CN105884841B

CN105884841B - A kind of preparation method of phenylpropanoids

Info

Publication number: CN105884841B
Application number: CN201610153958.3A
Authority: CN
Inventors: 刘逆夫; 龚云; 夏博候; 李亚梅; 林丽美; 伍实花
Original assignee: Zhuzhou Qianjin Pharmaceutical Co Ltd
Current assignee: Zhuzhou Qianjin Pharmaceutical Co Ltd
Priority date: 2016-03-17
Filing date: 2016-03-17
Publication date: 2018-09-25
Anticipated expiration: 2036-03-17
Also published as: CN105884841A

Abstract

The present invention relates to pharmaceutical technology fields, disclose a kind of preparation method of phenylpropanoids, more particularly to isolated a kind of phenylpropanoids from the dry root of Flemingia macrophylla, the phenylpropanoids are made through solvent extraction, column chromatography for separation, preparation liquid phase separation purifying, the phenylpropanoids obtained through the method for the present invention are to report for the first time, and purity is high.Experiments have shown that, obtained new phenylpropanoids can inhibit cellular inflammation factor TNF α, 1 β of IL, the expressional function of IL 6, with the inhibiting effect to hydroxyl radical free radical (OH), and then there is anti-inflammatory and antioxidant activity, it is beneficial to the treatment of the various diseases associated with inflammation such as cervicitis, endometritis, pelvic infecton, mastitis, sphagitis and/or arthritis, which can be developed into new drug.Heretofore described structural formula of compound is phenylpropanoids and its pharmaceutically acceptable salt shown in formula (I).

Description

A kind of preparation method of phenylpropanoids

Technical field

The present invention relates to pharmaceutical technology fields, more particularly, to a kind of preparation method of new phenylpropanoids.

Background technology

It is various, active notable that isolated constituent structure is extracted from natural drug, it is isolated and purified, structure Modification, transformation and it is fully synthetic, be always a main thought of new drug development.

TNF-α：Be it is a kind of can direct killing tumour cell and to cell factor of the normal cell without overt toxicity, be so far One of strongest bioactie agent of direct killing function of tumor found until the present, however its toxic side effect is also very tight Weight.

IL-1β：In local low concentration, collaboration stimulation APC and T cell activation, promote B cell proliferation and secretory antibody, into Row immunological regulation.There is endocrine effect when a large amount of generations：Induced liver acute phase protein synthesizes, and causes fever and cachexia.

IL-6：Mankind's IL-6 genes are located on No. 7 chromosome；IL-6 molecular weight is between 21~30KD.Mainly by list Core macrophage, Th2 cells, vascular endothelial cell, fibroblast generate.Activating B cell can be stimulated to be proliferated, secretion is anti- Body；Stimulate T cell proliferation and CTL activation；Cell cultured supernatant synthesized acute phase albumen participates in inflammatory reaction；Promote haemocyte hair It educates.

IL-6 can be synthesized by various kinds of cell, including the T cell of activation and B cell, monocytes/macrophages, endothelial cell, Epithelial cell and fibroblast etc..There are many target cell of IL-6 effects, including macrophage, liver cell, static T thin Born of the same parents, the B cell of activation and thick liquid cell etc.；Its biological effect is also sufficiently complex.

OH is most active reactive oxygen species in biosystem, can lead to DNA in cell and organism, protein and fat Matter oxidative damage.

Therefore, seek a kind of new preparation method, isolated new compound is extracted from natural plants, can inhibit thin Born of the same parents' inflammatory factor TNF-α, the expressional function of IL-1 β, IL-6 inhibit the activity of hydroxyl radical free radical (- OH), are applied to inflammatory disease The treatment of disease, is necessary.

Waras medicinal material is that pulse family (Leguminosae) Moghania (Flemingl.Roxb. or Moghania) plant is big The dry root of leaf waras (Moghaniamacrophylla (Willd.) O.Kuntze), the southeast is distributed mainly in China Area.The plant is in Chinese Plants will (1995,41:313), TaiWan, China flora (1977,3:258), Hainan flora (1965,2:311)、《Chinese Higher plant illustrated handbook》(1972,2:510), Chinese main plant figure is said (1955, pp707) and wide State flora is included in (1956, pp361).Waras medicinal material is the genunie medicinal materials of Guangxi province, and history is loaded in《Plant name is real Figure is examined》, there is extensive civil medication basis.Its nature and flavor is sweet, micro-puckery, puts down, and has removing damp-heat and other effects, is mainly used for treating The gynecological diseases such as more than treating rheumatic ostealgia, traumatic injury, chronic nephritis, dysmenorrhoea and leukorrhea.The medicinal material has been recorded at present into version in 2005 《Chinese Pharmacopoeia》Annex.

The ingredient that Flemingia macrophylla has been reported mainly has flavonoids, steroid, terpene, Anthraquinones, volatile oil ingredient, has There is certain pharmacological activity.

Flemingia macrophylla pharmacological activity is various, reports the more neuroprotection that has, anti-inflammatory, antioxidation, to disease Anthelmintic action, parahormone effect, cytotoxicity, antibacterial action and immunological enhancement, the antifatigue effect of pathogenic microorganism.

