AU747169B2

AU747169B2 - Synergistic gold-containing compositions

Info

Publication number: AU747169B2
Application number: AU47671/97A
Authority: AU
Inventors: Richard Edward Thomas
Original assignee: Psiron Ltd
Current assignee: Viralytics Ltd
Priority date: 1996-11-04
Filing date: 1997-11-04
Publication date: 2002-05-09
Anticipated expiration: 2017-11-04
Also published as: AU4767197A

Description

WO 98/19683 PCT/AU97/00747 -1- TITLE: SYNERGISTIC GOLD-CONTAINING COMPOSITIONS TECHNICAL FIELD The present invention relates to pharmaceutical compositions comprising a gold compound in combination with a corticosteroid and their use in the treatment of dermatological disorders.

BACKGROUND OF THE INVENTION The effectiveness of gold compounds in the treatment of rheumatoid arthritis has been known since the 1960s. More recently, gold complexes have been employed as therapeutic agents in the treatment of rheumatoid arthritis but their exact mechanism is still unknown. The most commonly used complexes have been water soluble, parenterally administered gold thiolates such as aurothiomalate (Myocrisin®) and aurothioglucose (Solganol Subsequently, a number of alkylphosphine gold complexes displayed anti-arthritic activity when administered orally to adjuvant arthritic rats. Auranofin (1-thio-P-D-glucopyranose 2,3,4.6-tetraacetato-S)-(triethylphosphine)- Au(I)) was among the most potent and efficacious of the compounds tested and is now used in the treatment of rheumatoid arthritis in man.

Gold compounds have also been administered by intravenous and oral routes for the treatment of asthma, tuberculosis, pemphigus vulgaris, various forms of arthritis, cancer and infection. However, treatment with gold compounds has been frequently associated with unacceptable and on occasions serious side effects.

Corticosteroids have also found similar therapeutic applications. The success of topical corticosteroids in the therapy of inflammatory and proliferative disorders of the skin has led to vigorous development of new corticosteroids since their first topical use.

An increase in potency has been achieved by chemical modification of the natural corticosteroid, hydrocortisone, without precise knowledge of the mechanism of action of corticosteroids. The development of more potent corticosteroids has extended their usefulness in a wide variety of skin diseases, but, especially with long term use, has led to unwanted effects. Systemic effects such as hypothalmic pituitary-adrenal-axis depression were already known from the systemic use of corticosteroids. Local side effects after topical application were observed only with the more potent synthetic steroids.

The most common serious side effects of topical corticosteroids are thinning of the skin, striae and telangiectasia. During long term treatment with very potent WO 98/19683 PCT/AU97/00747 -2corticosteroids, inflammatory cells are affected and the proliferation of keratinocytes and the activity of fibroblasts are also inhibited.

Fibroblasts synthesize important structural and functional components of the dermis, namely collagen, elastin and glycosaminoglycans. The inhibition of keratinocyte proliferation leads to thinning of the epidermis. Although the effect on the epidermis is usually reversible, the dermis can be irreversibly damaged.

Recently, topical formulations of gold organic complexes have found use in the treatment of skin disorders such as psoriasis. Thus, Australian Patent No. 616,755, describes the use of a topical formulation of auranofin in combination with a corticosteroid in the treatment of local inflammatory conditions such as those associated with psoriasis. In particular, treatment with a formulation comprising auranofin and betamethasone dipropionate demonstrated a remarkable synergy of action when compared to same concentrations of individual active ingredients. The finding that a gold compound can synergise with a corticosteroid enabled the use of considerably lower levels of both the gold compound and a corticosteroid in the formulations, thus enabling more effective therapy while obviating the well known side effects associated with the use of either gold compounds or corticosteroids alone.

Dermatological disorders are frequently associated with manifestations other than just inflammation. For example, psoriasis also contains a component of cellular hyperproliferation (hyperplasia), the mechanism of which is fundamentally different from that of inflammation and thus may not necessarily be affected by the topical gold/corticosteroid formulations. Furthermore, the inflammatory component of different dermatological conditions may range from very mild to very severe, necessitating variations in the formulation, in particular the choice of corticosteroid which would enable not only effective and appropriate treatment of the inflammatory component, but also provide the differential action in dermatological conditions where there is an additional component such as cellular hyperproliferation.

Other immune, autoimmune and infection disorders can also be associated with multiple manifestations, where effective treatment may rely on targeting only one of the manifestations of the disorder, or more than one, depending on the disorder treated and the assessment of the patient.

The present invention is based on a surprising finding that important differences exist between corticosteroids with respect to the degree of potentiation of effects and the type of effect potentiated, when combined with a gold compound. That is to say, different corticosteroids, when combined with a gold compound, do not all have the expected similarity of synergistic action against inflammation and also demonstrate differential synergistic action with respect to inflammation and hyperplasia. In the compositions of the present invention certain corticosteroids synergise with the gold compound to provide a greater effect on the inflammatory component of a disorder, such as psoriasis, while other corticosteroids give rise to compositions with preferential effects on cellular hyperproliferation. It is contemplated that the compositions of the present invention could be effectively used also for the treatment of a variety of systemic, tissue-specific or localised immune, autoimmune and inflammatory disorders.

SUMMARY OF THE INVENTION According to a first aspect the invention consists in a method of treating an immune-mediated disorder having an inflammatory component and/or a cellular hyperproliferation component, comprising the step of administering to a patient requiring such treatment a gold compound and at least one corticosteroid, wherein the at least one corticosteroid is selected to interact with the gold compound to exhibit preferential synergistic action towards one of the components of said disorder or to exhibit equal action towards each component of said disorder provided that said method does not include the administration of a combination of auranofin and betamethazone 20 dipropionate.

According to a preferred embodiment the present invention consists in a method of treating an immune mediated disorder according to the first aspect comprising the step of administering at least two corticosteroids, at least one of which is selected to interact mi with the gold compound to exhibit preferential synergistic action towards the inflammatory component, and at least another is selected to interact with the gold compound to exhibit preferential synergistic action towards the cellular hyperproliferation component of said disorder.

According to another preferred embodiment the present invention consists in a method of treating an immune-mediated disorder having multiple components, comprising the step of administering to a patient requiring such treatment one or more compositions comprising a gold compound and one or more corticosteroids, wherein the 20276-80.DOC/ -3acorticosteroid is selected to provide a composition with equal synergistic action towards each component of said disorder.

According to another preferred embodiment the present invention consists in a method of treating an immune-mediated disorder having one or more components, **1 oo ooo 20276-80.DOC/ u i/ U i i RECEIVED 2 2 SEP 1398 -4comprising the step of administering to a patient requiring such treatment a composition comprising a gold compound and one or more compositions comprising one or more corticosteroids wherein the corticosteroid is selected to provide a composition with preferential synergistic activity towards one of the components of said disorder and wherein the composition comprising a gold compound is administered orally and the one or more compositions comprising one or more corticosteroids is administered topically, in amounts effective to provide a composition of gold and a corticosteroid having preferential synergistic action towards said component.

