ATBECHDEDKESFRGBGRITLI..NLSE..PTIE..............................................*JDIM360 Ver 2.4 (29 Nov 2007) - 2999001/0The file contains technical information submitted after the application was filed and not included in this specification0938315CORRECTED EUROPEAN PATENT SPECIFICATIONB9B120080220W154deBibliographieenBibliographyfrBibliographiedeAnsprüche ENenClaims ENfrRevendications ENEP97946484.9199710241999052520011112enenen29301 P19961025US45331 P19970501US2008022020080819990901199935200707182007292005062320080220200808A61K 31/47 20060101AFI20050603BHEP A61K 31/435 20060101ALI20050603BHEP A61P 37/08 20060101ALI20050603BHEP A61P 31/08 20060101ALI20050603BHEP A61P 33/00 20060101ALI20050603BHEP A61P 37/00 20060101ALI20050603BHEP A61P 31/04 20060101ALI20050603BHEP deVERBINDUNGEN, DIE DIE IMMUNANTWORT MODIFIZIEREN, ZUR BEHANDLUNG VON TH2-VERMITTELTEN UND VERWANDTEN ERKRANKUNGENenIMMUNE RESPONSE MODIFIER COMPOUNDS FOR TREATMENT OF TH2 MEDIATED AND RELATED DISEASESfrCOMPOSES MODIFICATEURS DE LA REPONSE IMMUNITAIRE POUR LE TRAITEMENT DES MALADIES INDUITES PAR LES TH2 OU ASSOCIEESEP-A- 0 193 329VARNER ET AL: "effects of imiquimod on post-viral asthma-like syndrome" J OF ALLERGY AND CLINICAL IMMUNOLOGY, vol. 99, no. 1(2), 26 February 1996, page s127 XP002055521TOMAI, Mark, A.P.O. Box 33427Saint Paul, MN 55133-3427USHAMMERBECK, David, M.P.O. Box 33427Saint Paul, MN 55133-3427USSWINGLE, Karl, F.P.O. Box 33427Saint Paul, MN 55133-3427USMINNESOTA MINING AND MANUFACTURING COMPANY00300410C 1631 EP3M Center, P.O. Box 33427St. Paul, Minnesota 55133-3427USVossius & Partner00100314Siebertstrasse 481675 MünchenDEATBECHDEDKESFRGBGRIEITLINLPTSEUS199701999019971024enWO19980172791998043019981719990901199935

The present invention relates to the use of immunomodifying imidazoquinoline amines, imidazopyridine amines 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a pharmaceutical composition for the treatment of a non-viral and non-tumor T helper-type 2 (TH2) mediated disease. It also relates to the use of these compounds for the preparation of a pharmaceutical composition for the treatment of a non-viral and non-tumor disease, whereby the induction of interleukin (IL)-4 an IL-5, is inhibited, and to the use of these compounds for the preparation of a pharmaceutical composition for the treatment of eosinophilia.

Many imidazoquinoline amine, imidazopyridine amine, 6,7-fused cycloalkylimidazopyridine amine, and 1,2-bridged imidazoquinoline amine compounds have demonstrated potent immunostimulating, antiviral and antitumor (including anticancer) activity, and have also been shown to be useful as vaccine adjuvants to enhance protective immune system response to vaccines. These compounds are hereinafter sometimes collectively referred to as the "IRM" (immune response modifier) compounds useful in the invention. Such compounds are disclosed in, for example, U.S. Patents 4,689,338, 5,389,640, 5,268,376, 4,929,624, 5,266,575, 5,352,784, 5,494,916, 5,482,936, 5,346,905, 5,395,937, 5,238,944, and 5,525,612, WO 93/20847, and European Patent Application 90 30 1766.3, wherein their immunostimulating, antiviral and antitumor activities are discussed in detail, and certain specific diseases are identified as being susceptible to treatment therewith, including basal cell carcinoma, eczema, essential thrombocythaemia, hepatitis B, multiple sclerosis, neoplastic diseases, psoriasis, rheumatoid arthritis, type I herpes simplex, type II herpes simplex, and warts. One of these IRM compounds, known as imiquimod, has been commercialized in a topical formulation, Aldara, for the treatment ofanogenital warts associated with human papilloma virus.

The mechanism for the antiviral and antitumor activity of these IRM compounds is thought to be due in substantial part to enhancement of the immune response due to induction of various important cytokines (e.g., interferons, interleukins, tumor necrosis factor, etc.). Such compounds have been shown to stimulate a rapid release of certain monocyte/macrophage-derived cytokines and are also capable of stimulating B cells to secrete antibodies which play an important role in these IRM compounds' antiviral and antitumor activities. One of the predominant - immunostimulating responses to these compounds is the induction of interferon (IFN)-α production, which is believed to be very important in the acute antiviral and antitumor activities seen. Moreover, up regulation of other cytokines such as, for example, tumor necrosis factor (TNF), IL-1 and IL-6 also have potentially beneficial activities and are believed to contribute to the antiviral and antitumor properties of these compounds.

However, there are many diseases where the immune system itself actually appears to play a significant role in mediating the disease (i.e., the immune system action takes part in actually causing the disease or an inappropriate type of immune response prevents the correct response from irradicating the disease). Many such diseases are thought to involve a pathologic or inappropriate immune response by the humoral branch of the immune system, which is associated with TH2 cell activity (as opposed to TH1 cell mediated immunity).

