CA2309033C - Lacrimal gland specific emulsions for topical application to ocular tissue - Google Patents
Lacrimal gland specific emulsions for topical application to ocular tissue Download PDFInfo
- Publication number
- CA2309033C CA2309033C CA002309033A CA2309033A CA2309033C CA 2309033 C CA2309033 C CA 2309033C CA 002309033 A CA002309033 A CA 002309033A CA 2309033 A CA2309033 A CA 2309033A CA 2309033 C CA2309033 C CA 2309033C
- Authority
- CA
- Canada
- Prior art keywords
- cyclosporin
- emulsion
- polysorbate
- castor oil
- pharmaceutical composition
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired - Lifetime
Links
Abstract
A pharmaceutical composition is disclosed in the form of a nonirritating emulsion which includes at least one cyclosporin in admixture with a higher fatty acid glyceride and polysorbate 80. More particularly, the cyclosporin may be cyclosporin A and the higher fatty acid glyceride may be castor oil. Composition has been found to be of a high comfort level and low irritation potential suitable for delivery of medications to sensitive areas such as ocular tissues with enhanced absorption in the lacrimal gland. In addition, the composition has stability for up to nine months without crystallization of cyclosporin.
Description
'1~
LACRIMAL GLAND SPECIFIC EMULSIONS FOR TOPICAL
APPLICATION TO OCULAR TISSUE
The present invention generally relates to novel pharmaceutical compositions incorporating chemicals ZO Which are poorly soluble in water and is more particu larly related to a novel ophthalmic emulsion including cyclosporin in admixture with castor oil and polysor bate 80 with high comfort level and low irritation . potential.
Cyclosporins are a group of nonpolar cyclic oligopeptides with known immunosuppressant activity..
In addition, as set forth in U.S. Patent No.
4,839,342, cyclosporin (sometimes referred to in the literature as "cyclosporine") has been found as effective in treating immune medicated :keratoconjune-tivitis sicca (KCS or dry eye disease) in a patient suffering therefrom.
.As hereinabove noted, cyclosporin comprises a group of cyclic oligopeptides and the major component thereof is cyclosporin A (C~2H111N11012)Whzch has been identified along with several other minor metabolites, cyclosporin B through I. In addition, a number of ,30 synthetic analogs have been prepared.
In general, commercially available cyclosporins . may contain a mixture of several individual cyclo-sporins which all share a cyclic peptide structure consisting of eleven amino acid residues with a total molecular weight of about 1,200, but with different' substituents or configurations of some of the amino acids.
It should be appreciated that reference to the term "cyclosporin" or "cyclosporins" is used through-out the present specification in order to designate the cyclosporin component in the composition of the present invention.
However, this specific reference is intended to include any individual member of the cyclosporin group as well as admixtures of two or more individual cyclo-sporins, whether natural or synthetic.
The activity of cyclosporins, as hereinabove noted, is as an immunosuppressant and in the enhance-ment or restoring of lacrimal gland tearing.
This activity can be enhanced if it is possible to enhance the absorption of the cyclosporin in the lacrimal gland. The present invention provides for a formulation and method that produces optimal cyclo-sporin A concentrations in the lacrimal gland and other ocular surface tissues.
Unfortunately, the solubility of cyclosporin in water is extremely low and as elaborated in U.S.
Patent No. 5,051,402, it has been considered not merely difficult but practically impossible to prepare -30 a pharmaceutical composition containing cyclosporin dissolved in an aqueous medium.
As reported, the solubility of cyclosporin in water is between about 20 ug/ml to 30 ~g/ml for cyclosporin A. Hence, heretofore prepared formula-tions incorporating cyclosporin have been prepared as oily solutions containing ethanol. However, these preparations limit the bioavailability to oral prep arations and this is believed to be due to the separ ation of cyclosporin as a solid immediately after it comes into contact with water, such as in the mouth or eye of a patient.
In the case of injectable preparations of cyclo-sporin, they first must be diluted with physiological saline before intravenous administration but this is likely to result in the precipitation of cyclosporin and therefore may be considered undesirable for intravenous administration.
Surface active agents such as polyoxyethylated castor oil have been utilized as solubilizers to in-ject preparations in order to prevent cyclosporin from separating. However, this also may give rise to safety problems (see U.S: Patent No. 5,051,402).
The practical usefulness of cyclosporin would be greatly enhanced if administration thereof could be effective; for example, cyclosporin's effectiveness in the treatment of ocular symptoms of Behcet's Syndrome.
However, if it is administered orally for the treat-ment of these symptoms, the accompanying side effects due to systemic circulation may cause adverse reac-tions such as hypertrichosis or renal dysfunction.
On the other hand, if oily preparations contain-- 30 ing cyclosporin are applied directly to the eyes, ir ritation or a clouding of visual field may result.
This plus the difficulty in formulating cyclosporin limits its use in formulations that would be useful during keratoplasty as well in the treatment of herpetic keratitis and spring catarrh.
LACRIMAL GLAND SPECIFIC EMULSIONS FOR TOPICAL
APPLICATION TO OCULAR TISSUE
The present invention generally relates to novel pharmaceutical compositions incorporating chemicals ZO Which are poorly soluble in water and is more particu larly related to a novel ophthalmic emulsion including cyclosporin in admixture with castor oil and polysor bate 80 with high comfort level and low irritation . potential.
Cyclosporins are a group of nonpolar cyclic oligopeptides with known immunosuppressant activity..
In addition, as set forth in U.S. Patent No.
4,839,342, cyclosporin (sometimes referred to in the literature as "cyclosporine") has been found as effective in treating immune medicated :keratoconjune-tivitis sicca (KCS or dry eye disease) in a patient suffering therefrom.
.As hereinabove noted, cyclosporin comprises a group of cyclic oligopeptides and the major component thereof is cyclosporin A (C~2H111N11012)Whzch has been identified along with several other minor metabolites, cyclosporin B through I. In addition, a number of ,30 synthetic analogs have been prepared.
In general, commercially available cyclosporins . may contain a mixture of several individual cyclo-sporins which all share a cyclic peptide structure consisting of eleven amino acid residues with a total molecular weight of about 1,200, but with different' substituents or configurations of some of the amino acids.
It should be appreciated that reference to the term "cyclosporin" or "cyclosporins" is used through-out the present specification in order to designate the cyclosporin component in the composition of the present invention.
However, this specific reference is intended to include any individual member of the cyclosporin group as well as admixtures of two or more individual cyclo-sporins, whether natural or synthetic.
The activity of cyclosporins, as hereinabove noted, is as an immunosuppressant and in the enhance-ment or restoring of lacrimal gland tearing.