Preferably the component of the immune-mediated disorder is an inflammatory component and/or a cellular hyperproliferation component and the composition comprises at least two corticosteroids, one of which is selected to provide a composition with preferential synergistic action towards the inflammatory component and the second corticosteroid is selected to provide a composition with preferential synergistic action towards the cellular hyperproliferation component of said disorder.

Preferably the disorder to be treated is an immune-mediated dermatological disorder which is associated with more than one component. Examples of immunemediated dermatological disorders include psoriasis or dermatitis such as contact, atopic or seborrheic dermatitis. Other disorders include rheumatoid arthritis. Typical components of such disorders include an inflammatory component and/or a cellular hyperproliferation component. The corticosteroid can be selected to provide a composition with synergistic activity towards cellular hyperproliferation in preference to inflammation or vice versa. Such a corticosteroid can be, for example, betamethasone dipropionate, fluocinolone acetonide or hydrocortisone. In cases where inflammation needs to be targeted in preference to cellular hyperproliferation, the corticosteroid can be betamethasone dipropionate, fluocinolone acetonide or mometasone furoate.

The composition is suitably formulated for topical administration.

Where the immune-mediated disorder is characterised by a number of different components, the preferred method of treatment could employ one or more compositions comprising a gold compound and one or more corticosteroids, wherein the corticosteroids are selected to provide composition(s) with preferential activity towards only one of the components of said disorder. Thus the treatment of each individual LU rMENDED SHEET

IPEA/AU

Component is achieved through use of composition(s) comprising one or more selected corticosteroids, which may be applied in the form of two or more separate compositions or a single composition comprising two or more corticosteroids.

Preferably the gold compounds used in the present invention are lipid soluble.

Even more preferably the gold compounds used are formulated for topical application.

However, it will be understood that systemically or locally administered compositions are also within the scope of the present invention including those administered by injection, preferably intra-articularly. In this regard the corticosteroid can be formulated for oral, topical, systemic or local administration.

According to a second aspect the present invention consists a pharmaceutical composition comprising a gold compound and one or more corticosteroids, the corticosteroid being selected to interact with the gold compound to exhibit a preferential synergistic action towards an inflammatory component and/or a cellular hyperproliferation component of an immune-mediated disorder, in combination with a 15 pharmaceutically acceptable carrier, excipient, adjuvant or solvent provided that said composition does not include auranofin and betamethazone dipropionate.

Preferably the gold compound is auranofin and the corticosteroid is selected from the group comprising hydrocortisone acetate, hydrocortisone, betamethazone, *betamethazone dipropionate, dexamethasone, fluocortolone 21-pivalate, triamcinolone acetonide, betamethazone valerate, alclometasone dipropionate, halcinonide, mometasone furoate and fluocinolone acetonide. More preferably the corticosteroid is selected from the group comprising hydrocortisone, betamethazone dipropionate, mometasone furoate or fluocinolone acetonide.

eoco* o• *ooo^ 20276-80.DOC/ WO 98/19683 PCT/AU97/00747 -6- BRIEF DESCRIPTION OF FIGURES Figure 1: A histogram showing the effects of auranofin and glucocorticoids alone or in combination on TPA-induced epidermal hyperplasia. BMD: betamethasone dipropionate; HYD: hydrocortisone; FA: fluocinolone acetonide, MMF: mometasone furoate; AF: auranofin. Bars indicate standard error of the mean (SEM).

Figure 2: A histogram showing the effects of auranofin and glucocorticoids alone or in combination on TPA-induced inflammatory cell infiltration. BMD: betamethasone dipropionate; HYD: hydrocortisone; FA: fluocinolone acetonide; MMF: mometasone furoate; AF: auranofin. Bars indicate standard error of the mean (SEM).

DESCRIPTION OF THE PREFERRED EMBODIMENT For convenience, a TPA (12-O-tetradecanoylphorbol 13-acetate), model of psoriasis, as an example of an immune-mediated disorder which has an inflammatory as well as a cellular hyperproliferation component, will be used to demonstrate differential action of different corticosteroids as well as differential action of different formulations of a gold compound and a corticosteroid.

Although psoriasis does not occur in animals other than humans, studies have shown that the application of TPA produces an inflammatory reaction with epidermal thickening that resembles psoriasis in many ways. It produces epidermal hyperplasia and inflammatory cell infiltration into the dermis, both of these features are also characteristic of psoriasis.

TPA increases the activity of the phospholipase C/inositol trisphosphate/ diacylglycerol system. This system activates the protein kinase C and arachidonic acid pathways. Both these systems have been implicated in the pathogenesis of psoriasis.

TPA-treated mouse is believed to be a suitable model for psoriasis. This animal model will be used to show differential actions of different corticosteroids and the synergistic effects of compositions comprising a gold compound and a corticosteroid.

Three parameters have been measured: skin-fold thickness, epidermal hyperplasia and inflammatory cell infiltration into the dermis. These features, particularly the last two, are the hallmarks of psoriasis. It is noteworthy however, that the current findings clearly have implications beyond mere treatment of dermatological disorders. Systemic or tissue inflammatory and hyperplastic conditions could also benefit from treatment with the compositions of the present invention.

Topical Corticosteroids WO 98/19683 PCT/AU97/00747 -7- Topical corticosteroids can be grouped according to their strength: weak, medium, strong and very strong. Vasoconstriction assay is considered the best method of assessing the potency of various preparations. It is not known whether the measurement of vasoconstriction predicts anti-inflammatory activity. Other methods of assaying that are available include clinical trial, dermal thickness radiograph, biopsy for assessing epidermal thinning, and mitotic inhibition assays.

A useful clinical guide to the relative potencies of topical corticosteroid preparations is shown in Table 1, the rank order arrangement being approximately the same for ointments and creams. The preparations in each group are only roughly equipotent.