The humoral/TH2 branch of the immune system is generally directed at protecting against extracellular immunogens such as bacteria and parasites through the production of antibodies by B cells; whereas the cellular/TH1 branch is generally directed.at intracellular immunogens such as viruses and cancers through the activity of natural killer cells, cytotoxic T lymphocytes and activated macrophages. TH2 cells are believed to produce the cytokines IL-3, IL-4, IL-5, and IL-10, which are thought to stimulate production of IgE antibodies, as well as be involved with recruitment, proliferation, differentiation, maintenance and survival of eosinophils (i.e., leukocytes that accept an eosin stain), which can result in eosinophilia. Eosinophilia is a hallmark of many TH2 mediated diseases, such as asthma, allergy, and atopic dermatitis.

The interplay and importance of various aspects of immune system response, including interaction between TH1 and TH2 cell cytokines is discussed in WO 97/2688. Although WO 97/2688 is specifically concerned with the effects of a particular antiviral compound known as Ribavirin®, which is dissimilar to the IRM compounds useful in the present invention, it nonetheless illustrates some of the complex and unpredictable effects of drug compounds on the immune system.

EP-A-0 193 329 discloses certain pyrazolopyridines, their preparation and pharmaceutical compositions containing them.

It has now been found that in addition to their immunostimulatory, antiviral/antitumor effect on the immune system, the IRM compounds useful in the present invention-imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines-are also extremely useful for down regulating certain key aspects of the immune response. Specifically, the IRM compounds useful in the present invention have been found to inhibit TH2 immune response (in addition to enhancing TH1 immune response). This is extremely important for treating TH2 mediated diseases where an inappropriate TH2 response is causing the disease or preventing eradication of the disease by TH1 response. Thus, when administered in a therapeutically effective amount these IRM compounds can be used for treating TH2 mediated diseases. Accordingly, in a first embodiment, the present invention relates to the use of an immune response modifier compound selected from imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a pharmaceutical composition for the treatment of a non-viral and non-tumor, TH2 cell mediated disease with the proviso that said disease is other than eczema.

An apparently related effect of the IRM compounds useful in the present invention is to inhibit the induction of IL-4, IL-5, and perhaps other cytokines, which thereby allows for treatment of diseases associated with these cytokines. Accordingly, in a second embodiment, the present invention relates to the use of an immune response modifier compound selected form imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a pharmaceutical composition for the treatment of a non-viral and non-tumor disease, whereby the induction of IL-4 and/or IL-5 cytokines is inhibited, with the proviso that said disease is other than eczema. A further important and surprising effect of the compounds useful in the present invention is the suppression of eosinophils, which allows for treatment of eosinophilia and related diseases. Accordingly, in a third embodiment, the present invention relates to the use of an immune response modifier compound selected from imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a pharmaceutical composition for the treatment of eosinophilia, with the proviso that said disease is other than eczema.

Some diseases that are thought to be caused/mediated in substantial part by TH2 immune response, IL-4/IL-5 cytokine induction, and/or eosinophilia (and accordingly responsive to treatment by administering a therapeutically effective amount of the IRM compounds) include asthma, allergic rhinitis, systemic lupus erythematosis, Ommen's syndrome (hypereosinophilia syndrome), certain parasitic infections, for example, cutaneous and systemic leishmaniasis, toxoplasma infection and trypanosome infection, and certain fungal infections, for example candidiasis and histoplasmosis, and certain intracellular bacterial infections, such as leprosy and tuberculosis. These are examples of non-viral and non-tumor, TH2 mediated diseases for which effective treatment with the IRM compounds useful in the present invention clearly could not have been predicted. Additionally, it should also be noted that diseases having a viral or cancer related basis, but with a significant TH2 mediated pathology can also be beneficially treated with the IRM compounds useful in the present invention. In particulary preferred uses of the present invention, the pharmaceutical compositions are for the treatment of diseases associated with eosinophilia, such as asthma and allergic rhinitis.

The IRM compounds useful in the present invention may be administered via any suitable means, for example, parenterally, transdermally, and orally. One preferred delivery route is via a topical gel or cream formulation. For treatment of asthma and allergic rhinitis, it is preferred to deliver the IRM compound via oral and/or nasal inhalation from a metered dose inhaler.

Particularly preferred IRM compounds include 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol and 1-(2-methylpropyl)-1H-imidazo[4,5-c]quinolin-4-amine (known as Imiquimod).

Finally, it should be noted that the diseases identified as being treatable in the published patents referred to above (U.S. Patents 4,689,338, 5,389,640, 5,268,376, 4,929,624, 5,266,575, 5,352,784, 5,494, 916, 5,482,936, 5,346,905, 5,395,937, 5,238,944, and 5,525,612, WO 93/20847, and European. Patent Application 90 30 1766.3) are generally either viral/tumor based or, if not, are thought not to be TH2 mediated diseases. One exception is eczema, which, although a TH2 mediated disease, is believed to have been identified due to a susceptibility to treatment with interferon (which was then understood to be the main cytokine response induced by the compounds useful in the present invention. There was, however, no recognition at the time that any TH2, IL-4/5, or eosinophilia suppressing ability of these IRM compounds could be used for treating eczema.