This activity can be enhanced if it is possible to enhance the absorption of the cyclosporin in the lacrimal gland. The present invention provides for a formulation and method that produces optimal cyclo-sporin A concentrations in the lacrimal gland and other ocular surface tissues.
Unfortunately, the solubility of cyclosporin in water is extremely low and as elaborated in U.S.
Patent No. 5,051,402, it has been considered not merely difficult but practically impossible to prepare -30 a pharmaceutical composition containing cyclosporin dissolved in an aqueous medium.
As reported, the solubility of cyclosporin in water is between about 20 ug/ml to 30 ~g/ml for cyclosporin A. Hence, heretofore prepared formula-tions incorporating cyclosporin have been prepared as oily solutions containing ethanol. However, these preparations limit the bioavailability to oral prep arations and this is believed to be due to the separ ation of cyclosporin as a solid immediately after it comes into contact with water, such as in the mouth or eye of a patient.
In the case of injectable preparations of cyclo-sporin, they first must be diluted with physiological saline before intravenous administration but this is likely to result in the precipitation of cyclosporin and therefore may be considered undesirable for intravenous administration.
Surface active agents such as polyoxyethylated castor oil have been utilized as solubilizers to in-ject preparations in order to prevent cyclosporin from separating. However, this also may give rise to safety problems (see U.S: Patent No. 5,051,402).
The practical usefulness of cyclosporin would be greatly enhanced if administration thereof could be effective; for example, cyclosporin's effectiveness in the treatment of ocular symptoms of Behcet's Syndrome.
However, if it is administered orally for the treat-ment of these symptoms, the accompanying side effects due to systemic circulation may cause adverse reac-tions such as hypertrichosis or renal dysfunction.
On the other hand, if oily preparations contain-- 30 ing cyclosporin are applied directly to the eyes, ir ritation or a clouding of visual field may result.
This plus the difficulty in formulating cyclosporin limits its use in formulations that would be useful during keratoplasty as well in the treatment of herpetic keratitis and spring catarrh.
Heretofore, as for example in U.S. Patent No.
5,051,402, attempts have been made to dissolve suffi-cient cyclosporin in an aqueous solvent system so as to reach an effective concentration for treatment.
Importantly, this solvent system does not contain any surface active agent such as polyoxyethylated castor oil.
Conceptually, the purpose of dissolving the cyclosporin in an aqueous solvent system is to enable contact with body fluids which would merely constitute dilution of the aqueous solvent system which hopefully would eliminate the immediate precipitation of cyclo sporin when contacted with the water content of the body fluids.
For direct use in the eye, cyclosporin has been formulated with a number- of pharmaceutically accept-able excipients, for example, animal oil, vegetable oil, an appropriate organic or aqueous solvent, an artificial tear solution, a natural or synthetic poly-mer or an appropriate membrane.
Specific examples of these pharmaceutically acceptable excipients, which may be used solely or in combination, are olive oil, arachis oil, castor oil, mineral oil, petroleum jelly, dimethyl sulfoxide, chremophor, liposomes, or liposome-like products or a silicone fluid, among others.
In summary, a great deal of effort has been ex-pended in order to prepare a pharmaceutical composi-tion containing cyclosporin dissolved in an aqueous medium or cyclosporin prepared as an oily solution.
However, successful formulations have yet to be accom-plished as evidenced by the lack of commercial prod-ucts.
As hereinabove noted, it has been reported that cyclosporin has demonstrated some solubility in oily preparations containing higher fatty acid glycerides such as olive oil, peanut oil, and/or castor oil.
These formulations frequently produce an unpleasant sensation when applied to the eye because of stimula-tion or the viscousness which is characteristic of these oils.
Another drawback of these formulations is that they contain a high concentration of oils, and oils exacerbate the symptoms of certain ocular surface diseases such as dry eyes, indicated by cyclosporin.
Therefore, these oily formulations may not be clini-cally acceptable. Additionally, these formulations often suffer from physical instability due to cyclo-sporin°~ propensity to undergo conformational change and cr;~~stallize out. The-crystallization problem has been noticed in formulations containing corn oil or medium chain triglycerides. Lastly, these formula-tions often have a low thermodynamic activity (degree of saturation) of cyclosporin which leads to a poorer drug bioavailability.
It may be possible to minimize the problems related to unpleasant sensation and syndrome exacerba-tion by reducing the oil content and dispersing the oil phase in water into an emulsion. However, it is not an easy task to formulate an ophthalmic emulsion because one indispensable class of ingredients in an emulsion system is emulsifiers, and the majority of emulsifiers is highly irritating to the eyes.
The present invention is directed to an emulsion system which utilizes higher fatty acid glycerides but in combination with polysorbate 80 which results in an emulsion with a high comfort level and low irritation potential suitable for delivery of medications to sen-sitive areas such as ocular tissues. Further, the present invention provides a pharmaceutical composi-tion and method for causing preferential absorption of cyclosporin in the lacrimal gland. That is, for a given instillation of the composition into an eye, a greater amount of absorption occurs in the lacrimal gland for formulations made in accordance with the present invention than heretofore utilized formula tions.
SUMMARY OF THE INVENTION
In accordance with the present invention, a non-irritating pharmaceutical composition with high com-fort level and low irritation potential suitable for delivery to sensitive areas such as ocular tissues comprises cyclosporin in admixture with an emulsifying amount of a higher fatty acid glycerol and polysorbate 80. More particularly, the composition may comprise cyclosporin A and the higher fatty acid glyceride may comprise castor oil.
Preferably, the weight ratio of the castor oil to the polysorbate 80 is between about 0.3 to about 30 and a weight ratio of the cyclosporin to castor oil is below 0.16. More preferably, the weight ratio of castor oil to polysorbate 80 is between 0.5 and 12.5, and the weight ratio of cyclosporin to castor oil is between 0.12 and 0.02.
When cyclosporin is dissolved in the oil phase in accordance with the present invention, the emulsion is found to be physically stable upon long term storage.
No crystallization of cyclosporin was noticed after nine months at room temperature. Moreover, the cyclosporin emulsion is formulated in such a way that the drug has reasonably high thermodynamic activity, yet without the crystallization problem.
Importantly, the composition of the present in-vention provides for enhanced absorption of the cyclo-sporin in the lacrimal gland of the eye. In this manner, the activity of the cyclosporin in restoring lacrimal gland tearing is increased. That is, since a greater amount of cyclosporin is absorbed into the lacrimal gland, more of the cyclosporin is effective in producing lacrimal gland tearing than heretofore possible.
BRIEF DESCRIPTION OF THE DRAWINGS
The advantages and features of the present inven-tion will be better understood by the following description when consideYed in conjunction with the accompanying drawings in which:
Figure 1 is a bar chart of conjunctival concen-tration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye;
Figure 2 is a bar chart of cornea concentration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye;
Figure 3 is a bar chart of ciliary body concen-tration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye;
and Figure 4 is a bar chart of lacrimal gland concen-tration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye.