Table I Table I A guide to the clinical potencies of topical coticosteroids r I rVs- tfrn Weak MeGium I U111r, I t Dexamethasone 0.0 1% Fluocinolone acetonide 0.0025% Hydrocoutisone 0.5% and 0. 1% Hydrocortisone acetate 1% MethylIprednisolone acetate 0.25%

II

I

Aiclometasone dipropionate 0.05% Betamethasone valerate 0.025% Clobetasone butyrate 0.05% Dexamethasone 0.05% Flumetliasone pivatate 0.02% Fluocinolone acetonide 0.01% Fluocortin butylester 0.75% Fluocoitolone 0.2% Flurandrenolone 0.0 125%-0.025% Hydrocortisone 1% with urea Anicinonide 0. 1% Beclomethasone dipropionale 0.025% Betameihasone benzoate 0.025% Betamnethasone dipropionate 0.05% Ilelamethasone valerate 0. 1IV, Budcsonide 0.025% Desonide 0.05% Dexamethasone 0.25% Diflorasone diacelate 0.05% Diflucortolone valerate 0. 1% Fluclorolone acetonide 0.025% Fluocinolone acetonide 0.025% Fluocinonide 0.05% Flutocortolone Fluprednidene acetate 0. 1% Flurandrenolone 0.05% Halcinonide 0. 1% Ilydrocortisone butyrate 0. 1% Momnetasone furoate 0. 1% Triaincinolone acelonide 0. 1% Beclomelliasone dipropionate Clobetasol propionate 0.05% Diflucortolone valerate 0.3% Fluocinolone acetonide 0.2% I I. I WO 98/19683 PCT/AU97/00747 -9- The invention will now be more particularly described with reference to specific embodiments by way of non-limiting example only.

Example 1: Animal treatment and methods of measurement Materials Auranofin was kindly donated by Smith Kline and Beecham Pharmaceuticals, King of Prussia, Philadelphia, USA.

Alclometasone dipropionate, betamethasone dipropionate, betamethasone valerate, betamethasone (as free alcohol) and mometasone furoate were kindly donated by Schering-Plough Pty. Ltd., Baulkham Hills, NSW, Australia.

Halcinonide, Hydrocortisone and Triamcinolone acetonide were kindly donated by Bristol-Myers Squibb Pharmaceuticals Pty. Ltd.

Dexamethasone was kindly donated by Roussel Uclaf, Paris, France.

Fluocortolone 21-pivalate was kindly donated by Schering AG, Berlin, Germany.

12-O-Tetradecanoylphorbol 13-acetate, fluocinolone acetonide, aluminium potassium sulphate, sodium hydrogen carbonate, sodium iodate, magnesium sulphate, eosin Y, phloxine, calcium carbonate, formaldehyde acetic acid (17 thymol, xylene, haematoxylin and "Paraplast" tissue embedding medium were obtained from Sigma Chemical Company, Castle Hill, NSW, Australia.

Sorbolene cream A.P.F. was obtained from Wille Laboratories, Carole Park, Queensland, Australia.

Preparation of auranofin 0.2 solution Auranofin (20 mg) was dissolved in 10 mL of acetone to give the strength 0.2%.

Auranofin solution was freshly prepared for each experiment.

Preparation of auranofin ointment Various strengths of auranofin ointment were made according to the formula as shown below: strength w/w) auranofin propylene glycol white soft paraffin 0.20 40 mg 2 g to 20 g 0.50 100 mg 2 g to 20 g WO 98/19683 PCT/AU97/00747 Methods of animal treatment Female BALB/c mice aged 6 to 8 weeks were obtained from the University of Sydney, and treated according to a protocol approved by the University of Sydney Animal Care and Ethics Committee.

The mice were housed in stainless steel cages, 6 mice per cage under normal laboratory conditions (room temperature at about 22C) at least 7 days before the experiments for acclimatization. Food and water were allowed ad libilum throughout the experiment period. The backs of the mice were shaved with an electric clipper two days before each treatment and only those mice showing no hair regrowth were used the mice in the resting phase of the hair growth cycle were selected). During treatment, the mice were held with their tails and put on top of the cage so that they grasped the cage and rested there. The solutions were applied to an area approximately 2 cm x 2 cm on the shaved back of the mice by using a "Pipetman" to apply the solution. If auranofin ointment or ointment base was applied, the amount was standardized by using a microspatula whichfwas crimped at one end, the ointment was then put into the ridge and the excess removed by means of another microspatula and applied sparingly twice a day.

After a fixed time, the mice were killed routinely by cervical dislocation between 9 a.m.

and 11 a.m. to avoid variations due to circadian rhythms, and an area (1 cm x 1 cm) was excised from the centre of the treated area by scalpel and scissors. The rest of the tissues were disposed by combustion. The tissues were then fixed, embedded, sectioned and stained.

Methods of preparation of skin sections The method of preparation of skin sections was adapted from a method developed by the Department of pathology, University of Sydney and shown to be successful.

Fixation, embedding, sectioning and staining Standard preparation procedures were used. Briefly, the tissue was fixed in buffered formalin for 24 hours, washed in tap water for 10 minutes and then processed in an automatic tissue processor (Tissue-Tek VIP 200). In the automatic tissue processor, the tissue was dehydrated in a graded series of alcohol and xylene at room temperature, and was then infiltrated with 4 changes of paraffin wax ("Paraplast" tissue mounting medium) at 60'C- It was finally embedded in fresh paraffin wax.

WO 98/19683 PCT/AU97/00747 -11- Sections 5 !tm thick were cut on an American Optical Spencer "820" microtome.

The sections were then mounted on clean microscope slides using wood glue ("Selleys" Aquadhere, 1:100 dilution with water) as adhesive, and were allowed to dry in an oven at 0 C for at least 2 hours (usually overnight).

After the sections were blued in the Scott's blueing solution, they were examined under microscope to assess that nuclei were clearly stained and cytoplasm was unstained.

Measurement of skin-fold thickness The back skin of shaved mice was folded and measured by using a "Etalon" micrometer screw gauge. One measurement was taken for each mouse.

Measurement of epidermal thickness Epidermal thickness was determined by image analysis. This image analysis system was a minicomputer (Tracor Northern TN8500) attached to a light microscope (Zeiss Axioplan) and a camcorder (Sony DXC-3000P). Sections were taken from each tissue block and 20 measurements were taken at fixed intervals from each section. The average value for the 20 measurements was obtained and entered as one value for each mouse. The mean and SEM for the six mice in each treatment group were calculated.

Measurement of infiltration of inflammatory cells Infiltration of inflammatory cells was determined by the same image analysis system using the section taken from the block of mouse skin embedded in paraffin wax or Spurr's resin and stained with haematoxylin and eosin or toluidine blue respectively.

For each section, 10 fields, unless otherwise stated, were chosen randomly and the cell density per mm 2 of field determined. The average value for the 10 fields was obtained and entered as one value for each mouse. The mean and SEM for the six mice in each treatment group were calculated.

The measurement of the inflammatory cell infiltration included the background values which included other materials in the dermis stained in the same way. However, the increase, if there is any. reflects the migration of inflammatory cells.

