FIELD OF THE INVENTION

The current invention relates to novel p38 inhibitors, processes for the preparation thereof, the use thereof in treating p38 kinase mediated diseases and pharmaceutical compositions for use in such therapy.

BACKGROUND OF THE INVENTION

Mitogen-activated protein kinases ^(MAPK) are a family of proline-directed serine/threonine kinases that activate their substrates by dual phosphorylation. The kinases are activated by a variety of signals including nutritional and osmotic stress, UV light, growth factors, endotoxin and inflammatory cytokines.

One particularly interesting MAPK is p38, also known as cytokine suppressive antiinflammatory drug binding protein (CSBP). The p38 kinases are responsible for phosphorylating and activating transcription factors as well as other kinases They are activated by physical chemical and radiation stress like osmotic, anisomysin, UV etc. They are also activated by pro-inflammatory cytokines like IL-1 and TNF and bacterial lipopolysaccharide. More importantly, the products of the p38 phosphorylation activation have been shown to mediate the production of inflammatory cytokines, including TNF, IL-1 , IL-6 and cyclooxygenase-2. Each of these cytokines has been implicated in numerous disease states and conditions. p38-mediated condition includes any disease or deleterious condition in which upregulated p38 plays a role in pathogenesis of that condition and/or inhibition of p38 is useful in management of the same. p38-mediated conditions include inflammatory diseases, autoimmune diseases, destructive bone disorders, proliferative disorders including tumor progression, infectious diseases, neurodegenerative diseases, allergies, reperfusion/ischemia in stroke, heart attacks, angiogenic disorders, organ hypoxia, vascular hyperplasia cancer cachexia, cardiac hypertrophy, thrombin-induced platelet aggregation, and conditions associated with prostaglandin endoperoxidase synthase-2. p38 has been implicated in cancer, immunodeficiency disorders, cell death and osteoporosis.

Inhibition of p38 kinase leads to a blockade on the production of both IL-1 and TNF. IL-1 & TNF stimulate the production of other pro-inflammatory cytokines such as IL-6, and IL-8, which have been implicated in acute and chronic inflammatory diseases and in postmenopausal osteoporosis [R. B. Kimble et al., Endocrinol., 136, pp. 3054-61 (1995)]. The diseases characterized with abnormal regulation of these cytokines are amenable to treatment with p38 inhibitor.

IL-1 -mediated disease or condition includes rheumatoid arthritis, osteoarthritis, stroke, endotoxemia and/or toxic shock syndrome, inflammatory reaction induced by endotoxin, inflammatory bowel disease, tuberculosis, atherosclerosis, muscle degeneration, cachexia, psoriatic arthritis, Reiter's syndrome, gout, traumatic arthritis, rubella arthritis, acute synovitis, diabetes, pancreatic beta-cell disease and Alzheimer's disease.

TNF - α levels can be altered by varieties of pharmaceutical compositions are currently being used in mammal having TNF-α antagonist activity includes Infliximab, Adalulimb, Etamcept, Thalidomide, etc. They are used in management of rheumatoid arthritis, Crohn's disease, Ankylosing spondylitis, ulcerative colitis, apthous ulcer, systemic lupus erythematous, myeloma, uveitis, etc.

