US20140370101A1 - 2,2',6,6'-tetraisopropyl-4,4'-biphenol lipid microsphere preparations and preparation methods therefor - Google Patents

2,2',6,6'-tetraisopropyl-4,4'-biphenol lipid microsphere preparations and preparation methods therefor Download PDF

Info

Publication number
US20140370101A1
US20140370101A1 US14/374,220 US201214374220A US2014370101A1 US 20140370101 A1 US20140370101 A1 US 20140370101A1 US 201214374220 A US201214374220 A US 201214374220A US 2014370101 A1 US2014370101 A1 US 2014370101A1
Authority
US
United States
Prior art keywords
biphenol
injection
grade
homogenous
lipid microsphere
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.)
Abandoned
Application number
US14/374,220
Inventor
Rutao Wang
Tao Chen
Shupan Guo
Huijing Hu
Long An
Weijiao Wang
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.)
XI'AN LIBANG PHARMACEUTICAL CO Ltd
Original Assignee
XI'AN LIBANG PHARMACEUTICAL CO Ltd
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 XI'AN LIBANG PHARMACEUTICAL CO Ltd filed Critical XI'AN LIBANG PHARMACEUTICAL CO Ltd
Assigned to XI'AN LIBANG PHARMACEUTICAL CO., LTD reassignment XI'AN LIBANG PHARMACEUTICAL CO., LTD ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS). Assignors: AN, Long, CHEN, TAO, GUO, Shupan, HU, Huijing, WANG, RUTAO, WANG, WEIJIAO
Publication of US20140370101A1 publication Critical patent/US20140370101A1/en
Abandoned legal-status Critical Current

Links

Classifications

    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/48Preparations in capsules, e.g. of gelatin, of chocolate
    • A61K9/50Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals
    • A61K9/5005Wall or coating material
    • A61K9/5015Organic compounds, e.g. fats, sugars
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K31/00Medicinal preparations containing organic active ingredients
    • A61K31/045Hydroxy compounds, e.g. alcohols; Salts thereof, e.g. alcoholates
    • A61K31/05Phenols
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/02Inorganic compounds
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/06Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite
    • A61K47/08Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite containing oxygen, e.g. ethers, acetals, ketones, quinones, aldehydes, peroxides
    • A61K47/10Alcohols; Phenols; Salts thereof, e.g. glycerol; Polyethylene glycols [PEG]; Poloxamers; PEG/POE alkyl ethers
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/06Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite
    • A61K47/08Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite containing oxygen, e.g. ethers, acetals, ketones, quinones, aldehydes, peroxides
    • A61K47/12Carboxylic acids; Salts or anhydrides thereof
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/06Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite
    • A61K47/22Heterocyclic compounds, e.g. ascorbic acid, tocopherol or pyrrolidones
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/06Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite
    • A61K47/24Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite containing atoms other than carbon, hydrogen, oxygen, halogen, nitrogen or sulfur, e.g. cyclomethicone or phospholipids
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/44Oils, fats or waxes according to two or more groups of A61K47/02-A61K47/42; Natural or modified natural oils, fats or waxes, e.g. castor oil, polyethoxylated castor oil, montan wax, lignite, shellac, rosin, beeswax or lanolin
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/0012Galenical forms characterised by the site of application
    • A61K9/0019Injectable compositions; Intramuscular, intravenous, arterial, subcutaneous administration; Compositions to be administered through the skin in an invasive manner
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/10Dispersions; Emulsions
    • A61K9/107Emulsions ; Emulsion preconcentrates; Micelles
    • A61K9/1075Microemulsions or submicron emulsions; Preconcentrates or solids thereof; Micelles, e.g. made of phospholipids or block copolymers
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/14Particulate form, e.g. powders, Processes for size reducing of pure drugs or the resulting products, Pure drug nanoparticles
    • A61K9/16Agglomerates; Granulates; Microbeadlets ; Microspheres; Pellets; Solid products obtained by spray drying, spray freeze drying, spray congealing,(multiple) emulsion solvent evaporation or extraction
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/48Preparations in capsules, e.g. of gelatin, of chocolate
    • A61K9/50Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals
    • A61K9/5089Processes
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P25/00Drugs for disorders of the nervous system
    • A61P25/08Antiepileptics; Anticonvulsants