Waras is now widely used for the Chinese patent drug production of the types such as gynaecology, arthralgia pain due to rheumatism, such as FUKE QIANJIN PIAN, gynaecology A thousand pieces of gold capsule, infusion of cherokee rose and spatholobus stem, JINJI JIAONANG etc., such Chinese patent drug is mainly used for gynaecological disease, and (dysmenorrhoea, cold uterus be infertile, uterus Sagging, pelvic infecton, mastitis, leukorrhea be more, the postpartum deficiency of blood, arthralgia, postpartum waist and knee, hypogalactia and newborn sore etc.), weak anaemia (woman anemia, deficient qi and blood and after being ill deficiency of vital energy etc.).In recent years, what clinical report was more is that FUKE QIANJIN PIAN is scorching in treatment gynaecology Effect in terms of disease.

Currently, in the document of waras, report that the document of phenylpropanoids is few, finds a kind of new preparation side Method isolates effective Phenylpropanoid Glycosides class noval chemical compound from natural plants, is isolated and purified to it, structural modification and synthesis, Developing new drug is applied to the treatment of diseases associated with inflammation, significant.

Invention content

The purpose of the present invention is to provide a kind of Phenylpropanoid Glycosides classes isolated in a kind of dry root from Flemingia macrophylla The preparation method of compound, cellular inflammation factor TNF-α can be inhibited by extracting isolated compound by the preparation method, The expressional function of IL-1 β, IL-6 have the inhibiting effect to (- the OH) of hydroxyl radical free radical, and then with anti-inflammatory and anti-oxidant work Property, it is beneficial to the treatment of various diseases associated with inflammation, which can be developed into new drug.

Specifically, the preparation method of phenylpropanoids of the present invention includes the following steps：

S1. it is raw material to take the root of Flemingia macrophylla, and dry, stripping and slicing extracts through ethanol solution, extracting solution is merged, dense It is reduced to no alcohol taste, it is spare to obtain medicinal extract；

S2. gained medicinal extract in step S1 is dissolved in water, it is eluted using large pore resin absorption column, eluant, eluent is Ethanol-water system collects the eluent of preceding 3 column volumes, is named as MM-1, spare；

S3. the flow point MM-1 being collected into step S2 is eluted with reversed material ODS column chromatographies, eluant, eluent is first Alcohol-water system elutes 18 column volumes, and the eluent of a flow point is collected by every 3 column volumes, collects 6 flow points in order, It is respectively designated as MM-11, MM-12, MM-13, MM-14, MM-15, MM-16, it is spare；

S4. it is methanol-water-acetic acid system with liquid phase separation, mobile phase is prepared by the flow point MM-13 being collected into step S3 System collects eluent by peak sequence, collects 4 flow points altogether, be respectively designated as MM-131, MM-132, MM-133, MM-134, It is spare；

S5. the flow point MM-133 being collected into step S4 is purified with liquid phase is prepared, mobile phase is methanol-water-acetic acid system System collects eluent, the phenylpropanoids is obtained after recrystallization.The purity of the phenylpropanoids is 99.66%.Shown in the structural formula of the phenylpropanoids such as formula (1)：

Preferably, in step S1, a concentration of 50-80 volumes % of ethanol solution, further preferably ethanol solution concentration For 60 volume %.

Preferably, in step S1, the extraction time of ethanol solution is 2~4 times, is extracted 1~3 hour every time, further excellent The extraction time for being selected as ethanol solution is 3 times, every time 2 hours.

Preferably, in step S2, macroporous absorbent resin uses D101 macroporous absorbent resins.

Preferably, in step S2, the volume ratio of ethyl alcohol and water is 0:100~15:85.

Preferably, in step S3, the volume ratio of methanol and water is 20:80~30:70, further preferably 25:75.

Preferably, in step S4, the volume ratio of methanol-water-acetic acid is 10:90:0.01~35:65:0.01, further

Preferably 15:85:0.01.

Preferably, in step S4, preparative liquid chromatography column is YMC, and 20mm*250mm, flow rate of mobile phase is 5~10ml/ Min, further preferably flow velocity 5ml/min.

Preferably, in step S5, the volume ratio of methanol-water-acetic acid is 15:85:0.01.

Preferably, in step S5, preparative liquid chromatography column is YMC, 20mm*250mm, flow rate of mobile phase 5mL/min.

The present invention provides the phenylpropanoids that the preparation method is prepared.

And the phenylpropanoids being prepared through chemical synthesis process as raw material using the phenylpropanoids Salt.Shown in the structure of the salt such as formula (II) or formula (III)：

Wherein, R is inorganic acid, R₁Or R₂For in sulfonate radical, alkali metal ion or ammonium root any one or it is two kinds arbitrary.

Preferably, the inorganic acid is hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid or breast Acid；The sulfonate radical is the sulfonate radical with aryl；The alkali metal ion be potassium ion, sodium ion, calcium ion, magnesium ion or Lithium ion.

Preferably, the sulfonate radical with aryl is benzene sulfonic acid root or p-methyl benzenesulfonic acid root.

Preferably, the pharmaceutically acceptable salt is ammonium salt.

Beneficial effects of the present invention：

The present invention provides a kind of preparation method for new phenylpropanoids and its pharmaceutically acceptable salt, for the first time A kind of isolated new phenylpropanoids, compound obtained can inhibit cell from the dry root of Flemingia macrophylla Inflammatory factor TNF-α, the expressional function of IL-1 β, IL-6 have the inhibiting effect to (- the OH) of hydroxyl radical free radical, and then have Anti-inflammatory and antioxidant activity may be used as such as cervicitis, endometritis, pelvic infecton, mastitis, sphagitis and/or arthritis The medicine of equal diseases associated with inflammation.

