Formulations and methods for controlling the reproductive cycle and ovulation
10898432 · 2021-01-26
Assignee
- Proinvet Innovations S.A. (Ciudad Autonoma de Buenos Aires, AR)
- Proinvet Innovations LLC (Dover, DE, US)
Inventors
- Juan Andrés Colman (Buenos Aires, AR)
- Daniel Roberto Sammartino (Ciudad Autónoma de Buenos Aires, AR)
Cpc classification
A61K47/34
HUMAN NECESSITIES
A61K31/565
HUMAN NECESSITIES
A61K9/06
HUMAN NECESSITIES
A61K47/10
HUMAN NECESSITIES
A61K9/0024
HUMAN NECESSITIES
A61K31/568
HUMAN NECESSITIES
A61K47/44
HUMAN NECESSITIES
A61K9/0019
HUMAN NECESSITIES
A61K31/557
HUMAN NECESSITIES
A61K31/57
HUMAN NECESSITIES
A61K47/14
HUMAN NECESSITIES
A61K38/09
HUMAN NECESSITIES
International classification
A61K9/00
HUMAN NECESSITIES
A61K31/568
HUMAN NECESSITIES
A61P15/08
HUMAN NECESSITIES
A61K9/16
HUMAN NECESSITIES
A61K31/57
HUMAN NECESSITIES
A61K9/06
HUMAN NECESSITIES
A61K31/565
HUMAN NECESSITIES
A61K47/44
HUMAN NECESSITIES
A61K47/34
HUMAN NECESSITIES
A61K47/14
HUMAN NECESSITIES
A61K47/10
HUMAN NECESSITIES
A61K38/09
HUMAN NECESSITIES
Abstract
Hormone formulations, dosage units including the hormone formulations, and methods of use relate to a controlled release formulation, which includes hormones, e.g., progesterone. Formulations and methods are for controlling the reproductive cycle and/or ovulation of a female mammal, for example, to promote ovulation in a female mammal or synchronizing the ovulation or heat/estrus of a group of female mammals. In addition, formulations are for increasing the likelihood that a female mammal becomes pregnant, for example, after insemination or embryo transference. In addition, formulations are for reducing the anestrous period in a female mammal.
Claims
1. A controlled release injectable formulation, comprising one or more hormones comprising from about 1 mg/mL to about 250 mg/mL progesterone or an analogue or a salt thereof; one or more pharmaceutically acceptable organic solvents comprising about 1000 mg/mL or less benzyl alcohol, about 60 mg/mL or less benzyl benzoate, and about 300 mg/mL or less ethanol; one or more pharmaceutically acceptable fatty acids comprising about 60 mg/mL or less stearic acid; one or more pharmaceutically acceptable surfactants comprising about 120 mg/mL or less ethoxylated castor oil at 40 moles of ethylene oxide; one or more pharmaceutically acceptable gel forming agents comprising about 120 mg/mL or less poly(ethylene glycol)-block-poly(propylene glycol)-block-poly(ethylene glycol); and about 1000 mg/mL or less water; wherein a portion of said one or more hormones is dissolved in a mixture comprising said one or more pharmaceutically acceptable organic solvents to form a free portion, and a portion of said one or more hormones is enclosed by said one or more pharmaceutically acceptable fatty acids to form an enclosed portion, wherein said free and enclosed portions are included in a matrix, said matrix comprising said one or more pharmaceutically acceptable gel forming agents and said one or more pharmaceutically acceptable surfactants, and wherein the formulation is suitable for administration by an injection method selected from the group consisting of a subcutaneous, intravenous, intraparenteral, intramuscular and intradermal injection.
2. The controlled release injectable formulation of claim 1, further comprising a pharmaceutically acceptable oily carrier other than the said one or more pharmaceutically acceptable fatty acids, wherein the portion of said one or more hormones is dissolved in a mixture comprising said one or more pharmaceutically acceptable organic solvents and said pharmaceutically acceptable oily carrier.
3. The controlled release injectable formulation of claim 1, wherein the matrix further comprises one or more pharmaceutically acceptable structure forming agents.
4. The controlled release injectable formulation of claim 2, wherein the matrix further comprises one or more pharmaceutically acceptable structure forming agents.
5. The controlled release injectable formulation of claim 1, wherein the formulation is configured to increase the likelihood that a female mammal becomes pregnant, to synchronize the ovulation of a group of female mammals, to reduce the anestrous period in a female mammal, or combinations thereof.
6. The formulation of claim 2, wherein said pharmaceutically acceptable oily carrier is selected from the group consisting of flax oil, sesame oil, refined sesame oil, castor oil, palmitic acid, soybean oil, ethoxylated soybean oil, sunflower oil, corn oil, coconut oil, olive oil, almond oil, cotton oil, and combinations thereof.
7. The formulation of claim 6, wherein that said pharmaceutically acceptable oily carrier comprises refined sesame oil.
8. The formulation of claim 4, wherein said one or more pharmaceutically acceptable structure forming agents are selected from the group consisting of cellulose, a cellulose derivative, microcrystalline cellulose, ethylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, hydroxyethylpropylcellulose, carboxymethylcellulose, guar gum, gum arabic, xanthan gum, chitosan, alginate, gelatin, carbomer homopolymer or poly(acrylic acid) or 2-propenoic acid homopolymer, sodium starch glycolate, sodium corscarmelosa, alginic acid, pectin, and combinations thereof.
9. The formulation of claim 8, wherein said one or more pharmaceutically acceptable structure forming agents are selected from the group consisting of hydroxyethyl cellulose, gum arabic, xanthan gum and combinations thereof.
10. The formulation of claim 8, wherein said one or more pharmaceutically acceptable structure forming agents comprise hydroxyethyl cellulose.
11. The formulation of claim 1, further comprising about 50 mg/mL or less hydroxyethyl cellulose.
12. The formulation of claim 1, further comprising about 100 mg/mL or less refined sesame oil.
13. The formulation of claim 1, wherein the formulation has a pH from about 4.0 to about 8.0.
14. The formulation of claim 1, further comprising a pharmaceutically acceptable antioxidant agent selected from the group consisting of Vitamin E, d-a-tocopherol propylene glycol 1000 succinate, Butylhydroxytoluene (BHT), Butylhydroxyanisol (BHA), sodium bisulfite, ascorbic acid, ascorbyl palmitate, Vitamin A, propyl gallate, monothioglycerol, sodium sulfoxylate formal, and combinations thereof.
15. The formulation of claim 1, wherein the formulation is suitable for administration by intramuscular injection.
16. The formulation of claim 1, wherein upon administration to a female mammal there is a sustained blood concentration of said one or more hormones followed by a decrease in blood hormone concentration.
17. The formulation of claim 16, wherein the decrease in blood concentration of the hormone takes place from about 5 to about 10 days after administration of the formulation.
18. The formulation of claim 17, wherein the decrease in blood concentration of the hormone takes place from about 6 to about 8 days after administration of the formulation.
19. The formulation of claim 1, wherein from 1 to 20 mL of said formulation forms a dosage unit.
20. A prefilled syringe comprising a dosage unit according to claim 19.
21. A kit comprising a dosage unit according to claim 19, together with instructions for use.
22. A process for preparing the formulation according to claim 1, comprising: i) preparing a first solution comprising said one or more pharmaceutically acceptable surfactants and water; ii) preparing a second solution comprising said one or more hormones, said pharmaceutically acceptable fatty acid, said one or more pharmaceutically acceptable organic solvents, said one or more pharmaceutically acceptable gel forming agents and said water, wherein said second solution is prepared by combining mixtures I and II, wherein a) mixture I comprises said one or more hormones, said one or more pharmaceutically acceptable fatty acids and said one or more pharmaceutically acceptable organic solvents; and b) mixture II comprises said one or more pharmaceutically acceptable gel forming agents and water; iii) preparing a third solution comprising said one or more hormones and said one or more pharmaceutically acceptable organic solvents; iv) combining said first solution with said second solution; and v) incorporating into the mixture obtained in step iv) said third solution.
23. The process of claim 22, wherein the third solution further comprises a pharmaceutically acceptable oily carrier.
24. The process of claim 22, further comprising preparing a fourth solution including one or more pharmaceutically acceptable structure forming agents and water.
25. The process of claim 24, comprising adding to the mixture obtained in step v) said fourth solution.
26. A method for controlling the reproductive cycle and ovulation of a female mammal, increasing the likelihood that a female mammal becomes pregnant, synchronizing the ovulation of a group of female mammals, and/or reducing the anestrous period in a female mammal comprising administering the formulation according to claim 1 to said female mammal.
27. The method of claim 26, wherein said female mammal is selected from cattle, pigs, goats, sheep, horses or camels.
28. The method of claim 26, wherein said female mammal is a reproductively mature bovine animal.
29. The method of claim 26, wherein said formulation is administered to said female animal before insemination.
30. The method of claim 29, wherein the insemination is carried out from about 9 to about 11 days after the administration of said formulation.
31. The method of claim 26, further comprising administration of estradiol benzoate, wherein the administration of estradiol benzoate is performed the same day as the administration of said formulation.
32. The method of claim 26, further comprising administration of prostaglandin, an analogue or a salt thereof, wherein the administration of prostaglandin, an analog or a salt thereof is carried out from about 7 to about 8 days after administering said formulation, two days before administering said formulation, or both two days before administering said formulation and about 7 to about 8 days after administering said formulation.
33. The method of claim 29, further comprising administering the gonadotropin releasing hormone (GnRH), an analogue or a salt thereof, wherein the administration of the gonadotropin releasing hormone (GnRH), an analogue or a salt thereof is carried out on the same day as the insemination or a day before the insemination.
34. The method of claim 26, further comprising administering estradiol cypionate, wherein the administration of estradiol cypionate is carried out from about 7 to about 8 days after the administration of said formulation.
35. The formulation of claim 2, further comprising a pharmaceutically acceptable antioxidant agent selected from the group consisting of Vitamin E, d-a-tocopherol propylene glycol 1000 succinate, Butylhydroxytoluene (BHT), Butylhydroxyanisol (BHA), sodium bisulfite, ascorbic acid, ascorbyl palmitate, Vitamin A, propyl gallate, monothioglycerol, sodium sulfoxylate formal, and combinations thereof.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
(1)
(2)
DETAILED DESCRIPTION OF EMBODIMENTS OF THE DISCLOSURE
(3) Progestagens are hormones that have progestational activity. In the present application, the term progestagen includes progesterones and all natural or synthetic analogs (sometimes referred to as progestins), medroxyprogesterone acetate (medrysone), norethindrone, norethindrone acetate, megestrol acetate, 17--hydroxyprogesterone caproate, norgestrel, and derivatives thereof.
(4) The term pharmaceutically acceptable as used in the present application, means that the component is useful to prepare a pharmaceutical composition that generally is non-toxic and does not have undesirable biological effects and includes those accepted for veterinary use and/or pharmaceutical use in humans.
(5) The term surfactant as used in the present application refers to a compound that reduces the surface tension of the medium in which it is located.
(6) The term carrier as used in the present application means an inert medium in which there is an active agent, which facilitates its administration.
(7) The term pharmaceutically acceptable oily carrier as used in the present application means any conventional vegetal or synthetic oil or a mixture thereof, which are acceptable for veterinary use or for pharmaceutical use in humans.