Definitions

  • This invention relates to 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and the preparation methods therefor, in the field of pharmaceutical preparations.
  • biphenol 2,2′,6,6′-tetraisopropyl-4,4′-biphenol
  • biphenol is an anti-epileptic compound newly developed (Chinese patent CN 101804043A, Uses of biphenol and its derivatives in drugs for the treatment of epilepsy) for treating many epileptic symptoms such as generalized tonic-clonic seizures (grand mal), absence seizures (petit mal), simple partial seizures, complex partial seizures (psychomotor seizures), autonomic seizures (periodic seizures) and others.
  • Experimental studies have shown that biphenol has a strong affinity towards GABA receptors and is a GABA agonist, while it is an antagonist for NMDA receptors for regulating the Ca 2+ influx in Ca 2+ channels.
  • the present invention provides a 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparation and its preparation method.
  • 0.5 ⁇ 1% of antioxidants were added to the preparation to address the issue that biphenol is easily oxidizable.
  • vitamin E a potent, lipid soluble antioxidant, is used for ensuring the stability of the drug in the preparation.
  • This invention uses only phospholipid emulsifiers in an amount of 1 to 1.5% without any co-solvent so as to prevent hemolysis and production of substances that may otherwise cause thrombotic inflammation.
  • the emulsifiers of this invention are egg lecithin derived from the yolk of animal embryos which are easier and safer to be absorbed by the human body.
  • the lipid microsphere preparations of this invention are prepared by the processing of active ingredients comprising 2,2′,6,6′-tetraisopropyl-4,4′-biphenol (hereinafter referred as biphenol), injection-grade oil, emulsifier, and injection-grade water.
  • active ingredients comprising 2,2′,6,6′-tetraisopropyl-4,4′-biphenol (hereinafter referred as biphenol), injection-grade oil, emulsifier, and injection-grade water.
  • biphenol 2,2′,6,6′-tetraisopropyl-4,4′-biphenol
  • injection-grade oil injection-grade oil
  • emulsifier injection-grade water
  • injection-grade water injection-grade water.
  • All units are in percentage by weight.
  • the injection-grade oil is selected from one or more of soybean oil, medium chain triglyceride oil, sea buckthorn oil, and tea oil.
  • the emulsifier is selected from one or more of soy lecithin, hydrogenated lecithin, synthetic lecithin, and egg lecithin.
  • the antioxidant is selected from one or more of vitamin E, ascorbic acid, and sodium hydrogen sulfite.
  • the lipid microsphere preparation of this invention has the following composition.
  • Every 100 ml of lipid microsphere preparation comprises 1000 mg of biphenol, 10 g of soybean oil, 1.2 g of injection-grade egg lecithin for injection, 1 g of vitamin E, 2.5 g of glycerin, 0.5 g EDTA, and the remaining being injection-grade water.
  • This invention also aims to provide a method for preparing biphenol lipid microsphere preparations.
  • the preparation method of this invention comprises the following steps:
  • said method for preparing biphenol lipid microsphere preparations comprises the following steps:
  • the preparation of this invention is a lipid microsphere preparation for use in intravenous injections.
  • the particle size of the lipid microspheres of this invention is in the range of 100 nm ⁇ 800 nm with the average particle size being 150 nm ⁇ 300 nm.
  • biphenol is encapsulated within lipid microspheres which greatly increase its solubility in water, the amount of drug that can be loaded, and also the stability of the preparation. Further, being a novel drug carrier, lipid microspheres are non-toxic, non-immunogenic, reducing irritation due to the drug and decreasing the drug's toxic side effects.
  • This invention increases the stability of the injection, extends the drug's shelf life, improves its solubility and ensures its safeness. Moreover, the simple and feasible preparation process of the present invention is time and cost effective such that it is well suited for mass production. Furthermore, the formula and preparation methods for the preparation of this invention have been scientifically screened and proven.
  • the preparation of this invention relates to anti-epileptic preparations.
  • the anti-epileptic preparation of this invention has significantly higher efficacy in comparison to CMCNa-biphenol.
  • the method for administering the drug is switched from oral administration to intravenous injection which improves drug absorption and increases the therapeutic effect of the drug;
  • the preliminary emulsion was homogenized with a high-pressure homogenizer and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • Drugs and Excipients Amount (g) Biphenol 10.0 Injection-grade Soybean oil 300 Soy lecithin 15 Vitamin E 10 Glycerin 25 EDTA 5 Injection-grade water make up to 1000 ml
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • Drugs and Excipients Amount (g) Biphenol 10.0 Injection-grade Soybean oil 100 Hydrogenated Lecithin 12 Vitamin E 10 Glycerin 25 EDTA 5 Injection-grade water make up to 1000 ml
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • Drugs and Excipients Amount (g) Biphenol 10.0 Injection-grade Soybean oil 100 Synthetic phospholipids 12 Vitamin E 10 Glycerin 25 EDTA 5 Injection-grade water make up to 1000 ml
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the preliminary emulsion was homogenized with a high-pressure homogenizer for 5 ⁇ 8 times at 800 ⁇ 900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
  • the osmolarity of the final emulsion was determined to be 300 ⁇ 400 mOsm/L by an osmometer (freezing point depression method) which fulfilled the requirement for a lipid microsphere preparation to be used for intravenous injection.
  • the biphenol lipid microspheres prepared were kept at 4° C. for 6 months before subjected to 45° C. for 6 months and, after which, were placed at room temperature for 12 months.
  • the stability of the products was evaluated in terms of their appearance, pH and encapsulation efficiency. Results are shown in Table 1.
  • Example 0 mth Homogenous Homogenous Homogenous 7.85 7.86 7.84 98.45 98.35 98.46 1 1 mth Homogenous Homogenous Homogenous 7.74 7.71 7.68 98.45 98.38 98.45 2 mth Homogenous Homogenous Homogenous 7.66 7.64 7.55 98.40 98.36 98.44 3 mth Homogenous Homogenous Homogenous 7.54 7.66 7.46 98.41 98.37 98.45 6 mth Homogenous Homogenous Homogenous 7.32 7.52 7.29 98.38 98.25 98.36 9 mth — Homogenous — — 7.48 — — 98.26 — 12 mth — Homogenous — — 7.31 — — 98.23 — Example 0 mth Homogenous Homogenous Homogenous 7.94 7.84 7.91 98.54
  • the lipid microspheres of this invention have good stability. No significant change to their appearance and encapsulation efficiency was noticed after being placed at 4° C. for 6 months followed by 45° C. for 6 months and, subsequently, placed at room temperature for 12 months. Although there were some degrees of decrease in pH, this did not affect the stability of the preparations.
  • lipid microsphere preparations prepared according to this invention possessed good stability which met the requirements on the stability of preparations stipulated in China's National Guidelines on Novel Drug Research.
  • the biphenol content in this invention was determined by high performance liquid chromatography.
  • a C18 column (4.6 mm ⁇ 200 mm, 5 ⁇ m) was used with methanol-acetonitrile-water (60:22:18) as the mobile phase at a flow rate of 1.0 ml/min and UV detection at 275 nm.
  • Lipid microsphere preparations were centrifuged at 10000 r/min for 30 minutes by ultracentrifugation. 0.5 ml of the supernatant was obtained and dissolved with isopropyl alcohol and the biphenol content was characterized with high performance liquid chromatography to determine the encapsulated biphenol content, M1. The total biphenol content in lipid microsphere preparation is M0. The following formula was used for calculating the encapsulation efficiency which is the weight ratio of biphenol lipid microspheres to biphenol.
  • Three groups of 8 guinea pigs were randomly separated based on their weight. Each of the guinea pigs from group 1 and group 2 was given 3 successive peritoneal injections of the biphenol lipid microsphere preparations at a dose of 0.5 ml/guinea pig every other day to induce sensitization. On day 14 and day 21 after the first peritoneal injection, guinea pigs from groups 1 and 2 were given intravenous injections of the biphenol lipid microsphere preparations at the toe at a dose of 1.0 ml/guinea pig so as to cause stimulation.
  • the guinea pigs were given 3 successive peritoneal injections of 20% egg white at a dose of 0.5 ml/guinea pig every other day to induce sensitization and, after 14 days, were given intravenous injection of egg white at the toe at a dose of 1.0 ml/guinea pig so as to cause stimulation. All three groups were observed for 15 minutes after injection to notice for allergic reactions.
  • results The two groups of guinea pigs injected with biphenol lipid microspheres which received the stimulation dose of same drug on day 14 and day 21 respectively did not show any allergic response.
  • the guinea pigs in the positive control group had breathing difficulty and spasm within 2 minutes after injection before they died. The death of the guinea pigs were within 1 ⁇ 3 minutes after injection.
  • Biphenol lipid microsphere preparations were intravenously injected at the left ear of 2 New Zealand white rabbits at a dose of 5 ml/kg while 10% sucrose injections were intravenously injected at the right ear at a dose of 5 ml/kg.
  • the injections were given daily for a total of five days. The injection site was observed for any swelling or rashes since day 1. Within 24 hours after the last injection, the ears were removed and fixed in 10% formalin before being prepared for histopathological examination.
  • the allergy test, hemolytic test and irritation test on the lipid microsphere preparations of this invention showed that the lipid microsphere preparations of this invention are highly stable and do not cause any allergic, hemolytic or irritation effects. It therefore complies with the relevant requirements for clinically used drugs.

Abstract

This invention relates to a 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparation having 2,2′,6,6′-tetraisopropyl-4,4′-biphenol as its active ingredient and formed into said lipid microsphere preparation with common medically used injection-grade oil, emulsifier, and injection-grade water.