Data treatment The per cent inhibition of drug on TPA-induced skin responses epidermal hyperplasia, inflammatory cell infiltration and skin-fold thickness) was calculated by using the following formula: Total response due to TPA Total response due to drug Per cent inhibition x 100% Total response due to TPA Total response due to acetone WO 98/19683 PCT/AU97/00747 -12- It is commonly found that the relationship between dose (or concentration) and response may be satisfactorily described using the Michaelis Menton equation or a variant of it such as the Hill equation. This provides estimates of the potency, the efficacy or maximum effect and the slope of the log concentration-response curve by using Hill coefficient The Hill Equation may be expressed as follows: Emax x C'

ICS

0

C

Y

where ICs 0 is the drug concentration producing 50% of the maximal response and Emax refers to the maximal effect produced by the drug and is also termed efficacy. Efficacy is the measurement of the intrinsic ability of a drug to initiate a response once it occupies receptor sites. Measurement of both the and the ICo 0 (potency) are clearly crucial when comparing the activity of similar drugs. The Hill coefficient measures the slope of the dose-effect curve which can be markedly influenced by the shape of the curve that describes the binding of the drug to the receptor. For many drugs, y lies between 0.6 and 1.5. The use of the Hill coefficient not only improves the fit of the data, but also indicates the influence of changes in dose or concentration on response: for example, when y is greater than 1, the slope is very steep, meaning that a marked change in drug effect is associated with a small change in dose or concentration of drug. On the other hand, when y is less than 1, with a shallow hyperbolic concentration effect relationship, the activity occurs over a wide range of drug levels. Hence, the different values of y can dramatically affect the drug's clinical usefulness In the present study, concentration-response curves were obtained for a series of corticosteroids. In these experiments, curve fitting was accomplished using a computer programme called "The Scientist" (MicroMath Scientific Software, Salt Lake City, Utah, USA.) in which the parameters, Emax, IC 50 and Hill coefficient for each steroids were estimated by using non-linear regression and least square fits.

The overall significance of differences between treatments was determined by one way analysis of variance, while the Tukey HSD test was used to examine the significance level of specific contrasts. The Systat for Windows program (Systat Inc, Evanston, Illinois, USA.) was used.

Example 2: Effects of TPA on skin of mice This study was conducted to determine the time course of effects produced by applying TPA to mice and killing at intervals of 1. 2. 3. 5 and 8 days. Peak times for WO 98/19683 PCT/AU97/00747 -13epidermal hyperplasia, dermal inflammation and skin-fold thickness were determined.

The object of this study was to determine the best time to sacrifice TPA-treated mice so as to obtain the maximum response to TPA. The literature indicates that TPA-induced epidermal hyperplasia and dermal inflammation peak at different times. It was thus expected that a compromise time would have to be selected.

Forty two female BALB/c strain mice were divided into the treatment groups and the mice were treated with a single application (100 L) of TPA (0.01% in acetone) and sacrificed at days 1, 2, 3, 5 and 8 and the time course of TPA effects on epidermal hyperplasia, dermal inflammatory cell infiltration and skin-fold thickness measured as described in Example 1.

The skin responses to TPA are summarized below: Day l Day2 Day 3 Day 5 Day 8 Increase in epidermal thickness 326% 382% 393% 270% 130% Increase in dermal inflammatory 397% 296% 272% 280% 225% cell density Increase in skin-fold thickness 193% 142% 124% 116% 107% The experiment showed that a single application of TPA caused epidermal thickening, dermal inflammation and an increase in skin-fold thickness that lasted for at least 8 days. The peak effects were observed at 72 hours for epidermal hyperplasia and at 24 hours for dermal inflammation and skin-fold thickening.

Based on these results it was decided that an appropriate compromise, for most experiments, would be to sacrifice the animals 24 hours after a single application of TPA. This would result in maximum effects for inflammation and skin-fold thickness and near maximum effects for epidermal hyperplasia (over 80% of peak effect). Unless otherwise stated, mice were sacrificed 24 hours after the application of TPA.

Example 3: Action of Different Corticosteroids In the first instance the ability of corticosteroids alone to inhibit TPA lesions was investigated. The following groups of corticosteroids were tested (the classification of the potencies of corticosteroids is dependent on the concentration used, the composition of the vehicle and the effect being studied) (Table 1).

Low potency: betamethasone, dexamethasone, hydrocortisone, hydrocortisone acetate.

WO 98/19683 PCT/AU97/00747 -14- Medium potency: alclometasone dipropionate, fluocortolone 21-pivalate.

High potency: betamethasone dipropionate, betamethasone valerate, fluocinolone acetonide, halcinonide, mometasone furoate, triamcinolone acetonide Mice were divided into treatment groups. TPA and corticosteroids were premixed to the concentrations required and applied to the backs of mice immediately.

For those steroids not very soluble in acetone betamethasone, dexamethasone, hydrocortisone and hydrocortisone acetate), the drugs were dissolved in 100 |L dimethylformamide before further dilution with acetone. The efficacy of corticosteroids in inhibiting epidermal hyperplasia, inflammatory cell infiltration and skin-fold o1 thickness was assessed as described previously. Concentration-response curves were determined after computer-fitting of data. The curve fitting technique was generated by a computer programme called "The Scientist" in which the parameters in the Hill Equation were generated. These included Emax. ICso, and the Hill coefficient for each steroid.

Concentration-response curves for each steroid were plotted and the relative potencies were determined from the IC 50 values. Comparisons were made of variations in ratios of

IC

0 s for each corticosteroids tested. These values were compared with those in the literature and reflected the relative intrinsic potencies of steroids.

WO 98/19683 PTA9/04 PCT/AU97/00747 Table 2 A summary of the concentration -response curves for inhibition of TPA-induced -epidermal hyperplasia by various steroids showing the values of E.max, We., 0 and gamma with respect to the Hill equation.

Corticosteroids inhibition) JIC 5 I Gamma (y) Aiclometasone dipropionate Betamethasone Betamethasone dipropionate Betamethasone valerate Dexamethasone Fluocinolone acetonide Fluocortolone 21-pivalate Halcinonide Hydrocortisone Hydrocortisone acetate Mometasone furoate Triamcinolone acetonide 96.59 7.90 (76.28-1 16.90) 94.19 7.33 (75.35-113.04) 95.59 6.55 (82.14-109.04) 82.24 2.84 (75.69-88.78) 90.70 5.72 (76.72-104.69) 89.60 6.93 (70.36 108.85) 85.18 9.51 (58.79-111.58) 92.55 2.98 (85.25-99.85) 99.04 9.54 (72.56- 125 .51) 79.63 7.62 (60.04-99.23) 83.31 3.04 (76.11-90.51) 89.80 6.40 (74.14-105.46) 0.89 0.30 (0.16-1.67) 13.81 3.73 (4.22-23.39) 0.81 0.36 (0.49-1.13) 0.15 0.02 (0.10-0.20) 1.26 0.44 (0.85-1.67) 0.39 0.14 (0.043-0.78) 0.40 0.15 (0.12-0.68) 0.97 0. 13 (0.66-1.27) 46.18 ±13.22 (9.47-82.90) 36.67 12.01 (5.80-67.56) 0.23 0.04 (0.14-0.33) 1.13 0.35 (0.28-1.98) 0.67 0.12 (0.36-0.97) 0.81 0.11 (0.5 1-1.10) 0.54 0.06 (0.37-0.71) 0.94 0.12 (0.66-1.21) 0.50 0.08 (0.31-0.69) 0.75 0.23 (0.12-1.38) 0.97 0.30 (0.13-1.82) 0.78 0.06 (0.62-0.94) 0.96 0.17 (0.49-1.44) 0.79 0.13 (0.46-1.13) 0.79 0.11 (0.53-1.04) 0.75 0.15 (0.39-1.11) Results are presented as means SD. Figures in brackets are confidence intervals WO 98/19683 PTA9/04 PCT/AU97/00747 Table 3 16- A summary of the con centration-response curves for inhibition of TPA-induced- inflammatory cell infiltration by various steroids showing the values of EM ICj 0 and gamma with respect to the Hill equation.