The purpose of the present invention is from traditional prescriptions of traditional Chinese medicine, pass through the prescription from FUKE QIANJIN PIAN and ' Qianjin ' capsule to treat ganopathy In, by solvent extraction, column chromatography for separation, liquid phase separation, a kind of obtained new phenylpropanoids of purifying are prepared, and pass through reality Verification is real, diseases associated with inflammation is can be applied to, such as cervicitis, endometritis, pelvic infecton, mastitis, sphagitis and/or pass Save the treatment of the diseases such as inflammation.

Specifically, inventor is by the way that from the prescription of FUKE QIANJIN PIAN, ' Qianjin ' capsule to treat ganopathy, science chooses Flemingia macrophylla Dry root, by solvent extraction, column chromatography for separation, prepare liquid phase separation, purifying, obtain Phenylpropanoid Glycosides class chemical combination of the present invention Then object carries out test cell line to the compound, measure it to cellular inflammation factor TNF-α, the inhibition level of IL-1 β, IL-6, Experiment shows that the compound stimulates 264.7 cells of caused Raw scorching LPS in concentration (10.50-13.50 μ g/mL) range Inflammation factor TNF-α content has apparent inhibiting effect (p ＜ 0.05), and shows apparent dose-dependence；In concentration There is apparent inhibiting effect (p ＜ 0.05) to inflammatory factor IL-1 β contents in (4.50-13.50 μ g/mL) range, shows bright Aobvious dose-dependence；There is apparent inhibition to inflammatory factor IL-6 contents in concentration (7.50-13.50 μ g/mL) range It acts on (p ＜ 0.05), shows apparent dose-dependence.

Description of the drawings

Fig. 1 is the hydrogen nuclear magnetic resonance spectrogram of phenylpropanoids of the present invention.

Fig. 2 is the carbon-13 nmr spectra figure of phenylpropanoids of the present invention.

Fig. 3 is influence diagram of the phenylpropanoids of the present invention to cell activity.

Fig. 4 is inhibiting effect figure of the phenylpropanoids of the present invention to NO.

Fig. 5 is inhibiting effect figure of the phenylpropanoids of the present invention to TNF-α.

Fig. 6 is inhibiting effect figure of the phenylpropanoids of the present invention to IL-1 β.

Fig. 7 is inhibiting effect figure of the phenylpropanoids of the present invention to IL-6.

Fig. 8 is inhibiting effect figure of the phenylpropanoids of the present invention to OH.

Specific implementation mode

It is further illustrated the present invention below in conjunction with Figure of description and specific embodiment, but embodiment is not to the present invention It limits in any form.Unless stated otherwise, the present invention uses reagent, method and apparatus routinely try for the art Agent, method and apparatus.Unless stated otherwise, the raw material used in the present embodiment and equipment are the original of the art regular market purchase Material and equipment.

The compound of the present invention is the change shown in phenylpropanoids and formula (II) or formula (III) shown in the formula (I) Close object pharmaceutically acceptable salt.The method provided by the invention extracted as raw material using Flemingia macrophylla may be used in the compound It is prepared, can also be combined according to structural formula provided by the invention and be prepared using the methods of the chemical synthesis of this field.

As the salt of phenylpropanoids of the present invention, as long as pharmaceutically acceptable salt, can be enumerated as The inorganic acid salt formed with inorganic acids such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid；With The sulfonate that sulfonic acid is formed；The alkali metal salt formed with the hydroxide of the alkali metal such as potassium, sodium, calcium, magnesium, lithium is formed with ammonium Ammonium salt etc..

Phenylpropanoids of the present invention can be used as cervicitis, endometritis, pelvic infecton, mastitis, sphagitis and/ Or the medicine of the diseases associated with inflammation such as arthritis.

The compounds of this invention can be used as pharmaceutical composition together with the auxiliary material and/or carrier that pharmaceutically allow, can also Be added pharmaceutically allow auxiliary material and/or carrier in the case of with cherokee rose root, single side needle, Caulis Spatholobi, leatherleaf mahonia, Herba Andrographitis, The combination of one or more of Radix Angelicae Sinensis, Radix Codonopsis Chinese medicine or extract is used as pharmaceutical composition, and the compounds of this invention can be with With together with other pharmaceutically acceptable effective components be used as pharmaceutical composition.

Can be tablet, capsule, powder, granule, pill, solution, suspension, syrup as pharmaceutical composition Agent, injection, ointment, suppository, spray etc..

Further, tablet can be the manufactured sugar-coat in the case of auxiliary material and/or carrier that addition pharmaceutically allows Piece, Film coated tablets, enteric coatings ply or two-ply, multilayer tablet.

The auxiliary material and/or carrier of the present invention can be as follows：

Solid pharmaceutical preparation is made, additive, such as sucrose, lactose, cellulose sugar, maltitol, glucose, shallow lake can be used Powder class, agar, alginates, chitin, chitosan class, pectin class, gum arabic class, gelatin class, collagen class, junket egg In vain, albumin, calcium phosphate, D-sorbite, glycine, glycerine, polyethylene glycol, sodium bicarbonate, talcum etc..

Semisolid preparation is made, of animal or plant nature grease (olive oil, corn oil, castor oil etc.), mineral oil can be used It is fat (vaseline, albolene, solid paraffin etc.), wax class (jojoba oil, Brazil wax, beeswax etc.), partially synthetic or complete Fatty acid glyceride (lauric acid, myristic acid, palmitic acid etc.) of synthesis etc..

Liquid preparation is made, additive, such as sodium chloride, glucose, D-sorbite, glycerine, olive oil, the third two can be used Alcohol, ethyl alcohol etc..In the case of injection especially is made, aseptic aqueous solution, such as physiological saline, isotonic solution, oiliness can be used Liquid, such as sesame oil, soybean oil.Furthermore it is also possible to as needed, suspending agent appropriate, such as sodium carboxymethylcellulose, nonionic be used in combination Surfactant, cosolvent, such as Ergol, benzyl alcohol.