Description

    FIELD OF THE INVENTION
  • This invention relates to 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and the preparation methods therefor, in the field of pharmaceutical preparations.
    • BACKGROUND OF THE INVENTION
  • 2,2′,6,6′-tetraisopropyl-4,4′-biphenol (hereinafter referred to as biphenol) is an anti-epileptic compound newly developed (Chinese patent CN 101804043A, Uses of biphenol and its derivatives in drugs for the treatment of epilepsy) for treating many epileptic symptoms such as generalized tonic-clonic seizures (grand mal), absence seizures (petit mal), simple partial seizures, complex partial seizures (psychomotor seizures), autonomic seizures (periodic seizures) and others. Experimental studies have shown that biphenol has a strong affinity towards GABA receptors and is a GABA agonist, while it is an antagonist for NMDA receptors for regulating the Ca2+ influx in Ca2+ channels. Biphenol also offers protection against the excitotoxic effect induced by kainate (kainic acid). Studies have confirmed that biphenol is a significantly stronger antioxidant than propofol and has a stronger protective effect on the brain. Of particular importance is that biphenol does not cause the patients to lose consciousness and therefore has important clinical values in the treatment of patients with different types of epilepsy.
  • However, biphenol is a highly lipid soluble compound that is difficult to dissolve in water. Studies have shown that it is difficult to achieve a desired effect by using surfactants such as cyclodextrin, Tween 80, Vc or DMSO to assist or increase its dissolution and, thereby, its efficacy is affected and its clinical application becomes limited. In this invention, lipid microspheres are used as a drug carrier for the biphenol. This not only overcomes the problems due to insolubility of biphenol, but also allows the drug to be selectively accumulated in a lesion site and maximizes the amount of drug that is delivered to a targeted site so that the concentration of the drug at that site can be increased by several to hundred times above that of conventional preparations to improve its therapeutic effect. At the same time, there is minimal amount of drugs distributed in healthy tissues such that any cytotoxic side effects and adverse reactions are significantly reduced, and hence high efficacy with low toxicity would be achieved. Currently, there has been no report on biphenol lipid microsphere preparations. Therefore, the rational formulation of a preparation based on the physiochemical properties of biphenol for safe, stable and effective biphenol lipid microspheres is an issue this invention will address.
  • The present invention provides a 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparation and its preparation method. 0.5˜1% of antioxidants were added to the preparation to address the issue that biphenol is easily oxidizable. Particularly, vitamin E, a potent, lipid soluble antioxidant, is used for ensuring the stability of the drug in the preparation. This invention uses only phospholipid emulsifiers in an amount of 1 to 1.5% without any co-solvent so as to prevent hemolysis and production of substances that may otherwise cause thrombotic inflammation. Further, the emulsifiers of this invention are egg lecithin derived from the yolk of animal embryos which are easier and safer to be absorbed by the human body.
    • SUMMARY OF THE INVENTION
  • The present invention provides a 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparation, and preparation method therefor.
  • The lipid microsphere preparations of this invention are prepared by the processing of active ingredients comprising 2,2′,6,6′-tetraisopropyl-4,4′-biphenol (hereinafter referred as biphenol), injection-grade oil, emulsifier, and injection-grade water. In a specific embodiment, 0.1˜3% of biphenol, 10˜30% of injection-grade oil, 1˜1.5% of emulsifiers, 0.5˜1% of antioxidants, 0˜5% of additives with the remaining being injection-grade water. All units are in percentage by weight.
  • The chemical structure of said biphenol is:
  • Figure US20140370101A1-20141218-C00001
  • The injection-grade oil is selected from one or more of soybean oil, medium chain triglyceride oil, sea buckthorn oil, and tea oil.
  • The emulsifier is selected from one or more of soy lecithin, hydrogenated lecithin, synthetic lecithin, and egg lecithin.
  • The antioxidant is selected from one or more of vitamin E, ascorbic acid, and sodium hydrogen sulfite.
  • The additive is selected from one or more of pH adjusting agent, tonicity adjusting agents, complexing agents; said pH adjusting agent is hydrochloric acid or sodium hydroxide; said tonicity adjusting agent is glycerin; said complexing agent is EDTA; wherein their percentage by weight in an injection preparation are 0.01 to 1%, 0.1˜2.5% and 0.01 to 1% respective.
  • Preferably, the lipid microsphere preparation of this invention has the following composition.
  • Every 100 ml of lipid microsphere preparation comprises 1000 mg of biphenol, 10 g of soybean oil, 1.2 g of injection-grade egg lecithin for injection, 1 g of vitamin E, 2.5 g of glycerin, 0.5 g EDTA, and the remaining being injection-grade water.
  • Other preferred embodiments for the lipid microsphere preparation of this invention are disclosed in the Examples.
  • This invention also aims to provide a method for preparing biphenol lipid microsphere preparations.
  • The preparation method of this invention comprises the following steps:
    • 1) Dissolving the emulsifiers completely with the injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath; adding the antioxidants with stirring for dissolution before adding the biphenol with heat and stirring for dissolution to obtain an oil phase;
    • 2) Dissolving the tonicity adjusting agents and the complexing agents in the injection-grade water to obtain an aqueous phase;
    • 3) Adding the oil phase slowly to the aqueous phase while shearing under nitrogen for 5 minutes to obtain a preliminary emulsion;
    • 4) Homogenizing the preliminary emulsion with a high-pressure homogenizer before filtering with a microporous membrane filter, flushing with nitrogen, sealing and autoclaving at 115° C. to form the final product.
  • In the present invention, due to differences in water-solubility of antioxidants, there are different ways for adding the antioxidants. Lipid-soluble antioxidants are added to the oil phase while water-soluble antioxidants are added to the aqueous phase.
  • In a specific embodiment, said method for preparing biphenol lipid microsphere preparations comprises the following steps:
    • 1) Weighing the raw materials: 1 g˜30 g of biphenol, 100 ml˜300 ml injection-grade oil, 25 g of glycerin, 10 g˜15 g of emulsifiers, 5 g˜10 g of antioxidants, with the remaining being injection-grade water.
    • 2) Dissolving the emulsifiers and the antioxidants (Vitamin E) completely with the injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath, before adding the biphenol with heat and stirring for dissolution to obtain an oil phase;
    • 3) Dissolving the glycerin and the complexing agents in the injection-grade water and stir to obtain an aqueous phase;
    • 4) Adding the oil phase slowly to the aqueous phase while shearing under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion, and adjusting the pH to around 8.0 with NaOH;
    • 5) Homogenizing the preliminary emulsion 5˜8 times with a high-pressure homogenizer at 800˜900 bar before filtering with a microporous membrane filter, flushing with nitrogen, sealing and autoclaving at 115° C. to obtain the final product (1000 ml).
  • In another specific embodiment, said method for preparing biphenol lipid microsphere preparations comprises the following steps:
    • 1) Weighing the raw materials: 1 g˜30 g biphenol, 100 ml˜300 ml injection-grade oil, 25 g of glycerin, 10 g˜15 g of emulsifiers, 5 g˜10 g of antioxidants, with the remaining made up of injection-grade water.
    • 2) Dissolving the emulsifier completely in the injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath before adding the biphenol with heat and stirring for dissolution to obtain an oil phase;
    • 3) Dissolving the glycerin, the antioxidants (ascorbic acid or sodium bisulfite) and the complexing agents in injection-grade water and stirring to obtain an aqueous phase;
    • 4) Adding the oil phase slowly to the aqueous phase while shearing under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion, and adjusting pH to around 8.0 with NaOH;
    • 5) Homogenizing the preliminary emulsion 5˜8 times with a high-pressure homogenizer at 800˜900 bar before filtering with a microporous membrane filter, flushing with nitrogen, sealing and autoclaving at 115° C. to obtain the final product (1000 ml).
  • Other embodiments of the preparation method of this invention are disclosed in the Examples.
  • The preparation of this invention is a lipid microsphere preparation for use in intravenous injections.
  • The particle size of the lipid microspheres of this invention is in the range of 100 nm˜800 nm with the average particle size being 150 nm˜300 nm.