Glucocorticoids are known anti-inflammatory compounds. Commonly used glucocorticoids include hydrocortisone, prednisolene, betamethasone, dexamethasone, thaminolone, methyl prednisolene, prednisone. They suppress cytokines like IL-1 , IL-2, IL-3, IL-4, IL-5, IL-6, IL-8, IL-11 , IL-12, TNF-α, COX-2. IL-1 , ^" IL-2, IL-6, IL-8, IL-12, TNF-α are know as proinflammatory cytokines while IL-4, IL-5 etc are known as anti-inflammatory cytokines. Glucocorticoids are used in management of wide range of diseases which include rheumatoid arthritis, rheumatoid spondylitis, asthma, atopic dermatitis, drug hypersensitivity reactions, perennial or seasonal allergic rhinitis, serum sickness, bullous dermatitis herpetiformis, exfoliative erythroderma, mycosis fungoids, pemphigus, severe erythema multiforme(Stevenes), ulcerative colitis, idiopathic thrombocytopenic purpura, pure red cell aplasia, temporal arteritis, uveitis, proteinuria in idiopathic nephritis, idiopathic eosinophilic pneumonias, symptomatic sarcoidosis, acute gouty arthritis, ankylosing spondylitis, dermatomyositis, polymyositis, systemic lupus, refractory multiple myeloma, myelodysplastic syndromes, severe COPD, chronic granulomatous disease, angiogenesis, sarcoidosis. Transformed cells are the cells, which grow into continuous culture without mitogen stimuli. Eukaryotic cells are non transformed cells and do not grow in continuous culture. By transformation eukaryotic cells get converted from quiescent/stationary phase to unregulated growth and can be maintained in continuous culture. The p38 inhibitors are known to inhibit continuous growth of these transformed cells and trigger apoptosis. Following patents, patent applications describe p38 inhibitors and its uses,

Patent / Application No. Title Patent / Application No. Title

US7186737B2 Inhibitors of p38 US7169779B2 Inhibitors of p38

US6635644B2 Inhibitors of p38 US6608060B1 Inhibitors of p38 US6632945B2 Inhibitors of P38 US6528508B2 Inhibitors of p38

US6509363B2 Heterocyclic inhibitors of p38 40 US6147080A Inhibitors of p38 US6800626B2 Inhibitors of p38 US6093742A Inhibitors of p38

US6949560B2 Imidazo-substituted WO2000017175A1 Inhibitors of p38 compounds as p38 kinase inhibitors WO2000017204A1 Inhibitors of p38

WO1996021654A1 Novel Compounds WO1999058502A1 Heterocyclic inhibitors of

WO1999000357A1 Inhibitors of p38 p38 WO1999064400A1 Inhibitors of p38 US6162613A Methods for designing inhibitors of serine / threonine-kinases and tyrosine kinases

US7151010B2 Methods for assembling a stack package for high density integrated circuits

US6852740B2 Pyrazole derivatives as p38 kinase inhibitors

US6982270B1 3,4-dihydro-(1h)quinazolin-2-one compounds as csbp/p38 kinase inhibitors US6630485B2 p38 map kinase inhibitor

US7189400B2 Methods of treatment with antagonists of mu-1

US7115557B2 Use of certain drugs for treating nerve root injury

US7078431 B2 1 ,3-bis-(substituted-phenyl)-2-propen-1-ones and their use to treat vcam-1 mediated disorders US6759410B2 3,4-dihydro-(1h)-quinazolin-2ones and their use as csbp/p38 kinase inhibitors

US6696471 B2 Aminopyrrole compounds

US6696443B2 Piperidine / piperazine-type inhibitors of p38 kinase

US6649637B2 Inhibition of intracellular replication by pyridinylimidazoles US6638765B1 Platform for the differentiation of cells

US6509361 B1 1 ,5-diaryl substituted pyrazoles as p38 kinase inhibitors

US6479507B2 p38 map kinase inhibitors

US6444696B1 pyrazole derivatives p38 map kinase inhibitors

US6410540B1 Inhibitors of P38 alpha kinase US6376527B1 Pyrazole derivatives P38 Map kinase inhibitors

US6316466B1 Pyrazole derivatives P38 Map kinase inhibitors

US6316464B1 P38 Map Kinase Inhibitors

US6096711 A HSP 72 Induction And Applications

US6414150B1 & US6335336B1 describes inhibition of angiogenesis by suppression of TNF- alpha is useful in inhibition or prevention of metastasis.

US6994981 B2 describe modulators of para apoptosis and related methods. Several other prior art patents are also based on MAPK inhibitors are EP1208748A1 , WO2004089929,

WO2006117567.