Corticosteroids I inhibition) 1 1 C 50 (M x 1W 4 Ga mm a (Y) Alciometasone dipropionate Betamethasone Betamethasone dipropionate Betamethasone valerate Dexamethasone Fluocinolone acetonide Fluocortolone 21-pivalate Halcinonide Hydrocortisone Hydrocortisone acetate Mometasone furoate Triamcinolone acetonide 82.12 5.65 (67.58-96.66) 74.55 3.29 (66.09-83.01) 90.77 3 .71 (83.18-98.37) 73.52 1.76 (69.46-77.57) 99.05 10.98 (72.18-125.93) 79.60 2.41 (74.05-85.15) 97.91 12.16 (64.15±131.67) 90.34 ±6.29 (74.94-105.74) 100.29 ±9.36 (71.35-129.23) 79.36 11.49 (59.39-99.33) 89.98 4.88.

(78.45-101.51) 77.24 1.26 (74.15-80.33) 0.32 0.09 (0.1 0-0.54) 13.12 1.65 (8.87 17.37) 0.29 0.06 (0.16-0.41) 0.29 0.03 (0.22-0.34)) 4.44 ±1.02 (3.19-5.69)_ 0.16 0.02 (0.11-0.21) 1.10 0.40 (0.55-1.65) 0.31 0.05 (0.14-0.48) 61.48 9.66 (39.13-83.83) 77.33 13.85 (60.28-94.58) 0.20 0.05 (0.08-0.33) 0.39 0.03 (0.333-0.46) 0.97 0.26 (0.3 1-1.63) 1.28 0.17 (0.85-1.71) 0.52 0.06 (0.39-0.65) 0.93 0.07 (0.77-1.09) 0.73-± 0.19 (0.25-1.20) 1.05 0.14 (0.72-1.38) 0.94 0.21 (0.36-1.54) 0.60 0.11 (0.32-0.88) 0.57 0.26 (0.25-0. 89) 1.11 0.27 (0.42-1.80) 0.69 0.14 -01 1.42 0.11 (1.14-1.70) Results are presented as means ±SD. Figures in brackets are confidence intervals WO 98/19683 PCT/AU97/00747 -17- Tables 2 and 3 provide an estimate of the efficacies potencies (ICo) and slope of the concentration-response curve for the 12 corticosteroids investigated in this study. These values were obtained from the Hill equation which is a modified form of the Michaelis-Menton equation.

The apparent excellent correlations between ICSo values could indicate that inhibition of inflammation and epidermal hyperplasia are mediated by the same mechanism or else that the limiting factor in producing the two effects was the ability of the steroid to penetrate the skin. The fact that the maximum effects and slopes (y) of the concentration-response curves for the two effects were very poorly correlated suggests that different mechanisms are involved in suppressing inflammation and epidermal hyperplasia by the steroids. In addition, the correlations between ICo values are not so impressive when the effects of certain outlier drugs are removed. The effect of removing outliers is shown in Table 4: Table 4: ICso values (inflammation vs epidermal hyperplasia) r r Plot of ICs 0 values (derived from Hill (read from graph where IC 50 (inflammation vs equation) concentration that inhibits epidermal hyperplasia) half the effect of TPA) All drugs included 0.961 (p<0.0005) 0.909 (p<0.0005) Hydrocortisone and 0.959 (p<0.0005) 0.988 (p<0.0005) hydrocortisone acetate not included Hydrocortisone, 0.741 (p 0.057) 0.637 (p 0.072) hydrocortisone acetate, betamethasone dipropionate, dexamethasone and fluocortolone 21-pivalate not included From the above results it seems likely that the steroids inhibit the inflammatory and hyperplastic effects of TPA by different mechanisms, either inducing different biochemical responses or producing the same response in different cell lines. This conclusion is very relevant to the possible synergistic effects of auranofin are described.

The determination of Emax values from the Hill equation could be subject to error due to some uncertainty about measurements made at the top of the concentration- SUBSTITUTE SHEET (Rule 26) WO 98/19683 PCT/AU97/00747 18response curves. Therefore, ICso values were determined by two methods: using the Emax value generated from the Hill equation (Tables 5 and and directly from the concentration-response curve, taking the ICso value as that concentration that inhibited of the TPA-induced hyperplasia and inflammation (Tables 7 and The difference between ICso values, and hence relative potencies, determined by the two methods was not great. However, direct reading from the concentration-response curve was considered more reliable and these readings were used for calculating the "synergistic factors" given in Tables 9 and Table 5 Actual and relative potencies of topical corticosteroids for inhibition of TPA-induced epidermal hyperplasia Ivalues generated from the Hill equation where IC 5 0 is the concentration that produced 50% of the maximum inhibitory effect (Emax) 1 Corticosteroids IC 5 0 for inhibition of epidermal Relative thickening (M x 10- 4 potency Hydrocortisone acetate 36.67 Hydrocortisone 46.18 0.79 Betamethasone 27.25 1.35 Dexamethasone 1.26 29.10 Triamcinolone acetonide 1.13 32.45 Halcinonide 0.97 37.80 Alclometasone dipropionate 0.89 41.20 Betamethasone dipropionate 0.81 45.27 Fluocortolone 21-pivalate 0.4 91.68 Fluocinolone acetonide 0.39 94.03 Mometasone furoate 0.23 159.43 Betamethasone valerate 0.15 244.47 WO 98/19683 PCT/AU97/00747 Table 6 19- Actual and relative potencies of topical corticosteroids for inhibition of TPA-induced inflammatory cell infiltration into the dermis Ivalues generated from the Hill equation where ICso is the concentration that produced 50% of the maximum inhibitory effect Corticosteroids IC 50 for inhibition of Relative inflammatory cell infiltration in potency the dermis (M x Hydrocortisone acetate 77.33 Hydrocortisone 61.48 1.26 Betamethasone 13.12 5.89 Dexamethasone 4.44 17.42 Fluocortolone 21-pivalate 1.10 70.30 Triamcinolone acetonide 0.39 198.28 Alclometasone dipropionate 0.32 241.66 Halcinonide 0.31 249.45 Betamethasone dipropionate 0.29 266.66 Betamethasone valerate 0.29 266.66 Mometasone furoate 0.20 386.65 Fluocinolone acetonide 0.16 483.31 Table 7 Actual and relative potencies of topical corticosteroids for inhibition of TPA-induced epidermal hyperplasia (values taken from concentration-response curve where ICo 5 0 is the concentration that inhibited 50% of the TPA effect).