DETAILED DESCRIPTION
As hereinabove noted, cyclosporin is available as a mixture in which the principal ingredient is cyclo-_g_ sporin A with significant, but smaller, quantities of other cyclosporins such as cyclosporin B through I.
However, as also hereinabove noted, the present inven tion may be applied to either a pure cyclosporin or to a mixture of individual cyclosporins.
The discovery on which the present invention is founded relates to a combination of a higher fatty acid glyceride and an emulsifier and dispersing agent, polysorbate 80. The selection of these components could not have been anticipated on the basis of con-ventional thinking.
For example, although it is well known that cyclosporin may be used in combination with castor oil, this combination is irritating to sensitive tissues such as the eye. Thus, conventional teaching in the art is away from a formulation which utilizes a higher fatty acid glyceride, such as castor oil, and cyclosporin.
Stated another way, there is no way of deducing that the use of an emulsifier and dispersing agent such as polysorbate 80 will reduce the irritation po-tential of an emulsion utilizing castor oil. There are no examples of polysorbate in combination with castor oil which, when admixed to cyclosporin, pro-duces an emulsion with a high comfort level and low irritation potential suitable for the delivery of -30 medication to sensitive areas such as ocular tissues.
The present invention achieves a stable solution state of cyclosporin. This stable solution state is another important performance characteristic differ-entiating the present invention from the conventional oil systems. Cyclosporin is notorious for its ten-WO 95131211 P~.TfUS95/06302 _g_ dency to precipitate out in conventional oil systems in which it is fully dissolved initially.
In accordance with the present invention, the emulsions can be further stabilized using a polyelec-trolyte, or polyelectrolytes if more than one, from the family of cross-linked p.olyacrylates, such as carbomers and Pemulen~.
Pemulen~ is a polymeric emulsifier having a CTFA
name of Acryl~tes/C10-30 Alkyl Acrylate Cross-Polymer and is described in the "Garbomer 1342" monograph in the United States Pharmacopeial National Formuiary, United States Pharmacopeial Gonvention inc., 2002. ._ In addition, the tonicity of the emulsions can be further adjusted usincr a.lvcerine, mannitol, or sorbi-tol if desired. The pH of the emulsions can be ad-justed in a conventional manner using sodium hydroxide to a near physiological pH level and while buffering agents are not required, suitable buffers may include phosphates, citrates, acetates and borates.
While the preferable medications in accordance with the present invention include cyclosporin; other chemicals which are poorly soluble in water such as indomethacin and steroids such as androgens, predniso .lone, prednisolone acetate, fluorometholone, and dexamethasones, may be emulsified with castor oil and polysorbate 80 resulting in a composition with similar -30 low irritation potential.
The invention is further illustrated by the following =xamples with all parts and percentages expressed .by weight. The cyclosporin used in the examples was supplied by Sandoz.
WO 95/31211 PCTlUS95106302 Example 1 A B C D E
Cyclosporin 0.40% 0.20% 0.20% 0.10% 0.05%
A
Castor oil 5.00% 5.00% 2.50% 1.25% 0.625%
Polysorbate 1.00% 1.00% 1.00% 1.00% 1.00%
Pemulenm 0.05% 0.05% 0.05% 0.05% 0.05%
G1 cerine 2.20% 2.20% 2.20% 2.20% 2.20%
NaOH qs qs s s qs Purified waterqs qs qs qs qs pH 7.2-7.67.2-7.67.2-7.6 7.2-7.67.2-7.6'.
Example 2 A B C D
Castor oil 5.00% 2.50% 1.25% 0.625%
Pol sorbate 1.00% 1.00% 1.00% 1.00%
Pemulenm 0.05% 0.05% 0.05% 0.05%
Glycerine 2.20 2.20% 2.20% 2.20%
NaOH s s s s 2 0 Purified waters s s s pH 7.2-7.67.2-7.67.2-7.67.2-?.6' Example 3 A
Castor oil 2.50%
Polysorbate 80 0.75%
Carbomer 1382 0.05%
Glycerine 2.20%
3 0 NaOH qs Purified water qs pH 7.2-7.6 WO 95/31211 PC'TIUS95/06302 Example 4 A
Castor oil 5.00%
Polysorbate 80 0.75%
Carbomer 981 0.05%
G1 cerine 2.20%
NaOH s Purified water qs pH 7.2-7.6 The formulations set forth in Examples 1-4 were made for treatment of keratoconjunctivitis sicca (dry eye) syndrome with Examples 2, 3 and 4 without the active ingredient cyclosporin utilized to determine the toxicity of the emulsified components.
The formulations in Examples 1-4 were applied to rabbit eyes eight times a day for seven days and were found to cause only slight to mild discomfort and slight hyperemia in the rabbit eyes. Slit lamp exam-ination revealed no changes in the surface tissue. In addition, the cyclosporin containing castor oil emul-sion, as hereinabove set forth in Examples lA-1D, was also tested for ocular bioavailability in rabbits; and the therapeutic level of cyclosporin was found in the tissues of interest after dosage. This substantiates that cyclosporin in an ophthalmic delivery system is useful for treating dry eye as set forth in U.S.
'30 Patent No. 4,839,342.
In addition, no difference in toxicity was found between formulations with cyclosporin (Examples lA-1D) and formulations without cyclosporin (Examples 2-4).
The formulations set forth in Examples 1-4 were found to be physically stable upon long term storage.
pGTIUS95/06302 With regard to formulations lA-1D, no crystallization of cyclosporin was noticed after nine months at room temperature.
Further, other higher fatty acid glycerides such as olive oil, peanut oil and the like may also be utilized with the polysorbate 80 with similar results regarding biotoxicity.
The following examples demonstrate the activity of the composition in accordance with the present invention for enhanced absorption of cyclosporin A in the lacrimal gland.
Materials The [Mebmt-3H]-cyclosporin-A (lot #TRQ6553) was prepared by Amersham International (Buckinghamshire, England) with radiochemical purity of -98% (by reversed phase HPLC) and specific activity of 2.6 Ci/mmol (2.16 mCi/mg). The 3H-label is a metabolic-ally stable position as shown by the asterisk. The radiolabeled CsA was supplied as an ethanol solution (1 mCi/ml). All organic solvents used in the procedures described in this study were "HPLC grade".
all other chemicals and reagents were analytical grade unless otherwise noted.
The compositions of the six formulations tested - - 30 are listed in Table A.