(8) Prostaglandins are a group of substances of lipidic nature derived from 20-carbon fatty acids containing a cyclopentane ring and constitute a family of cellular mediators with diverse effects. In the present application, the term prostaglandin may refer to any existing natural or synthetic prostaglandin or any functional prostaglandin analogue, such as prostaglandin F2 or prostaglandin derivatives such as cloprostenol or a salt thereof
(9) The term dosage unit as used in the present application refers to any discrete physical unit suitable as unitary dosage for subjects to be treated; each of said units comprising a predetermined amount of active compound calculated to produce the desired therapeutic effect associated with the associated excipient or carrier.
(10) The term set of elements or kit as used in the present application defines a package, assembly or container including one or more components of an embodiment the present disclosure and/or any other component related to an embodiment of the disclosure. It may also include instructions for use of such components.
(11) The term structure forming agent as used in the present application refers to any excipient maintaining the physical stability of a formulation preventing the separation of its phases. Examples of structure forming agents of some embodiments of the present disclosure are, without limitation, cellulose, a cellulose derivative, microcrystalline cellulose, ethylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, hydroxyethylpropylcellulose, carboxymethylcellulose, guar gum, gum arabic, xanthan gum, chitosan, alginate, gelatin, carbopol, Carbopol 71G NF, Carbopol 971P NF, Carbopol 974P NF, Carbopol ETD 2020 NF, Carbopol 5984 ETD, Carbopol Ultrez 10, sodium starch glycolate, sodium corscarmelosa, alginic acid, pectin and combinations thereof.
(12) The term microparticle as used in the present application refers to particles having a size of about 1 m to 1000 m. Said particles can include microcapsules (reservoir system) and microcrystals. In the case of microcapsules, the active substance is enclosed by a polymer or coating, whereas in the case of microcrystals the active component may be in a defined form or in an amorphous form in a non-compatible solvent.
(13) The term microcapsule as used in the present application refers to a thin layer or coating of an amphipathic agent (comprising a hydrophobic portion and a hydrophilic portion, for example, a fatty acid), which may enclose an active substance both as a solid or dissolved in a solvent. Its size may vary between 1 and 500 microns and its aim may be, for example, to release the active ingredient into the surrounding environment in a slow or sustained manner over time.
(14) The term insemination as used in the present application refers to the introduction of sperm into a female reproductive system.
(15) The term artificial insemination as used in the present application refers to any reproductive technique consisting of depositing the sperm of a male inside the female reproductive system in order to fertilize it.
(16) The term fixed-time artificial insemination as used in the present application refers to the artificial insemination of one or more animals at the same fixed-time without needing to detect the heat of said animal.
(17) The term artificial insemination at detected heat detection as used in the present application refers to the artificial insemination of one or more animals where first the heat manifested by the animal is detected and then the animal is inseminated.
(18) Gonadotropin releasing hormone (GnRH) is a hormone released by the hypothalamus whose center of action is the pituitary gland. It is a decapeptide that stimulates the release of gonadotrophin (luteinizing hormone, LH, and follicle stimulating hormone, FSH) from the anterior pituitary. In the present disclosure, when we refer to GnRH, we intend to include all existing natural or synthetic functional analogs and salts, for example, buserelin or buserelin acetate.
(19) The term livestock as used in the present application refers to a group of animals that may be domesticated by humans for its exploitation and production.
(20) The term cattle as used in the present application refers to a group of cows, bulls and bullocks that may be domesticated by humans for its exploitation and production.
(21) The reproductive cycle of a female mammal is a number of physiological events occurring in the ovary at intervals of cyclic and regular time.
(22) The terms heat and estrous as used in the present application refer to the sexual receptivity behavior of an animal.
(23) The term anestrous as used in the present application refers to the state of sexual inactivity in female animals during which they exhibit no sexual receptivity behavior. Causes of anestrous include, for example, pregnancy, presence of offspring, season, stress, and pathologies, among others.
(24) Equine Chorionic Gonadotropin hormone (eCG) is a glycoprotein produced by the endometrial cups of a pregnant mare with FSH (follicle stimulating hormone) function. In the present disclosure, with reference to an eCG, we intend to include all existing natural or synthetic functional analogs and salts.
(25) The term pharmaceutically acceptable gel forming agent as used in the present application refers to any compound capable of gelling in a certain condition, which is acceptable for veterinary use or for pharmaceutical use in humans. Examples can include poloxamers, which are nonionic tri-block copolymer compounds of a central hydrophobic chain of polyoxypropylene flanked by two hydrophilic polyoxyethylene chains. Some known trademarks of polymers are Synperonics, Pluronics, and Kolliphor. As the lengths of the polymer blocks may vary, there are many poloxamers with different properties. The term poloxamer followed by three digits gives information, where the first two digits multiplied by 100 are the approximate molecular mass of the polyoxypropylene core and the last digit multiplied by 10 is the percentage of polyoxyethylene. For example, Poloxamer P407, means Poloxamer with a polyoxypropylene molecular mass of 4000 g/mol and 70% of polyoxyethylene. Kolliphor P407, for example, is a commercial form of Poloxamer P407.
(26) A first aspect of an embodiment of the present disclosure is to provide formulations for controlling the reproductive cycle and/or ovulation in a female mammal. For example, the formulations of the present disclosure can be used to reduce the anestrous period, promote ovulation in a female mammal and/or synchronizing the ovulation of a group of female mammals. In addition, they can be used to increase the likelihood that a female mammal gets pregnant, for example, after insemination or embryo transference. In an embodiment of this disclosure, the formulation comprises i) said one or more hormones; ii) said one or more pharmaceutically acceptable organic solvents; iii) optionally, said pharmaceutically acceptable oily carrier; iv) said one or more pharmaceutically acceptable fatty acids; v) optionally, said one or more pharmaceutically acceptable structure forming agents; vi) said one or more pharmaceutically acceptable surfactants; vii) said one or more pharmaceutically acceptable gel forming agents; and viii) water.
(27) In an embodiment of the present disclosure, the formulations may comprise one or more natural or synthetic progestins, for example progesterone (P4), or an analogue or a salt or combinations of said hormone. In other embodiments of the present disclosure, the formulations may also comprise other hormones such as, for example, an estrogen, estradiol benzoate, estradiol cypionate, d-cloprostenol sodium, DL cloprostenol sodium, buserelin acetate. In another embodiment of the present disclosure, the formulation comprises progesterone or a salt or an analogue of said hormone. The progesterone or analogue or a salt thereof may comprise, for example, progesterone of natural or synthetic origin. Further, the progesterone may comprise BP grade (British Pharmacopoeia) or USP grade (US Pharmacopoeia) progesterone or any other commercial analogue.
(28) In an embodiment of the present disclosure, said one or more pharmaceutically acceptable organic solvents may comprise, for example, ethanol, benzyl alcohol, benzyl benzoate, glycerol, glycerol formal, ethyl oleate, PEG400, propylene glycol, dimethylsulfoxide (DMSO), N-methylpyrrolidone, Miglyol, Miglyol 808, Miglyol 810, Miglyol 812, Miglyol 829, Miglyol 8108, Dynacetin 660, Softisan 649, Imwitor491, Imwitor 900 K, Imwitor 900 P, Imwitor 960 K, Imwitor 642, Imwitor 742, Imwitor 928, Imwitor 988, Imwitor 948, Softigen 701 or any other similar, or combinations thereof. In another embodiment of the present disclosure, the formulation comprises ethanol, benzyl alcohol, benzyl benzoate or a combination thereof, and even more preferably it comprises ethanol, benzyl alcohol and benzyl benzoate.
(29) In an embodiment of the present disclosure, said optional pharmaceutically acceptable oily carrier may comprise, for example, flax oil, sesame oil, refined sesame oil, castor oil, palmitic acid, soybean oil, ethoxylated soybean oil, sunflower oil, corn oil, coconut oil, olive oil, almond oil, cotton oil, or combinations thereof. In another embodiment of the present disclosure, the formulation comprises sesame oil, preferably, refined sesame oil.
(30) In an embodiment of the present disclosure, said one or more pharmaceutically acceptable fatty acids may comprise, for example, fatty acids of from 14 to 22 carbon atoms, and may be saturated or partially insaturated, but preferably saturated, fatty acids. In another embodiment, said one or more pharmaceutically acceptable fatty acids may comprise, for example, stearic acid, arachidonic acid, palmitic acid, miristic acid, oleic acid, linoleic acid, linolenic acid, arachidic acid, erucic acid or combinations thereof. In yet another embodiment, said one or more pharmaceutically acceptable fatty acids comprise stearic acid.
(31) In an embodiment of the present disclosure, said optional one or more pharmaceutically acceptable structure forming agents may comprise, for example, cellulose or its derivatives, for example, microcrystalline cellulose, ethylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, hydroxyethylpropylcellulose, carboxymethylcellulose, guar gum, gum arabic, xanthan gum, chitosan, alginate, gelatin, Carbopol, Carbopol 71G NF, Carbopol 971P NF, Carbopol 974P NF, Carbopol ETD 2020 NF, Carbopol 5984 ETD, Carbopol Ultrez 10, sodium starch glycolate, sodium corscarmelosa, alginic acid, pectin or combinations thereof. In another embodiment of the present disclosure, the formulation comprises hydroxyethyl cellulose. In yet another embodiment of the present disclosure, the formulation comprises hydroxyethyl cellulose, gum arabic and xanthan gum.
(32) In an embodiment of the present disclosure, said one or more pharmaceutically acceptable surfactants may comprise, for example, castor oil, for example, hydrogenated castor oil, ethoxylated castor oil, ethoxylated castor oil of from 15 to 60 moles of ethylene oxide, for example, ethoxylated castor oil at 40 moles of ethylene oxide, ethoxylated lauric alcohol of from 7 to 10 moles, Cremophor RH 40, Cremophor RH 60, Cremophor CO 455, Kolliphor EL, Lipocol oxo 650, Lipocol oxo 600, Solutol HS 15, Emulgin B1 PH, Lanette 20 PH, Lanette N PH, Polysorbate, Polysorbate 20 PH, Polysorbate 60 PH, Polysorbate 80 PH, ethoxylated fatty alcohols (of from 6 to 30 moles of ethylene oxide) derived from Capri alcohol, decyl alcohol, lauryl alcohol, isotridecyl alcohol, myristyl alcohol, ethyl alcohol, palmoleyl, stearyl, oleyl, elaidyl, petroselinyl, linolyl alcohol, linolenic, elaeostearyl alcohol, eicosyl, arachyl, gadoleyl, behenyl alcohol, erucyl alcohol, brassidyl or combinations thereof. In another embodiment, the formulation comprises castor oil, preferably, ethoxylated castor oil at 40 moles of ethylene oxide.
(33) In an embodiment of the present disclosure, said one or more pharmaceutically acceptable gel forming agents may comprise, for example, sucrose acetate isobutyrate (SAIB), oxyethylenated and propoxyethylenated block copolymers, Pluronic F 127, Poloxamer, for example, Poloxamer P407, Kolliphor P188, Kolliphor P237, Kolliphor P338, Kolliphor P407, maleic acid or anhydride and methyl vinyl ether copolymer, modified acrilic polymers, PEG 3000, Macrogol 4000, Macrogol 6000, Poloxamine or combinations thereof. In another embodiment, the formulation comprises a thermo sensitive gel forming agent, preferably, Poloxamer P407 (for example, Kolliphor P407).
(34) In another embodiment of the present disclosure, the formulation comprises: a) progesterone or an analogue or a salt thereof; b) benzyl alcohol; c) benzyl benzoate; d) ethanol; e) stearic acid; f) hydroxyethylcellulose; g) ethoxylated castor oil, at 40 moles of ethylene oxide; h) Poloxamer P407; i) refined sesame oil; and j) water.
(35) In another embodiment of the present disclosure, the formulation comprises: a) progesterone or an analogue or a salt thereof; b) benzyl alcohol; c) benzyl benzoate; d) ethanol; e) stearic acid; f) hydroxyethylcellulose; g) ethoxylated castor oil, at 40 moles of ethylene oxide; h) Poloxamer P407; and i) water.
(36) In another embodiment of the present disclosure, the formulation comprises: a) progesterone or an analogue or a salt thereof; b) benzyl alcohol; c) benzyl benzoate; d) ethanol; e) stearic acid; f) ethoxylated castor oil, at 40 moles of ethylene oxide; g) Poloxamer P407; h) refined sesame oil; and i) water.
(37) In another embodiment of this disclosure, the formulations are controlled release formulations, wherein a portion of said one or more hormones is dissolved in a mixture comprising said one or more pharmaceutically acceptable organic solvents and, optionally, said pharmaceutically acceptable oily carrier to form a free portion; and a portion of said one or more hormones is enclosed by said one or more pharmaceutically acceptable fatty acids to form a enclosed portion. Said free and enclosed portions of said one or more hormones may be comprised in a matrix comprising: i) optionally, said one or more pharmaceutically acceptable structure forming agents, ii) said one or more pharmaceutically acceptable gel forming agents and iii) said one or more pharmaceutically acceptable surfactants.
(38) In another embodiment of this disclosure, the controlled release formulation may comprise:
(39) 1) one or more natural or synthetic progestagens or salts thereof, preferably progesterone, dissolved in a mixture of i) said one or more pharmaceutically acceptable organic solvents, preferably ethanol, benzyl alcohol and benzyl benzoate, and ii) said pharmaceutically acceptable oily carrier, preferably refined sesame oil;
(40) 2) one or more natural or synthetic progestagens or salts thereof, preferably progesterone, forming microcapsules or microparticles enclosed by said one or more pharmaceutically acceptable fatty acid, preferably stearic acid; and
(41) 3) a matrix which includes said components 1) and 2), wherein said matrix comprises i) said one or more pharmaceutically acceptable structure forming agents, preferably hydroxyethylcellulose; ii) said one or more pharmaceutically acceptable gel forming agents, preferably Poloxamer P407; and iii) said one or more pharmaceutically acceptable surfactants, preferably ethoxylated castor oil, at 40 moles of ethylene oxide.
(42) The controlled release formulation of an embodiment of this disclosure allows a controlled release of one or more hormones, for example, progesterone, into the bloodstream of a female mammal after its administration. First, there is a sustained blood concentration of said one or more hormones followed by a decrease in hormone concentration. For example, the decrease in blood concentration of the hormone may take place from about 5 to about 10 days after administration, and preferably from about 6 to 8 days after administration of the formulation
(43) Hormone concentrations in the blood and release times after administration of the formulation of an embodiment of this disclosure may vary depending on the characteristics of the animal to which the formulation is administered, the route by which the formulation is applied, or various other factors.
(44) The formulations of an embodiment of this disclosure may optionally comprise a protective agent, for example, a pharmaceutically acceptable antioxidant agent. Said pharmaceutically acceptable antioxidant may comprise, for example, Vitamin E, Vitamin E TGPS (d--tocopherol propylene glycol 1000 succinate), Kolliphor TGPS, Butylated hydroxytoluene (BHT), butylated hydroxyanisole (BHA), sodium bisulphite, ascorbic acid, ascorbyl palmitate, Vitamin A, propyl gallate, monothioglycerol, sodium sulfoxilatoformal, or combinations thereof.
(45) The water in the formulations of an embodiment of this disclosure may be replaced by any other liquid or aqueous solution, for example, a saline solution. The water in the formulations of an embodiment of this disclosure may be, for example, water or any acceptable solution or aqueous liquid for injections.
(46) The formulations of an embodiment of this disclosure described above may comprise progesterone or an analogue or a salt thereof, at a concentration of from about 1 mg/mL to about 250 mg/mL, preferably from about 10 mg/mL to about 200 mg/mL, preferably from about 20 mg/mL to about 100 mg/mL, preferably from about 30 mg/mL to about 70 mg/mL, preferably from about 40 mg/mL to about 60 mg/mL, and more preferably about 50 mg/mL.
(47) The formulations of an embodiment of this disclosure may also comprise benzyl alcohol at a concentration of up to about 1000 mg/mL, or from about 5 mg/mL to about 500 mg/mL, or from about 10 mg/mL to about 250 mg/mL, or from about 20 mg/mL to about 150 mg/mL, or from about 30 mg/mL to about 100 mg/mL, or from about 40 mg/mL to about 60 mg/mL, and preferably about 40 mg/mL.
(48) The formulations of an embodiment of this disclosure may also comprise benzyl benzoate at a concentration of up to about 60 mg/mL, or from about 1 mg/mL to about 40 mg/mL, or from about 10 mg/mL to about 30 mg/mL, and preferably about 20 mg/mL.
(49) The formulations of an embodiment of this disclosure may also comprise ethanol at a concentration of up to about 300 mg/mL, or from about 10 mg/mL to about 250 mg/mL, or from about 50 mg/mL to about 200 mg/mL, or from about 100 mg/mL and about 150 mg/mL preferably about 120 mg/mL.
(50) The formulations of an embodiment of this disclosure may also comprise stearic acid at a concentration of up to about 60 mg/mL, or from about 1 mg/mL to about 40 mg/mL, or from about 10 mg/mL to about 30 mg/mL, preferably about 20 mg/mL.
(51) The formulations of an embodiment of this disclosure may also comprise, optionally, hydroxyethylcellulose at a concentration of up to about 50 mg/mL, or up to about 40 mg/mL or up to about 30 mg/mL, or up to about 20 mg/mL or up to about 10 mg/mL, or from about 2 mg/mL to about 8 mg/mL, preferably about 4 mg/mL.
(52) The formulations of an embodiment of this disclosure may also comprise ethoxylated castor oil, at 40 moles of ethylene oxide at a concentration of up to about 120 mg/mL, or from about 10 mg/mL to about 120 mg/mL, or from about 20 mg/mL to about 80 mg/mL, or from about 40 mg/mL to about 70 mg/mL, preferably about 100 mg/mL.
(53) The formulations of an embodiment of this disclosure may also comprise Poloxamer P407 (for example, Kolliphor P407) at a concentration of up to about 120 mg/mL, or from about 10 mg/mL to about 100 mg/mL, or from about 50 mg/mL to about 90 mg/mL, or preferably or from about 50 mg/mL to about 90 mg/mL, preferably about 70 mg/mL.
(54) The formulations of an embodiment of this disclosure may also comprise, optionally, refined sesame oil at a concentration of up to about 100 mg/mL, or from about 5 mg/mL to about 70 mg/mL, or from about 10 mg/mL to about 30 mg/mL, preferably about 20 mg/mL.
(55) The formulations of an embodiment of this disclosure may also comprise water in the formulation in an amount of up to about 1000 mg/mL, or from about 100 mg/mL to about 900 mg/mL, or from about 200 mg/mL to about 800 mg/mL, preferably from about 500 mg/mL to about 600 mg/mL.
(56) The formulations of an embodiment of this disclosure may comprise from about 1 mg/mL to about 250 mg/mL progesterone or an analogue or a salt thereof, up to about 1000 mg/mL benzyl alcohol, up to about 60 mg/mL benzyl benzoate, up to about 300 mg/mL ethanol, up to about 60 mg/mL stearic acid, up to about 50 mg/mL hydroxyethyl cellulose, up to about 120 mg/mL ethoxylated castor oil at 40 moles of ethylene oxide, up to about 120 mg/mL Poloxamer P407, up to about 100 mg/mL refined sesame oil, and up to about 1000 mg/mL water.
(57) The formulations of an embodiment of this disclosure may comprise from about 1 mg/mL to about 250 mg/mL progesterone or an analogue or a salt thereof, up to about 1000 mg/mL benzyl alcohol, up to about 60 mg/mL benzyl benzoate, up to about 300 mg/mL ethanol, up to about 60 mg/mL stearic acid, up to about 50 mg/mL hydroxyethyl cellulose, up to about 120 mg/mL ethoxylated castor oil at 40 moles of ethylene oxide, up to about 120 mg/mL Poloxamer P407, and up to about 1000 mg/mL water.
(58) The formulations of an embodiment of this disclosure may comprise from about 1 mg/mL to about 250 mg/mL progesterone or an analogue or a salt thereof, up to about 1000 mg/mL benzyl alcohol, up to about 60 mg/mL benzyl benzoate, up to about 300 mg/mL ethanol, up to about 60 mg/mL stearic acid, up to about 120 mg/mL ethoxylated castor oil at 40 moles of ethylene oxide, up to about 120 mg/mL Poloxamer P407. up to about 100 mg/mL refined sesame oil, and up to about 1000 mg/mL water.
(59) The formulation of an embodiment of this disclosure may also further comprise, optionally, a pH adjusting agent. In any case, the pH of the final formulation may be adjusted to a value from about 4.0 to about 8.0, or from about 4.5 to about 7.5, preferably from about 5.0 to about 7.0. The preferred final pH of the formulation may be, for example, 5.0, 5.1, 5.2, 5.3, 5.4, 5.5, 5.6, 5.7, 5.8, 5.9, 6.0, 6.1, 6.2, 6.3, 6.4, 6.5, 6.6, 6.7, 6.8, 6.9, 7.0.
(60) The formulation of an embodiment of this disclosure may be in the form of a solution, for example, a liquid solution, micellar solution, suspension, a two or more phase system, emulsion, for example, a microemulsion, miniemulsion, small particle emulsion or combinations thereof.
(61) The formulation of an embodiment of this disclosure may be a sterile formulation. The formulation or the separate components thereof of an embodiment of this disclosure may be sterilized using different methods. Sterilization methods are well known in the art and may comprise, as appropriate, heat sterilization, sterilization by filtration, sterilization by UV radiation, gamma radiation sterilization, among others.
(62) The formulations of an embodiment of this disclosure may be suitable for use as injectable formulations, but it should be understood that the formulations may be adapted for administration via different alternative routes. In the case of injectable formulations, these may be administered through the most appropriate route according to the characteristics of the animal, for example, parenteral, subcutaneous, intravenous, intradermal or intramuscular. One embodiment of this disclosure is an injectable formulation suitable for intramuscular administration.
(63) The formulations of an embodiment of this disclosure may be useful for controlling the reproductive cycle and/or ovulation in a female mammal. The formulations of an embodiment of this disclosure may also be used to promote ovulation. Another use of the formulations of an embodiment of this disclosure may be to synchronize the ovulation or the heat of a group of female mammals. In addition, the formulations of an embodiment of this disclosure may be used to reduce the anestrous period. In addition, the formulations of an embodiment of this disclosure may be used to increase the likelihood that a female mammal gets pregnant. For example, the formulations of an embodiment of this disclosure may be used to increase the likelihood that a female mammal gets pregnant after insemination, which may be artificial or natural insemination. For example, the formulations of an embodiment of this disclosure may be used together with a fixed-time artificial insemination (FTAI) protocol or a heat detection insemination protocol. The formulations of an embodiment of this disclosure may be used also in ovarian superstimulation protocols to superovulate, they also may be used in ovarian puncture protocols for subsequent in vitro fertilization or to increase the likelihood of success of embryo transfer process.
(64) Said female mammal may be, for example, a domestic or farm animal. For example, the female mammal may be a ruminant, such as cattle, pigs, goats, sheep, horses, camels, among others. For example, the female mammal may be a reproductively mature female bovine animal.
(65) The formulations of an embodiment of this disclosure may be used in coordination with other treatments, such as other hormone treatments to achieve the desired objectives.
(66) A second aspect of an embodiment of this disclosure provides a dosage unit comprising a formulation as described in the first aspect of an embodiment of the disclosure.
(67) In one embodiment, the dosage unit may have a volume from about 1 mL to about 20 mL, or from about 2 mL to about 10 mL or from about 4 mL to about 5 mL.
(68) The dosage unit in one embodiment may be housed in a container, for example, a bottle, vial, ampoule or syringe, among others. Therefore, an embodiment of the disclosure also provides a container prefilled with the required amount of the formulation described in the first aspect of an embodiment of the disclosure, for example, a syringe prefilled with the formulation.
(69) Another aspect of an embodiment of this disclosure provides a set of elements (kit) comprising the formulation, dosage unit or prefilled container, for example, a prefilled syringe, as described above. The set of components (kit) of an embodiment of this disclosure may further comprise, for example, the instructions for using some or all the elements comprising it.
(70) Still another aspect of an embodiment of this disclosure provides a process for preparing a formulation such as the one described in the first aspect of an embodiment of the disclosure. The process comprises combining each component of the formulation.
(71) In one embodiment of this disclosure, the process for preparing the formulation comprises combining i) said one or more hormones; ii) said one or more pharmaceutically acceptable organic solvents; iii) optionally, said pharmaceutically acceptable oily carrier; iv) said one or more pharmaceutically acceptable fatty acids; v) optionally, said one or more pharmaceutically acceptable structure forming agents; vi) said one or more pharmaceutically acceptable surfactants; vii) said one or more pharmaceutically acceptable gel forming agents; and viii) water.
(72) In another embodiment of this disclosure, the process for preparing the formulation comprises preparing mixtures comprising certain components separately which will be combined later. For example, the process for preparing the formulation of an embodiment of the present disclosure may comprise:
(73) 1) preparing a first solution (pre-product A) comprising said one or more pharmaceutically acceptable surfactants and water:
(74) 2) preparing a second solution comprising said one or more hormones, said one or more pharmaceutically acceptable fatty acids, said one or more pharmaceutically acceptable organic solvents, said one or more pharmaceutically acceptable gel forming agents and water, wherein said second solution is prepared by combination of mixture I (pre-product B) and mixture II (pre-product C), wherein a) mixture I (pre-product B) comprises said one or more hormones, said pharmaceutically acceptable fatty acids and said one or more pharmaceutically acceptable organic solvents; and b) mixture II (pre-product C) comprises said one or more pharmaceutically acceptable gel forming agents and water;
(75) 3) preparing a third solution (pre-product D) comprising said one or more hormones, said one or more pharmaceutically acceptable organic solvents and, optionally, said pharmaceutically acceptable oily carrier; and
(76) 4) optionally, preparing a fourth solution (pre-product E) comprising said one or more pharmaceutically acceptable structure forming agents and water;
(77) 5) combining said first solution with said second solution;
(78) 6) incorporating said third solution into the mixture obtained in step 5); and
(79) 7) optionally, adding said fourth solution to the mixture obtained in step 6).
(80) In the processes of an embodiment of this disclosure, said first solution may comprise, for example, ethoxylated castor oil, at 40 moles of ethylene oxide and water; said mixture I may comprise, for example, progesterone or an analogue or a salt thereof, stearic acid and ethanol; said mixture II may comprise, for example, Poloxamer P407 (for example, Kolliphor P407) and water; said third solution may comprise, for example, progesterone or an analogue or a salt thereof, ethanol, benzyl alcohol, benzyl benzoate and, optionally, refined sesame oil; and said optional fourth solution may comprise, for example, hydroxyethylcellulose and water.
(81) In the processes of an embodiment of this disclosure, optionally, a pharmaceutically acceptable antioxidant may be included in mixture I. The pharmaceutically acceptable antioxidant may be, for example, Vitamin E, Vitamin E TGPS (d--tocopherol propylene glycol 1000 succinate), Kolliphor TGPS, Butylated hydroxytoluene (BHT), Butylated hydroxyanisole (BHA), sodium bisulphite, ascorbic acid, ascorbyl palmitate, Vitamin A, propyl gallate, monothioglycerol, sodium sulfoxylate formal, or combinations thereof.
(82) The process for preparing the formulation in accordance with an embodiment of this disclosure may comprise the step of adjusting the pH. pH may be adjusted by adding a pH adjusting agent. In an alternative embodiment the pH of the final formulation may be adjusted using acidic or basic solutions. For example, the pH of the final formulation may be adjusted to a value from about 4.0 to about 8.0, or from about 4.5 to about 7.5, preferably from about 5.0 to about 7.0. The preferred final pH of the formulation may be, for example, 5.0, 5.1, 5.2, 5.3, 5.4, 5.5, 5.6, 5.7, 5.8, 5.9, 6.0, 6.1, 6.2, 6.3, 6.4, 6.5, 6.6, 6.7, 6.8, 6.9 or 7.0.
(83) The processes in accordance with an embodiment of this disclosure may further comprise one or more sterilization steps. Sterilization may be accomplished by any suitable method, for example, heat sterilization, sterilization by filtration, sterilization by UV radiation, gamma sterilization, among others. The formulation or its components in accordance with an embodiment of this disclosure may be sterilized separately.
(84) In even another aspect of an embodiment of this disclosure a method is provided for controlling the reproductive cycle and/or ovulation in a female mammal comprising administering a suitable dose of the formulation of an embodiment of this disclosure to said female mammal.
(85) In even another aspect of an embodiment of this disclosure a method is provided for synchronizing ovulation in a group of female mammals comprising administering a suitable dose of the formulation of an embodiment of this disclosure to said female mammals.
(86) In even another aspect of an embodiment of this disclosure a method is provided for promoting ovulation in female mammals comprising administering a suitable dose of the formulation of an embodiment of this disclosure to said female mammal.
(87) In even another aspect of an embodiment of this disclosure a method is provided for increasing the likelihood that a female mammal gets pregnant comprising administering a suitable dose of the formulation of an embodiment of this disclosure to said female mammals. For example, the method may comprise a method for increasing the likelihood that a female mammal gets pregnant after natural or artificial insemination thereof, or after the embryo transference.
(88) In even another aspect of an embodiment of this disclosure a method is provided for reducing the anestrous period in female mammals comprising administering a suitable dose of the formulation of an embodiment of this disclosure to said female mammal.
(89) In the methods in accordance with an embodiment of this disclosure, a suitable dose of the formulation of an embodiment of this disclosure is administered, wherein the dose of hormone required may be modified depending on the characteristics of the animal to be treated. In another embodiment, a dose of the formulation of an embodiment of this disclosure is administered comprising from about 50 mg to about 500 mg of progesterone or an analogue or a salt thereof, more preferably from about 150 mg to about 350 mg of progesterone or an analogue or a salt thereof, or preferably from about 200 mg to about 300 mg of progesterone or an analogue or a salt thereof, for example, 240 mg of progesterone or an analogue or a salt thereof.
(90) In the methods in accordance with an embodiment of this disclosure, the formulation of an embodiment of this disclosure may be administered by an injection or by different alternative routes. In addition, the formulations may be administered, for example, by a subcutaneous, intravenous, intraparenteral, intramuscular or intradermal injection. Preferably, the formulation is administered by intramuscular injection.
(91) The methods in accordance with an embodiment of this disclosure may comprise administering the formulation of an embodiment of this disclosure to a group of female mammals in an artificial insemination program, for example, a fixed-time artificial insemination (FTAI) program or a heat detection insemination program, which increases the proportion of animals that get pregnant after insemination. In one embodiment, insemination may be carried out from about 9 to about 11 days after administration of the formulation, for example, insemination may take place about 9, about 10 or about 11 days after administration of the formulation.
(92) The methods in accordance with an embodiment of this disclosure may optionally comprise the administration of estradiol benzoate. The administration of estradiol benzoate comprises, for example, a dose of up to about 3 mg of estradiol benzoate, for example, a dose from about 1 mg to about 3 mg of estradiol benzoate, preferably a dose of about 2 mg of estradiol benzoate. In other embodiments, it is possible to use any other suitable dose to cause atresia of the follicles existing at the beginning of the treatment and thus preventing the formation of persistent follicles that negatively interfere with fertility. The administration of estradiol benzoate may be carried out, for example, by instramuscular injection or by any other appropriate route of administration. The administration of estradiol benzoate is carried out, for example, the same day the formulation of an embodiment of this disclosure is administered. In another embodiment, the administration of estradiol benzoate may also be carried out one or more days before or one or more days after the administration of the formulation of an embodiment of this disclosure.
(93) The methods in accordance with an embodiment of this disclosure may optionally comprise the administration of a prostaglandin or a prostaglandin analogue or a salt thereof, for example, d-cloprostenol acetate. The administration of prostaglandin may comprise, for example, a dose of up to about 0.500 mg of prostaglandin, for example, a dose from about 0.075 mg to about 0.500 mg of prostaglandin, preferably a dose of about 0.150 mg of prostaglandin. In other embodiments, it is possible to use any other suitable dose to generate a luteolytic action, achieving the decrease of the progesterone concentration in blood. The administration of prostaglandin may be carried out, for example, by intramuscular injection or by any other appropriate route of administration. The administration of prostaglandin may be carried out, for example, a few days before and/or a few days after administering the formulation of an embodiment of this disclosure, for example, from about 4 days before to 10 days after application of said formulation. The administration of prostaglandin may be carried out, for example, about 2 days before and/or about 7 to about 9 days after administration of said formulation. The administration of prostaglandin may be carried out for example, about 2 days before and/or about 7 days after the administration of said formulation, and/or about 8 days after the administration of said formulation.
(94) The methods in accordance with an embodiment of this disclosure may optionally comprise the administration of gonadotropin-releasing hormone (GnRH), or an analogue or a salt thereof, for example, buserelin acetate. The administration of GnRH or an analogue or a salt thereof may comprise, for example, a dose of up to about 0.03 mg, or a dose from about 0.001 mg to about 0.03 mg, or a dose from about 0.005 mg to about 0.0150 mg, preferably a dose of about 0.0084 mg. In other embodiments, any other suitable dose may be used to control the synthesis and release of LH and FSH to help with the maturation and growth of the follicle to then produce the ovulation and formation of the corpus luteum. The administration of GnRH or an analogue or a salt thereof may be carried out, for example, by intramuscular injection or by any other appropriate route of administration. The administration of GnRH or an analogue or a salt thereof can be carried out, for example, some days after the formulation of an embodiment of this disclosure has been administered, for example, from about 9 and about 11 days after administration of the formulation for example, about 9, about 10 or about 11 days after administration of the formulation. In an artificial insemination program, the administration of GnRH or an analogue or a salt thereof may be carried out, for example, the same day of the insemination, or a different day, for example, one day before the day wherein the insemination is performed.
(95) The methods in accordance with an embodiment of this disclosure may optionally comprise the administration of Equine Chorionic Gonadotropin (eCG) hormone. The administration of eCG may comprise, for example, a dose of up to about 1000 IU of eCG, or a dose of from about 400 IU to about 800 IU of eCG, or a dose of from about 300 IU to about 400 IU of eCG, preferably a dose of about 500 IU of eCG. In other embodiments, any other suitable alternative dose may be used to control the synthesis and release of FSH and LH to help with the maturation and growth of the follicle. The administration of eCG may be carried out, for example, by intramuscular injection or by any other appropriate route of administration. The administration of eCG may be carried out, for example, some days after the formulation of an embodiment of this disclosure has been administered, for example, from about 6 to about 8 days after the administration of the formulation, for example, about 6, about 7 or about 8 days after the administration of the formulation.
(96) The methods in accordance with an embodiment of this disclosure may optionally comprise the administration of estradiol cypionate or an analogue thereof. The administration of estradiol cypionate may comprise, for example, a dose of up to about 1 mg of estradiol cypionate, preferably a dose of about 0.5 mg of estradiol cypionate. In other embodiments, any other suitable dose may be used to generate a preovulatory LH surge and prepare mature follicles to ovulate. The administration of estradiol cypionate may be carried out, for example, by intramuscular injection or by any other appropriate route of administration. The administration of estradiol cypionate may be carried out, for example, some days after the formulation of an embodiment of this disclosure has been administered, for example, from about 7 to about 8 days after the administration of said formulation, for example, about 7 after the administration of said formulation, or about 8 days after the administration of said formulation. In a method in accordance with an embodiment of this disclosure, if the method comprises administering prostaglandin, the administration of estradiol cypionate may be carried out, for example, the same day of administration of prostaglandin.
(97) The methods in accordance with an embodiment of this disclosure are primarily adapted for use in cattle, but may be modified in order to adapt them to any female mammal, for example, other domestic or farm animal. In other embodiments, said female mammal may be pigs, goats, sheep, horses, camels, among others.
(98) The methods in accordance with an embodiment of this disclosure may comprise, for example, without limitation, the protocols described below. The insemination step is optional and is included in the methods that aim to increase the likelihood that the female mammal gets pregnant after the insemination. Timing of insemination may be predetermined by knowing the pre-ovulation times, which can be detected by ultrasonography or by manifestation of heat.
(99) Protocol 1
(100) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(101) Day 7: Administration of prostaglandin.
(102) Day 9: Administration of gonadotropin releasing hormone (GnRH).
(103) Day 10: Insemination.
(104) Protocol 2
(105) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(106) Day 7: Administration of prostaglandin.
(107) Day 9: Administration of gonadotropin releasing hormone (GnRH). Insemination.
(108) Protocol 3
(109) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(110) Day 8: Administration of prostaglandin. Administration of estradiol cypionate.
(111) Day 10: Administration of gonadotropin releasing hormone (GnRH). Insemination.
(112) Protocol 4
(113) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(114) Day 8: Administration of prostaglandin.
(115) Day 10: Administration of gonadotropin releasing hormone (GnRH).
(116) Day 11: Insemination.
(117) Protocol 5
(118) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(119) Day 8: Administration of prostaglandin. Administration of estradiol cypionate.
(120) Day 11: Insemination.
(121) Protocol 6
(122) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(123) Day 7: Administration of prostaglandin. Administration of estradiol cypionate.
(124) Day 9: Administration of gonadotropin releasing hormone (GnRH).
(125) Day 10: Insemination.
(126) Protocol 7
(127) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(128) Day 8: Administration of prostaglandin. Administration of equine chorionic gonadotropin (eCG)
(129) Day 9: Administration of estradiol benzoate.
(130) Day 10 (68 hours after administration of prostaglandin): Insemination.
(131) Protocol 8
(132) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(133) Day 6: Administration of prostaglandin.
(134) Day 9 (68-72 hours after administration of prostaglandin): Insemination.
(135) Protocol 9
(136) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(137) Day 7 (in the morning): Administration of prostaglandin.
(138) Day 8 (in the morning): Administration of estradiol benzoate.
(139) Day 9 (68-72 hours after administration of prostaglandin): Fixed-time insemination.
(140) Protocol 10
(141) Day 0: Artificial Insemination.
(142) Day 13: Administration of the formulation of an embodiment of this disclosure.
(143) Day 21-25: Insemination at detected heat.
(144) Protocol 11
(145) Day 0: Administration of the formulation of an embodiment of this disclosure.
(146) Day 23: Administration of gonadotropin releasing hormone (GnRH).
(147) Day 30: Administration of prostaglandin.
(148) Day 30+52 hours: Detection of heat.
(149) Day 33: Administration of gonadotropin releasing hormone (GnRH). Insemination.
(150) Protocol 12
(151) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of gonadotropin releasing hormone (GnRH).
(152) Day 5: Administration of prostaglandin and repetition of dose at 12 hours.
(153) Day 5+52 hours: Detection of heat.
(154) Day 8: Administration of gonadotropin releasing hormone (GnRH). Insemination.
(155) Protocol 13
(156) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of gonadotropin releasing hormone (GnRH).
(157) Day 7: Administration of prostaglandin.
(158) Day 7-13: Detection of heat. Insemination.
(159) Protocol 14
(160) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of gonadotropin releasing hormone (GnRH).
(161) Day 7 (in the morning): Administration of prostaglandin.
(162) Day 7+72-84 hours: Detection of heat.
(163) Day 10: Administration of gonadotropin releasing hormone (GnRH). Insemination.
(164) Protocol 15
(165) Day 0: Administration of prostaglandin.
(166) Day 0-3: Detection of estrus. Insemination.
(167) Day 3: Administration of the formulation of an embodiment of this disclosure. Administration of gonadotropin releasing hormone (GnRH).
(168) Day 9: Administration of prostaglandin.
(169) Day 9-12: Detection of heat. Insemination.
(170) Protocol 16
(171) Day 0: Administration of prostaglandin.
(172) Day 0-3: Detection of heat. Insemination.
(173) Day 3: Administration of the formulation of an embodiment of this disclosure. Administration of gonadotropin releasing hormone (GnRH).
(174) Day 9: Administration of prostaglandin.
(175) Day 12: Administration of gonadotropin releasing hormone (GnRH). Insemination.
(176) Protocol 17
(177) Day 0: Administration of prostaglandin.
(178) Day 14: Administration of prostaglandin.
(179) Day 28: Administration of the formulation of an embodiment of this disclosure. Administration of gonadotropin releasing hormone (GnRH).
(180) Day 35: Administration of prostaglandin.
(181) Day 37: Administration of gonadotropin releasing hormone (GnRH).
(182) Day 38: Fixed-time insemination.
(183) Protocol 18
(184) Day 0: Administration of the formulation of an embodiment of this disclosure. Administration of estradiol benzoate.
(185) Day 6: Administration of prostaglandin. Administration of equine chorionic gonadotropin (eCG)
(186) Day 9 (72 hours post prostaglandin): Administration of gonadotropin releasing hormone (GnRH). Fixed-time insemination.
(187) The administration times and doses of the formulation of an embodiment of this disclosure as well as the administration times and doses of each hormone of the methods described above may be modified depending on the characteristics of the animal or group of animals to be treated.
EXAMPLES
Example 1: Formulations
(188) Some non-limiting examples of formulations of an embodiment of the present disclosure that were prepared and assayed comprise the compounds and concentrations as indicated in the following tables.
(189) Formulation 1
(190) TABLE-US-00001 Concentration Components (mg/mL) Progesterone 47 Benzyl alcohol 40 Benzyl benzoate 23 Ethanol 118 Stearic Acid 24 Hydroxyethyl cellulose 4 Ethoxylated castor oil, at 40 moles of ethylene oxide 99 Poloxamer P407 69 Refined sesame oil 17 Water 559
(191) Formulation 2
(192) TABLE-US-00002 Concentration Components (mg/mL) Progesterone 47 Benzyl alcohol 38 Benzyl benzoate 22 Ethanol 118 Stearic Acid 24 Hydroxyethyl cellulose 3.5 Ethoxylated castor oil, at 40 moles of ethylene oxide 64 Poloxamer P407 69 Refined sesame oil 16 d--tocopherol propylene glycol 1000 succinate 5 Xanthan gum 0.1 Water 599
(193) Formulation 3
(194) TABLE-US-00003 Concentration Components (mg/mL) Progesterone 50 Benzyl alcohol 40 Benzyl benzoate 20 Ethanol 120 Stearic Acid 20 Hydroxyethyl cellulose 4 Ethoxylated castor oil, at 40 moles of ethylene oxide 60 Poloxamer P407 70 Refined sesame oil 20 d--tocopherol propylene glycol 1000 succinate 5 BHA 1 BHT 1 Gum Arabic 1 Xanthan gum 0.1 Water 600
(195) Formulation 4
(196) TABLE-US-00004 Concentration Components (mg/mL) Progesterone 50 Benzyl alcohol 40 Benzyl benzoate 20 Ethanol 120 Stearic Acid 20 Hydroxyethyl cellulose 4 Ethoxylated castor oil, at 40 moles of ethylene oxide 60 Poloxamer P407 70 Refined sesame oil 20 d--tocopherol propylene glycol 1000 succinate 5 BHA 1 Gum Arabic 1 Water 600
(197) Formulation 5
(198) TABLE-US-00005 Concentration Components (mg/mL) Progesterone 50 Benzyl alcohol 40 Benzyl benzoate 20 Ethanol 120 Stearic Acid 20 Hydroxyethyl cellulose 4 Ethoxylated castor oil, at 40 moles of ethylene oxide 60 Kolliphor P407 70 Refined sesame oil 20 d--tocopherol propylene glycol 1000 succinate 5 BHT 2 Water 600
(199) Formulation 6
(200) TABLE-US-00006 Concentration Components (mg/mL) Progesterone 47.1 Benzyl alcohol 53.3 Benzyl benzoate 21.9 Ethanol 118 Stearic Acid 23.6 Hydroxyethyl cellulose 3.6 Ethoxylated castor oil, at 40 moles of ethylene oxide 100 Poloxamer P407 63.9 Water 556.7
(201) Formulation 7
(202) TABLE-US-00007 Concentration Components (mg/mL) Progesterone 47.1 Benzyl alcohol 37.6 Benzyl benzoate 21.9 Ethanol 118 Stearic Acid 23.6 Ethoxylated castor oil, at 40 moles of ethylene oxide 100 Poloxamer P407 63.9 Refined sesame oil 15.7 Water 566
Example 2: Process for Preparing an Injectable Formulation
(203) The process described below is an example of how to prepare one of the injectable formulations of an embodiment of the present disclosure (Formulation 1 of Example 1).
(204) The process for preparing the injectable formulation of the present disclosure consists, firstly, of preparing five pre-products A-E. The processes for the preparation of these pre-products are described below.
(205) Preparation of Pre-Product A Ethoxylated castor oil, at 40 moles of ethylene oxide, is dissolved in distilled water at a temperature of 70 C. to a concentration of about 30% by weight (m/m). Dissolution is carried out with slow stirring for 5 minutes or until complete dissolution. This pre-product may be stored at 4 C. until further use.
(206) Preparation of Pre Product B
(207) Firstly, stearic acid is added to a vessel containing ethanol at a temperature of 60 C., and stirred using a magnetic stirrer until complete dissolution. Next, progesterone is added and stirring is continued until its complete dissolution. Final concentrations of stearic acid and progesterone comprise about 14% by weight (m/m).
(208) Preparation of Pre-Product C
(209) Poloxamer P407, for example, Kolliphor P407, is added to distilled water at a temperature of about 70 C. to a concentration of about 25% by weight (m/m). The mixture is stirred continuously for a period of time. Then, the mixture is stored at a temperature of 4 C. until a clear and homogeneous liquid is formed.
(210) Preparation of Pre-Product D
(211) In the first place, a mixture of benzyl alcohol, benzyl benzoate, and ethanol is prepared. To this mixture progesterone is added and the mixture is stirred to its complete dissolution. Finally, refined sesame oil is included and stirred until a homogeneous mixture is obtained. The final half-finished product contains about 38% by weight (m/m) benzyl alcohol, about 22% by weight (m/m) benzyl benzoate, about 0.3% by weight (m/m) ethanol, about 16% by weight (m/m) sesame oil and about 24% by weight (m/m) progesterone. This pre-product may be stored at 4 C. until further use.
(212) Preparation of Pre-Product E
(213) Hydroxyethyl cellulose (HEC) is dissolved in distilled water at a temperature of 70 C. to a final concentration of about 3% by weight (m/m) HEC. Then, the solution is slowly stirred until a homogeneous gel is formed. This pre-product may be stored at 4 C. until further use.
(214) Final Preparation
(215) Once pre-products A-E are ready, preparation of the final formulation is carried out.
(216) For example, for preparing 5000 mg of formulation 1 of Example 1, firstly about 850 mg of pre-product B are mixed with about 1400 mg of pre-product C. Then, about 1650 mg of pre-product A and about 500 mg of pre-product D are added to this suspension. Finally, about 600 mg of pre-product E are added.
Example 3: Treatment Protocols
(217) Preliminary Considerations
(218) First, for the treatment protocols as described in the following assays, bovine animals were selected according to the criteria outlined below. This selection was made in order to work with cows that are suitable for a heat synchronization.
(219) Cows having reached sexual maturity were selected, that is, those of more than about 15 months of age and weighing more than about 260 kilograms.
(220) Regarding their body condition, preferably those animals scoring from about 2.5 to 3.5 points on a scale of 5 as described by Lowman et al., (The East of Scotland College of Agriculture; Edinburgh; 1976; pp. 1-31 (Vol. 6) were selected.
(221) The assessment by this scale is not exclusive since there were cases in which scoring was met but the animals were not fit for other reasons, for example, cows in anestrous phase. Furthermore, some animals which did not achieve the preferred scoring, for example, animals lacking weight but which were in a state of weight gaining, were selected. Moreover, animals with a preferred scoring, but having malformations which might prevent the animal from feeding correctly, for example, animals with crooked jaws, were discarded.
(222) Another aspect considered for selecting animals was their state of health.
(223) For example, cows showing purulent vaginal discharge caused by infections such as vaginitis, erratic behavior, wobbling, or sadness caused by internal or external parasites, lack or significant wear of teeth and cows with any other type of pathology, were discarded.
(224) Further, the nutritional state was assessed in a feeding history study of the last month to establish weight gain of the cows to be selected.
(225) Finally, an ultrasound was performed in all preselected animals and those cows having a size of corpus luteum or follicles equal or greater than 8 mm were selected. Cows with small ovaries, small follicles (indicative of anestrus), and pregnant cows were discarded.
(226) Protocols
(227) The protocols comprising administering the formulation of an embodiment of the present disclosure were adapted for use in cattle but may be modified as needed for use in other animals. Further, the assessed doses and application times may vary depending on the type of animal and other factors. The following protocols were tested:
(228) Protocol A
(229) Day 0 (in the morning):
(230) Application of intramuscular injection of the formulation of an embodiment of the present disclosure at a dose of 240 mg progesterone.
(231) Application of intramuscular injection of 2 mg estradiol benzoate.
(232) Day 7 (in the morning):
(233) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(234) Day 9 (in the morning):
(235) Application of intramuscular injection of 0.0084 mg buserelin.
(236) Day 10 (in the morning):
(237) Insemination.
(238) Protocol B
(239) Day 0 (in the morning):
(240) Application of intramuscular injection of the formulation of an embodiment of the present disclosure at a dose of 240 mg progesterone.
(241) Application of intramuscular injection of 2 mg estradiol benzoate.
(242) Day 7 (in the morning):
(243) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(244) Day 9 (in the morning):
(245) Application of intramuscular injection of 0.0084 mg buserelin.
(246) Insemination.
(247) Protocol B1
(248) Day 0 (in the morning):
(249) Insertion of a Bovine Intravaginal Device (DIB) with 1 g progesterone.
(250) Application of intramuscular injection of 2 mg estradiol benzoate.
(251) Day 7 (in the morning):
(252) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(253) Removal of DIB.
(254) Day 9 (in the morning):
(255) Application of intramuscular injection of 0.0084 mg buserelin.
(256) Insemination.
(257) Protocol C
(258) Day 0 (in the morning):
(259) Application of intramuscular injection of the formulation of an embodiment of the present disclosure at a dose of 240 mg progesterone.
(260) Application of intramuscular injection of 2 mg estradiol benzoate.
(261) Day 8 (in the morning):
(262) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(263) Application of intramuscular injection of 0.5 mg estradiol cypionate
(264) Day 10 (in the morning):
(265) Application of intramuscular injection of 0.0084 mg buserelin.
(266) Insemination.
(267) Protocol D
(268) Day 0 (in the morning):
(269) Application of intramuscular injection of the formulation of an embodiment of the present disclosure at a dose of 240 mg progesterone.
(270) Application of intramuscular injection of 2 mg estradiol benzoate.
(271) Day 8 (in the morning):
(272) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(273) Day 10 (in the morning):
(274) Application of intramuscular injection of 0.0084 mg buserelin.
(275) Day 11 (in the morning):
(276) Insemination.
(277) Protocol E
(278) Day 0 (in the morning):
(279) Application of intramuscular injection of the formulation of an embodiment of the present disclosure at a dose of 240 mg progesterone.
(280) Application of intramuscular injection of 2 mg estradiol benzoate.
(281) Day 8 (in the morning):
(282) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(283) Application of intramuscular injection of 0.5 mg estradiol cypionate
(284) Day 11 (in the morning):
(285) Insemination.
(286) Protocol E1
(287) Day 0 (in the morning):
(288) Insertion of a Bovine Intravaginal Device (DIB) with 0.5 g progesterone.
(289) Application of intramuscular injection of 2 mg estradiol benzoate.
(290) Day 8 (in the morning):
(291) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(292) Application of intramuscular injection of 0.5 mg estradiol cypionate
(293) Removal of DIB.
(294) Day 10 (in the morning):
(295) Insemination.
(296) Protocol F
(297) Day 0 (in the morning):
(298) Insertion of a Bovine Intravaginal Device (DIB) with 0.5 g progesterone.
(299) Application of intramuscular injection of 2 mg estradiol benzoate.
(300) Day 7 (in the morning):
(301) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(302) Application of intramuscular injection of 0.5 mg estradiol cypionate
(303) Removal of DIB.
(304) Day 9 (in the morning):
(305) Insemination.
(306) Protocol F1
(307) Day 0 (in the morning):
(308) Insertion of a Bovine Intravaginal Device (DIB) with 1 g progesterone.
(309) Application of intramuscular injection of 2 mg estradiol benzoate.
(310) Day 7 (in the morning):
(311) Application of an intramuscular injection of 0.150 mg d-cloprostenol acetate.
(312) Removal of DIB.
(313) Day 9 (in the morning):
(314) Insemination.
(315) Application of intramuscular injection of 0.0084 mg buserelin.
(316) In the case of heifers, the dose of the formulation of the present disclosure may be replaced by 192 g progesterone.
Example 4: Blood Progesterone Levels
(317) Cows of the following breeds were selected: Holando-Argentino (argentine dairy breed), Brangus (synthetic breed derived by crossing a British breed, such as Aberdeen Angus, with a cow of the Brahman breed at a relationship of , a crossing designated zebuine) and Aberdeen Angus, according to the criteria outlined in Example 3.
(318) Approximately 15 animals of each breed were selected and treated with the formulation of an embodiment of the present disclosure (Formulation 1 of Example 1) as described in Protocol A. In all cases, 0.150 mg d-cloprostenol acetate were applied two days before starting the treatment protocol in order to lyse the corpus luteus and allow for baseline progesterone on day 0.
(319) Blood extractions were performed from all animals as from two days before starting the treatment protocol. Then, blood extractions were conducted periodically up to day 14 after starting the treatment.
(320) Approximately 8 to 10 mL of venous blood were extracted preferably from the jugular vein or from the coccygeal vein, after previous cleaning of the extraction zone with 70% v/v ethanol or 10% v/v povidone-iodine solution. Blood was collected in 5 mL sterile tubes and left to stand at room temperature for 2 to 3 hours until clotting had occurred. Then it was centrifuged at 45000 rpm for 15 minutes to extract the serum. Finally, 2 aliquots of 1.5 mL serum were taken and deposited in 5 mL test tubes. These tubes may be stored at 18 C. for further analysis.
(321) Serum samples were analyzed to measure progesterone levels using the Immulite 2000 system (DPC/Siemens).
(322) The results obtained for the different groups of cows are summarized in the following tables. Average values of progesterone concentration in the blood from each group of animals are represented.
(323) The results shown in the following Tables 1 to 3 are also represented in
(324) TABLE-US-00008 TABLE 1 Holando-Argentino Day [P4] ng/mL 2 8.30 0 0.37 2 2.20 4 3.10 6 7.42 7 5.00 8 3.14 9 0.9 10 0.70 12 2.10 14 3.80
(325) TABLE-US-00009 TABLE 2 Brangus Day [P4] ng/mL 2 7.42 0 3.00 2 1.31 4 2.3 5 3.90 7 2.74 9 1.10 10 0.80 12 0.76 14 3.40
(326) TABLE-US-00010 TABLE 3 Aberdeen Angus Day [P4] ng/mL 2 3.00 0 0.80 2 2.20 4 2.30 5 4.20 7 1.18 9 0.60 10 0.57 12 2.80 14 4.00
(327) As may be observed from the above results, the formulation of an embodiment of the present disclosure allows for a delayed release of progesterone into the blood stream, thus generating a sustained concentration of said hormone about 5 to 7 days after starting the treatment protocol when there is a pronounced reduction of progesterone concentration.
(328) The results obtained in the present example show that the product an embodiment of the present disclosure defines a characteristic curve while maintaining the values required for a correct follicular growth. It should be noted that by the end of the treatment, i.e., after about 7 or 8 days, there is a reduction in progesterone levels, simulating what occurs with the removal of an intravaginal or implantable device. In other words, kinetics shown in
Example 5: Ovulation and Follicular Dynamics
Example 5A
(329) Cows of Holando-Argentino, Brangus and Aberdeen Angus breeds were selected according to the criteria outlined in Example 3.
(330) About 30 animals of each breed were selected and divided into two groups. A group of each breed was treated with the formulation of an embodiment of the present disclosure (Formulation 1 of Example 1) as described in Protocol A. The other group was treated using an intravaginal device as described in Protocol F (Brangus and Aberdeen Angus breeds) or in Protocol F1 (Holando-Argentino breed). In all cases, 0.150 mg d-cloprostenol acetate were applied two days before starting the treatment protocol in order to lyse the corpus luteus and allow for baseline progesterone on day 0.
(331) In order to monitor follicular dynamics in treated animals, scanning by transrectal ultrasound was performed using a DP-10 (Mindray Medical International Ltd.) of 6 to 8.5 Mhz with a lineal transducer. Ultrasounds were carried out on treatment days 0, 2, 4, 6, 7, 8, 9, 10 and 11 at the times indicated in the following table:
(332) TABLE-US-00011 TABLE 4 Days and times of ultrasound. Day Time 0 2 4 6 7 8 9 10 11 8:00 am X X X X X X X X X 12:00 pm X X X X 4:00 pm X X X X X 8:00 pm X X X
(333) The results of ultrasounds for each group of the selected animals are summarized below and shown in Tables 5 to 7.
(334) The results of the present example demonstrate that the formulation of an embodiment of the present disclosure provides an increase in the ovulation percentage. As may be seen in Table 5, a treatment with the formulation of an embodiment of the present disclosure produced higher ovulation percentages than a treatment with an intravaginal device in the three analyzed breeds. In addition, a greater average size of ovulatory follicles was observed (Table 6). Another important advantage when using the formulation of an embodiment of the present disclosure was that an improved synchronization of ovulation time as compared to the results obtained with the protocol using an intravaginal device was observed (Table 7). Most of the animals treated with the protocol including the formulation of an embodiment of the present disclosure ovulated during day 10 (that is, after 10 days of administering the formulation) in the afternoon. In contrast, when a treatment with an intravaginal device was used, ovulation times were more variable.
(335) TABLE-US-00012 TABLE 5 Ovulation percentage Breed Formulation 1 DIB Holando-Argentino 100% 56% Brangus 93% 61% Aberdeen Angus 100% 60%
(336) TABLE-US-00013 TABLE 6 Average size of ovulatory follicles Breed Formulation 1 DIB Holando-Argentino 17-18 mm.sup. 16 mm Brangus 16 mm 15 mm Aberdeen Angus 16 mm 14 mm
(337) TABLE-US-00014 TABLE 7 Ovulation times Day/Time of ovulation Formulation 1 DIB Holando-Argentina breed Day 9, in the afternoon 0% 31% Day 10, in the morning 0% 12.5%.sup. Day 10, in the afternoon 100% 12.5%.sup. No ovulation 0% 44% Brangus breed Day 9, in the afternoon 0% 27% Day 10, in the morning 0% 27% Day 10, in the afternoon 86% 7% Day 11, in the morning 7% 0% No ovulation 7% 39% Aberdeen Angus breed Day 9, in the afternoon 0% 40% Day 10, in the morning 0% 27% Day 10, in the afternoon 100% 0% No ovulation 0% 33%
(338) Further, the results shown in
(339) Ovulation percentages obtained by using the formulation of an embodiment of the present disclosure (about 100%) and enhanced synchronization of ovulation times are unexpected advantages as compared to intravaginal devices.
Example 5B
(340) A comparative assay was also performed to assess the ovulation percentages using formulations 1, 6 and 7 described in Example 1.
(341) For this assay, Aberdeen Angus cows without calves at foot were used.
(342) A minimum of three animals were treated with each one of formulations 1, 6 and 7, using the Protocol A described in Example 3. The results are shown in Table 8 below.
(343) TABLE-US-00015 TABLE 8 Ovulation percentage Fromulation # Ovulation % 1 100% 6 66% 7 100%
(344) The results show that the three assayed formulations produced acceptable ovulation percentages (about of the animals).
Example 6. Pregnancy Percentage
(345) Milking Yard Cows
(346) Cows of the Holando-Argentina breed were selected according to the criteria set out in Example 3, with the addition that all treated cows have had at least one calving and are producing milk.
(347) Nine batches of about 30 animals each were selected and each batch was divided into two groups. One group of each batch was treated with the formulation of an embodiment of the present disclosure (Formulation 1 of Example 1) as described in Protocol A and the other group was treated with an intravaginal device following Protocol B1.
(348) Pregnancy of animals treated during days 35 to 45 after starting the treatment was evaluated. Determination was carried out by ultrasound. The results thus obtained are shown in Table 9 below.
(349) TABLE-US-00016 TABLE 9 Pregnancy percentage Percentage of pregnant cows Batch No. Formulation 1 DIB 1 75% 33% 2 47% 38% 3 81% 31% 4 62% 42% 5 71% 38% 6 68% 51% 7 65% 49% 8 53% 42% 9 75% 37% Cumulative 67% 40%
(350) In addition, cows of the Holando-Argentina breed were selected according to the criteria set out in Example 3, except that the treated cows were only heifers.
(351) Forty five animals were selected and divided into two groups. One group of each batch was treated with the formulation of an embodiment of the present disclosure (Formulation 1 of Example 1) as described in Protocol A and the other group was treated with an intravaginal device following Protocol F.
(352) Pregnancy of animals treated during days 35 to 45 after starting the treatment was evaluated. Determination was carried out by ultrasound. The results thus obtained are shown in Table 10 below.
(353) TABLE-US-00017 TABLE 10 Pregnancy percentage of Holando-Argentina heifers Percentage of pregnant cows Formulation 1 DIB 77% 63%
(354) Meat Cows
(355) Fifty six cows of the Aberdeen Angus breed were selected according to the criteria set out in Example 3 and separated into two batches. The first batch comprised 30 cows which were treated with the formulation of an embodiment of the present disclosure (Formulation 1 of Example 1) as described in Protocol E and the second batch of 26 animals was treated with an intravaginal device as described in Protocol E1.
(356) Pregnancy of animals treated during days 35 to 45 after starting the treatment was evaluated by ultrasound.
(357) It was noted that 21 out of the 30 cows treated with the formulation of an embodiment of the present disclosure became pregnant before 45 days after starting the treatment, that is, a pregnancy percentage of 70% was obtained. On the other hand, only 14 out of the 26 cows treated with the intravaginal device became pregnant before 45 days after starting the treatment, that is, a pregnancy percentage of 54%.
(358) The above assay was repeated in 60 animals with the difference that in this case insemination was carried out with sexed semen. A first group of 40 animals was treated with the formulation of an embodiment of the present disclosure (Formulation 1 of Example 1) as described in Protocol E and the second group of 20 animals was treated with an intravaginal device as described in Protocol E1.
(359) It was noted that 24 out of the 40 cows treated with the formulation of the present disclosure (Protocol E) became pregnant before 45 days after starting the treatment, that is, a pregnancy percentage of 58% was obtained. On the other hand, only 7 out of the 20 cows treated with the intravaginal device (Protocol E1) became pregnant before 45 days after starting the treatment, that is, a pregnancy percentage of 35%.
(360) The above results are summarized in Table 11.
(361) TABLE-US-00018 TABLE 11 Pregnancy percentage for meat cows Percentage of pregnant cows Formulation 1 DIB Non-sexed semen 70% 54% Sexed semen 58% 35%
(362) In the above-described assays of this example, both for milking yard cows as for meat cows, the pregnancy percentages achieved were higher when the formulation of an embodiment of the present disclosure is used as compared to the use of intravaginal devices. These results show that the treatments comprising administration of the formulation of an embodiment of the present disclosure increase the likelihood of pregnancy in an animal, as compared to the treatments with intravaginal devices. It should be noted that these results were consistent with the high rate and ovulation synchronization obtained with all assessed breeds, as observed in Example 5.
NON-PATENT REFERENCES
(363) 1. N. Ahmad, F. N. Schrick, R. L. Butcher, E. K. Inskeep. Effect of persistent follicles on early embryonic losses in beef cows. Biol. Reprod. 52 (1995) 1129-1135. 2. Beck, L. R., Cowsar, D. R., Lewis, D. H., Cosgrove Jr, R. J., Riddle, C. T., Lowry, S. L., & Epperly, T. (1979). A new long-acting injectable microcapsule system for the administration of progesterone. Fertility and sterility, 31(5), 545-551. 3. S. Burggraaf, M. J. Rathbone, C. R. Bunt, C. R. Burke, K. L. Pickering. Effect of Shore hardness, inert fillers and progesterone particle size upon the relase of progesterone from a controlled relase intravaginal drug delivery system. Proc. Int. Symp. Control. Re. Bioact. Mater. 24 (1997) 147-148. 95. 4. C. R. Bunt, M. J. Rathbone, S. Burggraaf, C. Ogle. Development of a QC relase assessment method for a physically large veterinary product containing a highly water insoluble drug and the effect of formulation variables upon relase. Proc. Int. Symp. Control. Rei. Bioact. Mater. 24 (1997) 145-146. 5. C. R. Burke, M. Mihm, K. L. Macmillan, J. F. Roche. Some effects of prematurely elevated concentrations of progesterone on luteal and follicular characteristics during the oestrus cycle in heifers. Anim. Reprod. Sci. 35 (1994) 27-39. 6. C. R. Burke, S. Burggraaf, C. R. Bunt, M J. Rathbone, K. L. Macmillan. Use of pregnant dairy cows in product development of the intravaginal progesterone releasing (CIDR) device. Proc. NZ Soc. Anim. Prod., 57 (1997). 7. M. J. Carrick, J. N. Shelton. The synchronisation of oestrus in cattle with progestogen impregnated intravaginal sponges. J. Reprod. Frtil. 14 (1967) 21-32. 8. S. E. Curl, W. Durfey, R. Patterson, D. W. Zinn. Synchronization of estrus in cattle with subcutaneous implants. J. Anim. Sci. 27 (1968) 1189. 9. S. R. Davis, R. A. S. Welch, M. G. Pierce, A. J. Peterson. Induction of lactation in nonpregnant cows by oestradiol 17b and progesterone from an intravaginal sponge. J. Dairy Sci. 66 (1983) 450{circumflex over ()}157. 10. G. F. Duirs, K. L. Macmillan, D. G. McCall, W. H. McMillan, A. M. Day. CIDR systems in suckling beef cows. Proc. Aust. Soc. Reprod. Biol. 19 (1987) 59. 11. Espinosa, M. Efecto de Diferentes Protocolos para IATF sobre las tasas de preez aplicados en Ganado lechero. IRAC Cordoba 2010. 12. D. H. Hale, R. B. Symington. Control of sexual activity in ranch cows by intramuscular and intravaginal administration of progestogens. J. Reprod. Frtil. 18 (1969) 193-199. 13. Heba F Salem. Sustained-release progesterone nanosuspension following intramuscular injection in ovariectomized rats. International Journal of Nanomedicine 9 noviembre 2010. 14. P. G. Hignett, H. Boyd, D. F. Wishart. Syncronisation of oestrus in Ayrshire heifers by the use of progestinated intravaginal pessaries. Vet. Rec. 86 (1970) 528-531. 15. Th. Hornykiewytsch. Intra-vaginal application system (INVAS) for controlled drug relase in animis. Acta Pharm. Technol. 34 (1988) 68. 145 D. Hiller. 16. Th. Hornykiewytsch. Process for preparing an intravaginal application system. U.S. Pat. No. 5,398,698 (1995). 17. Y. Iwazumi, Y. Fukui, R. B. Vargas, C. Nakano, N. Sato, M. Furudate, K. Ohsaki, S. Matsuzaki. Superovulation using CIDR in Holstein cows. J. Reprod. Dev. 40 (1994) 259-266. 18. D. R. Kerr, M. R. McGowan, C. L. Carroll, F. C. Baldock. Evaluation of three estrus synchronization regimens for use in extensively managed Bos indicus and Bos indicus/taurus heifers in Northern Australia. Theriogenology 36 (1991) 129-141. 19. Lowman, B. G., Scott, N., & Somerville, S. (1976). Condition scoring of cattle. East of Scotland College of Agriculture, Edinburgh. Vol 6 pp. 1-31. 20. S. McDougall, C. R. Burke, K. L. Macmillan, N. B. Williamson. The effect of pretreatment with progesterone on the oestrus response to oestradiol-17b benzoate in the postpartum dairy cow. Proc. NZ Soc. Anim. Prod. 52 (1992) 157-160. 21. W. H. McMillan, K. L. Macmillan. CIDR-B for managed reproduction in beef cows and heifers. Proc. NZ Soc. Anim. Prod. 49 (1989) 85-89. 22. W. H. McMillan, K. L. Macmillan, A. J. Peterson. Is uterine function compromised in heifers synchronised with a long duration progesterone treatment? Proc. Aust. Soc. Reprod. Biol. 25 (1993) 18. 23. K. L. Macmillan, A. M. Day, V. K. Taufa, B. R. Barnes, T. J. Braggins. Plasma progesterone concentration and oestrus or ovulation in heifers treated with CIDR-type B for at least 7 weeks. Proc. Aust. Soc. Reprod. Biol. 19 (1987) 61. 24. K. L. Macmillan, D. R. Barnes, V. K. Taufa, S. N. Duncan. Plasma progesterone concentrations (PPC) in heifers treated with the CIDR type-B. Proc. Asian/Aust. Assoc. Anim. Prod. 4 (1987) 229. 25. K. L. Macmillan, V. K. Taufa. Effects of using bovine CIDR after first insemination on pregnancy rate and subsequent synchrony. Proc. Asian/Aust. Assoc. Anim. Prod. 4 (1987) 224. 26. K. L. Macmillan, V. K. Taufa, A. M. Day. Onset of oestrus and fertility in heifers synchronised with progesterone from a CIDR-Type B for fifteen days. Proc. 1 lth Int. Cong. Anim. Reprod. 4 (1988) 444. 27. K. L. Macmillan, V. K. Taufa, D. R. Barnes, A. M. Day, R. Henry. Detecting estrus in synchronized heifers using tailpaint and an aerosol raddle. Theriogenology 30 (1988) 1099-1114. 28. K. L. Macmillan, S. P. Washburn, H. V. Henderson, S. F. Petch. Effects of varying the progesterone conten of CIDR intravaginal devices and mltiple CIDR treatments on plasma hormone concentrations and residual hormone conten. Proc. NZ Soc. Anim. Prod. 50 (1990) 471-472. 29. K. L. Macmillan, V. K. Taufa, A. M. Day, A. J. Peterson. Effects on supplemental progesterone on pregnancy rates in cattle. J. Reprod. Frtil. 43 (1990) 304. 30. K. L. Macmillan, V. K. Taufa, A. M. Day, D. R. Barnes. Some effects of administering progesterone per vaginum during metoestrus on oestrous cycle length in heifers. Proc. Aust. Soc. Reprod. Biol. 21 (1989) 105.36 (1991) 4. 31. K. L. Macmillan, V. K. Taufa, A. M. Day. Combination treatments for synchronising oestrus in dairy heifers. Proc. NZ Soc. Anim. Prod. 53 (1993) 267-270. 32. K. L. Macmillan, V. K. Taufa, A. M. Day, S. McDougall. Some effects of using progesterone and oestradiol benzoate to stimulate oestrus and ovulation in dairy cows with anovulatory anoestrus. Proc. NZ Soc. Anim. Prod. 55 (1995) 239-241. 33. S. R. McPhee, C. J. Hughes, L. D. Staples, M. B. White, A. H. Williams, I. F. Davis, L. P. Cahill. Synchronisation of oestrus in dairy cows using progesterone administered by controlled internal drug relase (CIDR) devices. Proc. Aust. Soc. Anim. Prod. 16 (1976) 103-106. 34. R. W. Moore, J. F. Smith. Effect of progestogen intravaginal sponges and PMSG on synchronization of oestrus in maiden heifers and on interval from calving to oestrus in beef cows. NZ J. Expt. Agrie. 8 (1980) 199-203. 35. A. J. Peterson, H. C. Henderson. Plasma progesterone concentrations in ovariectomized dairy cows treated with a CIDR-B breeding device. J. Reprod. Frtil. Suppl. 43 (1990) 315. 36. Rathbone, M. Delivering drugs to farmed animals using controlled relase science and technology. (2012). 37. J. F. Roche, J. P. Crowley, The use of implants containing steroids for growth promotion and control of oestrus in cattle. Anim. Prod. 13 (1971) 385. 38. J. F. Roche, J. P. Crowley. The long-term suppression of heat in cattle with implants of melengestrol actate. Anim. Prod. 16 (1973) 245-250. 39. J. F. Roche. Effect of short-term progesterone treatment on estrus response and fertility in heifers. J. Reprod. Frtil. 40 (1974) 433-440. 40. J. F. Roche, Synchronisation of oestrus in heifers with implants of progesterone. J. Reprod. Frtil. 41 (1974) 337-344. 41. J. F. Roche. Control of time of ovulation in heifers treated with progesterone and gonadotrophin releasing hormone. J. Reprod. Frtil. 43 (1975) 471-477. 42. J. F. Roche. Retention rate in cows and heifers of intravaginal silastic coils impregnated with progesterone. J. Reprod. Frtil. 46 (1976) 253-255. 43. J. F. Roche. Fertility in cows after treatment with a prostaglandin analogue with or without progesterone. J. Reprod. Frtil. 46 (1976) 341-345. 44. J. F. Roche. Control of oestrus in cattle. World Rev. Anim. Prod. 15 (1979) 49-76. 45. J. F. Roche, J. J. Ireland. Effect of exogenous progesterone on time of occurrence of the LH surge in heifers. J. Anim. Sci. 52 (1981) 580-586. 46. J. D. Savio, W. W. Thatcher, G. R. Morris, K. Entwistle, M. Drost, M. R. Mattiacci. Effects of induction of low plasma progesterone concentrations with a progesterone-releasing intravaginal device on follicular turnover and fertility in cattle. J. Reprod. Frtil. 98 (1993) 77-84. 47. P. F. Scanlon, T. D. Burgess. Subcutaneous and oral applications of progestogens for control of estrus in heifers. Can. J. Anim. Sci. 51 (1971) 540-541. 48. P. F. Scanlon, W. J. Neville, T. G. Burgess, J. W. Macpherson. Synchronisation of oestrus in cattle by intravaginal application of progesterone with oestrogen administration. Can. J. Anim. Sci. 51 (1971) 250-251. 49. P. F. Scanlon, B. Sreenan, I. Gordon. Synchronization of oestrus in heifers by intravaginal application of progesterone. Vet. Rec. 90 (1972) 440{circumflex over ()}41. 50. H. Shimizu, Y. Toyoda, S. Takeuchi, T. Kawai, S. Adachi. Synchronisation of oestrus and subsequent fertility of beef cattle following the intravaginal administration of gestagen. J. Reprod. Frtil. 13 (1967) 555-558. 51. R. E. Short, R. A. Bellows, J. B. Carr, R. B. Staigmiller, R. D. Randel. Induced or synchronized puberty in heifers. J. Anim. Sci. 43 (1976) 1254-1258. 52. J. Sirois, J. E. Fortune. Lengthening the bovine estrus cycle with low levis of exogenous progesterone: a model for studying ovarian follicular dominance. Endocrinology 127 (1990) 916-925. 53. J. F. Smith. Synchronisation of oestrus in cattle. NZ J. Agrie. Aug. (1974) 26-30. 54. J. F. Smith, R. J. Fairclough, A. J. Peterson. Plasma levis of progesterone provera oestradiol-17b and 13, 14 dihydro-15-keto-prostaglandin F in cows treated with Provera-impregnated intravaginal sponges. J. Reprod. Frtil. 55 (1979) 359-364. 55. R. D. Smith, R. J. Pomerantz, W. E. Beale, J. P. McCann, T. E. Pilbeam, W. Hansel. Insemination of Holstein heifers at a preset time after estrus cycle synchronization using progesterone and prostaglandin. J. Anim. Sci. 58 (1984) 792-800. 56. J. Sreenan. Retention of intravaginal sponge-pessaries by cattle. Vet. Rec. 94 (1974) 45-47. 57. L. V. Swanson, B. W. Wickham, K. L. Macmillan. Effect of exogenous progesterone (P4) on follicular waves in dairy beef heifers. J. Dairy Sci. 73 (1990) 177. 58. Valderrama, R. U., & Vlez, E. R. (2014). Uso de dispositivos auriculares de nogestomet en inseminacin artificial a tiempo fijo en bovinos doble propsito, con amamantamiento permanente (Using nogestomet ear devices fixed-time insemination artificial in cattle double purpose, permanent nursing c. Revista CES Medicina Veterinaria y Zootecnia, 7(1), 63-71. 59. J. Van Cleeff, K. L. Macmillan, W. W. Thatcher, M. C. Lucy. Estrus synchronization and fertility in heifers with CIDR before and after insemination. J. Anim. Sci. 67 (1989) 383. 60. J. van Cleeff, M. C. Lucy, C. J. Wilcox, W. W. Thatcher. Plasma and milk progesterone and plasma LH in ovariectomized lactating cows treated with new or used controlled internal relase devices. Anim. Reprod. Sci. 27 (1992) 91-106. 61. S. P. Washburn, H. G. Howard, W. Jochle, K. L. Macmillan. Control of estrus cycles in mature dairy heifers with a progesterone-releasing device. J. Anim. Sci. 67 (1989) 382. 62. R. A. S. Welch. Mating heifers with CIDR. Proc. Ruakura Farmers Conf. 37 (1985) 105-107. 63. J. N. Wiltbank, J. C. Sturges, D. Wideman, D. G. LeFever, L. C. Faulkner. Control of estrus and ovulation using subcutaneous implants and estrogens in beef cattle. J. Anim. Sci. 33 (1971) 600-606. 64. V. W. Winkler, S. Borodkin, S. K. Webel, J. T. Mannebach. In vitro and in vivo considerations of a novel matrix controlled bovine progesterone-releasing intravaginal device. J. Pharm. Sci. 66 (1977) 816-818. 65. D. F. Wishart, B. D. Hoskin. Synchronization of oestrus in heifers using intra-vaginal pessaries impregnated with SC-9880 and PMSG. J. Reprod. Frtil. 17 (1968) 285-289. 66. C. O. Woody, R. A. Pierce, Influence of day of estrus cycle at treatment on response to estrus cycle regulation by norethanrolone implants and estradiol valerate injections, J. Anim. Sci. 39 (1974) 903-906. 67. Z. Z. Xu, L. J. Burton, K. L. Macmillan. Reproductive performance of synchronised lactating dairy cows. Proc. NZ Soc. Anim. Prod. 55 (1995) 242-244.
PATENT REFERENCES
(364) 1. CN101152186 2. CN101856361 3. CN103284955 4. MX PA06015172 5. U.S. Pat. No. 7,157,102 6. U.S. Pat. No. 4,599,227 7. WO1991019484 8. WO1999042110 9. WO 2003065924 10. WO2005048930 11. WO2007062483 12. WO2001070200 13. WO 2010085363 14. WO 2011074931 15. WO2012156561 16. WO2013192250 17. US2003/0077297A1 18. US2002/0013304A1 19. YS2014/0271882A1 20. US2013/0108737A1 21. US2009/0220613A1 22. US2003/0180368A1