Corticosteroids IC 5 0 for inhibition of epidermal Relative thickening (M x 10 potency Hydrocortisone acetate 70.00 Hydrocortisone 45.10 1.55 Betamethasone 50.00 1.40 Dexamethasone 2.00 35.0 Triamcinolone acetonide 1.40 50.0 Betamethasone dipropionate 1.40 50.0 Halcinonide 1.10 63.64 Alclometasone dipropionate 1.00 70.0 Fluocortolone 21-pivalate 0.60 116.67 Mometasone furoate 0.40 175.0 Betamethasone valerate 0.22 318.18 Fluocinolone acetonide 0.21 333.33 WO 98/19683 PCT/AU97/00747 Table 8 Actual and relative potencies of topical corticosteroids for inhibition of TPA-induced inflammatory cell infiltration into the dermis (values taken from concentration-response curve where ICso is the concentration that inhibited 50% of the TPA effect).

Corticosteroids ICs0 for inhibition of Relative inflammatory cell infiltration in potency the dermis (M x 10 4 Hydrocortisone acetate 110.0 Hydrocortisone 60.0 1.83 Betamethasone 21.0 5.23 Dexamethasone 4.10 26.83 Fluocortolone 21-pivalate 1.10 100.0 Triamcinolone acetonide 0.70 157.14 Betamethasone valerate 0.65 169.23 Alclometasone dipropionate 0.60 183.33 Halcinonide 0.60 183.33 Betamethasone dipropionate 0.40 275.0 Mometasone furoate 0.30 366.67 Fluocinolone acetonide 0.25 440.0 In the present study, hydrocortisone, hydrocortisone acetate, betamethasone and dexamethasone had low to medium potencies with respect to both inhibition of TPAinduced epidermal hyperplasia and TPA-induced inflammatory cell infiltration. This ranking was consistent with corresponding potencies in clinical setting that was shown in Table 1.

Halcinonide, triamcinolone acetonide, alclometasone dipropionate, betamethasone dipropionate, fluocortolone 21-pivalate were found to have medium to strong potencies in inhibition of TPA-induced epidermal hyperplasia and inflammatory cell infiltration, and these values were consistent with the clinical potencies.

Finally, mometasone furoate, betamethasone valerate, betamethasone dipropionate, and fluocinolone acetonide had strong to very strong potencies for TPAinduced epidermal hyperplasia. Amongst them, betamethasone valerate was shown to be the most potent agent. When their potencies for inhibition of TPA-induced inflammatory cell infiltration were investigated, they were also shown to have strong to very strong anti-inflammatory effect. Fluocinolone acetonide was found to be the most potent agent, with a relative potency of 483 (Table 6) or 440 (Table 8).

When comparisons were made between the relative potencies of the steroids tested in this study and their respective clinical potencies, the order of potency was generally the same.

WO 98/19683 PCT/AU97/00747 -21- It might be expected that a particular corticosteroid would have equal potency with respect to anti-hyperplastic and anti-inflammatory actions. Our results showed that these reactions were not necessarily closely related. Linear regression of the relative potencies for inhibition of the hyperplastic effects of the steroids vs relative potencies for suppression of inflammation gave a value r 0.573 (p =0.51) for data from tables 5 and 6 and a value of r 0.658 (p<0.0 2 for values in tables 7 and 8. Thus, about 65% of the variance between the two actions seems to be due to some common property (which could be lipid solubility) but a significant component of these actions differs with respect to suppression of hyperplasia and suppression of inflammation. This is also illustrated by comparing the rank orders of potency in Tables 7 and 8. Only six of the 12 steroids have the same rank for both effects and, of these steroids, four are the four least potent.

Example 2: Synergistic Effect Of Auranofin And Corticosteroids With Different Clinical Potencies Results of preliminary studies indicated that auranofin, under certain conditions, can inhibit some of the effects of TPA, although it is not particularly potent in this regard.

The present study examines whether combinations of auranofin and corticosteroids had a synergistic effect in suppressing TPA lesions.

Four corticosteroids with different clinical potencies ranging from weak to strong were chosen, namely, hydrocortisone, fluocinolone acetonide, betamethasone dipropionate and mometasone furoate. TPA was premixed with the corticosteroids in the presence or absence of a fixed concentration of auranofin to produce the required concentrations and applied to the backs of mice immediately. Concentration-response curves were determined by non-linear regression using least squares fitting. IC 50 values were determined by reading the value from the graph that corresponded to 50% of the effect produced by TPA (Tables 9 and The term 'apparent ICs 5 refers to the value for the combination of steroid and auranofin.

WO 98/19683 PCT/AU97/00747 22 Table 9 Apparent ICs( values obtained from the computer fitted graph for the effects -on TPA-induced epidermal hyperplasia of four corticosteroids in the absence and presence of auranofin Apparent ICs (M x 10 4 Corticosteroids without with auranofin Synergistic auranofin factor Betamethasone dipropionate 1.40 0.36 0.025 0.003 56.0 Hydrocortisone 45.00 13.22 22.00 11.23 2.05 Fluocinolone acetonide 0.21 0.14 0.016 0.002 13.13 Mometasone furoate 0.40 0.04 0.31 0.05 1.29 Results are presented as means SD.

Table 10 Apparent ICso values obtained from the computer fitted graph for the effects on TPA-induced dermal inflammatory cell infiltration of four corticosteroids in the absence and presence of auranofin Apparent ICo (M x 10" 4 Corticosteroids without with auranofin Synergistic auranofin factor Betamethasone dipropionate 0.40 0.06 0.090 0.016 4.44 Hydrocortisone 60.00 9.66 31.00 4.12 1.94 Fluocinolone acetonide 0.25 0.002 0.11 0.013 2.27 Mometasone furoate 0.30 0.05 0.008 0.001 37.50 Results are presented as means SD.

The value termed the 'synergistic factor' is defined as the IC 5 s value for the steroid determined in the absence of auranofin divided by the ICso for the same steroid Sdetermined in the presence of auranofin Synergism refers to situations in which a combination of two drugs produces an effect that is significantly greater than the algebraic sum of the effects when the same dose or concentration of each drug is observed separately in the same test system.

Synergism can result in a multifold potentiation of the effects of one or both drugs or it can give rise to effects that are qualitatively different from those elicited by the drugs when used separately.