  • In the preparation of this invention, biphenol is encapsulated within lipid microspheres which greatly increase its solubility in water, the amount of drug that can be loaded, and also the stability of the preparation. Further, being a novel drug carrier, lipid microspheres are non-toxic, non-immunogenic, reducing irritation due to the drug and decreasing the drug's toxic side effects.
  • This invention increases the stability of the injection, extends the drug's shelf life, improves its solubility and ensures its safeness. Moreover, the simple and feasible preparation process of the present invention is time and cost effective such that it is well suited for mass production. Furthermore, the formula and preparation methods for the preparation of this invention have been scientifically screened and proven.
  • The preparation of this invention relates to anti-epileptic preparations.
  • The anti-epileptic preparation of this invention has significantly higher efficacy in comparison to CMCNa-biphenol.
  • In this invention, the method for administering the drug is switched from oral administration to intravenous injection which improves drug absorption and increases the therapeutic effect of the drug;
  • Detailed experimental results on the anti-epileptic effect of the preparation of this invention can be found in the Examples.
  • Obviously, further embodiments can be devised by means of modification, replacement or alteration of the invention described above with common knowledge and skills in the art without steering away from the basic concepts of this invention.
  • The following specific embodiments in the Examples aim to provide further explanation of the above description. One should not interpret this as a means to limit the scope of this invention to only the embodiments which follow. All embodiments based on the above description should fall into the scope of this invention.
    • DETAILED DESCRIPTION OF THE INVENTION
  • The following examples further illustrate the present invention but in no way limit the scope of the present invention. Those skilled in the art will appreciate that the present invention is not limited to the embodiments and methods of preparation described with reference to the following examples. Further, those equivalent embodiments that skilled person in the art can make by modification, replacement or alteration of the present invention should also fall into the scope of the present invention.
    • Part 1) Lipid Microsphere Preparation Prepared with Different Concentrations of Biphenol Example 1 1% Biphenol Lipid Microsphere Preparation
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Soybean oil (Injection-grade) 100
    Egg lecithin 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 20 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtained an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 2 0.1% Biphenol Lipid Microsphere Preparation
  • Drugs and Excipients Amount (g)
    Biphenol 1.0
    Sea buckthorn oil (Injection- 100
    grade)
    Hydrogenated Lecithin 12
    Ascorbic acid 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of hydrogenated lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 1 g of biphenol was then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin, 10 g ascorbic acid and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain the aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 3 3% Biphenol Lipid Microsphere Preparation
  • Drugs and Excipients Amount (g)
    Biphenol 30
    Injection-grade Medium-chain 100
    triglyceride oil
    Soy lecithin 12
    Sodium bisulfite 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of soy lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 30 g of biphenol was then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin, 10 g of sodium bisulfite and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtained an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Part 2) Lipid Microsphere Preparation Prepared with Different Types of Injection Oil and Contents Example 4 Lipid Microsphere Preparation with 20% Soybean Oil
  • Drugs and Excipients The amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 200
    (Injection-grade)
    Egg lecithin 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 200 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain the aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 5 Lipid Microsphere Preparation with 10% Medium-Chain Glyceride Oil
  • Drugs and their accessories The amount (g)
    Biphenol 10.0
    Injection-grade Medium chain 100
    triglyceride oil (Injection-
    grade)
    Egg lecithin 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 200 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 6 Lipid Microsphere Preparation with 30% Sea Buckthorn Oil
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Sea buckthorn 300
    oil
    Egg lecithin 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 200 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were the added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 7 Lipid Microsphere Preparation with 10% Tea Oil
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Tea oil 100
    Egg lecithin 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 200 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Part 3) Lipid Microsphere Preparations with Different Type and Amount of Emulsifier Example 8 Lipid Microsphere Preparation with 30% Sea Buckthorn Oil
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Egg lecithin 10
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 10 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 9 Lipid Microsphere Preparation with 1.5% Soy Lecithin
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 300
    Soy lecithin 15
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 15 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 10 Lipid Microsphere Preparation with 1.2% Hydrogenated Lecithin
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Hydrogenated Lecithin 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of hydrogenated lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 11 Lipid Microsphere Preparation with 1.2% Synthetic Phospholipid
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Synthetic phospholipids 12
    Vitamin E 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of synthetic phopholipid was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Part 4) Lipid Microsphere Preparation with Different Types and Amount of Antioxidant Example 12 Lipid Microsphere Preparation with 0.5% Vitamin E
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Egg lecithin 12
    Vitamin E 5
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath, 10 g of biphenol and 5 g of vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin and 5 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 13 Lipid Microsphere Preparation with 1% Ascorbic Acid
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Egg lecithin 12
    Ascorbic acid 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol was then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin, 5 g of EDTA and 10 g of ascorbic acid were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 14 Lipid Microsphere Preparation with 1% Sodium Bisulfite
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Egg lecithin 12
    Sodium bisulfite 10
    Glycerin 25
    EDTA 5
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol was then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 25 g of glycerin, 5 g of EDTA and 10 g of sodium bisulfite were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Part 5) Lipid Microsphere Preparation with Different Types and Amount of Additives Example 15 Lipid Microsphere Preparation with 1.5% Glycerin and 0.3% EDTA
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Egg lecithin 12
    Vitamin E 10
    Glycerin 15
    EDTA 3
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 10 g vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 15 g of glycerin and 3 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 16 Lipid Microsphere Preparation with 2% Glycerin and 1% EDTA
  • Drugs and Excipients Amount (g)
    Biphenol 10.0
    Injection-grade Soybean oil 100
    Egg lecithin 12
    Vitamin E 10
    Glycerin 20
    EDTA 10
    Injection-grade water Make up to 1000 ml
    • Preparation Method
  • 1) 12 g of egg lecithin was completely dissolved in 100 g of injection-grade oil under a nitrogen atmosphere and in a 70° C. water bath. 10 g of biphenol and 5 g vitamin E were then added and nitrogen gas was fed in for protection before being dissolved, with heat and stirring, to obtain an oil phase.
  • 2) 20 g of glycerin and 10 g of EDTA were dissolved, with stirring, in the injection-grade water to obtain an aqueous phase.
  • 3) The oil phase was added slowly to the aqueous phase while sheared under nitrogen (10000 r, 5 min) to obtain a preliminary emulsion which was then adjusted to around pH 8.0 with sodium hydroxide.
  • 4) The preliminary emulsion was homogenized with a high-pressure homogenizer for 5˜8 times at 800˜900 bar and filtered with a microporous membrane filter before being flushed with nitrogen, sealed, autoclaved at 115° C. to obtain the final product.
    • Example 17 Experiment for Screening of Formulations 1) Selection of Injection-Grade Oil