WO 95/31211 . PCTfi3S9510G302 TABLE A
Castor Miglyol Aqueous- Polyoxyl ngredients astor Oil-in- ~ Cyclo-Oil-in.-olyoxyl40 with Oil Water dextrinWater 40 Edetate j Emulsion Emulsion C clos orin-A 0.20 0.20 0.10 0.20 0.05 0.05 C clodextrin 14 Castor Oil 99.8 1.25 Miglyoi* OiI
Pluronic* i_121 0.75 ~- P123 Tween* 80 I . 00 Gl cerin 2.20 2.20 Pemulen~ TR-2 0.05 Carbopol* 981 0 . 05' Polyoxyl 40 20 20 Steavate (mg) FiPMC 0.3 0.3 Butylated H drox toluene 0.001 0.001 Ethanol(9200 rood) 0.1 Sodium Chloride 0.73 0.73 Sodium Mono hos hate 0.2 0.2 Disodium Edetate 0.1 ~~
Water QS QS QS QS QS
Batch Size 1 g 5 g 1 g 5 g 1 g 1 g The radiolabeled formulations were formulated to ensure that the radioactivity was homogeneous throughout the vehicle. The, expected radioactivity concentrations of the radiolabeled drug formulations were 1-2 mCi/ml. The expected specific activity of radiolabeled cyclosporin A (CsA) formulations was 0.5-2 mCi/mg. All test articles were stored at ambient temperature.
* Trade mark Analysis of Test Drug Formulations The test formulations were analyzed in triplicate by HPLC to determine the concentration of CsA and radiochemical purity of the CsA dosing solutions (>93%) before dosing. The radioactive concentrations of the test formulations were quantified by liquid scintillation counting (LSC).
l0 Chromatographic Conditions Pump: Beckman Model 126 (Beckman Instruments, San Ramon, CA) Mobile phase: Acetonitrile: 0.03a H3POq in water, pH 3 (65:35 v/v) Flow rate: 1.0 ml/min Column: Supercosil C8, 7.5 cm x 4.6 mm, 3 ~cm (Supelco, Bellefonte, PA) Superguard LC-8 (Supelco) Column heater (Bio-rad, Richmond, CA) at 60-70C
Injector: WISP 712B (Waters Associates, Milford, MA) 1aC detector: Radio Isotope 171 Detector (Beckman Instruments) Scintillant: Ready Flow III (Beckman Instruments), Flow Rate of '4 ml/min W detector: Model 166 (Beckman Instruments), 2 0 2 nm - Data processor: Beckman System Gold (Beckman Instruments) Run Time: 15 min Retention Time: 6 min (cyclosporin A) Animals Female New Zealand albino rabbits were obtained and quarantined for at least five days before procedures. Animals were housed in temperature- and humidity-controlled rooms. Food and tap water were provided ad libitum. Fifty-eight rabbits (2-3 kg) were selected Pram the colony to minimize bias. They were individually identified by ear tags and appeared to be healthy.
Dos inct The animals were divided into six groups of nine I5 rabbits; each group was treated with one of the six CsA formulations. During dosing, the lower eyelid of each rabbit was gently pulled away from the eye and 35 ~cl of the formulation were administered in the lower conjunctival cul-de-sac of each eye. After dosing, the upper and lower eyelid were handheld closed for '5 seconds and released. The animals were observed visually for any signs of tearing or ocular discomfort.
Samr~li,ng Tissues were collected at 20-min., 6-hr. and 24-hr. post-dose for each group. Three rabbits (six eyes) were used at each time point. At the specific sampling times, the animals were euthanized by an intravenous injection of 0.5-1 ml Eutha-6 (Western Supply Co., Arcadia, California) via marginal ear vein. Each eye was then rinsed with normal saline.
The aqueous humor ('200 ~1) was removed by means of a 0.5~m1 tuberculin syringe. The orbital lacrimal gland ('400 mg) , upper and lower bulbar conjunctivae ('S0 mg each), corneal ('50 mg) and iris-ciliary body ('S0 mg) were dissected. The tissues dissected were blotted dry and weighed. Ocular tissue and aqueous humor samples from both eyes were collected from four untreated animals to be used as blank samples.
Analysis of Radioactivity An aliquot of aqueous humor (50-175 ~.1) was counted directly in 10 ml of Ready-Solv HP by LSC.
Tissue and blood samples were weighed into combustion cones prior to combustion in a Model 307 Packard Tissue Oxuduzer (Packard Co., Downers Grove, Illinois). After combustion of the tissue samples, 3H20 was trapped in the Monophase-S solution (Packard) and the radioactivity of the samples was determined by LSC in a Beckman Model 1801 or 3801 scintillation counter (Beckman Instruments, San Ramon, California).
Data Analyses Excel software (version 4.0, Microsoft Corp, Redmond, Washington) was used for data analysis.
concentrations of total radioactivity in the tissue samples were expressed as dpm/g or dpm/ml and converted to ng equivalents (eq) of CsA/g or ml, using the specific activity of the dosing formulations.
Mean, standard deviation (SD) or standard error of the mean (SEM) was calculated according to standard methods. Radioactivity levels were not considered - -30 significant unless the dpm was greater than twice that of background b=(blanks).
Comparisons of tissue drug concentrations at each time point for the formulations were determined by one-factor ANOVA. All statistical comparisons were made using StatView~ (version 1.03, Abacus Concepts, Inc., Berkeley, California). the Fisher and Scheffe F tests were used to determine significant differences between formulations at the 95% level (a = 0.05). The rejection criteria for excluding any outlier data was based on standard outlier tests. No mere than one outlier was eliminated from any data set.
results aid ~i~scuss~on The radioactivity concentrations in ocular tissues at 20 minutes, 6 hours, and 24 hours after a single topical application of various formulations are depicted in Figures 1-4. In general, the concentra-tions in the ocular tissues were greatest at the earl-iest time point of 20 minutes as reported in~previous single dose studies, The radioactivity concen tration was highest in the conjunctiva and cornea for each formulation. The relatively low aqueous humor and iris-ciliary body concentrations suggest low in traocular absorption of CsA, consistent with the low 2o CsA corneal permeability of -1.0 x 10'6 cm/sec., The decline of radioactivity concentrations from the cornea was slower than those from the conjunctiva, lacrimal gland, and aqueous humor. The obse~~-ved blood radioactivity concentrations (<3 ng-eq/ml) were much , lower than trough plasma CsA concentrations of 80-250 ng/ml observed after oral dosing to humans, The dependence of CsA corneal and conjunctival penetration on the formulation was interpreted in -30 terms of CsA concentration in formulation and the release rate of CsA from formulation into tear film.
