dosage blank NS high dosage low dosage blank NS high dosage low dosage low dosage
Average 8.185 8.371 8.3055 8.5073 10.242 10.28 10.645 10.627 153.42 155.6 156.9 158.5 670 805.4 719.6 827
Standard deviation 0.5948 0.3175 0.2232 0.4834 1.8278 2.143 1.647 3.6598 10.638 3.502 4.989 8.347 174 88.92 103.6 89.8
P value 0.3857 0.5384 0.171 0.964 0.585 0.7491 0.543 0.543 0.223 0.038 0.423 0.01
Annotate: the RBC red blood cell count(RBC); The WBC white blood cell count(WBC); The HGB oxyphorase; The PLT thrombocyte
Table 19 amygdaloside long term injections is to the influence of rat blood picture
HCT (%) MCV (fL) MCH (pg) MCHC (g/L)
The blank NS high dosage of blank NS high dosage low dosage blank NS high dosage low dosage blank NS high dosage low dosage low dosage
Average 46.708 48.37 47.973 48.445 57.142 57.77 57.782 56.955 18.75 18.61 18.88 18.65 329 322.1 327.1 327
Standard deviation 2.8353 1.1889 1.3799 2.8115 2.1377 1.217 1.4063 1.4638 0.6245 0.576 0.615 0.216 15.1 8.569 6.625 6.91
P value 0.0998 0.1949 0.1554 0.42 0.4105 0.8107 0.594 0.612 0.604 0.243 0.766 0.78
Annotate: HCT blood cell specific volume: MCV MCV; MCH mean corpuscular hemoglobin: MCHC mean corpuscular hemoglobin concentration (MCHC)
Table 20 amygdaloside long term injections is to the influence of rats'liver function
ALT (U/L) TP (g/l) ALB (g/l) T-BIL umol/l)
The blank NS high dosage of blank NS high dosage low dosage blank NS high dosage low dosage blank NS high dosage low dosage low dosage
Average 168.5 114.1 98.818 100 67.983 75.65 75.355 76.273 38.825 41.26 41.74 41.1 0.95 0.648 0.564 0.84
Standard deviation 72.393 24.786 24.624 23.277 4.9101 5.609 5.6828 5.4575 2.5385 2.851 2.953 2.717 0.76 0.291 0.479 0.44
P value 0.0351 0.0064 0.0069 0.003 0.0031 0.001 0.047 0.019 0.05 0.248 0.162 0.67
Annotate: the ALT alanine aminotransferase; The TP total protein: ALB albumin: T-BIL is total-bilirubin
Table 23 amygdaloside long term injections is to the influence of rat heart coefficient (x ± s)
Internal organs control group physiological saline high dosage low dosage
Heart 0.0034 ± 0.00043 0.0034 ± 0.00026 0.0033 ± 0.00024 0.0035 ± 0.00031
Liver 0.035 ± 0.0023 0.034 ± 0.0023 0.029 ± 0.01 0.026 ± 0.01
Spleen 0.0024 ± 0.0002 0.0024 ± 0.0003 0.0024 ± 0.0003 0.0061 ± 0.0089
Lungs 0.0095 ± 0.0023 0.0076 ± 0.0018 0.0053 ± 0.0008 0.0062 ± 0.0013
Kidney 0.0065 ± 0.0005 0.0066 ± 0.0003 0.0067 ± 0.0004 0.0066 ± 0.0006
Testis 0.0092 ± 0.0005 0.0096 ± 0.0006 0.0080 ± 0.0039 0.0091 ± 0.0019
Ovary 0.0006 ± 0.0001 0.0004 ± 0.0003 0.0006 ± 0.0009 0.0006 ± 0.0001
6. pathological tissue check result:
Blank group, physiological saline group and amygdaloside is low and the heart of high dose group animal, liver,spleen,kidney and sexual gland (testis or ovary) all do not have any pathological change.Intra-alveolar hemorrhage (may be the result that disconnected neck sucks when putting to death), slight interstitial cell hyperplasia, alveolar septum broadening, organizing consolidation etc. all to exist to some extent in each group, therefore think the problem of animal itself, is not the chronic toxicity effect of amygdaloside.
Four. conclusion
The continuous abdominal injection of amygdaloside, 1ml/d. (3% or 9%) in totally 2 weeks, does not produce chronic toxicity effect * to rat.
* to recommend clinical using dosage be that this uses the dosage of chronic toxicity test once to inject as 1ml to 2ml/kg/h (still use dosage for experiment at present, carry out the clinical trial treatment and the time also must further weigh), so dosage is possible bigger than normal to amygdaloside.Lung pathology checks that the finding slight abnormality is perhaps relevant therewith.The conversion method of a transfusion dosage and an implantation dosage is still very not clear and definite.The applied dosage of chronic toxicity test is because may be bigger than normal, gained test-results (free of toxic effects) thereby more reliable.