  • This experiment was conducted with biphenol lipid microsphere preparations prepared separately with soybean oil, medium chain triglyceride oil, sea buckthorn oil and tea oil. The final emulsions appeared homogenous with no layering or floating oil. 1 ml of each of the lipid microsphere injections was obtained separately and diluted by a factor of 1000 and their particle sizes were determined by dynamic light scattering particle size analyzer (Marvelen, US). Results showed that the particle sizes of the microspheres prepared using the above mentioned injection-grade oil were evenly distributed with 70% having a particle size smaller than 500 nm and 100% having a particle size smaller than 1 μm which fulfilled the requirement for a lipid microsphere preparation to be used for intravenous injections. Soybean oil and medium chain triglyceride oil fared the best with 90% having a particle size smaller than 500 nm and 100% having a particle size smaller than 1 μm.
    • 2) Selection of Emulsifier
  • This experiment was conducted with biphenol lipid microsphere preparations prepared separately with egg lecithin, soy lecithin and hydrogenated lecithin. The final emulsions appeared homogenous with no layering or floating oil. 1 ml of each of the lipid microsphere injections was obtained separately and diluted by a factor of 1000 and their particle sizes were determined by dynamic light scattering particle size analyzer (Marvelen, US). Results showed that the particle sizes of the microspheres prepared using the above mentioned injection-grade oil were evenly distributed with 70% having a particle size smaller than 500 nm and 100% having a particle size smaller than 1 μm which fulfilled the requirement for a lipid microsphere preparation to be used for intravenous injections.
    • 3) Selection of Tonicity Adjusting Agent
  • This experiment was conducted with glycerin as the tonicity adjusting agent so as to ensure that the microspheres would be isotonic inside the human body. The osmolarity of the final emulsion was determined to be 300˜400 mOsm/L by an osmometer (freezing point depression method) which fulfilled the requirement for a lipid microsphere preparation to be used for intravenous injection.
    • 4) Antioxidant
  • This experiment was conducted with vitamin E as the antioxidant so as to prevent any instability due to oxidation. The final emulsions appeared homogenous with no layering or floating oil. 1 ml of the lipid microsphere injections was obtained separately and diluted by a factor of 1000 and the particle size was determined by dynamic light scattering particle size analyzer (Marvelen, US). Results showed that the microspheres obtained with the above mentioned injection-grade oil was evenly distributed with 70% having a particle size smaller than 500 nm and 100% having a particle size smaller than 1 μm which fulfills the requirement for a lipid microsphere preparation to be used in intravenous injection.
    • 5) Complexing Agent
  • This experiment was conducted with biphenol lipid microsphere preparations prepared with EDTA, a common complexing agent, so as to decrease the concentration of free positive ions in the microspheres and increase the stability of lipid microsphere preparation. The final emulsions appeared homogenous with no layering or floating oil. 1 ml of each of the lipid microsphere injections was obtained separately and diluted by a factor of 1000 and their particle sizes were determined by dynamic light scattering particle size analyzer (Marvelen, US). Results showed that the microspheres prepared using the above mentioned injection-grade oil were evenly distributed with 70% having a particle size smaller than 500 nm and 100% having a particle size smaller than 1 μm which fulfills the requirement for a lipid microsphere preparation to be used for intravenous injections.
  • The following experiments characterized the physiochemical properties and safeness of the lipid microsphere preparation prepared in accordance to above description.
    • Experiment 1 Stability Test
  • The biphenol lipid microspheres prepared were kept at 4° C. for 6 months before subjected to 45° C. for 6 months and, after which, were placed at room temperature for 12 months. The stability of the products was evaluated in terms of their appearance, pH and encapsulation efficiency. Results are shown in Table 1.
  • TABLE 1
    Results of the Stability Test on the biphenol lipid microspheres of this invention
    Encapsulation
    Appearance pH efficiency
    Sample Time 4° C. 25° C. 45° C. 4° C. 25° C. 45° C. 4° C. 25° C. 45° C.
    Example 0 mth Homogenous Homogenous Homogenous 7.85 7.86 7.84 98.45 98.35 98.46
    1 1 mth Homogenous Homogenous Homogenous 7.74 7.71 7.68 98.45 98.38 98.45
    2 mth Homogenous Homogenous Homogenous 7.66 7.64 7.55 98.40 98.36 98.44
    3 mth Homogenous Homogenous Homogenous 7.54 7.66 7.46 98.41 98.37 98.45
    6 mth Homogenous Homogenous Homogenous 7.32 7.52 7.29 98.38 98.25 98.36
    9 mth Homogenous 7.48 98.26
    12 mth  Homogenous 7.31 98.23
    Example 0 mth Homogenous Homogenous Homogenous 7.94 7.84 7.91 98.54 98.38 98.44
    3 1 mth Homogenous Homogenous Homogenous 7.80 7.73 7.82 98.39 98.44 98.54
    2 mth Homogenous Homogenous Homogenous 7.74 7.66 7.60 98.39 98.45 98.33
    3 mth Homogenous Homogenous Homogenous 7.62 7.62 7.47 98.64 98.38 98.31
    6 mth Homogenous Homogenous Homogenous 7.39 7.53 7.33 98.55 98.31 98.35
    9 mth Homogenous 7.44 98.34
    12 mth  Homogenous 7.28 98.29
    Example 0 mth Homogenous Homogenous Homogenous 7.88 7.92 7.93 99.12 98.85 98.65
    6 1 mth Homogenous Homogenous Homogenous 7.86 7.85 7.80 98.57 98.74 98.37
    2 mth Homogenous Homogenous Homogenous 7.79 7.81 7.74 98.65 98.75 98.29
    3 mth Homogenous Homogenous Homogenous 7.68 7.75 7.63 98.36 98.63 98.54
    6 mth Homogenous Homogenous Homogenous 7.59 7.62 7.44 98.54 98.68 98.47
    9 mth Homogenous 7.46 98.58
    12 mth  Homogenous 7.31 98.71
    Example 0 mth Homogenous Homogenous Homogenous 7.87 7.93 7.89 99.02 98.99 98.66
    8 1 mth Homogenous Homogenous Homogenous 7.80 7.82 7.80 98.72 98.47 98.87
    2 mth Homogenous Homogenous Homogenous 7.76 7.79 7.77 98.56 98.65 98.25
    3 mth Homogenous Homogenous Homogenous 7.65 7.73 7.66 98.63 98.66 98.48
    6 mth Homogenous Homogenous Homogenous 7.58 7.60 7.48 98.44 98.84 98.43
    9 mth Homogenous 7.45 98.63
    12 mth  Homogenous 7.30 98.42
    Example 0 mth Homogenous Homogenous Homogenous 8.03 7.96 7.88 99.03 98.69 98.42
    12 1 mth Homogenous Homogenous Homogenous 7.98 7.88 7.85 98.72 98.77 98.68
    2 mth Homogenous Homogenous Homogenous 7.78 7.75 7.73 98.33 98.64 98.84
    3 mth Homogenous Homogenous Homogenous 7.72 7.68 7.65 98.34 98.58 98.62
    6 mth Homogenous Homogenous Homogenous 7.55 7.47 7.41 98.65 98.79 98.79
    9 mth Homogenous 7.42 98.99
    12 mth  Homogenous 7.36 98.45
    Example 0 mth Homogenous Homogenous Homogenous 7.96 7.84 7.94 99.62 98.64 98.41
    16 1 mth Homogenous Homogenous Homogenous 7.90 7.80 7.78 98.54 98.84 98.89
    2 mth Homogenous Homogenous Homogenous 7.84 7.76 7.68 98.80 98.62 99.03
    3 mth Homogenous Homogenous Homogenous 7.75 7.71 7.60 98.67 98.87 98.74
    6 mth Homogenous Homogenous Homogenous 7.60 7.58 7.24 98.43 98.59 98.66
    9 mth Homogenous 7.51 98.44
    12 mth  Homogenous 7.29 98.63
  • As shown in Table 1, the lipid microspheres of this invention have good stability. No significant change to their appearance and encapsulation efficiency was noticed after being placed at 4° C. for 6 months followed by 45° C. for 6 months and, subsequently, placed at room temperature for 12 months. Although there were some degrees of decrease in pH, this did not affect the stability of the preparations.
  • Although the above only listed the results for the embodiments in this part of the specification, it should be noted that other embodiments of this invention also possess the same or similar beneficial effects.
  • In conclusion, lipid microsphere preparations prepared according to this invention possessed good stability which met the requirements on the stability of preparations stipulated in China's National Guidelines on Novel Drug Research.
    • Experiment 2 Method for Quality Control
  • The biphenol content in this invention was determined by high performance liquid chromatography. A C18 column (4.6 mm×200 mm, 5 μm) was used with methanol-acetonitrile-water (60:22:18) as the mobile phase at a flow rate of 1.0 ml/min and UV detection at 275 nm. The results showed that the average recovery rate was 99.35% with RSD=0.75% (n=11). Good linear relationship (r=0.9999) was found between concentration and the area under the peak for biphenol in the range 1˜100 μg/ml.
    • Experiment 3 Determining the Encapsulation Efficiency of the Lipid Microsphere Preparations
  • Lipid microsphere preparations were centrifuged at 10000 r/min for 30 minutes by ultracentrifugation. 0.5 ml of the supernatant was obtained and dissolved with isopropyl alcohol and the biphenol content was characterized with high performance liquid chromatography to determine the encapsulated biphenol content, M1. The total biphenol content in lipid microsphere preparation is M0. The following formula was used for calculating the encapsulation efficiency which is the weight ratio of biphenol lipid microspheres to biphenol.