The aqueous formulations demonstrated a greater propensity to release CsA for diffusion across. the surface tissue epithelia. The 0.2% straight castor oil was formulated below the CsA solubility and therefore the release rate could be hampered by the less than maximal CsA thermodynamic activity, The ocular surface tissues contained a higher fraction of the CsA dose than the other tissues and was used to discriminate among the aqueous, emulsion and the straight castor oil formulations. The poly-oxyl 4o formulation produced higher ocular surface tissue concentrations than the emulsions and straight castor oil. The emulsions were also effective in delivery of CsA to the tissues of interest, lacrimal gland, cornea, and conjunctiva. The castor oil emul-lo sion showed higher lacrimal gland concentrations than the modified Santen and the miglyol* ~ emulsion. The straight castor oil showed the lowest concentrations in surface ocular tissues. Apparently, the factors influencing CsA penetration into the lacrimal gland and the surface tissues are different.
Although there has been hereinabove described a particular pharmaceutical composition in the form of a nonirritating emulsion for the purpose of illustrat-ing the manner in which the invention may be used to advantage, it should be appreciated that the invention is not limited thereto. Accordingly, any and all mod-ifications, variations, or equivalent arrangements, which may occur,to those skilled in the art, should be considered to be within the scope of the present in-vention as defined in the appended claims.
* Trade mark
Importantly, this solvent system does not contain any surface active agent such as polyoxyethylated castor oil.
Conceptually, the purpose of dissolving the cyclosporin in an aqueous solvent system is to enable contact with body fluids which would merely constitute dilution of the aqueous solvent system which hopefully would eliminate the immediate precipitation of cyclo sporin when contacted with the water content of the body fluids.
For direct use in the eye, cyclosporin has been formulated with a number- of pharmaceutically accept-able excipients, for example, animal oil, vegetable oil, an appropriate organic or aqueous solvent, an artificial tear solution, a natural or synthetic poly-mer or an appropriate membrane.
Specific examples of these pharmaceutically acceptable excipients, which may be used solely or in combination, are olive oil, arachis oil, castor oil, mineral oil, petroleum jelly, dimethyl sulfoxide, chremophor, liposomes, or liposome-like products or a silicone fluid, among others.
In summary, a great deal of effort has been ex-pended in order to prepare a pharmaceutical composi-tion containing cyclosporin dissolved in an aqueous medium or cyclosporin prepared as an oily solution.
However, successful formulations have yet to be accom-plished as evidenced by the lack of commercial prod-ucts.
As hereinabove noted, it has been reported that cyclosporin has demonstrated some solubility in oily preparations containing higher fatty acid glycerides such as olive oil, peanut oil, and/or castor oil.
These formulations frequently produce an unpleasant sensation when applied to the eye because of stimula-tion or the viscousness which is characteristic of these oils.
Another drawback of these formulations is that they contain a high concentration of oils, and oils exacerbate the symptoms of certain ocular surface diseases such as dry eyes, indicated by cyclosporin.
Therefore, these oily formulations may not be clini-cally acceptable. Additionally, these formulations often suffer from physical instability due to cyclo-sporin°~ propensity to undergo conformational change and cr;~~stallize out. The-crystallization problem has been noticed in formulations containing corn oil or medium chain triglycerides. Lastly, these formula-tions often have a low thermodynamic activity (degree of saturation) of cyclosporin which leads to a poorer drug bioavailability.
It may be possible to minimize the problems related to unpleasant sensation and syndrome exacerba-tion by reducing the oil content and dispersing the oil phase in water into an emulsion. However, it is not an easy task to formulate an ophthalmic emulsion because one indispensable class of ingredients in an emulsion system is emulsifiers, and the majority of emulsifiers is highly irritating to the eyes.
The present invention is directed to an emulsion system which utilizes higher fatty acid glycerides but in combination with polysorbate 80 which results in an emulsion with a high comfort level and low irritation potential suitable for delivery of medications to sen-sitive areas such as ocular tissues. Further, the present invention provides a pharmaceutical composi-tion and method for causing preferential absorption of cyclosporin in the lacrimal gland. That is, for a given instillation of the composition into an eye, a greater amount of absorption occurs in the lacrimal gland for formulations made in accordance with the present invention than heretofore utilized formula tions.
SUMMARY OF THE INVENTION
In accordance with the present invention, a non-irritating pharmaceutical composition with high com-fort level and low irritation potential suitable for delivery to sensitive areas such as ocular tissues comprises cyclosporin in admixture with an emulsifying amount of a higher fatty acid glycerol and polysorbate 80. More particularly, the composition may comprise cyclosporin A and the higher fatty acid glyceride may comprise castor oil.
Preferably, the weight ratio of the castor oil to the polysorbate 80 is between about 0.3 to about 30 and a weight ratio of the cyclosporin to castor oil is below 0.16. More preferably, the weight ratio of castor oil to polysorbate 80 is between 0.5 and 12.5, and the weight ratio of cyclosporin to castor oil is between 0.12 and 0.02.
When cyclosporin is dissolved in the oil phase in accordance with the present invention, the emulsion is found to be physically stable upon long term storage.
No crystallization of cyclosporin was noticed after nine months at room temperature. Moreover, the cyclosporin emulsion is formulated in such a way that the drug has reasonably high thermodynamic activity, yet without the crystallization problem.
Importantly, the composition of the present in-vention provides for enhanced absorption of the cyclo-sporin in the lacrimal gland of the eye. In this manner, the activity of the cyclosporin in restoring lacrimal gland tearing is increased. That is, since a greater amount of cyclosporin is absorbed into the lacrimal gland, more of the cyclosporin is effective in producing lacrimal gland tearing than heretofore possible.
BRIEF DESCRIPTION OF THE DRAWINGS
The advantages and features of the present inven-tion will be better understood by the following description when consideYed in conjunction with the accompanying drawings in which:
Figure 1 is a bar chart of conjunctival concen-tration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye;
Figure 2 is a bar chart of cornea concentration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye;
Figure 3 is a bar chart of ciliary body concen-tration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye;
and Figure 4 is a bar chart of lacrimal gland concen-tration of cyclosporin A after a single topical instillation of various formulations in a rabbit eye.
DETAILED DESCRIPTION
As hereinabove noted, cyclosporin is available as a mixture in which the principal ingredient is cyclo-_g_ sporin A with significant, but smaller, quantities of other cyclosporins such as cyclosporin B through I.
However, as also hereinabove noted, the present inven tion may be applied to either a pure cyclosporin or to a mixture of individual cyclosporins.
The discovery on which the present invention is founded relates to a combination of a higher fatty acid glyceride and an emulsifier and dispersing agent, polysorbate 80. The selection of these components could not have been anticipated on the basis of con-ventional thinking.