Preferred IRM Compounds

As noted above, many of the imidazoquinoline amine, imidazopyridine amine, 6,7-fused cycloalkylimidazopyridine amine, and 1,2-bridged imidazoquinoline amine IRM compounds useful in the present invention have demonstrated significant immunomodulating activity. Preferred immune response modifier compounds include 1H-imidazo[4,5-c]quinolin-4-amines defined by one of Formulas I-V below: wherein

wherein wherein wherein wherein or a pharmaceutically acceptable salt of any of the foregoing.

Preferred 6.7 fused cycloalkylimidazopyridine amine IRM compounds are defined by Formula VI below: wherein

and pharmaceutically acceptable salts thereof.

Preferred imidazopyridine amine IRM compounds are defined by Formula VII below: wherein

and pharmaceutically acceptable salts thereof.

Preferred 1,2-bridged imidazoquinoline amine IRM compounds are defined by Formula VIII below: wherein

and pharmaceutically acceptable salts thereof,

The compounds recited above are disclosed in the patents and applications noted above.

The substituents R11 - R17 above are generally designated "1-substituents" herein. The preferred 1-substituents are alkyl containing one to six carbon atoms and hydroxyalkyl containing one to six carbon atoms. More preferably the 1 - substituent is 2-methylpropyl or 2-hydroxy-2-methylpropyl.

The substituents R21 - R27 above are generally designated "2-substituents" herein. The preferred 2-substituents are hydrogen, alkyl of one to six carbon atoms, alkoxyalkyl wherein the alkoxy moiety contains one to four carbon atoms and the alkyl moiety contains one to four carbon atoms, and hydroxyalkyl of one to four carbon atoms. More preferably the 2-substituent is hydrogen, methyl, butyl, hydroxymethyl, ethoxymethyl or methoxyethyl.

In instances where n can be zero, one, or two, n is preferably zero or one:

The amounts of these IRM compounds that will be therapeutically effective in a specific situation will of course depend on such things as the activity of the particular compound, the mode of administration, and the disease being treated. As such, it is not practical to identify specific administration amounts herein; however, those skilled in the art will be able to determine appropriate therapeutically effective amounts based on the guidance provided herein, information available in the art pertaining to these compounds, and routine testing.

Immune System Mechanisms

Recent evidence indicates that the immune system can be broken down into two major arms, the humoral and cellular arms. The humoral arm is important in eliminating extracellular pathogens such as bacteria and parasites through production of antibodies by B cells. On the other hand, the cellular arm is important in the elimination of intracellular pathogens such as viruses through the activity of natural killer cells, cytotoxic T lymphocytes and activated macrophages. In recent years it has become apparent that these two arms are activated through distinct T helper cell (TH) populations and their distinct cytokine production profiles. T helper type 1 (TH1) cells are believed to enhance the cellular arm of the immune response and produce predominately the cytokines IL-2 and IFN-γ; whereas, T helper 2 (TH2) cells are believed to enhance the humoral arm of the immune response and produce cytokines, such as interleukin-3 (IL-3), interleukin-4 (IL-4), interleukin-5 (lL-5) and granulocyte-macrophage colony-stimulating factor (GM-CSF). In the TH2 case, IL-3, IL-5 and GM-CSF are thought to stimulate eosinophilopoiesis. In addition, IL-5 facilitates terminal differentiation and cell proliferation of eosinophils and promotes survival, viability and migration of eosinophils, while IL-4 stimulates production of antibodies of the IgE class. IgE is an important component in allergies and asthma. IL-5 may also prime eosinophils for the subsequent actions of other mediators.

In contrast, the TH 1 cytokines, IL-2 and IFN-γ, are important in activating macrophages, NK cells and CTL (cytotoxic T lymphocytes). IFN-γ also stimulates B cells to secrete specifically cytophilic antibody for the elimination of virally-infected cells. Interestingly, IFN-α, a macrophage-derived cytokine has been shown to antagonize TH2-type responses. IFN-α also appears to inhibit the proliferation and cytokine production of TH2 cells and enhances IFN-γ production by TH1 cells. In addition, IFN-α also appears to inhibit IgE production and antigen-induced increases in IL4 mRNA levels.

TH1 stimulation versus TH2 down regulation

IRM compounds useful in the present invention have been shown in a number of models to augment cell mediated immunity, which is consistent with stimulation of TH1 cells. Surprisingly, in models of eosinophilia (TH2/humoral immune mediated process) these compounds actually inhibit the eosinophilia. Further studies indicate that the way in which these compounds are achieving this is in part by their ability to inhibit TH2 cell production of the cytokine IL-5. We have shown in both in vitro and in vivo models, inhibition of IL-5 production by imidazoquinolines. For example, as shown in Table 1, an exemplary IRM compound 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol dramatically inhibits IL-5 production in spleen cell cultures stimulated with antigen. Spleen cells from OVA-sensitized CFW mice (2x106/ml) were cultured for 96 hr with OVA (100µg/ml). Some cultures also received this IRM compound over a range of concentrations. Culture supernatants were collected and analyzed by ELISA (Endogen) for IL-5. Results are presented as the mean of triplicate cultures±SEM. IL-5 concentration is in pg/ml. <b>Table 1</b> Inhibition of Mouse Spleen Cell Production of IL-5 Treatment IRM Compound Concentration IL-5 Concentration (pg/ml) OVA alone 240±20 OVA + IRM Compound 10µg/ml 12±2 OVA + IRM Compound 1µg/ml 22±3 OVA + IRM Compound 0.1µg/ml 25±8 OVA + IRM Compound 0.01µg/ml 125±46 Medium 57±27

As can be seen from Table 1, concentrations of IRM compound as low as 0.01 µg/ml inhibit IL-5 production by greater than 60%; whereas, higher concentrations inhibit IL-5 production by 100%.