  • Q=M 1 /M 0×100%
  • The results showed that the encapsulation efficiency of the lipid microsphere preparation for intravenous injection prepared in this invention is greater than 98% when using biphenol as an indicator.
    • Experiment 4 Sterility Test
  • Sterility test was conducted on the lipid microsphere preparations of this invention in accordance to the method described in the appendix of the Chinese Pharmacopoeia 2010 edition. All lipid microsphere preparations of this invention passed the sterility test.
    • Experiment 5 Pyrogen Test
  • Pyrogen test was conducted on the lipid microsphere preparations of this invention in accordance to the method described in the appendix of the Chinese Pharmacopoeia 2010 edition. All lipid microsphere preparations of this invention passed the pyrogen test.
    • Experiment 6 Allergy Test
  • Method: Three groups of 8 guinea pigs were randomly separated based on their weight. Each of the guinea pigs from group 1 and group 2 was given 3 successive peritoneal injections of the biphenol lipid microsphere preparations at a dose of 0.5 ml/guinea pig every other day to induce sensitization. On day 14 and day 21 after the first peritoneal injection, guinea pigs from groups 1 and 2 were given intravenous injections of the biphenol lipid microsphere preparations at the toe at a dose of 1.0 ml/guinea pig so as to cause stimulation. For group 3, the guinea pigs were given 3 successive peritoneal injections of 20% egg white at a dose of 0.5 ml/guinea pig every other day to induce sensitization and, after 14 days, were given intravenous injection of egg white at the toe at a dose of 1.0 ml/guinea pig so as to cause stimulation. All three groups were observed for 15 minutes after injection to notice for allergic reactions.
  • Results: The two groups of guinea pigs injected with biphenol lipid microspheres which received the stimulation dose of same drug on day 14 and day 21 respectively did not show any allergic response. The guinea pigs in the positive control group had breathing difficulty and spasm within 2 minutes after injection before they died. The death of the guinea pigs were within 1˜3 minutes after injection.
  • Conclusion: The biphenol lipid microsphere preparation did not cause allergic reaction to guinea pigs under the current set of experimental conditions.
    • Experiment 7 Hemolysis Test
  • Method: 0.1 ml, 0.2 ml, 0.3 ml 0.4 ml and 0.5 ml of biphenol lipid microsphere preparations were separately added to 5 test tubes and diluted with 10% sucrose injection to 2.5 ml. 2.5 ml of 10% sucrose injection was added to a sixth test tube. 2.5 ml of distilled water was added to a seventh test tube (Control for complete hemolysis). 2.5 ml of 2% rabbit red blood cell suspension was added to each test tube and gently shaken before being placed in a 37° C. water bath. The hemolysis and coagulation in each test tube was recorded at 15 min, 30 min, 45 min, 1 h, 2 h, 3 h, and 4 h.
  • Results: The five test tubes with biphenol lipid microsphere preparations did not cause hemolysis or coagulation in 4 hours.
  • Conclusion: The biphenol lipid microsphere preparation did not cause hemolysis and coagulation under the current set of experimental conditions.
    • Experiment 8 Irritation Test
  • Method: Biphenol lipid microsphere preparations were intravenously injected at the left ear of 2 New Zealand white rabbits at a dose of 5 ml/kg while 10% sucrose injections were intravenously injected at the right ear at a dose of 5 ml/kg. The injections were given daily for a total of five days. The injection site was observed for any swelling or rashes since day 1. Within 24 hours after the last injection, the ears were removed and fixed in 10% formalin before being prepared for histopathological examination.
  • Results: No rashes or swelling was observed on both rabbit ears that were injected with biphenol lipid microsphere preparation daily for consecutive 5 days. Histopathologically, the epidermises of the rabbit ears appeared normal. No inflammatory cells or blood were exudating in the papillary layer and reticular layer. There were also no blood clots formed in the blood vessels and other structures also appeared normal.
  • Conclusion: The biphenol lipid microsphere preparation had no irritation effect on the veins of the rabbit ear.
  • The following animal model experiments characterized the anti-epileptic effects of the lipid microsphere preparation prepared in accordance to above description.
  • In this experiment, there were 5 groups of 20 Kunming mice each namely, model group, control group (CMC-NA-biphenol group), drug test group 1, drug test group 2 and drug test group 3.
    • Experiment 1 Anti-Epileptic Effect of Different Concentrations of Biphenol Lipid Microsphere Preparations on PTZ Induced Seizures in Mice
  • The mode of administration, type of drug and dose administered in each of the five groups are summarized in the following table. One hour after the drugs were administered, an intraperitoneal injection of PTZ (75 mg/kg) was used for inducing epileptic seizure. Results are summarized in the following table.
  • Mode of Dose Seizure Severity Efficacy
    Group Administration Type of Drug (mg/kg) 0 I II III IV V (≦III)
    Model Group Intravenous Non-loaded lipid 100 0 0 0 0 18 2  0%
    (n = 20) microspheres
    Control Group Gavage CMCNa- 100 0 0 0 2 18 0  10%
    (n = 20) biphenol
    Drug Test Intravenous Biphenol lipid 100 20 0 0 0 0 0 100%
    Group 1 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 50 20 0 0 0 0 0 100%
    Group 2 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 20 15 3 2 0 0 0 100%
    Group 3 (n = 20) microspheres
    Seizure severity of the animal models was evaluated based on the Racine Stages (Stage 0 No response Stage I Mouth or facial rhythmic movement Stage II Head nodding or tail flicking Stage III Clonus of a single limb Stage IV Clonus or rearing in multiple limbs Stage V Full scale clonic-tonic seizure
    • Experiment 2 Anti-Epileptic Effect of Different Concentrations of Biphenol Lipid Microsphere Preparations on Bicuculline Induced Seizures in Mice
  • The mode of administration, type of drug and dose administered in each of the five groups are summarized in the following table. One hour after the drugs were administered, a subdermal injection of Bic (2.7 mg/kg) was used for inducing epileptic seizure. Results are summarized in the following table.
  • Mode of Dose Seizure Severity Efficacy
    Group Administration Type of Drug (mg/kg) 0 I II III IV V (≦III)
    Model Group Intravenous Non-loaded lipid Equal 0 0 0 0 0 0  0%
    (n = 20) microspheres Volume
    Control Group Gavage CMCNa— 100 0 0 0 0 4 4  40%
    (n = 20) biphenol
    Drug Test Intravenous Biphenol lipid 100 20 0 0 0 0 0 100%
    Group 1 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 50 12 1 2 3 2 0 100%
    Group 2 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 20 10 2 3 4 1 0 100%
    Group 3 (n = 20) microspheres
    Evaluation of bicuculline based model: The death rate for this model is 100%, therefore surivival after drug administration would indicate efficacy.
    • Experiment 3 Anti-Epileptic Effect of Different Concentrations of Biphenol Lipid Microsphere Preparations on 3-Mercaptopropionic Acid Induced Seizures in Mice
  • The mode of administration, type of drug and dose administered in each of the five groups are summarized in the following table. One hour after the drugs were administered, a subdermal injection of 3-MP (60 mg/kg) was used for inducing epileptic seizure. Results are summarized in the following table.
  • Mode of Dose Seizure Severity Efficacy
    Group Administration Type of Drug (mg/kg) 0 I II III (≦III)
    Model Group Intravenous Non-loaded lipid Equal 0 0 0 20  0%
    (n = 20) microspheres Volume
    Control Group Gavage CMCNa— 100 1 1 3 15 25%
    (n = 20) biphenol
    Drug Test Intravenous Biphenol lipid 100 20 0 0 0 100% 
    Group 1 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 50 20 0 0 0 100% 
    Group 2 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 20 18 0 1 1 95%
    Group 3 (n = 20) microspheres
    Evaluation of 3-mercaptopropionic acid based model: Stage I Incubation Stage II Clonic Seizure Stage III Tonic Seizure
    • Experiment 4 Anti-Epileptic Effect of Different Concentrations of Biphenol Lipid Microsphere Preparations on Maximal Electroshock Induced Seizures in Mice
  • The mode of administration, type of drug and dose administered in each of the five groups are summarized in the following table. One hour after the drugs were administered, MES was used for inducing epileptic seizure. Results are summarized in the following table.
  • Mode of Dose Seizure Severity Efficacy
    Group Administration Type of Drug (mg/kg) No Seizure Seizure (≦III)
    Model Group Intravenous Non-loaded lipid Equal 0 20  0%
    (n = 20) microspheres Volume
    Control Group Gavage CMCNa— 100 2 18 10%
    (n = 20) biphenol
    Drug Test Intravenous Biphenol lipid 100 18 2 90%
    Group 1 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 50 15 5 75%
    Group 2 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 20 12 8 60%
    Group 3 (n = 20) microspheres
    Evaluation of maximal electroshock based model: Assessed based on whether the animal exhibited rigidity of all four limbs
    • Experiment 5 Anti-Epileptic Effect of Different Concentrations of Biphenol Lipid Microsphere Preparations on Penicillin Induced Seizures in Mice
  • The mode of administration, type of drug and dose administered in each of the five groups are summarized in the following table. One hour after the drugs were administered, an intraperitoneal injection of penicillin (6 million U/kg) was used for inducing epileptic seizure. Results are summarized in the following table.
  • Mode of Dose Seizure Severity Efficacy
    Group Administration Type of Drug (mg/kg) 0 I II III IV V (≦III)
    Model Group Intravenous Non-loaded lipid 100 0 0 0 0 2 18  0%
    (n = 20) microspheres
    Control Group Gavage CMCNa— 100 0 1 2 1 3 13  10%
    (n = 20) biphenol
    Drug Test Intravenous Biphenol lipid 100 18 2 0 0 0 0 100%
    Group 1( n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 50 18 1 1 0 0 0 100%
    Group 2 (n = 20) microspheres
    Drug Test Intravenous Biphenol lipid 20 15 2 0 1 1 1 100%
    Group 3 (n = 20) microspheres
    Seizure severity of the animal models was evaluated based on the Racine Stages (Stage 0 No response Stage I Mouth or facial rhythmic movement Stage II Head nodding or tail flicking Stage III Clonus of a single limb Stage IV Clonus or rearing in multiple limbs Stage V Full scale clonic-tonic seizure
  • Experimental results showed that the efficacy of biphenol lipid microsphere preparation improved several to dozens of times as compared to CMC-NA-biphenol.
  • It could be observed from the above results that the preparations of this invention are safe and reliable and do not induce any allergic, hemolytic or irritation effects. It therefore complies with the relevant requirements for clinically used drugs.
  • Although the above only selected the drug described in example 1 as the test drug, it should be noted that other embodiments of this invention also possess the same or similar beneficial effects.
  • The allergy test, hemolytic test and irritation test on the lipid microsphere preparations of this invention showed that the lipid microsphere preparations of this invention are highly stable and do not cause any allergic, hemolytic or irritation effects. It therefore complies with the relevant requirements for clinically used drugs.