For example, although it is well known that cyclosporin may be used in combination with castor oil, this combination is irritating to sensitive tissues such as the eye. Thus, conventional teaching in the art is away from a formulation which utilizes a higher fatty acid glyceride, such as castor oil, and cyclosporin.
Stated another way, there is no way of deducing that the use of an emulsifier and dispersing agent such as polysorbate 80 will reduce the irritation po-tential of an emulsion utilizing castor oil. There are no examples of polysorbate in combination with castor oil which, when admixed to cyclosporin, pro-duces an emulsion with a high comfort level and low irritation potential suitable for the delivery of -30 medication to sensitive areas such as ocular tissues.
The present invention achieves a stable solution state of cyclosporin. This stable solution state is another important performance characteristic differ-entiating the present invention from the conventional oil systems. Cyclosporin is notorious for its ten-WO 95131211 P~.TfUS95/06302 _g_ dency to precipitate out in conventional oil systems in which it is fully dissolved initially.
In accordance with the present invention, the emulsions can be further stabilized using a polyelec-trolyte, or polyelectrolytes if more than one, from the family of cross-linked p.olyacrylates, such as carbomers and Pemulen~.
Pemulen~ is a polymeric emulsifier having a CTFA
name of Acryl~tes/C10-30 Alkyl Acrylate Cross-Polymer and is described in the "Garbomer 1342" monograph in the United States Pharmacopeial National Formuiary, United States Pharmacopeial Gonvention inc., 2002. ._ In addition, the tonicity of the emulsions can be further adjusted usincr a.lvcerine, mannitol, or sorbi-tol if desired. The pH of the emulsions can be ad-justed in a conventional manner using sodium hydroxide to a near physiological pH level and while buffering agents are not required, suitable buffers may include phosphates, citrates, acetates and borates.
While the preferable medications in accordance with the present invention include cyclosporin; other chemicals which are poorly soluble in water such as indomethacin and steroids such as androgens, predniso .lone, prednisolone acetate, fluorometholone, and dexamethasones, may be emulsified with castor oil and polysorbate 80 resulting in a composition with similar -30 low irritation potential.
The invention is further illustrated by the following =xamples with all parts and percentages expressed .by weight. The cyclosporin used in the examples was supplied by Sandoz.
WO 95/31211 PCTlUS95106302 Example 1 A B C D E
Cyclosporin 0.40% 0.20% 0.20% 0.10% 0.05%
A
Castor oil 5.00% 5.00% 2.50% 1.25% 0.625%
Polysorbate 1.00% 1.00% 1.00% 1.00% 1.00%
Pemulenm 0.05% 0.05% 0.05% 0.05% 0.05%
G1 cerine 2.20% 2.20% 2.20% 2.20% 2.20%
NaOH qs qs s s qs Purified waterqs qs qs qs qs pH 7.2-7.67.2-7.67.2-7.6 7.2-7.67.2-7.6'.
Example 2 A B C D
Castor oil 5.00% 2.50% 1.25% 0.625%
Pol sorbate 1.00% 1.00% 1.00% 1.00%
Pemulenm 0.05% 0.05% 0.05% 0.05%
Glycerine 2.20 2.20% 2.20% 2.20%
NaOH s s s s 2 0 Purified waters s s s pH 7.2-7.67.2-7.67.2-7.67.2-?.6' Example 3 A
Castor oil 2.50%
Polysorbate 80 0.75%
Carbomer 1382 0.05%
Glycerine 2.20%
3 0 NaOH qs Purified water qs pH 7.2-7.6 WO 95/31211 PC'TIUS95/06302 Example 4 A
Castor oil 5.00%
Polysorbate 80 0.75%
Carbomer 981 0.05%
G1 cerine 2.20%
NaOH s Purified water qs pH 7.2-7.6 The formulations set forth in Examples 1-4 were made for treatment of keratoconjunctivitis sicca (dry eye) syndrome with Examples 2, 3 and 4 without the active ingredient cyclosporin utilized to determine the toxicity of the emulsified components.
The formulations in Examples 1-4 were applied to rabbit eyes eight times a day for seven days and were found to cause only slight to mild discomfort and slight hyperemia in the rabbit eyes. Slit lamp exam-ination revealed no changes in the surface tissue. In addition, the cyclosporin containing castor oil emul-sion, as hereinabove set forth in Examples lA-1D, was also tested for ocular bioavailability in rabbits; and the therapeutic level of cyclosporin was found in the tissues of interest after dosage. This substantiates that cyclosporin in an ophthalmic delivery system is useful for treating dry eye as set forth in U.S.
'30 Patent No. 4,839,342.
In addition, no difference in toxicity was found between formulations with cyclosporin (Examples lA-1D) and formulations without cyclosporin (Examples 2-4).
The formulations set forth in Examples 1-4 were found to be physically stable upon long term storage.
pGTIUS95/06302 With regard to formulations lA-1D, no crystallization of cyclosporin was noticed after nine months at room temperature.
Further, other higher fatty acid glycerides such as olive oil, peanut oil and the like may also be utilized with the polysorbate 80 with similar results regarding biotoxicity.
The following examples demonstrate the activity of the composition in accordance with the present invention for enhanced absorption of cyclosporin A in the lacrimal gland.
Materials The [Mebmt-3H]-cyclosporin-A (lot #TRQ6553) was prepared by Amersham International (Buckinghamshire, England) with radiochemical purity of -98% (by reversed phase HPLC) and specific activity of 2.6 Ci/mmol (2.16 mCi/mg). The 3H-label is a metabolic-ally stable position as shown by the asterisk. The radiolabeled CsA was supplied as an ethanol solution (1 mCi/ml). All organic solvents used in the procedures described in this study were "HPLC grade".
all other chemicals and reagents were analytical grade unless otherwise noted.
The compositions of the six formulations tested - - 30 are listed in Table A.
WO 95/31211 . PCTfi3S9510G302 TABLE A
Castor Miglyol Aqueous- Polyoxyl ngredients astor Oil-in- ~ Cyclo-Oil-in.-olyoxyl40 with Oil Water dextrinWater 40 Edetate j Emulsion Emulsion C clos orin-A 0.20 0.20 0.10 0.20 0.05 0.05 C clodextrin 14 Castor Oil 99.8 1.25 Miglyoi* OiI
Pluronic* i_121 0.75 ~- P123 Tween* 80 I . 00 Gl cerin 2.20 2.20 Pemulen~ TR-2 0.05 Carbopol* 981 0 . 05' Polyoxyl 40 20 20 Steavate (mg) FiPMC 0.3 0.3 Butylated H drox toluene 0.001 0.001 Ethanol(9200 rood) 0.1 Sodium Chloride 0.73 0.73 Sodium Mono hos hate 0.2 0.2 Disodium Edetate 0.1 ~~
Water QS QS QS QS QS
Batch Size 1 g 5 g 1 g 5 g 1 g 1 g The radiolabeled formulations were formulated to ensure that the radioactivity was homogeneous throughout the vehicle. The, expected radioactivity concentrations of the radiolabeled drug formulations were 1-2 mCi/ml. The expected specific activity of radiolabeled cyclosporin A (CsA) formulations was 0.5-2 mCi/mg. All test articles were stored at ambient temperature.