With respect to effects on epidermal hyperplasia, only two of the four steroids tested could be regarded as showing a synergistic reaction with auranofin, namely betamethasone dipropionate and fluocinolone acetonide. From results depicted in Tables 9 and 10 it can be seen that in the case of betamethasone dipropionate and fluocinolone acetonide, the per cent increase in the apparent potencies of the steroids is 5,600% and 1,300%, respectively. However, in the case of the least potent of the four steroids, namely, hydrocortisone. the apparent increase in potency was 100%. A more effective WO 98/19683 PCT/AU97/00747 -23way of demonstrating the presence of true synergism is to compare separately the following: 1) auranofin alone, 2) a low concentration of steroid alone (sufficient to inhibit about 20% of the effects of TPA this value can be read from the concentration-response curve for the steroid when studied alone), 3) the same concentration of steroid as in combined with auranofin this value can be obtained from the dose-response curve for steroid in the presence of auranofin, and 4) a concentration of the same steroid used in but in sufficient concentration as to produce the same effect as that achieved in If the effects of appear to be the summation of and the result is not synergism. If the effects of greatly exceed those of and if added arithmetically, the result is synergism according to our definition.

The results for epidermal hyperplasia are displayed in Figure 1. Auranofin alone inhibited TPA-induced epidermal hyperplasia by about 10% in all four studies.

Betamethasone dipropionate 1 x 10 5 M alone caused about 20% inhibition of TPA effect. The combination of betamethasone dipropionate (1 x 10 5 M) and auranofin produced about 65% inhibition of TPA effect. To gauge the significance of the increased effect that resulted when auranofin was added to betamethasone dipropionate, comparison should be made with the concentration of betamethasone dipropionate that, in the absence of auranofin, produced the same effect. This value was 5 x 10" 4 M or times the concentration that produced the same effect in the presence of auranofin.

With respect to epidermal hyperplasia, the studies demonstrate that: a massive synergism results when auranofin is added to betamethasone dipropionate and to fluocinolone acetonide; a minor degree of synergism may result from the combination of hydrocortisone and auranofin; and that no synergism or even additive effect results when auranofin is co-administered with mometasone furoate.

With respect to inflammatory cell infiltration into the dermis, the results in Table 10 indicate that the effects of a combination of auranofin and mometasone furoate is the result of synergism since the apparent IC 50 is increased by about 3,800%. It is also possible that a lesser degree of synergism occurs with respect to the anti- WO 98/19683 PCT/AU97/00747 24 inflammatory action of betamethasone dipropionate in the presence of 0.2% auranofin.

Here the increase in apparent ICso is of the order of 400-500% (Table The results in Figure 2 show a massive synergism between mometasone furoate x 10.6 M) and auranofin This combination produced an effect that was equal to that produced by 1 x 10.3 M mometasone in the absence of auranofin. Figure 2 also indicates that synergism may exist for the combination of auranofin with betamethasone dipropionate and fluocinolone acetonide, but not with hydrocortisone.

The results of these studies indicate that extensive synergism results from the combination of auranofin with certain corticosteroids, such as for example betamethasone dipropionate and fluocinolone acetonide as regards reduction of epidermal hyperplasia, and with others such as for example mometasone furoate as regards reduction of inflammation. Lesser degrees of synergism may exist between auranofin and other steroids.

Gold compounds and corticosteroids, as well as their formulations, which can be suitably used in the present invention have been discussed in detail in the present application or in Australian patent No. 616 755, which is incorporated herein by reference.

Claims

1. A method of treating an immune-mediated disorder having an inflammatory component and/or a cellular hyperproliferation component, comprising the step of administering to a patient requiring such treatment a gold compound and at least one corticosteroid, wherein the at least one corticosteroid is selected to interact with the gold compound to exhibit preferential synergistic action towards one of the components of said disorder or to exhibit equal action towards each component of said disorder provided that said method does not include the administration of a combination of auranofin and betamethazone dipropionate.

2. A method of treating an immune-mediated disorder according to claim 1 wherein the disorder has an inflammatory component and a cellular hyperproliferation component.

3. A method of treating an immune-mediated disorder according to any one of the preceding claims wherein the gold compound and the at least one corticosteroid are 15 administered simultaneously.

4. A method of treating an immune-mediated disorder according to any one of the preceding claims wherein the gold compound and the at least one corticosteroid are administered sequentially.

5. A method of treating an immune-mediated disorder according to claim 4 wherein 20 the at least one corticosteroid is administered after the gold compound.

6. A method of treating an immune-mediated disorder according to any one of the preceding claims comprising the step of administering at least two corticosteroids, at least one of which is selected to interact with the gold compound to exhibit preferential synergistic action towards the inflammatory component,-and at least another is selected to interact with the gold compound to exhibit preferential synergistic action towards the cellular hyperproliferation component of said disorder.

7. A method according to any one of the preceding claims, wherein the disorder is an immune-mediated dermatological disorder.