In vivo, the exemplary IRM compound 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol was shown to inhibit antigen induced IL-5 production in a dose dependent manner, as shown in Table 2. CFW male mice were sensitized with OVA as described above. 14 days after the last sensitization animals were challenged with 100 µg OVA sc. Some animals received the free-base of 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol po either at the same time of OVA challenge or 24 hrs before. Serum was collected 7 hrs after OVA and analyzed for IL-5 and IFN-γ concentrations. Results are expressed as the mean cytokine concentration ±SEM. <b>Table 2</b> Effects of IRM Compounds on IL-5 and IFN-γ Production IRM Compound Dose (mg/kg) Cytokine Concentration (pg/mL) ±SEM -24.hr IL-5 (pg/mL) 0 hr IL-5 (pg/mL) 0.01 78 96 0.1 49 62 1.0 38 40 10.0 8 29 Sen. Control 213 270 Normal Control 1 1

It can thus be seen that 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol was active when given either at the same time of antigen challenge or when given a day before antigen. Doses as low as 0.01 mg/kg inhibited IL-5 production by at least 65%.

One common feature of many TH2 mediated diseases is an accumulation of eosinophils, referred to as eosinophilia. For example, chronic pulmonary inflammation involving eosinophil infiltration is a characteristic hallmark feature of bronchial asthma. Increased numbers of eosinophils have been observed in blood, bronchoalveolar lavage fluid and pulmonary tissue in patients with asthma, but the mechanism(s) responsible for their recruitment into and regulation within pulmonary tissues undergoing allergic or pro-inflammatory reactions has not been fully understood. Mediators and cytokines from T-lymphocytes and effector cells such as basophils, mast cells, macrophages and eosinophils have been implicated in enhancing cell maturation, chemotaxis and activation of eosinophils. Evidence suggests that an association exists between the immune system, especially CD4+ T cells, and eosinophils and eosinophil recruitment. Studies in asthmatics and in animal models of allergic pulmonary responses support this notion with the evidence of close correlations between the relative numbers of T cells and activated eosinophils in the airways. The importance of T-lymphocyte in eosinophil recruitment is strengthened by studies with T cell-selective immunosuppressive agents like cyclosporin A, FK506 and cyclophosphamide. These agents have been shown to reduce eosinophilia. Immunostimulants on the other hand have generally not been shown to clearly reduce eosinophilia. However, this may be a reflection on how these immunostimulants are affecting the immune system.

The following three sets of studies clearly indicate that the IRM compounds useful in the present invention can be used to suppress eosinophilia.

The first set of studies evaluate the IRM compound 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol for its ability to inhibit antigen-induced eosinophilia in the lung after aerosol challenge with antigen. Results in Table 3 show that 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol at 1 mg/kg is capable of inhibiting antigen-induced eosinophilia in the lung of mice by 78% when given 15 minutes prior to antigen challenge. Concentrations of IL-4 were reduced in the BAL of these mice by 43% when compared to animals receiving antigen alone. Also, the lRM compound induced inhibition of eosinophilia correlated with a significant inhibition in BAL concentrations of IL-5. which were reduced by 78%. CFW mice were sensitized on day 0 with 10 µg ofovalbumin (OVA) ip in 1% alum and then boosted 7 days later with the same regimen. Fourteen days after boosting animals were dosed by nebulization for 30 minutes using a 1% OVA solution. This was repeated on days 17 and 20. Twenty-four hours after the final nebulized dose animals were sacrificed and bronchoalveolar lavage (BAL) was performed using 1.0 ml of PBS containing 1% fetal bovine serum. BAL was stored at -70°C before analyzed. Lungs were then removed and placed in 0.5% cetrimide, 0.05 M KH2PO4 for homogenization of 4 X 30 seconds with 30 second cooling intervals between on ice. Centrifugation was then done at 1300 rpm (400 X g) for 30 minutes at 4C. Pellet was collected and resuspended in 4 ml 0.5 % cetrimide, 0.05 M KH2PO4 buffer. Samples were then frozen until sonication and the EPO assessment. This was followed by sonication for 3 X 15 seconds with 30 second intervals on ice.

An EPO (eosinophil peroxidase, an eosinophil protein used as a marker of eosinophil presence) assay consisted of determining the levels of EPO in the lung tissue (or supernatant of BAL fluid) from each individual guinea pig sample. 50 ul of the "sample solution" consisting of 375 ul PBS (pH 7, RT) + 25 ul 0.05 M TRIS-HCL containing 2 % Triton (pH 8, RT) + 50 ul of sonicated lung lobe was added to 860 ul 0.05 M TRIS-HCL containing 0.1 % Triton (pH 8, RT) in combination with 8.5 ul mM 0-phenylenediaminedihydrochloride (OPD). To start the reaction, I ul of 30 % hydrogen peroxide was added to the cuvette. The optical density reading was measured spectrophotometrically over a 4 minute time interval at 490 nm in a Beckman Du-64 spectrophotometer.