The amount of the active ingredient of these preparations is 0.01~80 weight % of preparation, is suitably 1~50 weight %, dosage Symptom, weight, age according to patient etc. are different and change.

The preparation of 1 phenylpropanoids of embodiment

The present embodiment provides a kind of preparation methods of phenylpropanoids shown in formula (I), include the following steps：

S1. Flemingia macrophylla 50kg is taken, it is dry using root as raw material, it is cut into small pieces.Alcohol reflux through 8 times of amounts 60% Extraction 3 times, 2 hours every time, extracting solution is merged, is concentrated into no alcohol taste, it is spare to obtain medicinal extract；

S2. the medicinal extract after being concentrated in step S1 is dissolved in 10L water, it is washed using D101 large pore resin absorption columns De-, eluant, eluent is water, elutes 3 column volumes, collects eluent, is named as MM-1, spare；

S3. the flow point MM-1 being collected into step S2 is eluted with reverse phase ODS column chromatographies, eluant, eluent is methanol-water System, volume ratio 25:75,18 column volumes are eluted, the eluent of a flow point are collected by every 3 column volumes, in order 6 flow points are collected, are respectively designated as：MM-11, MM-12, MM-13, MM-14, MM-15, MM-16 are spare；

S4. it is with liquid phase separation, preparative liquid chromatography column is prepared by the flow point MM-13 being collected into step S3：YMC, 20mm*250mm, flow velocity：5ml/min, mobile phase are methanol-water-acetic acid system, methanol：Water：The volume ratio of acetic acid is 25:75: 0.01, eluent is collected by peak sequence, 4 flow points is collected altogether, is respectively designated as MM-131, MM-132, MM-133, MM- 134, it is spare；

S5. the flow point MM-133 being collected into step S4 is purified with liquid phase is prepared, preparative liquid chromatography column is：YMC, 20mm*250mm, flow velocity：5ml/min, mobile phase are methanol-water-acetic acid system, methanol：Water：The volume ratio of acetic acid is 15:85: 0.01, eluent is collected, the phenylpropanoids are obtained after recrystallization.

The preparation of 2 phenylpropanoids of embodiment

S1. Flemingia macrophylla 40kg is taken, it is dry using root as raw material, it is cut into small pieces.Alcohol reflux through 6 times of amounts 50% Extraction 2 times, 1 hour every time, extracting solution is merged, is concentrated into no alcohol taste, it is spare to obtain medicinal extract；

S2. the medicinal extract after being concentrated in step S1 is dissolved in 5L water, it is washed using D101 large pore resin absorption columns De-, eluant, eluent is that the volume ratio of ethyl alcohol and water is 15:85,3 column volumes are eluted, eluent is collected, is named as MM-1, it is spare；

S3. the flow point MM-1 being collected into step S2 is eluted with reverse phase ODS column chromatographies, eluant, eluent is methanol-water System, volume ratio 20:80,18 column volumes are eluted, the eluent of a flow point are collected by every 3 column volumes, in order 6 flow points are collected, are respectively designated as：MM-11, MM-12, MM-13, MM-14, MM-15, MM-16 are spare；

S4. it is with liquid phase separation, preparative liquid chromatography column is prepared by the flow point MM-13 being collected into step S3：YMC, 20mm*250mm, flow velocity：10ml/min, mobile phase are methanol-water-acetic acid system, methanol：Water：The volume ratio of acetic acid is 35: 65:0.01, eluent is collected by peak sequence, 4 flow points is collected altogether, is respectively designated as MM-131, MM-132, MM-133, MM- 134, it is spare；

The preparation of 3 phenylpropanoids of embodiment

S1. Flemingia macrophylla 60kg is taken, it is dry using root as raw material, it is cut into small pieces.The alcohol reflux of 7 times of amounts 70% carries It takes 4 times, 3 hours every time, extracting solution is merged, be concentrated into no alcohol taste, it is spare to obtain medicinal extract；

S2. the medicinal extract after being concentrated in step S1 is dissolved in 8L water, it is washed using D101 large pore resin absorption columns De-, eluant, eluent is that the volume ratio of ethyl alcohol and water is 10:90,3 column volumes are eluted, eluent is collected, is named as MM-1, it is spare；

S3. the flow point MM-1 being collected into step S2 is eluted with reverse phase ODS column chromatographies, eluant, eluent is methanol-water System, volume ratio 30:70,18 column volumes are eluted, the eluent of a flow point are collected by every 3 column volumes, in order 6 flow points are collected, are respectively designated as：MM-11, MM-12, MM-13, MM-14, MM-15, MM-16 are spare；

S4. it is with liquid phase separation, preparative liquid chromatography column is prepared by the flow point MM-13 being collected into step S3：YMC, 20mm*250mm, flow velocity：10ml/min, mobile phase are methanol-water-acetic acid system, methanol：Water：The volume ratio of acetic acid is 30: 70:0.01, eluent is collected by peak sequence, 4 flow points is collected altogether, is respectively designated as MM-131, MM-132, MM-133, MM- 134, it is spare；

The preparation of 4 phenylpropanoids of embodiment

S1. Flemingia macrophylla 50kg is taken, it is dry using root as raw material, it is cut into small pieces.The alcohol reflux of 8 times of amounts 60% carries It takes 2 times, 1.5 hours every time, extracting solution is merged, be concentrated into no alcohol taste, it is spare to obtain medicinal extract；