Claims (3)

1-10. (canceled)
11. A 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparation for use in intravenous injections, wherein every 100 ml of said preparation comprises 0.1 to 0.3 weight % of 2,2′,6,6′-tetraisopropyl-4,4′-biphenol, 10 to 30 weight % of soybean oil, 1 to 1.5 weight % of injection-grade egg lecithin, 0.5 to 1 weight % of vitamin E, 0.01 to 1 weight % of sodium hydroxide, 0.1 to 2.5 weight % of glycerin, 0.01 to 1 weight % of EDTA, and the remaining being injection-grade water; and wherein the average particle size is 150 nm to 300 nm.
12. A method for preparing the 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparation of claim 1 for use in intravenous injections, comprising the steps of:
1) Dissolving appropriate amounts of injection-grade egg lecithin and vitamin E completely in injection-grade soybean oil under a nitrogen atmosphere in a 70° C. water bath before adding 2,2′,6,6′-tetraisopropyl-4,4′-biphenol, with heat and stirring for dissolution, to obtain an oil phase;
2) Dissolving appropriate amounts of glycerin and EDTA in injection-grade water, with stirring, to obtain an aqueous phase;
3) Adding said oil phase slowly to said aqueous phase while shearing under nitrogen at 10000 r for 5 minutes to obtain a preliminary emulsion, and adjusting the pH to around 8.0 with NaOH; and
4) Homogenizing said preliminary emulsion 5 to 8 times under a pressure of 800 to 900 bar before filtering with a microporous membrane filter, flushing with nitrogen, sealing and autoclaving at 115° C. to obtain said lipid microsphere preparation.
US14/374,220 2012-02-06 2012-03-07 2,2',6,6'-tetraisopropyl-4,4'-biphenol lipid microsphere preparations and preparation methods therefor Abandoned US20140370101A1 (en)

Applications Claiming Priority (3)

Application Number Priority Date Filing Date Title
CN2012100256112 2012-02-06
CN2012100256112A CN102525921B (en) 2012-02-06 2012-02-06 2,2',6,6'-tetraisopropyl-4,4'-bigeminy phenol lipid microsphere preparation and preparation method thereof
PCT/CN2012/072031 WO2013117022A1 (en) 2012-02-06 2012-03-07 2,2',6,6'-tetraisopropyl-4,4'-2-biphenol lipid microsphere preparation and preparation method therefor

Related Parent Applications (1)

Application Number Title Priority Date Filing Date
PCT/CN2012/072031 A-371-Of-International WO2013117022A1 (en) 2012-02-06 2012-03-07 2,2',6,6'-tetraisopropyl-4,4'-2-biphenol lipid microsphere preparation and preparation method therefor

Related Child Applications (1)

Application Number Title Priority Date Filing Date
US15/141,517 Continuation US10154967B2 (en) 2012-02-06 2016-04-28 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and preparation methods therefor

Publications (1)

Publication Number Publication Date
US20140370101A1 true US20140370101A1 (en) 2014-12-18

Family

ID=46334755

Family Applications (2)

Application Number Title Priority Date Filing Date
US14/374,220 Abandoned US20140370101A1 (en) 2012-02-06 2012-03-07 2,2',6,6'-tetraisopropyl-4,4'-biphenol lipid microsphere preparations and preparation methods therefor
US15/141,517 Active US10154967B2 (en) 2012-02-06 2016-04-28 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and preparation methods therefor

Family Applications After (1)

Application Number Title Priority Date Filing Date
US15/141,517 Active US10154967B2 (en) 2012-02-06 2016-04-28 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and preparation methods therefor

Country Status (6)

Country Link
US (2) US20140370101A1 (en)
EP (1) EP2813215B1 (en)
JP (1) JP5748926B2 (en)
CN (1) CN102525921B (en)
CA (1) CA2865777C (en)
WO (1) WO2013117022A1 (en)

Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20180185299A1 (en) * 2015-01-13 2018-07-05 Xi'an Libang Pharmaceutical Co., Ltd The use of diphenol in preparation of medicines for prevention and treatment of cerebral ischemia
US10154967B2 (en) 2012-02-06 2018-12-18 Xi'an Libang Pharmaceutical Co., Ltd 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and preparation methods therefor
US10329243B2 (en) * 2015-01-13 2019-06-25 Xi'an Libang Pharmaceutical Co., Ltd Biphenyl derivative and uses thereof

Families Citing this family (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN112336868A (en) * 2020-10-28 2021-02-09 西安力邦医美科技有限公司 Polyethylenimine matrine lipid microsphere antifungal preparation and application thereof

Citations (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5714520A (en) * 1994-03-22 1998-02-03 Zeneca Limited Propofol compostion containing edetate
US20020025337A1 (en) * 1995-07-20 2002-02-28 Lisbeth Illum Lipid vehicle drug delivery composition containing vitamin e
US6572884B1 (en) * 1999-07-28 2003-06-03 Daftary Gautam Vinod Parenteral Cisplatin emulsion
US20040137049A1 (en) * 2001-03-01 2004-07-15 Pai Srikanth Annappa Amphotericin b aqueous composition
US20060148776A1 (en) * 2003-03-13 2006-07-06 Conforma Therapeutics Corporation Drug formulations having long and medium chain triglycerides
US20070026058A1 (en) * 2004-05-11 2007-02-01 Lena Pereswetoff-Morath Method and composition for treating rhinitis
CN101804043A (en) * 2010-04-30 2010-08-18 西安力邦制药有限公司 Application of 2-phenylphenol and derivatives thereof to medicine for treating epilepsia