BAL were analyzed by ELISA (Endogen) for IL-5 and IL-4 concentrations with data being presented as the average from 11 animals ± SEM. Results are presented as the mean of triplicate cultures±SEM. IL-5 concentration is in pg/ml. <b>Table 3</b> Inhibition of Antigen-induced Lung Eosinophilia, IL-5 and IL-4 Treatment EPO Concentration in Lune (ABS) IL-5 Concentration in BAL (pg/ml) IL-4 Concentration in BAL (pg/ml) Non sensitized Control 258±28 0.8±0.3 30±3 Antigen Sensitized 600±87 (100) 59±18 (100) 70±10(100) IRM Compound + Antigen 352±30 (78)* 13±2(78)* 53±8 (42) *=Significant difference from ovalbumin control group at α=0.05

The second set of studies evaluated the two IPM compounds 4-amino-α,α,-2-trimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol (Cmpd 1) and 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol (Cmpd 2) for their ability to inhibit sephadex-induced eosinophilia in the lung intravenous sephadex challenge. Results in Table 4 show that oral administration or intratracheal instillation of IRM Cmpd Ex. 1 at ≥0.7mg/kg and oral administration of Cmpd 2 at ≥0.01 mg/kg are capable of inhibiting sephadex-induced eosinophilia in the lung of rats when given 60 minutes prior to challenge. A maximum inhibition of 95% occurred with Cmpd I and 87% occurred with Cmpd 2.

Male Sprague Dawley rats were injected on day 0 with sephadex G-200 particles in a lateral tail vein (0.5 mg/rat). On days 14-16, the rats were lightly anesthetized with halothane and subsequently dosed with either drug or vehicle (1.0 mg/kg, orally) 24 hours and I hour before a second sephadex challenge on day 14. A booster of Sephadex G-200 particles was administered intravenously in a lateral tail vein (0.5 mg/rat) at I hour post-drug (i.e., following either drug or vehicle) on day 14 only. The animals are sacrificed on day 17 at 72 hrs. post-sephadex dosing by lethal injection of sodium pentobarbital (100-125 mg/kg, ip). Lungs were exanguinated, lavaged, and removed. They were then placed in 0.5 % cetrimide, 0.05 M KH2PO4 for homogenization of 4 X 30 seconds with 30 second cooling intervals between on ice. Centrifugation was then done at 1300 rpm (400 X g) for 30 minutes at 4C. Pellet was collected and resuspended in 4 ml 0.5 % cetrimide, 0.05 M KH2PO4 buffer. Samples were then frozen until sonication and the EPO assessment. This was followed by sonication for 3 X 15 seconds with 30 second intervals on ice.

The EPO (eosinophil peroxidase, an eosinophil protein used as a marker of eosinophil presence) assay consisted of determining the levels of EPO in the lung tissue (or supernatant of BAL fluid) from each individual rat sample. 50 ul of the "sample solution" consisting of 375 ul PBS (pH 7, RT) + 25 ul 0.05 M TRIS-HCL containing 2 % Triton (pH 8, RT) + 50 ul of sonicated lung lobe was added to 860 ul 0.05 M TRIS-HCL containing 0.1 % Triton (pH 8, RT) in combination with 8.5 ul mM 0-phenylenediaminedihydrochloride (OPD). To start the reaction, ul of 30 % hydrogen peroxide was added to the cuvette. The optical density reading was measured spectrophotometrically over a 4 minute time interval at 490 nm in a Beckman Du-64 spectrophotometer. <b>Table 4</b> Inhibition of Sephadex-induced Lung Eosinophilia in Rats Treatment Drug mg/k EPO Concentration in the Lungb,c (χ±SE) % Inhibition Group 1: Cmpd 1 Intratracheal Instillation Non-Sephadex Control 0.0 0.0923 ± 0.017 Sephadex Challenged 0.0 0.5456 ± 0.085 Drug + Sephadex Challenged 0.03 0.7107 ± 0.129 0% 0.1 0.5030 ± 0.089 9% 0.3 0.3440 ± 0.201 44% 0.7 0.1967 + 0.080* 77% Group 2: Cmpd 1 Oral Administration Non-Sephadex Control 0.0 0.0390 ± 0.008 Sephadex Challenged 0.0 0.3453 ± 0.100 Drug + Sephadex Challenged 0.1 0.4240 ± 0.138 0% 0.7 0.1497 ± 0.030* 64% 1.0 0.0780 ± 0.039* 87% 5.0 0.0790 + 0.030* 87% 30.0 0.0550 + 0.013 * 95% Group 3: Cmpd 2 Oral Administration Non-Sephadex Control 0.0 0.1072 ± 0.020 Sephadex Challenged 0.0 0.6738 ± 0.100 Drug + Sephadex Challenged 0.001 0.6775 ± 0.140 0% 0.01 0.4908 ± 0.070* 32% 0.1 0.2000 ± 0.060* 84% 1.0 0.1824 + 0.060* 87% *= Significant difference from ovalbumin control group at α=0.05

The third set of studies evaluated 4-amino-α,α,-2-trimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol (Cmpd 1) and 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinoline-1-ethanol (Cmpd 2) for their ability to inhibit ovalbumin-induced eosinophilia in the lung aerosol antigen challenge. Results in Table 5 show that intraperitoneal administration or aerosol inhalation of Cmpd 1 at 0.01 mg/kg and oral administration of Cmpd 2 at 0.01 mg/kg are capable of inhibiting ovalbumin-induced eosinophilia in the lung of guinea pigs when given either 15 or 60 minutes prior to challenge, respectively. A maximum inhibition of 92% occurred with IRM Cmpd 1 and 96% occurred with IRM Cmpd 2. In the guinea pig, these two imidazoquinoline compounds produce approximately equivalent effects on ovalbumin-induced lung eosinophilia.