Claims (3)

1. the preparation method of an amygdaloside is characterized in that squeezing Semen Armeniacae Amarum 1Kg after the deoiling 4000-5000ml that adds diethyl ether and divides 2 reflux degreasings, filters standby; Add 95% alcohol reflux three times after the dregs of a decoction are waved most ether, each 3000-5000ml, filtered while hot, merging filtrate, decompression recycling ethanol is doubly measured volume to the 1-2 of crude drug amount, is placed to room temperature, adds the ether of 1/2 amount again, the container bottom chromatography goes out to be stained with the oily precipitation of wall, produce supernatant liquor, place, separate out crystallization, suction filtration gets the amygdaloside crude product; The amygdaloside crude product is added 20-40 times of dissolve with ethanol, filtration, places, separates out the crystallization of amygdaloside white plates, and filtration under diminished pressure with the crystallization of 100-200mL washing with alcohol, promptly gets the pure product of amygdaloside, and yield is more than 4%, and purity reaches more than 90%.
2. preparation method according to claim 1, but it is characterized in that in case of necessity amygdaloside crude product repeated treatments 1-2 time, but each amount of alcohol must reduce by half.
3. application in preparation promotion heart brain pancreas and the sanguimotor amygdaloside preparation of wound is characterized in that:
A. amygdaloside is to the effect of cerebral blood circulation:
I. treat and prevent because of the cerebral ischemia of blood viscosity due to raising, the circulation blood flow at the input all can increasing of amygdaloside vein rat's pial and brain essence two positions, the vasodilation reaction that two positions are described has synchronism, effect manifests later, and after the intravenous injection 30 minutes, effect is increase progressively, in the time of 60 minutes and before the administration, notable difference is arranged, for this reason, before causing the blood flow reduction, give amygdaloside, the pathogenic effects of energy antagonism dextran;
II. to the influence of brain microcirculation disorder, be used for prevention and treatment as injection suprarenin, Pituitrin and mesencephalic arteries ligation;
B. the amygdaloside treatment is in heart failure:
Amygdaloside can be kept contract power and contraction frequency of isolated rat heart coronary flow, the heart in a long time and remain unchanged, and uses the amygdaloside perfusion and can make isolated heart keep the heart normal function in the long period, and cardiac failure is had provide protection;
C. amygdaloside is treated acute pancreatitis:
Amygdaloside has influence preferably to pancreatic blood flow and oxygen consumption, and white corpuscle rolls and the increase of adhesion number in the time of reducing heavy acute pancreatitis, can increase velocity of blood flow and wall is cut rate; By suppressing white corpuscle endotheliocyte excessive adhesion, reduce white corpuscle in in-house gathering, thereby the outer internal organs of pancreas are shielded; The excessive rising of rat blood serum NO has the reduction effect during to acute pancreatitis;
D. amygdaloside promotes wound healing:
Amygdaloside improves the subcutis oxygen partial pressure, increases the skin histology microcirculation blood flow, and the quickening that cicatrizes a wound improves the otch breaking tenacity, is of value to the healing of ischemic skin incision.
CNB2003101193893A 2003-12-24 2003-12-24 Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound Expired - Fee Related CN1318439C (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
CNB2003101193893A CN1318439C (en) 2003-12-24 2003-12-24 Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
CNB2003101193893A CN1318439C (en) 2003-12-24 2003-12-24 Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound

Related Child Applications (1)

Application Number Title Priority Date Filing Date
CNB2006101702971A Division CN100486584C (en) 2003-12-24 2003-12-24 Application of amygdalin in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound

Publications (2)

Publication Number Publication Date
CN1631895A true CN1631895A (en) 2005-06-29
CN1318439C CN1318439C (en) 2007-05-30

Family

ID=34843896

Family Applications (1)

Application Number Title Priority Date Filing Date
CNB2003101193893A Expired - Fee Related CN1318439C (en) 2003-12-24 2003-12-24 Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound

Country Status (1)

Country Link
CN (1) CN1318439C (en)

Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN102048856A (en) * 2010-12-03 2011-05-11 南方医科大学 Medicine for relieving cough and asthma and preparation method thereof
CN102234298A (en) * 2010-04-23 2011-11-09 华东理工大学 Method for extracting and purifying amygdalin from peach seeds
WO2019047848A1 (en) * 2017-09-05 2019-03-14 石家庄以岭药业股份有限公司 Method for separating eighteen components in traditional chinese medicine composition
WO2020001166A1 (en) * 2018-06-27 2020-01-02 上海和黄药业有限公司 Glycoside compound and preparation method therefor, composition, application, and intermediate
CN111012789A (en) * 2020-01-10 2020-04-17 上海中医药大学附属曙光医院 Application of amygdalin in preparing medicine for treating fatty liver disease