* Trade mark Analysis of Test Drug Formulations The test formulations were analyzed in triplicate by HPLC to determine the concentration of CsA and radiochemical purity of the CsA dosing solutions (>93%) before dosing. The radioactive concentrations of the test formulations were quantified by liquid scintillation counting (LSC).
l0 Chromatographic Conditions Pump: Beckman Model 126 (Beckman Instruments, San Ramon, CA) Mobile phase: Acetonitrile: 0.03a H3POq in water, pH 3 (65:35 v/v) Flow rate: 1.0 ml/min Column: Supercosil C8, 7.5 cm x 4.6 mm, 3 ~cm (Supelco, Bellefonte, PA) Superguard LC-8 (Supelco) Column heater (Bio-rad, Richmond, CA) at 60-70C
Injector: WISP 712B (Waters Associates, Milford, MA) 1aC detector: Radio Isotope 171 Detector (Beckman Instruments) Scintillant: Ready Flow III (Beckman Instruments), Flow Rate of '4 ml/min W detector: Model 166 (Beckman Instruments), 2 0 2 nm - Data processor: Beckman System Gold (Beckman Instruments) Run Time: 15 min Retention Time: 6 min (cyclosporin A) Animals Female New Zealand albino rabbits were obtained and quarantined for at least five days before procedures. Animals were housed in temperature- and humidity-controlled rooms. Food and tap water were provided ad libitum. Fifty-eight rabbits (2-3 kg) were selected Pram the colony to minimize bias. They were individually identified by ear tags and appeared to be healthy.
Dos inct The animals were divided into six groups of nine I5 rabbits; each group was treated with one of the six CsA formulations. During dosing, the lower eyelid of each rabbit was gently pulled away from the eye and 35 ~cl of the formulation were administered in the lower conjunctival cul-de-sac of each eye. After dosing, the upper and lower eyelid were handheld closed for '5 seconds and released. The animals were observed visually for any signs of tearing or ocular discomfort.
Samr~li,ng Tissues were collected at 20-min., 6-hr. and 24-hr. post-dose for each group. Three rabbits (six eyes) were used at each time point. At the specific sampling times, the animals were euthanized by an intravenous injection of 0.5-1 ml Eutha-6 (Western Supply Co., Arcadia, California) via marginal ear vein. Each eye was then rinsed with normal saline.
The aqueous humor ('200 ~1) was removed by means of a 0.5~m1 tuberculin syringe. The orbital lacrimal gland ('400 mg) , upper and lower bulbar conjunctivae ('S0 mg each), corneal ('50 mg) and iris-ciliary body ('S0 mg) were dissected. The tissues dissected were blotted dry and weighed. Ocular tissue and aqueous humor samples from both eyes were collected from four untreated animals to be used as blank samples.
Analysis of Radioactivity An aliquot of aqueous humor (50-175 ~.1) was counted directly in 10 ml of Ready-Solv HP by LSC.
Tissue and blood samples were weighed into combustion cones prior to combustion in a Model 307 Packard Tissue Oxuduzer (Packard Co., Downers Grove, Illinois). After combustion of the tissue samples, 3H20 was trapped in the Monophase-S solution (Packard) and the radioactivity of the samples was determined by LSC in a Beckman Model 1801 or 3801 scintillation counter (Beckman Instruments, San Ramon, California).
Data Analyses Excel software (version 4.0, Microsoft Corp, Redmond, Washington) was used for data analysis.
concentrations of total radioactivity in the tissue samples were expressed as dpm/g or dpm/ml and converted to ng equivalents (eq) of CsA/g or ml, using the specific activity of the dosing formulations.
Mean, standard deviation (SD) or standard error of the mean (SEM) was calculated according to standard methods. Radioactivity levels were not considered - -30 significant unless the dpm was greater than twice that of background b=(blanks).
Comparisons of tissue drug concentrations at each time point for the formulations were determined by one-factor ANOVA. All statistical comparisons were made using StatView~ (version 1.03, Abacus Concepts, Inc., Berkeley, California). the Fisher and Scheffe F tests were used to determine significant differences between formulations at the 95% level (a = 0.05). The rejection criteria for excluding any outlier data was based on standard outlier tests. No mere than one outlier was eliminated from any data set.
results aid ~i~scuss~on The radioactivity concentrations in ocular tissues at 20 minutes, 6 hours, and 24 hours after a single topical application of various formulations are depicted in Figures 1-4. In general, the concentra-tions in the ocular tissues were greatest at the earl-iest time point of 20 minutes as reported in~previous single dose studies, The radioactivity concen tration was highest in the conjunctiva and cornea for each formulation. The relatively low aqueous humor and iris-ciliary body concentrations suggest low in traocular absorption of CsA, consistent with the low 2o CsA corneal permeability of -1.0 x 10'6 cm/sec., The decline of radioactivity concentrations from the cornea was slower than those from the conjunctiva, lacrimal gland, and aqueous humor. The obse~~-ved blood radioactivity concentrations (<3 ng-eq/ml) were much , lower than trough plasma CsA concentrations of 80-250 ng/ml observed after oral dosing to humans, The dependence of CsA corneal and conjunctival penetration on the formulation was interpreted in -30 terms of CsA concentration in formulation and the release rate of CsA from formulation into tear film.
The aqueous formulations demonstrated a greater propensity to release CsA for diffusion across. the surface tissue epithelia. The 0.2% straight castor oil was formulated below the CsA solubility and therefore the release rate could be hampered by the less than maximal CsA thermodynamic activity, The ocular surface tissues contained a higher fraction of the CsA dose than the other tissues and was used to discriminate among the aqueous, emulsion and the straight castor oil formulations. The poly-oxyl 4o formulation produced higher ocular surface tissue concentrations than the emulsions and straight castor oil. The emulsions were also effective in delivery of CsA to the tissues of interest, lacrimal gland, cornea, and conjunctiva. The castor oil emul-lo sion showed higher lacrimal gland concentrations than the modified Santen and the miglyol* ~ emulsion. The straight castor oil showed the lowest concentrations in surface ocular tissues. Apparently, the factors influencing CsA penetration into the lacrimal gland and the surface tissues are different.