Male Hartley guinea pigs (~250-500 g), sensitized to ovalbumin (50 mg/kg, ip, greater than or equal to 14 days) were dosed with chlorpheniramine (5 mg/kg, ip) and drug or vehicle intratracheally (or by another route) at 15 minutes pre-challenge. Animals were placed inside an inverted dessicator jar which was placed onto a plexiglass platform. The platform allowed for aerosolization of H2O or ovalbumin (50 mg/ml) for 5 minutes via a No. 40 DeVilbiss nebulizer, and for providing a constant flow of air into the chamber from a continuous air source. Animals were sacrificed at 24 hrs. post-challenge by lethal injection of sodium pentobarbital (100-125 mg/kg, ip). Lungs were exanguinated, lavaged, and removed. They were then placed in 0.5 % cetrimide, 0.05 M KH2PO4 for homogenization of 4 X 30 seconds with 30 second cooling intervals between on ice. Centrifugation was then done at 1300 rpm (400 X g) for 30 minutes at 4C. Pellet was collected and resuspended in 4 ml 0.5 % cetrimide, 0.05 M KH2PO4 buffer. Samples were frozen until assayed. This was followed by sonication for 3 X 15 seconds with 30 second intervals on ice.

The EPO (eosinophil peroxidase, an eosinophil protein used as a marker of eosinophil presence) assay consisted of determining the levels of EPO in the lung tissue (or supernatant of BAL fluid) from each individual guinea pig sample. 50 ul of the "sample solution" consisting of 375 ul PBS (pH 7, RT) + 25 ul 0.05 M TRIS-HCL containing 2 % Triton (pH 8, RT) + 50 ul of sonicated lung lobe was added to 860 ul 0.05 M TRIS-HCL containing 0. 1 % Triton (pH 8, RT) in combination with 8.5 ul mM 0-phenylenediaminedihydrochloride (OPD). To start the reaction, I ul of 30 % hydrogen peroxide was added to the cuvette. The optical density reading was measured spectrophotometrically over a 4 minute time interval at 490 nm in a Beckman Du-64 spectrophotometer. <b>Table 5</b> Inhibition of Ovalbumin-Induced Lung Eosinophilia in the Guinea Pig Treatment Drug mg/kg EPO Concentration in the Lungb,c (χ±SE) % Inhibition Group 1: Cmpd 1 Aerosol Inhalation Non-Ovalbumin Control 0.0 0.0312 ± 0.005 Ovalbumin Challenged 0.0 0.2959 ± 0.035 Drug + Ovalbumin Challenged 0.003 0.2620 ± 0.116 13% 0.01 0.1806 ± 0.035* 44% Group 2: Cmpd 1 Intraperitoneal Administration Non-Ovalbumin Control 0.0 0.0338 ± 0.004 Ovalbumin Challenged 0.0 0.3268 ± 0.046 Drug + Ovalbumin Challenged 0.003 0.2435 ± 0.0515 28% 0.01 0.1690 ± 0.053* 54% 0.03 0.1693 ± 0.060* 54% 3.0 0.0580 + 0.018* 92% Group 3: Cmpd 2 Oral Administration Non-Ovalbumin Control 0.0 0.0203 ± 0.008 Ovalbumin Challenged 0.0 0.2307 ± 0.010 Drug + Ovalbomin Challenged 0.001 0.1862 ± 0.030 19% 0.01 0.1181± 0.020* 49% 0.1 0.0118 ± 0.005* 95% 1.0 0.0084 ± 0.005* 96% *=Significant difference from ovalbumin control group at α=0.05

The above studies indicate that the IRM compounds useful in the present invention can be used for treatment of TH2 mediated diseases by inhibiting TH2 immune responses, and suppressing IL-4 and IL-5 induction and eosinopilia. Examples of such diseases include asthma, allergy, atopic dermatitis, early HIV disease, infectious mononucleosis, and systemic lupus erythematosis. There is also an association with an increased TH2 response in Hodgkin's and non-Hodgkin's lymphoma as well as embryonal carcinoma. Moreover, the ability of the IRM compounds useful in the present invention to inhibit TH2 response and augment TH I response indicates that these compounds will be useful in treating parasitic infections, for example, cutaneous and systemic leishmaniasis, Toxoplasma infection and Trypanosome infection, certain fungal infections, for example Candidiasis and Histoplasmosis, and intracellular bacterial infections, such as leprosy and tuberculosis. Studies in mice infected with leishmania major have shown that a TH I response correlates with resistance, whereas a TH2 response correlates with susceptibility. Also studies in mice have shown that parasites that live in macrophages, for example, leishmania major, are killed when the host cells are activated by interferon-γ, which is known to be a TH1 cell product. In mice infected with candida and histoplasma, it is known that a TH1 response correlates with resistance, whereas a TH2 response correlates with susceptibility.