Family Cites Families (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN1084518A (en) * 1993-05-07 1994-03-30 张伯熙 The preparation technology of total gypenosides
CN1156485C (en) * 2002-02-01 2004-07-07 河北药都制药集团有限责任公司 Process for extracting, separating and refining amygdalin

Cited By (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN102234298A (en) * 2010-04-23 2011-11-09 华东理工大学 Method for extracting and purifying amygdalin from peach seeds
CN102048856A (en) * 2010-12-03 2011-05-11 南方医科大学 Medicine for relieving cough and asthma and preparation method thereof
WO2019047848A1 (en) * 2017-09-05 2019-03-14 石家庄以岭药业股份有限公司 Method for separating eighteen components in traditional chinese medicine composition
US11458417B2 (en) 2017-09-05 2022-10-04 Shijiazhuang Yiling Pharmaceutical Co., Ltd. Method for separating eighteen components in traditional Chinese medicine composition
WO2020001166A1 (en) * 2018-06-27 2020-01-02 上海和黄药业有限公司 Glycoside compound and preparation method therefor, composition, application, and intermediate
US11325937B2 (en) 2018-06-27 2022-05-10 Shanghai Hutchison Pharmaceuticals Limited Glycoside compound and preparation method therefor, composition, application, and intermediate
CN111012789A (en) * 2020-01-10 2020-04-17 上海中医药大学附属曙光医院 Application of amygdalin in preparing medicine for treating fatty liver disease

Also Published As

Publication number Publication date
CN1318439C (en) 2007-05-30

Similar Documents

Publication Publication Date Title
CN1245198C (en) Chinese medicine composition for treating diabetes and its preparing method
CN101049324A (en) Composition of medication prepared from ginkgo leaves and puerarin
CN1711099A (en) Extract with anti-tumor and anti-poisonous activity
CN1631895A (en) Preparation method of amygdalin and its application in preparation of amygdalin preparation for promoting the blood circulation of heart, brain, pancreas and wound
CN1586533A (en) Composition for strengthening body resistance and restoring and function, strengthening spleen and kidney, relieving metal stress and promoting blood circulation to remove blood stasis
CN100341492C (en) Ginseng-astragalus blood-sugar lowering soft capsule, and its preparing and detecting method
CN100335102C (en) Chinese medicina composition for treating algomenorrhea and its preparation method
CN1241577C (en) Medicine use of cyclodextrin derivs. and medicine composition thereof
CN1931233A (en) Medicine composition of red sage and epimedium for treating cardiac and cerebral vascular diseases
CN101049293A (en) Medication composition of acetyl cysteine or its pharmaceutical salt and asarin
CN1557352A (en) Novel usage of chicory aqueous extract
CN101040886A (en) Medicine compound of erigeron breviscapus and tanshinone IIA sodium sulfoacid
CN1559549A (en) Medicine for treating diabetes and its preparation method
CN1923228A (en) Pharmaceutical composition comprising notoginseng extract, Danshen extract and ligustrazine
CN1923229A (en) Pharmaceutical composition comprising notoginseng extract, Danshen extract and puerarin
CN1256081C (en) Method for preparing injection of oleum functus brucease
CN1287835C (en) Pharmaceutical composition for treating coronary heart disease and angina pectoris and its preparing process
CN101049355A (en) Composition of medication prepared from safflower and leaves of hawthorn
CN1709238A (en) Power for intravenous injection with liver-protecting action, and its preparation and quality control method
CN100341490C (en) Ginseng and astragalis blood glucose lowering dispersion tablet and its preparing and detecting method
CN1557395A (en) Collateral channels clearing arthralgia dredging prescription for treating rheumatoid arthritis and its preparing process
CN1238038C (en) Medicine for tonifying kidney, strengthening spleen, replenishing esseuce and invigorating marrow and its preparing method
CN1168739C (en) Narcissus seed glycopeptide and its application
CN1813822A (en) Natural medicinal composition for preparing diabete drug
CN1593500A (en) Kidney benefiting, Chong collateral reinforcing and menstruation regulating hemostat

Legal Events

Date Code Title Description
C06 Publication
PB01 Publication
C10 Entry into substantive examination
SE01 Entry into force of request for substantive examination
C14 Grant of patent or utility model
GR01 Patent grant
CF01 Termination of patent right due to non-payment of annual fee

Granted publication date: 20070530

Termination date: 20161224

CF01 Termination of patent right due to non-payment of annual fee