S2. the medicinal extract after being concentrated in step S1 is dissolved in 6L water, it is washed using D101 large pore resin absorption columns De-, eluant, eluent is that the volume ratio of ethyl alcohol and water is 5:95,3 column volumes are eluted, eluent is collected, is named as MM-1, it is spare；

S4. it is with liquid phase separation, preparative liquid chromatography column is prepared by the flow point MM-13 being collected into step S3：YMC, 20mm*250mm, flow velocity：10ml/min, mobile phase are methanol-water-acetic acid system, methanol：Water：The volume ratio of acetic acid is 25: 75:0.01, eluent is collected by peak sequence, 4 flow points is collected altogether, is respectively designated as MM-131, MM-132, MM-133, MM- 134, it is spare；

The preparation of 5 phenylpropanoids of embodiment

S1. Flemingia macrophylla 50kg is taken, it is dry using root as raw material, it is cut into small pieces.The alcohol reflux of 8 times of amounts 80% carries It takes 2 times, 1.5 hours every time, extracting solution is merged, be concentrated into no alcohol taste, it is spare to obtain medicinal extract；

S2. the medicinal extract after being concentrated in step S1 is dissolved in 6L water, it is washed using D101 large pore resin absorption columns De-, eluant, eluent is that the volume ratio of ethyl alcohol and water is 10:90,3 column volumes are eluted, eluent is collected, is named as MM-1, it is spare；

S3. the flow point MM-1 being collected into step S2 is eluted with reverse phase ODS column chromatographies, eluant, eluent is methanol-water System, volume ratio 28:72,18 column volumes are eluted, the eluent of a flow point are collected by every 3 column volumes, in order 6 flow points are collected, are respectively designated as：MM-11, MM-12, MM-13, MM-14, MM-15, MM-16 are spare；

S4. it is with liquid phase separation, preparative liquid chromatography column is prepared by the flow point MM-13 being collected into step S3：YMC, 20mm*250mm, flow velocity：10ml/min, mobile phase are methanol-water-acetic acid system, methanol：Water：The volume ratio of acetic acid is 10: 90:0.01, eluent is collected by peak sequence, 4 flow points is collected altogether, is respectively designated as MM-131, MM-132, MM-133, MM- 134, it is spare；

The compound that embodiment 1 to embodiment 5 is prepared carries out mass spectrum, nuclear magnetic resonance spectroscopy, carbon-13 nmr spectra Detection, as a result prove gained compound be：The 3 '-glucosyl groups of hydroxyl -4 ' -3-hydroxybutyrate methyl esters.Its structural formula such as formula (I) It is shown：

Its mass spectrum, nuclear magnetic resonance spectroscopy, the spectral data of carbon-13 nmr spectra are as follows：

HR-ESIMS shows [M+Na]+be m/z 397.1267, and in conjunction with nuclear-magnetism feature, it is C that can obtain molecular formula₁₆H₂₂O₁₀, no Saturation degree is 6.

¹H-NMR(600MHz,CD₃OD):7.43(dd,1H),7.12(dd,1H),6.81(dd,1H),4.84(d,1H), 4.12(t,2H),3.56(m,1H),1.14(s,3H)。

¹³C-NMR(150MHz,CD₃OD):179.3(C-1),168.8(C-5'),150.1(C-1'),144.7(C-3'), 129.9(C-2'),116.4(C-4'),114.8(C-6'),103.6(C-1”),76.6-61.4(C2”-6”),42.9(C-2), 21.8(C-3),17.0(-CH₃)。

The preparation of 6 phenylpropanoids salt of embodiment

The preparation of phenylpropanoids hydrochloride：

Saturation hydrochloric acid will be added dropwise under stirring in the Phenylpropanoid Glycosides compound methanol solution to pH value 2-3, stir lower dropwise addition acetonitrile, It filters, is dried to obtain white powder solid, the as hydrochloride of Phenylpropanoid Glycosides compound.

The preparation of phenylpropanoids sulfonate：

Alkali metal is added in the reaction system containing the phenylpropanoids, solvent, sulfonic acid, neutral oil and accelerating agent Hydroxide, solvent, lower alcohol and kicker is added, is passed through carbon dioxide, isolated white powder solid, as benzene The sulfonate of C prime compound.

The preparation of phenylpropanoids sylvite or sodium salt：

The KOH being dissolved in ethyl alcohol or NaOH are added in the Phenylpropanoid Glycosides compound, lower heating reflux reaction, cold room processed are stirred Temperature, stir it is lower acetonitrile is added dropwise, filter, dry white solid, the as sylvite or sodium salt of the Phenylpropanoid Glycosides compound.

The preparation of phenylpropanoids ammonium salt：

Saturation ammonium hydroxide will be added dropwise under stirring in the Phenylpropanoid Glycosides compound methanol solution to pH value 9-11, stir lower dropwise addition second Nitrile filters, is dried to obtain white solid, the as ammonium salt of phenylpropanoids.