Accordingly, from all of the above, it is apparent that the imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines useful in the present invention are useful for treating TH2 mediated and other related diseases. Although the invention has been presented in terms of preferred embodiments and specific examples, there is no intention to limit the invention to such embodiments and examples.

 Use of an immune response modifier compound selected from imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a Pharmaceutical Composition for the treatment of a non-viral and non-tumor, TH2 cell mediated disease with the proviso that said disease is other than eczema. The use of claim 1, wherein said disease is a parasitic infection, a bacterial infection, or a fungal infection. The use of claim 1, wherein said disease is selected from asthma, allergy, leprosy, systemic lupus erythematosis, Ommen's syndrome, leishmaniasis, toxoplasma infection, trypanosome infection, candidiasis, and histoplasmosis. The use of claim 1, wherein said disease is selected from asthma and allergic rhinitis. Use of an immune response modifier compound selected from the group consisting of imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a pharmaceutical composition for the treatment of a non-viral and non-tumor disease, whereby the induction of IL-4 and/or IL-5 cytokines is inhibited, with the proviso that said disease is other than eczema. Use of an immune response modifier compound selected from the group consisting of imidazoquinoline amines, imidazopyridine amines, 6,7-fused cycloalkylimidazopyridine amines, and 1,2-bridged imidazoquinoline amines for the preparation of a pharmaceutical composition for the treatment of eosinophilia, with the proviso that said disease is other than eczema. The use of claim 1 or 6, wherein said composition is adapted to be administered via oral or nasal inhalation. The use of claim 1 or 6, wherein said composition is adapted to be administered via a topical cream or gel. The use of claim 1 or 6, wherein said compound is selected from 4-amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]quinolin-1-ethanol and 1-(2-methylpropyl)-1H-imidazo[4,5-c]quinolin-4-amine. The use of claim 1 or 6, wherein said immune response modifier compound is a compound of Formula IX or a pharmaceutically acceptable salt thereof,
wherein R19 is selected from alkyl containing one to six carbon atoms and hydroxyalkyl containing one to six carbon atoms; and R29 is selected from hydrogen, alkyl containing one to six carbon atoms, alkoxyalkyl wherein the alkoxy moiety contains one to four carbon atoms and the alkyl moiety contains one to four carbon atoms, and hydroxyalkyl containing one to four carbon atoms. The use according to Claim 10, wherein said R19 is 2-methylpropyl or 2-hydroxy-2-methylpropyl. The use according to Claim 10, wherein said R29 is selected from hydrogen, methyl, butyl, hydroxymethyl, ethoxymethyl, and methoxymethyl. Verwendung einer Verbindung, die die Immunantwort modifiziert, ausgewählt aus Imidazochinolinaminen, Imidazopyridinaminen, 6,7-kondensierten Cycloalkylimidazopyridinaminen und 1,2-verbrückten Imidazochinolinaminen zur Herstellung einer pharmazeutischen Zusammensetzung zur Behandlung einer nichtviralen und nichttumorösen, durch TH2-Zellen vermittelten Erkrankung, mit der Maßgabe, daß die Erkrankung nicht Ekzem ist. Verwendung nach Anspruch 1, wobei die Erkrankung eine parasitäre Infektion, eine bakterielle Infektion oder eine Pilzinfektion ist. Verwendung nach Anspruch 1, wobei die Erkrankung ausgewählt ist aus Asthma, Allergie, Lepra, systemischem Lupus erythematodes, Omenn-Syndrom, Leishmaniase, Toxoplasmoseinfektion, Trypanosomeninfektion, Candidose und Histoplasmose. Verwendung nach Anspruch 1, wobei die Erkrankung ausgewählt ist aus Asthma und allergischer Rhinitis. Verwendung einer Verbindung, die die Immunantwort modifiziert, ausgewählt aus Imidazochinolinaminen, Imidazopyridinaminen, 6,7-kondensierten Cycloalkylimidazopyridinaminen und 1,2-verbrückten Imidazochinolinaminen zur Herstellung einer pharmazeutischen Zusammensetzung zur Behandlung einer nichtviralen und nichttumorösen Erkrankung, wodurch die Induktion von IL-4- und/oder IL-5-Cytokinen gehemmt wird, mit der Maßgabe, daß die Erkrankung nicht Ekzem ist. Verwendung einer Verbindung, die die Immunantwort modifiziert, ausgewählt aus Imidazochinolinaminen, Imidazopyridinaminen, 6,7-kondensierten Cycloalkylimidazopyridinaminen und 1,2-verbrückten Imidazochinolinaminen zur Herstellung einer pharmazeutischen Zusammensetzung zur Behandlung von Eosinophilie, mit der Maßgabe, daß die Erkrankung nicht Ekzem ist. Verwendung nach Anspruch 1 oder 6, wobei die Zusammensetzung so angepaßt ist, daß sie mittels oraler oder nasaler Inhalation zu verabreichen ist. Verwendung nach Anspruch 1 oder 6, wobei die Zusammensetzung so angepaßt ist, daß sie als topische Creme oder Gel zu verabreichen ist. Verwendung nach Anspruch 1 oder 6, wobei die Verbindung ausgewählt ist aus 4-Amino-2-ethoxymethyl-α,α-dimethyl-1H-imidazo[4,5-c]chinolin-1-ethanol und 1-(2-Methylpropyl)-1H-imidazo[4,5-c]chinolin-4-amin. Verwendung nach Anspruch 1 oder 6, wobei die die Immunantwort modifizierende Verbindung eine Verbindung der Formel IX oder ein pharmazeutisch verträgliches Salz davon ist,