Family Cites Families (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
SE0001865D0 (en) * 2000-05-19 2000-05-19 Astrazeneca Ab Management of septic shock
US20040225022A1 (en) * 2003-05-09 2004-11-11 Desai Neil P. Propofol formulation containing reduced oil and surfactants
CN1478465A (en) * 2003-07-14 2004-03-03 丽 佟 Biphenyl diester liquid medicinal composition containing fat
WO2007052288A2 (en) * 2005-08-05 2007-05-10 Bharat Serums & Vaccines Ltd. Intravenous propofol emulsion compositions having preservative efficacy
WO2008023384A1 (en) * 2006-08-24 2008-02-28 Bharat Serums & Vaccines Ltd. Propofol emulsion compositions for intravenous administration
CN101940549B (en) * 2010-08-27 2012-04-25 北京中海康医药科技发展有限公司 Flurbiprofen axetil medium-chain and long-chain fat emulsion and preparation method thereof
CN102525921B (en) 2012-02-06 2013-08-07 西安力邦制药有限公司 2,2',6,6'-tetraisopropyl-4,4'-bigeminy phenol lipid microsphere preparation and preparation method thereof

Patent Citations (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5714520A (en) * 1994-03-22 1998-02-03 Zeneca Limited Propofol compostion containing edetate
US20020025337A1 (en) * 1995-07-20 2002-02-28 Lisbeth Illum Lipid vehicle drug delivery composition containing vitamin e
US6572884B1 (en) * 1999-07-28 2003-06-03 Daftary Gautam Vinod Parenteral Cisplatin emulsion
US20040137049A1 (en) * 2001-03-01 2004-07-15 Pai Srikanth Annappa Amphotericin b aqueous composition
US20060148776A1 (en) * 2003-03-13 2006-07-06 Conforma Therapeutics Corporation Drug formulations having long and medium chain triglycerides
US20070026058A1 (en) * 2004-05-11 2007-02-01 Lena Pereswetoff-Morath Method and composition for treating rhinitis
CN101804043A (en) * 2010-04-30 2010-08-18 西安力邦制药有限公司 Application of 2-phenylphenol and derivatives thereof to medicine for treating epilepsia

Non-Patent Citations (6)

* Cited by examiner, † Cited by third party
Title
Barros et al. (2007). "Effects of the vitamin E in catalase activities in hippocampus after status epilepticus induced by pilocarpine in Wistar rats." Neuroscience Letters, 416: 227-230. *
Ogata et al. (2005). "Mechanism of Action of Dipropofol and Synergistic Action with Other Antibacterial Agents in Vitro." Biol. Pharm. Bull, 28(9): 1773-1775. *
Ogata et al. (2007). "Solubilization of Dipropofol, an Antibacterial Agent, Using Saccharide and Ascorbic Acid." Biol. Pharm. Bull, 30(8): 1565-1568. *
Ogata et al. (2007). "Solubilization of Dipropofol, and Antibacterial Agent, Using Saccharide and Ascorbic Acid." Biol. Pharm. Bull, 30(8): 1565-1568. *
Ogunmekan et al. (1989). "A Randomized, Double-Blind, Placebo-Controlled, Clinical Trial of D-a-Tocopheryl Acetate (Vitamin E), as Add-On Therapy, for Epilepsy in Children." Epilepsia, 30(1): 84-89. *
Ogunmekan et al. (1989). "A Randomized, Double-Blind, Placebo-Controlled, Clinical Trial of D-a-Tocopheryl Acetate (Vitamin E), as Add-On Therapy, for Epilepsy in Children." Epilepsia, 30(1):84-89. *

Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US10154967B2 (en) 2012-02-06 2018-12-18 Xi'an Libang Pharmaceutical Co., Ltd 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and preparation methods therefor
US20180185299A1 (en) * 2015-01-13 2018-07-05 Xi'an Libang Pharmaceutical Co., Ltd The use of diphenol in preparation of medicines for prevention and treatment of cerebral ischemia
US10329243B2 (en) * 2015-01-13 2019-06-25 Xi'an Libang Pharmaceutical Co., Ltd Biphenyl derivative and uses thereof

Also Published As

Publication number Publication date
EP2813215A4 (en) 2015-07-08
EP2813215A1 (en) 2014-12-17
EP2813215B1 (en) 2016-07-13
CN102525921A (en) 2012-07-04
JP5748926B2 (en) 2015-07-15
US20160235684A1 (en) 2016-08-18
WO2013117022A1 (en) 2013-08-15
CA2865777C (en) 2015-09-22
CN102525921B (en) 2013-08-07
CA2865777A1 (en) 2013-08-15
JP2015506378A (en) 2015-03-02
US10154967B2 (en) 2018-12-18

Similar Documents

Publication Publication Date Title
US20220280446A1 (en) Stable cannabinoid formulations
US10154967B2 (en) 2,2′,6,6′-tetraisopropyl-4,4′-biphenol lipid microsphere preparations and preparation methods therefor
KR102465046B1 (en) A composition comprising 5-cholestene-3, 25-diol, 3-sulfate (25HC3S) or a pharmaceutically acceptable salt thereof, and at least one cyclic oligosaccharide
JP2003535884A (en) Improved injectable dispersion of propofol
KR102268710B1 (en) Aqueous suspension containing nanoparticles of glucocorticosteroid
CN107970208B (en) Butylphthalide injection and preparation method thereof
AU2016371598A1 (en) Method for preventing and/or treating aging-associated cognitive impairment and neuroinflammation
JP2018503637A (en) Biphenyl derivatives and uses thereof
EP3329940A1 (en) Non-irritant ophthalmic composition containing cyclosporin, and convenient preparation method
CN112912066B (en) Nimodipine injection composition and preparation method thereof
CN115804771A (en) Lipid drug delivery system with long-acting sustained release effect and preparation method thereof
CN100502850C (en) Medicinal composition of total capsicine compounds and beta-cyclodextrin or derivative of beta-cyclodextrin
CN107405503A (en) Ellagic acid dihydrate adjusts the purposes of blood sugar level in pharmaceutical preparation
US20140329774A1 (en) Injectable composition containing phosphatidylcholine devoid of sodium deoxycholate and preparing method thereof
KR20150112975A (en) Stable pharmaceutical composition of clopidogrel free base for oral and parenteral delivery
US9161981B2 (en) Non-aqueous oily injectable formulation exhibiting preservative efficacy
EP4176869A1 (en) Preparation and use of cannabis nano-formulation
US20160228387A1 (en) Solubilized formulation of coq10 for use in treatment of parkinson's disease
KR20170099911A (en) Injectable formulations of paracetamol
CN116209427A (en) Formulations for delivery of lipophilic active ingredients
BR102016005548B1 (en) THERMOREVERSIBLE MICELLAR FORMULATION CONTAINING QUERCETIN AND VILDAGLIPTIN FOR ORAL ADMINISTRATION IN TYPE 1 DIABETES

Legal Events

Date Code Title Description
AS Assignment

Owner name: XI'AN LIBANG PHARMACEUTICAL CO., LTD, CHINA

Free format text: ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNORS:WANG, RUTAO;CHEN, TAO;GUO, SHUPAN;AND OTHERS;REEL/FRAME:033550/0280

Effective date: 20140815

STCB Information on status: application discontinuation

Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION