Title of Invention

SELFEMULSIFIABLE FORMULATION HAVING ENHANCED BIOABSORPTION AND IMMUNOSUPPRESSION ACTIVITIES AND METHOD OF PREPARATION THEREOF

Abstract

Abstract A selfemulsifiable formulation for oral administration essentially comprising of immunosuppression agent, hydrophilic agent, lipophilic agent, surfactants, antioxidant and preservative is disclosed, wherein immunosuppression agent is lactam macrolide having immunosuppression activity and present in an amount of about 2 to 10% by weight of the formulation; hydrophilic agent is ethanol present in a weight ratio of about 1:0.5 to about 1:2.5 with respect to immunosuppression agent; lipophilic agent is medium chain triglycerides of caprylic and/or capric acids; surfactants are the combination of transesterified caprylic and capric glycerides, polysorbate 80, and cremophor RH 40; antioxidant is selected from a group consisting of alpha-tocopherol, ascorbyl palmitate, butyl hydroxy anisole, butyl hydroxy toluene, propyl gallate; and preservative is selected from a group consisting of ethanol and benzyl alcohol.

Full Text

FORM 2 THE PATENTS ACT, 1970 (39 of 1970) & THE PATENTS RULES, 2003 PROVISIONAL/COMPLETE SPECIFICATION (See Section 10 and Rule 13) 1. Title of the Invention :- Selfemulsifiable formulation having enhanced bioabsorption and immunosuppression Activities and Method of Preparation Theredf. 2. Applicant(s):- (a) Name: RPG LIFE SCIENCES LIMITED (b) Nationality: An Indian Company (c) Address: Ceat Mahal, 463, Dr. Annie Besant Road, Worli, MUMBAI - 400 030, Maharashtra, INDIA 3. Preamble to the Description:- Complete Specification: The following specification particularly describes the Invention and the manner in which it is to be performed. ORIGINAL 254/MUMNP/2003 GRANTED 27/1/2006 Technical Field of Invention The present invention relates to a formulation, particularly to a selfemulsifiable formulation for oral administration having enhanced bioabsorption and immunosuppression activities, more particularly it relates to a selfemulsifiable formulation for early delivery of drug, even more particularly it relates to a selfemulsifiable formulation, which will form thermodynamically stable oil in water emulsion preferably in upper part of gastrointestinal tract and facilitate the early delivery of drug, particularly of the immunosuppression agent, still more particularly it relates to a selfemulsifiable formulation not only having the improved bioavailability and bioabsorption but also has improved capability to release the drug in reduced time with reduced toxicity and variability that is inter and intra patient bioabsorption variability. The present invention particularly relates to a selfemulsifiable formulation, which facilitates increased solubility, transport rate, bioavailability and bioabsorption of an agent having immunosuppression activity. Background Art of Invention The immunosuppression activity of a drug acting as an immunosuppression agent is achieved by inhibiting the growth and differentiation of T-cells. Such immunosuppression agents also have other pharmacological activities like anti¬inflammatory and/or antiparasitic, in particular antiprotozoal, like antimalerial activities. The commonly used immunosuppression agents include cyclosporine. There are many cyclosporines known in the art, like cyclosporine A, cyclosporine B, cyclosporine C, cyclosporine D, cyclosporine E etc. The cyclosporine A is preferably used in the clinical field due to its proven pharmacological activity and clinical indication and effectiveness. This immunosuppression agent, that is, cyclosporine A has been found useful in various other areas, like in autoimmune diseases, inflammatory conditions, particularly in inflammatory conditions with an aetiology including an autoimmune component like arthritis. Further, this immunosuppression agent is applicable in rheumatoid arthritis, arthritis chronica, and progredientic and arthritis deformana. Further, this immunosuppression agent is also applicable in rheumatic diseases. The immunosuppression therapy using this immunosuppression agent has been proposed or applied in autoimmune hematological disorder, like hemolytic anemia, aplastic anaemia, pure red cell anaemia and idiopathic thrombocytopaenia, systemic lupus erythematosus, dematomyositis, chronic active hepatitis, myasthenia gravis, psoriasis, Steven-Johnson syndrome, idiopathic spure, autoimmune inflammatory bowel disease including ulcerative colitis and Crohn's disease, endocrine opthalmopathy, Graves disease, sarcoidosis, multiple sclerosis, primary billiary cirrhosis, juvenile diabetes, like diabetes mellitus Type I, anterior and posterior uveitis, and keratoconjuncativities sicca an vernal keratoconjuncativities, intestinal lung fibrosis, psoriatic arthritis and glomerulonephritis -with or without nephrotic syndrome, like idiopathic nephrotic syndrome or minimal change nephropathy. Therefore, this immunosuppression agent is widely acceptable immunosuppression agent. This agent is made available in the form of pharmaceutical formulation. The clinical acceptance of such formulations comprising of this immunosuppression agent has suffered due to low solubility and low transport rate and delayed bioavailability and bioabsorption of the immunosuppression agent. Therefore, in recent past the research has been directed to improve its solubility and transport rate. In addition efforts have been on to improve its early bioavailability, particularly in the upper part of the gastrointestinal tract and bioabsorption. Various formulations, comprising this immunosuppression agent as one of the essential ingredients, have been developed and made available. Although there are many formulations to form microemulsions, but many of them do not have satisfactorily acceptable bioavailability and bioabsorption. The formation of microemulsions of the clinically acceptable particle size that is of less than 200 nm, particularly of less than 100 nm, is one of the desired requirements for the formulation to be clinically acceptable. Therefore, the efforts are still on to develop new formulations, particularly the formulations which will have better bioavailability, particularly in the upper part of the gastrointestinal tract and better bioabsorption and at the same time will have better solubility and reduced variability, that is inter and intra patient bioabsorption variability, and form the microemulsions of the clinically acceptable particle size. The another parameter controlling the applicability of formulations of the immunosuppression agent is its manner of administration. The formulation comprising of the immunosuppression agent, particularly of this immunosuppression agent is generally administered after filling it in a soft or hard shell, known as capsule, or in the form of solution for oral administration. The solution form of formulation of the immunosuppression agent is taken after dilution with flavored milk or fruit juice. The mixing with milk or the juice forms the emulsion, particularly microemulsions of varying particle sizes, generally varying above 100 nm, preferably varying above 150 run. The preferred form of administration of the formulation of this immunosuppression agent is after filling the formulation in a shell, which may be soft or hard shell. The major problem arises, when the immunosuppression agent or its formulation is administered after filling in a hard or soft-shell. It has been generally observed that, the availability of the immunosuppression agent will depend upon the rupture time of the shell. The known formulations of the immunosuppression agent, which are made available in the shell, have rupture time of shell varying from 12 minutes to 15 minutes or above. The problem arises due to this longer rupture time, which delays the availability of the immunosuppression agent, which in-turn effects its bioabsorption. The desired rupture time of the shell in order to make the availability of the immunosuppression agent at an early time, preferably in the upper part of the gastrointestinal tract is less than 12 minutes, preferably less than 10 minutes. Need of Invention Therefore, there is a need to have a formulation, particularly a selfemulsifiable formulation for oral administration, which can overcome all or some of the disadvantages and limitations of the prior art, as described herein above and more particularly of a selfemulsifiable formulation, which facilitates increased solubility, transport rate, bioavailability and bioabsorption of the immunosuppression agent. Objects of Invention This is the main object of the present invention to make a complete disclosure of a formulation, particularly of a selfemulsifiable formulation for oral administration, which can overcome all or some of the disadvantages and limitations of the prior art, as described herein above and more particularly of a selfemulsifiable formulation, which can facilitate the increased solubility, transport rate, bioavailability and bioabsorption of the immunosuppression agent. Another object of this invention is to propose for a selfemulsifiable formulation capable of making early bioavailability of the immunosuppression agent, particularly in the upper part of the gastrointestinal tract. Still another object of this invention is to propose a selfemulsifiable formulation, which can satisfactorily meet the clinical requirements. Still further an object of the present invention is to disclose a selfemulsifiable formulation, which can form microemulsions of particle size less than 200 nm, preferably less than 100 nm. Yet another object of this invention is to propose a selfemulsifiable formulation, which can administered orally after filling in a soft or hard shell, or in the form of solution. This is further an object of this invention to disclose a selfemulsifiable formulation, which can form microemulsions of particle size less than 200 nm, preferably less than 100 nm and a clear solution when administered orally in the form of microemulsions mixed with fruit juice, milk or any aqueous medium. This is still an object of this invention to disclose a selfemulsifiable formulation, which can form microemulsions of particle size less than 200 nm, preferably less than 100 nm when administered orally after filling in a soft or hard shell. This is yet an object of this invention to disclose a selfemulsifiable formulation, which on administration in a shell, particularly in a soft shell is made available at an early time, preferably in the upper part of the gastrointestinal tract in less than 12 minutes, more preferably in less than 10 minutes, by rupturing the shell in desired time of less than 12 minutes. This is still an object of this invention to disclose a selfemulsifiable formulation, which has better solubility and reduced variability, that is inter and intra patient bioabsorption variability. Still another an object of this invention is to disclose a selfemulsifiable formulation, which can be stored in the tropical countries for a longer time and can forms thermodynamically stable oil in water microemulsions in-situ, which are stable for more than 24 hrs. Yet another an object of this invention is to disclose a selfemulsifiable formulation and the method of preparation thereof. Further objects, advantages and preferred embodiments of the present invention will be more apparent from the following description when read in conjunction with the accompanying drawings, which are not intended to limit the scope of the present invention. Description of the Figures Figure 1 shows the phase diagram of the selfemulsifiable formulation in accordance to the preferred embodiments of the present invention. Figure 2 shows the phase diagram representing the relative concentration of oil phase, water phase and mixture of surfactants of the selfemulsifiable formulation in accordance to the preferred embodiments of the present invention. Figure 3 shows the comparative dissolution profile of experiments XIII, XIV and XV of the selfemulsifiable formulation in accordance to the preferred embodiments of the present invention and of Sandimmun Neoral, which is taken as standard. Figure 4 shows the percent amount of normalized particle size in experiment XV, the best preferred experiment of the selfemulsifiable formulation in accordance to the preferred embodiments of the present invention. Figure 5 shows the mean plasma concentration of the immunosuppression agent after administration of formulation, after filled in soft-shell, of experiment XV, the best preferred experiment of the selfemulsifiable formulation in accordance to the preferred embodiments of the present invention. Figure 6 shows the compositions of formulations prepared in accordance to the preferred method of the present invention. Brief Description of Invention Accordingly this invention provides a complete disclosure of a formulation, particularly of a selfemulsifiable formulation for oral administration, which has enhanced bioabsorption and immunosuppression activities, more particularly of a selfemulsifiable formulation for early delivery of drug, even more particularly of a selfemulsifiable formulation, which will form thermodynamically stable oil in water emulsion preferably in upper part of gastrointestinal tract and facilitate the early delivery of drug, particularly of the immunosuppression agent, still more particularly of a selfemulsifiable formulation not only having the improved bioavailability and bioabsorption but also the improved capability to release the drug in reduced time with reduced toxicity and variability, that is inter and intra patient bioabsorption variability. In accordance to the present invention a selfemulsifiable formulation is disclosed, which facilitates the increased solubility, transport rate, bioavailability and bioabsorption of an immunosuppression agent, wherein said formulation essentially comprises of an immunosuppression agent, hydrophilic agent, lipophilic agent, surfactants, antioxidant and preservatives. In accordance with one of the preferred embodiments of the present invention the formulation is made available in a shell, preferably a soft shell, wherein the shell essentially comprises gelatin, glycerin, water, one or more preservatives and one or more colorants. The formulation of the present invention can be prepared by known method. In accordance with a preferred embodiment of the present invention the preferred method, for preparation of the presently disclosed selfemulsifiable formulation comprises of dissolution of an immunosuppression agent in a hydrophilic agent followed by entrapping of solubilised immunosuppression agent with lipophilic agent, which in-tum is followed by treatment of oil entrapped solubilised form of drug with surfactants and the resulted solubilised drug entrapped with oil and surfactants is treated with preservative and antioxidant. Accordingly, the present relates to a selfemulsifiable formulation for oral administration, said formulation essentially comprises of immunosuppression agent, hydrophilic agent, lipophilic agent, surfactants, antioxidant and preservative, characterized in that :- said immunosuppression agent is lactam macrolide having immunosuppression activity and is present in an amount of about 2 to 10% by weight of the formulation; said hydrophilic agent is ethanol which is present in a weight ratio of about 1:0.5 to about 1:2.5 with respect to said immunosuppression agent; said lipophilic agent is medium chain triglycerides of caprylic and/or capric acids; said surfactants are the combination of transesterified caprylic and/or capric glycerides having a hydrophilic lipophilic balance (HLB) of about 14 and saponification value of about 85 to 105, polysorbate 80, and cremophor RH 40; said antioxidant is selected from a group consisting of alpha-tocopherol, ascorbyl palmitate, butyl hydroxy anisole, butyl hydroxy toluene, propyl gallate; and said preservative is selected from a group consisting of ethanol and benzyl alcohol. Accordingly, the present invention also relates to a method of preparation of selfemulsifiable formulation for oral administration, wherein said method comprises the following steps: -a) dissolution of the immunosuppression agent in the hydrophilic agent, b) entrapping the resulting solubilised immunosuppression agent with the lipophilic agent, c) treatment the resulting oil entrapped solubilised form of immunosuppression agent with the combination of surfactants, and d) treatment of the solubilised immunosuppression agent entrapped with oil and combination of surfactants with preservative and antioxidant. Accordingly, the present invention also relates to a process for preparation of a soft shell for the selfemulsifiable formulation for oral administration prepared in accordance with the presently disclosed process, wherein the shell is prepared by mixing gelatin, glycerin, water and one or more of preservatives and one or more of colorants. Detailed Description and Preferred Embodiments of Invention In accordance with this invention a selfemulsifiable formulation for oral administration, as described herein above, is disclosed, wherein said formulation essentially comprise of immunosuppression agent, hydrophilic agent, lipophilic agent, surfactants, antioxidant and preservative, wherein the immunosuppression agent is a lactam macrolide having irnmunosuppression activity; the hydrophilic agent is ethanol; the lipophilic agent is medium chain triglycerides of caprylic and/or capric acids; the surfactants are the combination of transesterified caprylic and/or capric glycerides (Labrasol®), polysorbate 80 and cremophore RH 40; the antioxidant is selected from a group consisting of alpha-tocopherol, ascorbyl palmitate, butyl hydroxy anisole, butyl hydroxy toluene, and propyl gallate; and the preservative is selected from a group consisting of ethanol and benzyl alcohol. In accordance with the most preferred embodiment of the present invention, it has been surprisingly found that particularly stable microemulsions of clinically acceptable particle size with enhanced bioavailability and reduced variability in inter and intra-patient dose response, are obtained by using as the lipophilic agent, medium chain triglycerides of caprylic acid and capric acid, named labrafac lipophile. In accordance with the preferred embodiment of the present invention the medium chain triglycerides of caprylic acid and capric acid, which is used as the lipophilic agent can be obtained by any known method, for example esterification of glycerol by caprylic acid and capric acid at high temperature. The medium chain triglyceride of caprylic acid and capric acid, which is selected for use as lipophilic agent has a specific gravity of about 0.93 to 0.96, a refractive index of about 1.44 to 1.46, an acid value of less than about 0.2, a saponification value of about 310 to 360 and an iodine value of less than about 1 and water content of less than about 0.5% by weight. In accordance with one of the preferred embodiments of the present invention the immunosuppression agent is cyclosporine, particularly cyclosporine A having immunosuppression activity. The polyglycolised transesterified caprylic and capric glycerides (Labrasol®) surfactant has hydrophilic lipophilic balance (HLB) of about 14 and a saponification value ofabout 85 to 105. The preservative, to protect the formulation during storage and use from any microbial growth, particularly in tropical regions, is selected from ethanol and benzyl alcohol. In accordance with the present invention the immunosuppression agent is taken in an amount of about 2 to 10%, preferably in an amount of about 5 to 10% by weight of the formulation. The immunosuppression agent is preferably present in a ratio of about 1:0.5 to 1:2.5 by weight or about 1:1.25 by weight with respect to the hydrophilic agent. The hydrophilic agent is ethanol, which is present in a weight ratio of about 1:0.5 to about 1:2.5 with respect to the immunosuppression agent. The ratio of immunosuppression agent to lipophilic agent, medium chain triglyceride of caprylic and capric acids is about 1:1.5 or 1:1.78 by weight for entrapment of solubilised immunosuppression agent, particularly cyclosporine, more particularly cyclosporine A. Still other lipophilic agent of the present invention includes combination of labrafac and labrasol, for example are present in a ratio of about 1:3, preferably of about 1:3.5, and more preferably of about 1:4 by weight. In accordance with the present invention labrasol acts as a surfactant. The surfactants, in accordance with the present invention, include polyglycolised transesterified caprylic and capric acids (Labrasol®) which is present in a ratio of about 2.2:1 or about 3.3:1 or about 4:1 by weight with respect to the lipophilic agent of the present invention. In accordance with the preferred embodiment of the present invention the combination of Labrasol® and cremophore RH 40 is present in a ratio of about 1.2:1 or about 2.5:1 by weight, and the combination of Labrasol® and polysorbate 80 is present in a ratio of about 2.7:1 or about 4.3:1 by weight. In accordance with one of the preferred embodiments of this invention the combination of Labrasol®, polysorbate 80 and cremophor RH 40 are present in a weight ratio of about 4.3:1:1.8 or about 2.7:1:2.3 respectively which give clear translucent microemulsions with a bluish tinge and a particle size less than 100 nm. The preservative, in accordance with the present invention includes benzyl alcohol in an amount of about 0.5 to 1% by weight of the formulation. The antioxidant, in accordance with the present invention includes alpha-tocopherol in an amount of about 0.00007 to 0.0009% by weight of the formulation. The formulations of the present invention can be prepared by known methods. The preferred method, in accordance with one of the preferred embodiments of this invention comprises the following steps ;- a) dissolution of the immunosuppression agent in the hydrophilic agent, b) entrapping the resulting solubilised immunosuppression agent with the lipophilic agent, c) treatment of the resulting oil entrapped solubilised form of the drug with the combination of surfactants, and d) treatment of the solubilised drug entrapped with oil and combination of surfactants with preservative and antioxidant. In accordance with the preferred method of the present invention the first step involves dissolution of a selected amount of immunosuppression agent in a selected amount of hydrophilic agent. The concentration of hydrophilic agent is optimized to such a level in the present invention, that it will keep the immunosuppression agent in solubilized form for the shelf life of the formulation. The solubilisation step of the presently disclosed method is followed by entrapping with a selected amount of the lipophilic agent, which acts as a carrier during absorption of the immunosuppression agent in the gastrointestinal tract. The third step of the presently disclosed process for manufacture of presently disclosed formulation involves treatment of oil entrapped solubilised form of drug with a selected amount of combination of the surfactants. The fourth step of the process involves treatment of solubilised drug entrapped with oil and the surfactants with a selected amount of the preservative and antioxidant. In accordance with one of the preferred embodiments of the present invention the formulation is made available in a shell, preferably soft shell, wherein the said shell essentially comprises of gelatin, glycerin, water and one or more preservatives, like methyl paraben or propyl paraben, and one or more colorants, like iron oxide black or titanium dioxide. In a preferred embodiment of the present invention, a formulation having presently disclosed composition and prepared in accordance with the preferred method, as described herein above is filled in a shell, preferably in a soft shell, and more preferably in a disintegrating soft gelatin shell, which becomes part of the formulation for oral administration and it cannot be separate entity of the medicament taken by the patient. However, the present invention is not restricted by making availability of the formulation filled in the presently disclosed shell. It is obvious to those who have knowledge of the art that the presently disclosed formulations can also be administered in the form of a solution or after filling in any of the known shells, which may be soft or hard shell. It is further obvious to those who have knowledge of the art that the presently disclosed shell can also be used for filling any other formulation including similar formulations. Therefore, in accordance with one of the preferred embodiments of the present invention a disclosure is made of shell essentially comprising gelatin, glycerin, water and one or more preservatives, like methyl paraben or propyl paraben, and one or more colorants, like iron oxide black or titanium dioxide, wherein gelatin is taken in an amount of about 35 to 50% by weight of the shell, glycerin is taken in an amount of about 15 to 30% by weight of the shell, the preservatives, like methyl paraben or propyl paraben are taken in an amount of about 0.2% to about 0.8% by weight of the shell, water is taken in an amount of about 30 to 45% by weight of the shell, and colorants, like iron oxide black or titanium dioxide are taken in an amount of about 0.5% by weight of the shell. It is obvious from the foregoing description that the advantages of the presently disclosed selfemulsifiable formulations for oral administration, as disclosed and described herein above includes increased solubility, transport rate, bioavailability and bioabsorption of the immunosuppression agent; capability of making early bioavailability of the immunosuppression agent, particularly in the upper part of the gastrointestinal tract; capability to meet satisfactorily the clinical requirements; capability to form microemulsions of particle size less than 200 run, preferably less than 100 nm whether administered orally in the form of microemulsions mixed with fruit juice, milk or any aqueous medium, or administered orally after filling in a soft or hard shell; capability to facilitate the availability of the immunosuppression agent, preferably in the upper part of the gastrointestinal tract in less than 12 minutes, more preferably in less than 10 minutes by rupturing the shell; reduced inter and intra patient bioabsorption variability; capability to be stored in the tropical countries for a longer time; capability to form thermodynamically stable oil in water microemulsions in-situ, which are stable for more than 24 hrs and also having capability to be administered orally after filling in a soft or hard shell, or in the form of solution. Formulations in accordance with preferred embodiments of the present invention have shown enhanced bioabsorption, bioavailability and immunosuppression activities as a result of entrapping the solubilised immunosuppression agent with the lipophilic agent and subsequent treatment with surfactants, preservatives and antioxidants before being filled into soft-gelatine shell which are capable of rupturing preferably in less than 10 minutes to deliver the formulation in upper part of gastrointestinal tract. The formation of thermodynamically stable oil in water microemulsions in-situ provides enhanced bioavailability and bioabsorption of the immunosuppression agent, which can as a result provide enhanced immunosuppression to be achieved. Experiments The presently disclosed formulations were prepared in accordance with the preferred method of preparation, as described herein above, and phase diagrams (Figure 1), relative concentrations of various phases, i.e. oil phase, water phase and mixture of surfactants (Figure 2), rupture identification test in dissolution medium by analysing the percent drug content at different time intervals (Figure 3), percent amount of normalised particle size (Figure 4) and mean plasma concentration of the drug (cyclosporine) after administration of the shell (Figure 5) were studied/carried out in case of selected preparations XIII, XIV and XV. Formulations of experiments I to XIII are not in accordance with the present invention and are for comparison purposes. The scope of the present invention is restricted by the formulations of experiments XIV and XV. It was observed that all formulations were clear solutions, some formulations were slightly turbid in contact with aqueous media but when subjected to particle size analysis, passes the microemulsion properties. The formulations were filled in soft gelatin shell of the present invention. The formulations were prepared having compositions as given in figure 6. For experimental purpose only different combinations of said agents were used. However, the combination of experiments XIII, XIV and XV, particularly of XIV and XV were observed to better and were according to the preferred embodiments of the present invention. These experimental formulations were subjected to microemulsion tests. From these experiments it was observed that presence of labrafac lipophile as lipopholic agent in combination with other selected agents improves the microemulsion quality significantly. Now referring to accompanying figures, the figure 1 shows the two way plot for cyclosporine microemulsion - phase behaviour. These phases are mixture of surfactants (I), oil phase (II) and water phase (III). Point 1 represents water in oil microemulsion existence, while point 2 represents oil in water microemulsion existence part and point 3 is coarse emulsion part while point 4 is micelle phase. According to this phase diagram, the oil phase (II) contains 10% of cyclosporine-A dissolved in hydrophilic agent and then entrapped in oil. The oil phase (II) concentration increase from 0% along the left-hand margin to 100% as shown by arrow. The concentration of aqueous phase (HI) increase from 0% along the right hand margin to 100% as shown by arrow, while the concentration of surfactants mixture (I) increase from 0% at the base line of the plot to 100% as shown by arrow. The relative portion of oil, surfactants and water phases will suitably lie with the area (2), i.e. microemulsion existence field as shown in the figure 1. All the experiments were carried out in the laboratory at a temperature less than 25°C having relative humidity less than 60%. The figure 2 shows three way plot for cyclosporine microemulsion. This figure represents the relative concentration of oil phase (II), water phase (III) and mixture of surfactants (I). The point A represents the preferred concentration of microemulsion that is oil phase (II), water phase (III) and surfactant phase (I). The figure 3 represents the comparative dissolution profile of experiments XIII, XIV, XV and standard experiment for which Sandimmun Neoral was taken as standard. The X-axis represents time in minutes required to rupture the shell as USP-specification for cyclosporine shells. The rupture time was identified by content analysis in the dissolution fluid. The Y-axis represents the percentage of cyclosporine dissolved in dissolution fluid, which was analysed by high performance liquid chromatography (HPLC). In view of stringent dissolution test specification of cyclosporine capsule USP in USP/NF 24 that each capsule should rupture within 15 minutes, the presently disclosed formulation of immunosuppression agent, particularly cyclosporine was also subjected to dissolution tests as per USP specifications and tested for rupture test and shell stability test. The soft gelatin shells having following compositions were used in four set of experiments for these studies :- Experiment No. -►A B C O Ingredient 4- | Composition Gelatin 35% 40% 45% 45% Glycerine 15% 25% 25% 20% Sorbitol 18.7% — — — Propyl Paraben 0.04% 0.04% 0.04% 0.04% Methyl Paraben 0.76% 0.76% 0.76% 0.76% Colorants 0.5% 0.5% 0.5% 0.5% Water 30.0% 33.7% 28.7% 33.7% The soft gelatin shells having above compositions were prepared in accordance to the preferred method of the present invention and were cured at lower humidity and temperature for less than 25°C for sufficient time. The cured shells were subjected to rupture test. The in-vitro dissolution conditions were maintained as follows :- Apparatus USP Type-II (paddle) Medium Water (500 ml) Rotation per minute (RPM) 50 Temperature of medium 37°C Time 15 mins As per USP dissolution test of cyclosporine, it mentions the rupture of the shell should be within 15 mins. In the present invention, the efforts were taken not only to comply with the dissolution but also to quantify the rupture time, which gives clear identification of the rupture. The rupture identification tests have been designed and were performed in dissolution medium by analysing the percent drug content at different time intervals, viz. 8, 12 and 15 minutes by HPLC. The percent drug contents for each rupture time interval are given in figure 3, as described herein above. The percent drug contents in case of experiments XIII, XIV, XV and standard (Sandimmun Neoral) were observed to be 30, 31.8, 35 and 0 respectively at time interval of 8 mins, and 75, 70.86, 75 and 28.73 respectively at time interval of 12 mins, and 90, 86.83, 95 and 91.01 respectively at time interval of 15 mins. This data clearly shows that the shell of the present invention releases higher amount of the drug as compared to the standard. The figure 4 represents percent amount of normalised particle size in experiment XV, the best mode of the present invention. The X-axis represents the particle diameter in nm and Y-axis represents the amount of normalised particle size in percent. It is observed from the figure that the mean particle size is less than 100 nm. The figure 5 represents the mean plasma concentration of cyclosporine after administration of shells of the present invention of experiment XV. The X-axis represents the time in hours and Y-axis represents mean plasma concentration in ng/ml. It is observed from the figure that the mean plasma concentration that is the bioavailability of the drug is more than the standard at the early part of the gastrointestinal tract and having the less variability in the inter and intra patient for the dose response. The presently disclosed formulation (experiment XV) was subjected to bioequivalence study and the results were compared with the standard - Sandimmun Neoral. The bioequivalence study of formulation of experiment XV, best mode of performing the present invention, was carried out on 24 healthy male subjects using 50 mg of sample of this preparation and the results were compared with 50 mg of sample of Sandimmun Neoral. All the subjects were adult, healthy, non-smoking males. The mean (+S.E.) age and weight for the subjects were 27.42 + 0.97 years and 63.63 + 1.38 kg respectively. Subjects were selected for the participation in the study after providing informed written consent and successfully completing a battery of medically related examinations including medical history, complete physical examination, electrocardiogram and a laboratory profile with hematological, urine and biochemical, tests. Subjects were excluded if they had received any drug that are known to induce the drug-metabolising enzymes within three months of study entry. History of hypersensitivity to any drug was ruled out. In a randomized cross over and comparative study designed, 24 subjects received these two preparations on two occasions with a wash out period of two weeks. Subjects reported to the test facility in the evening before drug administration. No food was permitted for at least 10 hrs before the administration of the drug. Next morning after attending to the morning routine, subjects were made to lie to supine. An indwelling teflon needle was introduced in the left fore arm vein and fasting blood sample was collected. Two shells of either formulations were administered with 240 ml of water. Blood was collected in centrifuge tube containing 0.1 ml of 10% ETDA. Post dose sampling time after drug administration were 0.50, 1.00, 1.50, 2.00, 2.50, 3.00, 3.50, 4.00, 5.00, 6.00, 8.00 10.00, 12.00, 24.00 and 48.00 hrs. Blood samples were centrifuged in cooling centrifuge, maintained at -20°C + 5°C; with appropriate labels, identifying subject numbers, study day and time of blood collection. Fluid intake was controlled and consistent for the first four hours following drug administration as follows : drug was administered with 240 ml of water, 280 ml of a non-caffeine containing soft drink provided 4.0 hrs post dose. Water was allowed ad libitum there after. Standarised breakfast, lunch and dinner were served to the subjects at 4.0, between 7 to 8 hrs and 14 hrs respectively. Emergence of symptoms, if any were noted by the subjects at the end of the study in the symptom check list formed. The subjects were housed in the laboratory for the entire period. It was randomised comparative study with a two way cross over design. Plasma cyclosporine levels were measured by HPLC method. The drug was extracted from plasma and injected on HPLC system. The chromatography was carried out on C18 column using acetonitrile:distilled water in the ratio of 70:30 (v/v) at flow rate of 1.0 ml per min at 80°C. The detection was carried out using a UV-detector. The lowest limit of qualification of the drug from plasma 20 ng/ml. Administration of standard formulation (Sandimmun Neoral) showed a miximum concentration of cyclosporine 218.2 ± 16.9 ng/ml in plasma (Cmax) (In Cmax 5.2979 + 0.0936) at 2.42 ± 0.16 hrs (Tmax), while that of test formulation (Experiment XV) showed a maximum concentration of cyclosporine 208.5 ± 12.8 ng/ml (Cmax) (In Cmax 5.2912 + 0.0673) at 2.29 ±0.11 hrs (Tmax). The AUC(o-t) for standard formulation was 518.35 + 50.15 ng/ml x hr (In AUC(0-t) 6.1406 + 0.1010) and for test formulation, it was 518.71 ± 46.97 ng/ml x hr (In AUC(0-t) 6.1238 + 0.1163). The AUC(0-oo) for standard formulation was 611.64 + 54.55 ng/ml x hr (In AUC(0-oo) 6.3262 + 0.0897) and for test formulation, it was 597.27 + 50.13 ng/ml x hr (In AUC(0-oo) 6.2847 ±0.1062). The elimination rate constants for standard and test formulations were 0.140 ± 0.023 hr-1 and 0.168 ± 0.028 hr-1 and elimination half-lives were 7.98 ± 0.97 hrs and 7.34 + 1.44 hrs respectively. In this study, with both the formulations, standard and experiment XV, cyclosporine was detected in plasma in few subjects at 0.50 hrs after ingestion of formulation. Cyclosporine was detected up to 8 hrs in some of the subjects post-dose with both the formulations. Cmax values, time at which they were achieved Tmax were comparable with both the formulations, so also were When ANOVA was applied with the subjects, period and treatment as variables no significant variation was observed for Tmax, whereas subject parameter was found significant for The 90% confidence interval for cyclosporine for the values were 87.26% to 104.34%, 84.10% to 117.23% and 81.76% to 114.60% respectively. For the log-transformed data they were 90.54% to 109.69%, 82.24% to 118.00% and 80.21% to 115.57% respectively. The ratio of the least squares means of the of the test/standard were 95.56%, 100.07% and 97.65% respectively. For the log-transformed data the ratios were 99.87%, 99.73% and 99.34% respectively. The power of test for cyclosporine for the value was 97.44% and for log-transformed data it was 91.15%. The inter-subject variability for cyclosporine for values were 17.54%, 33.18% and 33.31% respectively. For log-transformed data the values were 19.46%, 37.51% and 37.98% respectively. When of both the formulations were compared, experiment XV and Standimmun Neoral showed bioavailability of 100.07%. The bioequivalence data of both the formulations - standard and experiment XV using 50 mg shells is given below. The mean (ng/ml), S.D., S.E. and COV (%) were measured at time intervals of 0.00, 0.50, 1.00, 1.50, 2.00,2.50, 3.00, 3.50,4.00, 5.00,6.00, 8.00,10.00,12.00, 24.00 and 48.00 hrs. Time in Sandimmun Neoral Experiment XV hrs Mean (ng/ml) S.D. S.E. COV (%) Mean (ng/ml) S.D. S.E. COV (%) 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.50 19.1 56.4 11.5 295.81 22.8 42.0 8.6 184.41 1.00 66.7 95.3 19.5 142.81 71.8 51.4 10.5 71.58 1.50 137.2 92.1 18.8 67.13 121.0 62.1 12.7 51.34 2.00 150.6 77.5 15.8 51.50 160.6 74.2 15.1 46.17 2.50 163.4 78.4 16.0 48.01 164.9 62.5 12.8 37.89 3.00 159.8 92.2 18.8 57.72 157.2 72.6 14.8 46.17 3.50 114.7 57.6 11.8 50.25 109.8 64.7 13.2 58.96 4.00 75.3 62.7 12.8 83.27 73.2 58.1 11.9 79.41 5.00 37.9 39.6 8.1 104.54 42.3 43.9 9.0 103.96 6.00 21.4 27.9 5.7 130.08 19.0 25.6 5.2 134.78 8.00 4.6 10.7 2.2 232.42 7.0 14.3 2.9 203.34 10.00 1.2 5.7 1.2 489.71 0.0 0.0 0.0 0.0 12.00 1.1 5.5 1.1 490.04 0.0 0.0 0.0 0.0 24 0.0 0.0 0.0 0.0 0.0 0.0 0.0 0.0 48 0.0 0.0 0.0 0.0 0.0 0.0 0.0 0.0 AUCm n 518.35 245.75 50.16 47.41 518.72 230.14 46.98 44.37 AUC(o.i) 611.64 267.32 54.57 43.70 597.27 245.61 50.14 41.12 The above bioequivalence data shows that the trial of composition of formulation of experiment XV has less percentage of Coefficient of Variation (COV) and standard error (SE) than the standard formulation. From this data, it can be concluded that the presently disclosed formulation shows significantly less variability in inter and intra patient dose response than the standard formulation, which is a unique characteristic required for the formulation, particularly for the cyclosporine formulation microemulsions. From the above bioequivalence data, one another advantage of the presently disclosed formulation which is apparent, is that the soft gelatin shell having very low rupture time, that is, about 8 mins, will give fast release of the drug out of the formulation for the immediate bioavailability of the drug, that is, of the immunosuppression agent, that is, of the cyclosporine, i.e. 22.8 ng/ml in 30 mins as against standard formulation i.e. 19.1 ng/ml. We Claim: 1. A selfemulsifiable formulation for oral administration, said formulation essentially comprises of immunosuppression agent, hydrophilic agent, lipophilic agent, surfactants, antioxidant and preservative, characterized in that :- said immunosuppression agent is lactam macrolide having immunosuppression activity and is present in an amount of about 2 to 10% by weight of the formulation; said hydrophilic agent is ethanol which is present in a weight ratio of about 1:0.5 to about 1:2.5 with respect to said immunosuppression agent; said lipophilic agent is medium chain triglycerides of caprylic and/or capric acids; said surfactants are the combination of transesterified caprylic and/or capric glycerides having a hydrophilic lipophilic balance (HLB) of about 14 and saponification value of about 85 to 105, polysorbate 80, and cremophor RH 40; said antioxidant is selected from a group consisting of alpha-tocopherol, ascorbyl palmitate, butyl hydroxy anisole, butyl hydroxy toluene, propyl gallate; and said preservative is selected from a group consisting of ethanol and benzyl alcohol. 2. A selfemulsifiable formulation as claimed in claim 1, wherein said medium chain triglyceride of caprylic acid and capric acid has specific gravity of about 0.93 to 0.96, refractive index of about 1.44 to 1.46, acid value of less than about 0.2, saponification value of about 310 to 360 and an iodine value of less than about 1 and water content of less than about 0.5% by weight. 3. A selfemulsifiable formulation as claimed in claim 1, wherein said immunosuppression agent is cyclosporine-A having immunosuppression activity. 4. A selfemulsifiable formulation as claimed in claim 1, wherein said immunosuppression agent is taken in an amount of about 5 to 10% by weight of the formulation. 5. A selfemulsifiable formulation as claimed in claim 1, wherein said immunosuppression agent is taken in ratio of about 1:0.5 to 1:2.5 by weight or about 1:1.25 by weight with respect to said hydrophilic agent. 6. A selfemulsifiable formulation as claimed in claim 1, wherein the ratio of immunosuppression agent to lipophilic agent is about 1:1.5 or about 1:1.78 by weight. 7. A selfemulsifiable formulationas claimed in claim 1, wherein said transesterified caprylic acid and capric glyceride [labrasol®] is taken in the ratio of about 2.2:1, or about 3.3:1, or about 4:1 by weight with respect to said lipophilic agent. 8. A selfemulsifiable formulation as claimed in claim 1, wherein said transesterified caprylic acid and capric glyceride [labrasol®] and cremophore RH 40 are taken in the ratio of about 1.2:1 or about 2.5:1 by weight, and said transesterified caprylic acid and capric glyceride [labrasol®] and polysorbate 80 are taken in the ratio of about 2.7:1 or about 4.3:1 by weight. 9. A selfemulsifiable formulation as claimed in claim 1, wherein said transesterified caprylic acid and capric glyceride [labrasol®], polysorbate 80 and cremophor RH 40 are taken in the ratio of about 4.3:1:1.8 or about 2.7:1:2.3 by weight respectively. 10. A selfemulsifiable formulation as claimed in claim 1, wherein said preservative is benzyl alcohol and is taken in the amount of about 0.5 to 1% by weight of the formulation. 11. A selfemulsifiable formulation as claimed in claim 1, wherein said antioxidant is alpha-tocopherol and is taken in the amount of about 0.00007 to 0.0009% by weight of the formulation. 12. A selfemulsifiable formulation as claimed in claim 1, wherein said formulation forms microemulsions of particle size less than 200 nm or less than 100 nm on contact with gastric juice or aqueous medium. 13. A selfemulsifiable formulation for oral administration substantially as hereinbefore described with reference to the accompanying examples XIV and XV. 14. A method of preparation of selfemulsifiable formulation for oral administration according to claims 1 to 13, wherein said method comprises the following steps ;- a) dissolution of the immunosuppression agent in the hydrophilic agent, b) entrapping the resulting solubilised immunosuppression agent with the lipophilic agent, c) treatment the resulting oil entrapped solubilised form of immunosuppression agent with the combination of surfactants, and d) treatment of the solubilised immunosuppression agent entrapped with oil and combination of surfactants with preservative and antioxidant. 15. A method of preparation of selfemulsifiable formulation for oral administration substantially as hereinbefore described with reference to the accompanying examples XIV and XV. 16. A selfemulsifiable formulation as claimed in any one of the preceding claims 1 to 13, wherein said formulation is in a soft shell, wherein the said shell essentially comprises of gelatin, glycerin, water and one or more of preservatives, like methyl paraben, propyl paraben, and one or more of colorants, like iron oxide black, titanium dioxide. 17. A selfemulsifiable formulation in a soft shell as claimed in claim 16, wherein gelatin forms about 35 to 50% by weight of the shell. 18. A selfemulsifiable formulation in a soft shell as claimed in claim 16, wherein glycerin forms about 15 to 30% by weight of the shell. 19. A selfemulsifiable formulation in a soft shell as claimed in claim 16, wherein the preservatives forms about 0.2% to about 0.8% by weight of the shell. 20. A selfemulsifiable formulation in a soft shell as claimed in claim 16, wherein water forms about 30 to 45% by weight of the shell. 21. A selfemulsifiable formulation in a soft shell as claimed in claim 16, wherein colorant forms about 0.5% by weight of the shell. 22. A shell for selfemulsifiable formulation for oral administration substantially as hereinbefore described with reference to the accompanying examples XIV and XV. Dated this 18th day of September, 2000 Dr. Ramesh Kr. MEHTA Patent Attorney for the Applicants MEHTA & MEHTA ASSOCIATES

Documents:

254-mumnp-2003-abstract(27-01-2006).doc

254-mumnp-2003-abstract(27-01-2006).pdf

254-MUMNP-2003-ABSTRACT(AMENDED)-(27-1-2006).pdf

254-MUMNP-2003-ABSTRACT(GRANTED)-(7-12-2006).pdf

254-mumnp-2003-cancelled page(27-01-2006).pdf

254-MUMNP-2003-CANCELLED PAGES(27-1-2006).pdf

254-mumnp-2003-claim(granted)-(27-01-2006).doc

254-mumnp-2003-claim(granted)-(27-01-2006).pdf

254-MUMNP-2003-CLAIMS(24-2-2003).pdf

254-MUMNP-2003-CLAIMS(AMENDED)-(13-10-2005).pdf

254-MUMNP-2003-CLAIMS(GRANTED)-(7-12-2006).pdf

254-MUMNP-2003-CORRESPONDENCE(17-5-2006).pdf

254-MUMNP-2003-CORRESPONDENCE(27-9-2012).pdf

254-mumnp-2003-correspondence(ipo)-(07-12-2006).pdf

254-MUMNP-2003-CORRESPONDENCE(IPO)-(22-12-2006).pdf

254-mumnp-2003-correspondence1(19-05-2004).pdf

254-mumnp-2003-correspondence2(10-01-2007).pdf

254-MUMNP-2003-DESCRIPTION(COMPLETE)-(24-2-2003).pdf

254-MUMNP-2003-DESCRIPTION(GRANTED)-(7-12-2006).pdf

254-MUMNP-2003-DRAWING(24-2-2003).pdf

254-mumnp-2003-drawing(27-01-2006).pdf

254-MUMNP-2003-DRAWING(AMENDED)-(27-1-2006).pdf

254-MUMNP-2003-DRAWING(GRANTED)-(7-12-2006).pdf

254-mumnp-2003-form 1(04-04-2005).pdf

254-MUMNP-2003-FORM 1(11-3-2003).pdf

254-MUMNP-2003-FORM 1(24-2-2003).pdf

254-mumnp-2003-form 1(27-01-2006).pdf

254-mumnp-2003-form 13(03-08-2005).pdf

254-mumnp-2003-form 13(16-08-2005).pdf

254-mumnp-2003-form 13(27-01-2006).pdf

254-MUMNP-2003-FORM 13(27-9-2012).pdf

254-mumnp-2003-form 19(19-05-2004).pdf

254-MUMNP-2003-FORM 2(COMPLETE)-(24-2-2003).pdf

254-mumnp-2003-form 2(granted)-(27-01-2006).doc

254-mumnp-2003-form 2(granted)-(27-01-2006).pdf

254-MUMNP-2003-FORM 2(GRANTED)-(7-12-2006).pdf

254-MUMNP-2003-FORM 2(TITLE PAGE)-(24-2-2003).pdf

254-MUMNP-2003-FORM 2(TITLE PAGE)-(GRANTED)-(7-12-2006).pdf

254-mumnp-2003-form 26(04-04-2005).pdf

254-mumnp-2003-form 3(04-04-2005).pdf

254-mumnp-2003-form 3(16-08-2005).pdf

254-MUMNP-2003-FORM 3(24-2-2003).pdf

254-mumnp-2003-form 3(27-01-2006).pdf

254-mumnp-2003-form 5(04-04-2005).pdf

254-MUMNP-2003-FORM 5(24-2-2003).pdf

254-mumnp-2003-other document(13-10-2005).pdf

254-mumnp-2003-pct-ipea-409(24-02-2003).pdf

254-mumnp-2003-pct-isa-210(24-02-2003).pdf

254-MUMNP-2003-PETITION UNDER RULE 137(3-10-2005).pdf

254-mumnp-2003-power of attorney(03-03-2003).pdf

254-mumnp-2003-power of attorney(24-02-2003).pdf

254-MUMNP-2003-SPECIFICATION(AMENDED)-(27-1-2006).pdf

254-MUMNP-2003-SPECIFICATION(AMENDED)-(3-8-2005).pdf

254-MUMNP-2003-SPECIFICATION(AMENDED)-(4-4-2005).pdf

254-MUMNP-2003-WO INTERNATIONAL PUBLICATION REPORT(24-2-2003).pdf