Although there has been hereinabove described a particular pharmaceutical composition in the form of a nonirritating emulsion for the purpose of illustrat-ing the manner in which the invention may be used to advantage, it should be appreciated that the invention is not limited thereto. Accordingly, any and all mod-ifications, variations, or equivalent arrangements, which may occur,to those skilled in the art, should be considered to be within the scope of the present in-vention as defined in the appended claims.
* Trade mark
Claims (15)
PROPERTY OR PRIVILEGE IS CLAIMED ARE AS FOLLOWS:
1. A composition comprising a nonirritating emulsion of a higher fatty acid glyceride, polysorbate 80 and an emulsion stabilizing amount of Pemulen® in water suitable for topical application to ocular tissue.
2. The pharmaceutical composition according to claim 1 wherein the weight ratio of the higher fatty acid glyceride to the polysorbate 80 is between about 0.3 and about 30.
3. A pharmaceutical composition comprising castor oil, polysorbate 80 and an emulsion-stabilizing amount of Pemulen® in water suitable for topical application to ocular tissue.
4. The pharmaceutical composition according to claim 3 wherein the weight ratio of castor oil to the polysorbate 80 is between about 0.3 and about 30.
5. A stable, nonirritating ophthalmic composition comprising an emulsifying amount of a higher fatty acid glyceride, polysorbate 80 and an emulsion-stabilizing amount of Pemulen®.
6. A pharmaceutical emulsion comprising castor oil, Pemulen®, a higher fatty acid glyceride , polysorbate 80 and water, said pharmaceutical emulsion being suitable for topical application to ocular tissue.
7. A pharmaceutical emulsion according to claim 6 wherein the castor oil is present in an amount of between about 0.625% and about 5.0% by weight, the polysorbate 80 is present in an amount of about 1.0%
by weight, Pemulen® is present in an amount of about 0.05% by weight and the glyceride is present in an amount of about 2.2% by weight.
by weight, Pemulen® is present in an amount of about 0.05% by weight and the glyceride is present in an amount of about 2.2% by weight.
8. A pharmaceutical emulsion consisting of between about 0.625%
and about 5.0% by weight of castor oil, about 1.0% by weight .of polysorbate 80, about 0.05% by weight of Pemulen® and about 2.2% by weight of glycerine in water with a pH of between about 7.2 and 7.6 suitable for topical application to ocular tissue.
and about 5.0% by weight of castor oil, about 1.0% by weight .of polysorbate 80, about 0.05% by weight of Pemulen® and about 2.2% by weight of glycerine in water with a pH of between about 7.2 and 7.6 suitable for topical application to ocular tissue.
9. A pharmaceutical composition suitable for instillation into an eye, said pharmaceutical composition comprising a non-irritating emulsion of a drug selected from cyclosporin, an indomethacin and a steroid drug, polysorbate 80, Pemulen®
and castor oil in an amount causing enhanced lacrimal gland absorption.
and castor oil in an amount causing enhanced lacrimal gland absorption.
10. The pharmaceutical composition according to claim 9 wherein the drug is selected from the group consisting of indomethacin and steroids.
11. The pharmaceutical composition according to claim 10 further comprising an emulsion-stabilizing amount of Pemulen® in water suitable for topical application in the eye.
12. The pharmaceutical composition according to claim 11 further comprising glycerin.
13. A nonirritating pharmaceutical composition suitable for instillation into an eye, said pharmaceutical composition comprising an emulsion-stabilizing amount of Pemulen®, polysorbate 80 and castor oil in an amount causing enhanced lacrimal gland absorption.
14. Use of a composition according to claim 13 for instillation into the eye for causing enhanced absorption in the lacrimal gland of an eye.
15. Use of a composition according to claim 11 for instillation into the eye for causing enhanced absorption in the lacrimal gland of an eye.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US08/243,279 | 1994-05-17 | ||
| US08/243,279 US5474979A (en) | 1994-05-17 | 1994-05-17 | Nonirritating emulsions for sensitive tissue |
| CA002190485A CA2190485C (en) | 1994-05-17 | 1995-05-17 | Lacrimal gland specific emulsions for topical application to ocular tissue |
Related Parent Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002190485A Division CA2190485C (en) | 1994-05-17 | 1995-05-17 | Lacrimal gland specific emulsions for topical application to ocular tissue |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CA2309033A1 CA2309033A1 (en) | 1995-11-23 |
| CA2309033C true CA2309033C (en) | 2003-08-26 |
Family
ID=25678827
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002309033A Expired - Lifetime CA2309033C (en) | 1994-05-17 | 1995-05-17 | Lacrimal gland specific emulsions for topical application to ocular tissue |
Country Status (1)
| Country | Link |
|---|---|
| CA (1) | CA2309033C (en) |
-
1995
- 1995-05-17 CA CA002309033A patent/CA2309033C/en not_active Expired - Lifetime
Also Published As
| Publication number | Publication date |
|---|---|
| CA2309033A1 (en) | 1995-11-23 |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| CA2190485C (en) | Lacrimal gland specific emulsions for topical application to ocular tissue | |
| US5182258A (en) | Systemic delivery of polypeptides through the eye | |
| US4990337A (en) | Cyclosporin formulations of mono or diglyceride fatty acid | |
| RU2331423C2 (en) | Delivery system with controlled release for intranasal applying | |
| US5951971A (en) | Ophthalmic compositions | |
| US5789375A (en) | Pernasal composition and pernasal preparation containing the same | |
| KR20090053797A (en) | Cyclosporin compositions | |
| KR20100107462A (en) | Stable aqueous cyclosporin compositions | |
| SK282714B6 (en) | Hydrophilic binary systems for the administration of cyclosporin | |
| US5278142A (en) | Systemic delivery of polypeptides through the eye | |
| US20150045309A1 (en) | Cyclosporin emulsions | |
| AU2003247976A1 (en) | Ophthalmic compositions containing loratadine | |
| TANIGUCHI et al. | Efficacy of a liposome preparation of anti-inflammatory steroid as an ocular drug-delivery system | |
| CA2309033C (en) | Lacrimal gland specific emulsions for topical application to ocular tissue | |
| MXPA96005599A (en) | Specific emulsions for the lagrimal gland, for the topic application to the ocu tissue | |
| US4623664A (en) | Oil suspended phenylephrine | |
| Tsuji et al. | Hydrolysis of prednisolone succinate by esterase in rabbit ocular tissue | |
| JP2632010B2 (en) | Cyclosporine preparation | |
| US6225332B1 (en) | Compositions containing histamine H2 agonists and methods of use in treating allergy and inflammation | |
| RU2634267C2 (en) | Aqueous ophthalmic solution based on cyclosporin a | |
| MXPA06005325A (en) | Controlled release delivery system for nasal applications |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| EEER | Examination request | ||
| MKEX | Expiry |
Effective date: 20150519 |