The spectral data of above compound salt：

Phenylpropanoids hydrochloride：ESIMS shows m/z 410.62, nuclear-magnetism feature¹H-NMR(600MHz, CD3OD):7.40(dd,1H),7.07(dd,1H),6.77(dd,1H),4.64(d,1H),4.02(t,2H),3.46(m,1H), 1.11(s,3H)。

Phenylpropanoids sulfonate：ESIMS is shown as m/z 438.22, nuclear-magnetism feature¹H-NMR(600MHz, CD3OD):7.54(dd,1H),7.13(dd,1H),6.80(dd,1H),4.83(d,1H),4.10(t,2H),3.54(m,1H), 1.13(s,3H)。

Phenylpropanoids sylvite or sodium salt：

Sylvite：ESIMS shows m/z 412.42, nuclear-magnetism feature¹H-NMR(600MHz,CD3OD):7.55(dd,1H), 7.11(dd,1H),6.86(dd,1H),4.83(d,1H),4.11(t,2H),3.56(m,1H),1.14(s,3H)。

Sodium salt：ESIMS display m/z 396.54,7.51 (dd, 1H), 7.10 (dd, 1H), 6.87 (dd, 1H), 4.85 (d, 1H),4.12(t,2H),3.57(m,1H),1.14(s,3H)。

Phenylpropanoids ammonium salt：ESIMS shows m/z 389.26, nuclear-magnetism feature¹H-NMR(600MHz,CD3OD): 7.46(dd,1H),7.17(dd,1H),6.80(dd,1H),4.84(d,1H),4.13(t,2H),3.51(m,1H),1.11(s, 3H)。

Shown in the structural formula such as formula (IV) of above-mentioned Phenylpropanoid Glycosides compound salt~formula (VIII).

Wherein, formula (IV) is the phenylpropanoids hydrochloride being prepared, and formula (V) is the Phenylpropanoid Glycosides being prepared The one of which sulfonate of class compound, formula (VI) are the one of which sylvite for the phenylpropanoids being prepared, formula (VII) it is the one of which sodium salt for the phenylpropanoids being prepared, formula (VIII) is the phenylpropanoids being prepared One of which ammonium salt.

7 application test of experimental example

Compound of the present invention and salt stress be with the shadows of inflammation to LPS 264.7 oxidative macrophages of RAW induced It rings.(it is convenient in order to be recorded in experimentation, below by phenylpropanoids of the present invention marked as：Drug MM-133, I.e. heretofore described drug MM-133 refers to phenylpropanoids shown in formula (I) or its is pharmaceutically acceptable Salt.)

1 materials and methods

1.1 drugs and instrument

Lipopolysaccharides (lipopolysaccharide, LPS), MTT are purchased from Sigma companies；Mouse macrophage Raw264.7 Purchased from the refined cell bank in Hunan；PBS；DMEM high glucose mediums, fetal calf serum, penicillin and streptomysin；Full-automatic microplate reader；Constant temperature CO2 incubators.

Mouse IL 1-β (IL-1- β) ELISA detection kit, lot number：2014/06(96T)；Small mIL6 (IL-6) ELISA detection kit, lot number：2014/06(96T)；Murine tumor necrosis factor-α (TNF-α) ELISA detection examinations Agent box, lot number：2014/06(96T)；Mouse nitrous oxide (NO) ELISA detection kit, lot number：2014/10(96T)；Mouse Hydroxyl radical free radical (OH) ELISA detection kit, lot number：2014/10(96T).

1.2 medicine preparation

It is dissolved first with a small amount of DMSO, certain concentration is then diluted to DMEM, DMSO contents in final concentration is made to be less than 1‰。

1.3 cell culture

Mouse macrophage Raw 264.7 be incubated at containing 10% heat inactivation (56 DEG C, 30min) fetal calf serum (FBS), 10U/mL Benzylpenicillin sodium salts, 100 μ g/mL streptomysins DMEM culture mediums in, 37 DEG C, 5%CO₂Growth is incubated in constant incubator.

1.4 cell viabilities measure

Cell viability is measured by mtt assay.Cell suspension inoculation is made in cell to incubate in 96 orifice plates (1 × 104/hole) It educates for 24 hours, resynchronization for 24 hours, then by the drug effect of various concentration in cell 2h, then adds LPS (30 μ g/mL) stimulations For 24 hours, it inhales and abandons former culture medium, the MTT (0.5mg/mL) that 100 μ L are added per hole continues to be incubated 4h, and culture medium is abandoned in suction, is added per hole The DMSO of 150 μ L, shaking table shake 10min, and absorbance is measured at 490nm.

1.5NO assay

264.7 cell inoculations of Raw in 96 orifice plates for 24 hours, resynchronization for 24 hours, then by the drug effect of various concentration in thin Then born of the same parents 2h adds LPS (30 μ g/mL) stimulations for 24 hours, finally collect supernatant, and on 10000rpm centrifugation 5min, packing Clearly -80 DEG C are placed in save backup.Pass through mouse NO kit measurement NO contents.

1.6 inflammatory factor TNF-α, IL-1 β, IL-6 measurements

Sample takes 1.5 samples prepared for subsequent inflammation factor determination.Cell generation TNF-α, IL-1 β, IL-6's By mouse TNF-α, IL-1 β, IL-6 kits measure for amount.

1.7OH assay

Sample takes 1.5 samples prepared for OH factor determinations.Pass through OH kit measurement contents.

1.8 statistical analysis

Using SPSS17.0 softwares, experimental data is indicated with x ± s；The data obtained is by with one-way analysis of variance, variance Homogeneous is examined with LSD, and heterogeneity of variance is examined with Dunnett T3.

2 experimental results

2.1 cell viability

Influence of the drug to cell viability is evaluated by mtt assay.As shown in figure 3, drug MM-133 is in 1.50-13.50 μ 264.7 cell viabilities of Raw are had no significant effect in g/mL concentration ranges；Therefore the drug concentration pair under this range of concentrations It is suitable in subsequent experimental.