wobei R19 ausgewählt ist aus Alkyl enthaltend ein bis sechs Kohlenstoffatome und Hydroxyalkyl enthaltend ein bis sechs Kohlenstoffatome; und R29 ausgewählt ist aus Wasserstoff, Alkyl enthaltend ein bis sechs Kohlenstoffatome, Alkoxyalkyl, wobei die Alkoxygruppe ein bis vier Kohlenstoffatome enthält und die Alkylgruppe ein bis vier Kohlenstoffatome enthält, und Hydroxyalkyl enthaltend ein bis vier Kohlenstoffatome. Verwendung nach Anspruch 10, wobei R19 für 2-Methylpropyl oder 2-Hydroxy-2-methylpropyl steht. Verwendung nach Anspruch 10, wobei R29 ausgewählt ist aus Wasserstoff, Methyl, Butyl, Hydroxymethyl, Ethoxymethyl und Methoxymethyl. Utilisation d'un composé modifiant la réponse immunitaire choisi parmi les amines imidazoquinoléine, les amines imidazopyridine, les amines cycloalkylimidazopyridine à noyaux condensés en 6,7 et les amines imidazoquinoléine pontées en 1,2, pour la préparation d'une composition pharmaceutique destinée au traitement d'une maladie non virale et non tumorale ayant pour médiateur les cellules TH2, à condition que ladite maladie soit autre que l'eczéma. Utilisation selon la revendication 1, dans laquelle ladite maladie est une infection parasitaire, une infection bactérienne ou une infection fongique. Utilisation selon la revendication 1, dans laquelle ladite maladie est choisie parmi l'asthme, l'allergie, la lèpre, le lupus érythémateux aigu disséminé, le syndrome d'Omenn, la leishmaniose, la toxoplasmose, la trypanosomose, la candidose et l'histoplasmose. Utilisation selon la revendication 1, dans laquelle ladite maladie est choisie parmi l'asthme et la rhinite allergique. Utilisation d'un composé modifiant la réponse immunitaire choisi parmi les amines imidazoquinoléine, les amines imidazopyridine, les amines cycloalkylimidazopyridine à noyaux condensés en 6,7 et les amines imidazoquinoléine pontées en 1,2, pour la préparation d'une composition pharmaceutique destinée au traitement d'une maladie non virale et non tumorale ainsi inhibant le déclenchement de cytokines IL-4 et/ou IL-5, à condition que ladite maladie soit autre que l'eczéma. Utilisation d'un composé modifiant la réponse immunitaire choisi parmi les amines imidazoquinoléine, les amines imidazopyridine, les amines cycloalkylimidazopyridine à noyaux condensés en 6,7 et les amines imidazoquinoléine pontées en 1,2, pour la préparation d'une composition pharmaceutique destinée au traitement de l'éosinophilie, à condition que ladite maladie soit autre que l'eczéma. Utilisation selon la revendication 1 ou 6 dans laquelle ladite composition est conçue pour être administrée par inhalation orale ou nasale. Utilisation selon la revendication 1 ou 6 dans laquelle ladite composition est conçue pour être administrée au moyen d'une crème ou d'un gel à usage local. Utilisation selon la revendication 1 ou 6 dans laquelle ledit composé est choisi parmi le 4-amino-2-éthoxyméthyl-α,α-diméthyl-1H-imidazo[4,5-c]quinoléine-1-éthanol et la 1-(2-méthylpropyl)-1H-imidazo[4,5-c]-quinoléine-4-amine. Utilisation selon la revendication 1 ou 6 dans laquelle ledit composé modifiant la réponse immunitaire est un composé de formule IX ou un sel pharmaceutiquement acceptable de ce composé,
formule dans laquelle R19 est choisi parmi un groupe alkyle contenant un à six atomes de carbone et un groupe hydroxyalkyle contenant un à six atomes de carbone ; et R29 est choisi parmi un atome d'hydrogène et les groupes alkyle contenant un à six atomes de carbone, alcoxy-alkyle dont le groupement alcoxy contient un à quatre atomes de carbone et le groupement alkyle contient un à quatre atomes de carbone, et hydroxyalkyle contenant un à quatre atomes de carbone. Utilisation selon la revendication 10 dans laquelle ledit radical R19 est un groupe 2-méthylpropyle ou 2-hydroxy-2-méthylpropyle. Utilisation selon la revendication 10 dans laquelle ledit radical R29 est choisi parmi un atome d'hydrogène et les groupes méthyle, butyle, hydroxy-méthyle, éthoxyméthyle et méthoxyméthyle. REFERENCES CITED IN THE DESCRIPTION

This list of references cited by the applicant is for the reader's convenience only. It does not form part of the European patent document. Even though great care has been taken in compiling the references, errors or omissions cannot be excluded and the EPO disclaims all liability in this regard.

Patent documents cited in the description