8. A method according to claim 7, wherein the disorder is psoriasis.

9. A method according to claim 7, wherein the disorder is dermatitis.

20276-80.DOC/ A method according to any one of claims 1 to 6 wherein the disorder is rheumatoid arthritis. 11. A method according to any one of the preceding claims, wherein the gold compound is lipid soluble. 9 9 *9* e 20276-80.DOC/ PCT/AU 9 7/ 0 0 7 4 7 RECEIVED 2 2 SEP 1998 -26- 12. A method according to any one of the preceding claims, wherein the at least one corticosteroid is selected to interact with the gold compound to exhibit synergistic activity towards cellular hyperproliferation in preference to inflammation. 13. A method according to claim 12, wherein the at least one corticosteroid is selected from the group consistin of betamethasone dipropionate, fluocinolone acetonide and hydrocortisone. 14. A method according to any one of the preceding claims, wherein the at least one corticosteroid is selected to interact with the gold compound to exhibit synergistic activity towards inflammation in preference to cellular hyperproliferation. 15. A method according to claim 14, wherein the at least one corticosteroid is selected from the group consisting of betamethasone dipropionate, fluocinolone acetonide and mometasone furoate. 16. A method according to claim 10 wherein the corticosteroid is selected from the group comprising hydrocortisone acetate, hydrocortisone, betamethasone, betamethasone dipropionate, dexamethasone, fluocortolone 21-pivalate, triamcinolone acetonide, betamethasone valerate, alclometasone dipropionate, halcinonide, mometasone furoate and fluocinolone acetonide. 17. A method according to claim 16 wherein the corticosteroid is selected from the group comprising hydrocortisone, betamethasone dipropionate, mometasone furoate and fluocinolone acetonide. 18. A method according to any one of the preceding claims wherein the gold compound is auranofin. 19. A method according to any one the preceding claims, wherein the gold compound is administered systemically. 20. A method according to any one of claims 1 to 18, wherein the gold compound is administered orally. 21. A method according to any one of claims 1 to 18, wherein the gold compound is administered locally. 22. A method according to any one of claims 1 to 18, wherein the gold compound is administered topically. 23. A method according to any one of claims 1 to 18, wherein the gold compound is administered by intra-articular injection. SlzuED SHEET !PEA/AU -27- 24. A method according to anyone of the preceding claims, wherein the at least one corticosteroid is administered systemically. A method according to anyone of claims 1 to 23, wherein the at least one corticosteroid is administered orally. 26. A method according to any one of claims 1 to 23, wherein the at least one corticosteroid is administered locally. 27. A method according to any one of claims 1 to 23, wherein the at least one corticosteroid is administered topically. 28. A method according to any one of claims 1 to 23, wherein the at least one corticosteroid is administered by intra-articular injection. 29. A pharmaceutical composition comprising a gold compound and one or more corticosteroids, the corticosteroid being selected to interact with the gold compound to exhibit a preferential synergistic action towards an inflammatory component and/or a cellular hyperproliferation component of an immune-mediated disorder, in combination 15 with a pharmaceutically acceptable carrier, excipient, adjuvant or solvent provided that said composition does not include auranofin and betamethazone dipropionate. 30. A pharmaceutical composition according to claim 29, wherein the composition is formulated for systemic administration. S31. A pharmaceutical composition according to claim 29, wherein the composition is 20 formulated for oral administration. 32. A pharmaceutical composition according to claim 29, wherein the composition is formulated for local administration. 33. A pharmaceutical composition according to claim 29, wherein the composition is formulated for topical administration. 34. A pharmaceutical composition according to claim 29, wherein the composition is formulated for administration by intra-articular injection. A pharmaceutical composition according to any one of claims 29 to 34, wherein the corticosteroid is selected from the group comprising hydrocortisone acetate, Rhydrocortisone, betamethazone, betamethazone dipropionate, dexamethasone, fluocortolone 21-pivalate, triamcinolone acetonide, betamethazone valerate, 20276-80.DOC/ -28- alclometasone dipropionate, halcinonide, mometasone furoate and fluocinolone acetonide. 36. A pharmaceutical of treating an immune mediated disorder according to any one of claims 29 to 34 comprising the administration of a pharmaceutical composition according to claim 35, wherein the corticosteroid is selected from the group comprising hydrocortisone, betamethasone dipropionate, mometasone furoate and flucinolone acetonide. 37. A pharmaceutical according to any one of claims 29 to 34 and claim 36, wherein the gold compound is auranofin. 38. Use of a gold compound and at least one corticosteroid for the manufacture of a medicament for treating an immune-mediated disorder having an inflammatory component and/or a cellular hyperproliferation component, wherein the at least one corticosteroid is selected to interact with the gold compound to exhibit preferential synergistic action towards one of the components of said disorder or to exhibit equal 15 action towards each component of said disorder. 39. Use according to claim 38, wherein the disorder has an inflammatory component and a cellular hyperproliferation. Use according to claim 38 or claim 39, wherein the gold compound and the at least ne corticosteroid are to be administered simultaneously. 20 41. Use according to any one of claims 38 to 40, wherein the gold compound and the at least one corticosteroid are to be administered sequentially. 42. Use according to claim 41, wherein the at least one corticosteroid is to be administered after the gold compound. 43. Use according to any one of claims 38 to 42, wherein the medicament comprises at least two corticosteroids, at least one of which is selected to interact with the gold compound to exhibit preferential synergistic action towards the inflammatory component, and at least another is selected to interact with the gold compound to exhibit 20276-80.DOC -29- preferential synergistic action towards the cellular hyperproliferation component of said disorder. 44. Use according to any one of claims 38 to 43, wherein the disorder is an immune- mediated dermatological disorder. 45. Use according to claim 44, wherein the disorder is psoriasis. 46. Use according to claim 44, wherein the disorder is dermatitis. 47. Use according to any one of claims 38 to 43, wherein the disorder is rheumatoid arthritis. 48. Use according to any one of claims 38 to 47, wherein the gold compound is lipid 10 soluble. 49. Use according to any one of claims 38 to 48, wherein the at least one corticosteroid i is selected to interact with the gold compound to exhibit synergistic activity towards cellular hyperproliferation in preference to inflammation. 50. Use according to claim 49, wherein the at least one corticosteroid is selected from 15 the group consisting of betamethasone dipropionate, fluocinolone acetonide and hydrocortisone. S* 51. Use according to any one of claims 38 to 50, wherein the at least one corticosteroid is selected to interact with the gold compound to exhibit synergistic activity towards inflammation in preference to cellular hyperproliferation. 52. Use according to claim 51, wherein the at least one corticosteroid is selected from the group consisting of betamethasone dipropionate, fluocinolone acetonide and mometasone furoate. 20276-80.DOC 53. Use according to claim 47, wherein the corticosteroid is selected from the group comprising hydrocortisone acetate, hydrocortisone, betamethasone, betamethasone dipropionate, dexamethasone, fluocortolone 21-pivalate, triamcinolone acetonide, betamethasone valerate, alclometasone dipropionate, halcinonide, mometasone furoate and fluocinolone acetonide. 54. Use according to claim 53, wherein the corticosteroid is selected from the group comprising hydrocortisone, betamethasone dipropionate, mometasone furoate and fluocinolone acetonide. Use according to any one of claims 38 to 54, wherein the gold compound is 10 auranofin. 56. Use according to any one of claims 38 to 55, wherein the gold compound is to be administered systemically. 57. Use according to any one of claims 38 to 55, wherein the gold compound is to be o: 0administered orally. *o. Is. 58. Use according to any one of claims 38 to 55, wherein the gold compound is to be administered locally. S59. Use according to any one of claims 38 to 55, wherein the gold compound is to be administered topically. Use according to any one of claims 38 to 55, wherein the gold compound is to be administered by intra-articular injection. 61. Use according to any one of claims 38 to 60, wherein the at least one corticosteroid is to be administered systemically. 20276-80.DOC -31- 62. Use according to any one of claims 38 to 60, wherein the at lease one corticosteroid is to be administered orally. 63. Use according to any one of claims 38 to 60, wherein the at least one corticosteroid is to be administered locally. 64. Use according to any one of claims 38 to 60, wherein the at least one corticosteroid is to be administered topically. Use according to any one of claims 38 to 60, wherein the at least one corticosteroid is to be administered by intra-articular injection. 66. A method of treating an immune-mediated disorder having an inflammatory 10 component and/or a cellular hyperproliferation component, substantially as herein described with reference to any one of the examples. i 67. A pharmaceutical composition comprising a gold compound and one or more •corticosteroids, substantially as herein described with reference to any one of the S examples. DATED this 28th day of January 2000 MEDICAL INNOVATIONS LIMITED **ee F Attorney: IVAN A. RAJKOVIC Fellow Institute of Patent Attorneys of Australia of BALDWIN SHELSTON WATERS 20276-80.DOC