The generation of 2.2 Drug inhibition NO

As shown in figure 4, by LPS stimulate 264.7 cells of Raw, generate NO (65.81 ± 2.93IU/mL) contents with just Often group NO (33.61 ± 2.19IU/mL) is compared significantly raised (p ＜ 0.01).Drug MM-133 is under the concentration to caused by LPS NO contents increase no apparent inhibiting effect.

2.3 Drug inhibition TNF-α, the generation of IL-1 β, IL-6

As shown in Figures 5 to 7,264.7 cells of Raw, 264.7 cellular inflammation factor TNF-α of Raw are stimulated by LPS (132.16 ± 5.28pg/mL), IL-1 β (358.80 ± 24.64pg/mL), IL-6 (198.39 ± 5.97pg/mL) contents with just Often group TNF-α (65.41 ± 6.29pg/mL), IL-1 β (172.67 ± 10.06pg/mL), IL-6 (103.34 ± 2.88pg/mL) It is significantly raised (p ＜ 0.01) compared to content；Illustrate that LPS can stimulate 264.7 cells of Raw to generate a large amount of inflammatory factors.

Raw264.7 cells caused by drug MM-133 stimulates LPS in concentration (10.50-13.50 μ g/mL) range are scorching Inflammation factor TNF-α content has apparent inhibiting effect (p ＜ 0.05), and shows apparent dose-dependence；In concentration There is apparent inhibiting effect (p ＜ 0.05) to inflammatory factor IL-1 β contents in (4.50-13.50 μ g/mL) range, shows bright Aobvious dose-dependence；There is apparent inhibition to inflammatory factor IL-6 contents in concentration (7.50-13.50 μ g/mL) range It acts on (p ＜ 0.05), shows apparent dose-dependence.

The generation of 2.4 Drug inhibition OH

As shown in figure 8, by LPS stimulate 264.7 cells of Raw, generate OH (113.58 ± 6.03ng/mL) contents with Normal group OH (63.40 ± 1.19ng/mL) is compared significantly raised (p ＜ 0.01).

Drug MM-133 has significantly OH changes of contents caused by LPS in (7.50-13.50 μ g/mL) concentration range Inhibiting effect (p ＜ 0.05), and show dose-dependence.

This experiment has studied drug MM-133 to mouse macrophage NO, TNF-α, IL-1 β, IL-6, OH through in vitro culture The influence of generation.

Drug MM-133 has apparent suppression in higher concentration to factor NO unrestraint activity to cellular inflammation factor TNF-α System activity, to IL-1 β, IL-6 inhibitory activity is stronger, and after illustrating its generation by inhibiting TNF-α, to IL-1 β, IL-6's contains Amount produces influence, illustrates that its anti-inflammatory activity is preferable, certain antioxidant activity is shown in middle and high concentration.

Embodiment 8

The preparation of tablet：Phenylpropanoids shown in formula (I) are first made by 1 method of embodiment, and utilize the change Close object and inorganic acid (such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid) or sulfonic acid or alkali Salt made of the hydroxide (such as potassium hydroxide, sodium hydroxide, calcium hydroxide, magnesium hydroxide, lithium hydroxide) or ammonium of metal, is pressed The compound or its any one salt and excipient weight ratio are 1:Excipient, pelletizing press sheet is added in 10 ratio.

Embodiment 9

The preparation of powder：Phenylpropanoids shown in formula (I) are first made by 1 method of embodiment, and utilize the change Close object and inorganic acid (such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid) or sulfonic acid or alkali Salt made of the hydroxide (such as potassium hydroxide, sodium hydroxide, calcium hydroxide, magnesium hydroxide, lithium hydroxide) or ammonium of metal, is pressed Powder is made in conventional powder preparation method.

Embodiment 10

The preparation of capsule or granule：Phenylpropanoids shown in formula (I) are first made by 1 method of embodiment, with And utilize the compound and inorganic acid (such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid) Or the hydroxide (such as potassium hydroxide, sodium hydroxide, calcium hydroxide, magnesium hydroxide, lithium hydroxide) or ammonium of sulfonic acid or alkali metal Manufactured salt is 1 by the compound or its any one salt and excipient weight ratio:Excipient is added in 10 ratio, and glue is made Wafer or granule.

Embodiment 11

The preparation of injection：Phenylpropanoids shown in formula (I) are first made by 1 method of embodiment, and utilizing should Compound and inorganic acid (such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid) or sulfonic acid or Salt made of the hydroxide (such as potassium hydroxide, sodium hydroxide, calcium hydroxide, magnesium hydroxide, lithium hydroxide) or ammonium of alkali metal, Injection is made in routinely water for injection, refined filtration, embedding sterilizing.

Embodiment 12

A kind of pharmaceutical composition is made phenylpropanoids shown in formula (I) containing 1 method of embodiment, and utilizes The compound and inorganic acid (such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid) or sulfonic acid Or made of the hydroxide (such as potassium hydroxide, sodium hydroxide, calcium hydroxide, magnesium hydroxide, lithium hydroxide) or ammonium of alkali metal Salt and cherokee rose root, single side needle, Caulis Spatholobi, leatherleaf mahonia, Herba Andrographitis, Radix Angelicae Sinensis, powder and auxiliary material made of Radix Codonopsis.

Embodiment 13

Phenylpropanoids shown in formula (I), and golden cherry is made containing 1 method of embodiment in a kind of pharmaceutical composition Root, single side needle, Caulis Spatholobi, leatherleaf mahonia, Herba Andrographitis, Radix Angelicae Sinensis, powder and auxiliary material made of Radix Codonopsis.

Embodiment 14

Phenylpropanoids shown in formula (I), and golden cherry is made containing 1 method of embodiment in a kind of pharmaceutical composition Root, single side needle, Caulis Spatholobi, leatherleaf mahonia, Herba Andrographitis, Radix Angelicae Sinensis, Radix Codonopsis extract and auxiliary material.Extract is by patent announcement number CN1078079C、CN1170549C、CN1158087C、CN1330335C、CN1296071C、CN1321631C、CN1296072C、 Extracting method is prepared in any one of CN1296073C or several patent documents.

Embodiment 15

A kind of pharmaceutical composition is made phenylpropanoids shown in formula (I) containing 1 method of embodiment, and utilizes The compound and inorganic acid (such as hydrochloric acid, hydrobromic acid, hydrofluoric acid, hydroiodic acid, sulfuric acid, nitric acid, carboxylic acid, phosphoric acid, lactic acid) or sulfonic acid Or made of the hydroxide (such as potassium hydroxide, sodium hydroxide, calcium hydroxide, magnesium hydroxide, lithium hydroxide) or ammonium of alkali metal Salt and cherokee rose root, single side needle, Caulis Spatholobi, leatherleaf mahonia, Herba Andrographitis, Radix Angelicae Sinensis, Radix Codonopsis extract and auxiliary material.Extract be by Patent announcement CN1078079C, CN1170549C, CN1158087C, CN1330335C, CN1296071C, CN1321631C, Extracting method is prepared in any one of CN1296072C, CN1296073C or several patent documents.

The advantage of the basic principles and main features and the present invention of the present invention has been shown and described above.The technology of this field Personnel are it should be appreciated that the present invention is not limited to the above embodiments, and the above embodiments and description only describe this The principle of invention, without departing from the spirit and scope of the present invention, various changes and improvements may be made to the invention, this is to this It is for field technology personnel it will be apparent that these changes and improvements all fall within the protetion scope of the claimed invention.This hair Bright claimed range is defined by the appending claims and its equivalent thereof.

Claims

1. a kind of preparation method of phenylpropanoids, which is characterized in that the structural formula of the phenylpropanoids such as formula (I) shown in,

The preparation method includes the following steps：

S1. it is raw material to take the root of Flemingia macrophylla, dry, and stripping and slicing extracts through ethanol solution, extracting solution is merged, is concentrated into Without alcohol taste, it is spare to obtain medicinal extract；

S2. gained medicinal extract in step S1 is dissolved in water, it is eluted using large pore resin absorption column, eluant, eluent is second Alcohol-water system collects the eluent of preceding 3 column volumes, is named as MM-1, spare；

S3. the flow point MM-1 being collected into step S2 is eluted with reversed material ODS column chromatographies, eluant, eluent is methanol-water System elutes 18 column volumes, and the eluent of a flow point is collected by every 3 column volumes, collects 6 flow points in order, respectively It is named as MM-11, MM-12, MM-13, MM-14, MM-15, MM-16, it is spare；

S4. it is methanol-water-acetic acid system with liquid phase separation, mobile phase is prepared by the flow point MM-13 being collected into step S3, presses Peak sequence collects eluent, collects 4 flow points altogether, is respectively designated as MM-131, MM-132, MM-133, MM-134, spare；

S5. the flow point MM-133 being collected into step S4 is purified with liquid phase is prepared, mobile phase is methanol-water-acetic acid system, is received Collect eluent, the phenylpropanoids are obtained after recrystallization.

2. preparation method according to claim 1, it is characterised in that：In step S1, a concentration of the 50~80 of ethanol solution Volume %.

3. preparation method according to claim 2, it is characterised in that：In step S1, a concentration of 60 body of ethanol solution Product %.

4. preparation method according to claim 1, it is characterised in that：In step S1, the extraction time of ethanol solution is 2~ It 4 times, extracts 1-3 hours every time.

5. preparation method according to claim 4, it is characterised in that：In step S1, the extraction time of ethanol solution is 3 It is secondary, it extracts 2 hours every time.

6. preparation method according to claim 1, it is characterised in that：In step S2, macroporous absorbent resin is big using D101 Macroporous adsorbent resin.

7. preparation method according to claim 1, it is characterised in that：In step S2, the volume ratio of ethyl alcohol and water is 0:100 ~15:85.

8. preparation method according to claim 1, it is characterised in that：In step S3, the volume ratio of eluant, eluent methanol and water It is 20:80~30:70.

9. preparation method according to claim 8, it is characterised in that：In step S3, the volume ratio of eluant, eluent methanol and water It is 25:75.

10. preparation method according to claim 1, it is characterised in that：In step S4, the volume ratio of methanol-water-acetic acid is 10:90:0.01~35:65:0.01.

11. preparation method according to claim 10, it is characterised in that：In step S4, the volume ratio of methanol-water-acetic acid It is 15:85:0.01.

12. preparation method according to claim 1, it is characterised in that：In step S4, the chromatographic column for preparing liquid phase is YMC, 20mm*250mm, flow rate of mobile phase are 5~10mL/min.

13. preparation method according to claim 12, it is characterised in that：In step S4, the chromatographic column for preparing liquid phase is YMC, 20mm*250mm, flow rate of mobile phase 5mL/min.

14. preparation method according to claim 1, which is characterized in that in step S5, the volume ratio of methanol-water-acetic acid is 15:85:0.01。

15. preparation method according to claim 1, it is characterised in that：In step S5, the chromatographic column for preparing liquid phase is YMC, 20mm*250mm, flow rate of mobile phase 5mL/min.