US6852740B2 describes pyrazole derivatives as p38 kinase inhibitors. WO95/31451 describes pyrazole compositions that inhibit MAPKs, and, in particular, p38. The efficacy of these inhibitors in vivo is still being investigated.

Other p38 inhibitors have been produced, including those described in WO98/27098, WO99/00357, WO99/10291 , WO99/58502, WO99/64400, WO00/17175 and WO00/17204. In addition, WO97/24328, WO98/34920, WO98/35958 and US5145857A disclose amino- substituted heterocycles having therapeutic uses. Accordingly, there is a need to develop inhibitor of p38 that are useful in treating various conditions associated with p38 mediated activity.

SUMMARY OF THE INVENTION:

The main object of the invention is to provide Mw cells and/or its constituents for p38 kinase inhibition.

It is another object of the invention to provide methods for treatment or prevention of a p38-mediated condition.

It is yet another object of the invention to provide a method for the treatment of condition or disease state mediated by p38 kinase activity, or mediated by cytokines produced by the activity of p38 kinase, which comprises administering to a subject (e.g. mammals) therapeutically effective amount of Mycobacterium w and/or constituents thereof. It is yet another object of the invention to provide use of Mycobacterium w and/or constituents thereof, for the preparation of a medicament for the treatment of a condition or disease state mediated by p38 kinase activity or medicated by cytokines produced by p38 kinase activity.

DETAILED DESCRIPTION OF THE INVENTION:

The invention relates to the use of Mycobacterium w(Mw) cells and/or its constituents for inhibition of p38 protein kinase. The said invention also includes the use of Mw cells and/or its constituents for inhibition of cytokine production.

The said invention also encompasses compositions comprising Mw cells and/or its constituents are inhibitors of serine/threonine kinase p38 and cytokine production.

In accordance with the invention Mycobacterium w (Mw) cells and/or its constituents are useful in treating p38 mediated disorders.

The invention comprises compositions having therapeutically effective amount of Mw cells and/or its constituents for the treatment of p38 kinase mediated disorder, TNF mediated disorder, inflammation and/or arthritis.

The present invention provides a method of treating a cytokine-mediated disease which comprises administering an effective cytokine interfering amount of compositions containing Mw and/or its constituents. The use include but not limited to rheumatoid arthritis, rheumatoid spondylitis, asthma, atopic dermatitis, drug hypersensitivity reactions, perennial

or seasonal allergic rhinitis, serum sickness, bullous dermatitis herpetiformis, exfoliative erythroderma, mycosis fungoids, pemphigus, severe erythema multiforme (Stevenes), ulcerative colitis, idiopathic thrombocytopenic purpura, pure red cell aplasia, temporal arthritis, uvetitis, proteinuria in idiopathic nephritis, idiopathic eosinophilic pneumonias, symptomatic sarcoidosis, acute gouty arthritis, ankylosing spondylitis, dermatomyositis, polymyositis, systemic lupus, refractory multiple myeloma, myelodysplastic syndromes, severe COPD, chronic granulomatous disease, angiogenesis, sarcoidosis

Mw cells are useful for the treatment of p38 kinase mediated disorder including inflammatory diseases, autoimmune diseases, destructive bone disorders, proliferative disorders including tumor progression, infectious diseases, neurodegenerative diseases, allergies, reperfusion, ischemia in stroke, heart attacks, angiogenic disorders, organ hypoxia, vascular hyperplasia cancer cachexia, cardiac hypertrophy, thrombin-induced platelet aggregation, conditions associated with prostaglandin endoperoxidase synthase-2, cancer, immunodeficiency disorders, cell death, osteoporosis. Mw cells may be used for the treatment of TNF-alfa mediated disease or condition including rheumatoid arthritis, Crohn's disease, ankylosing spondylitis, ulcerative colitis, apthous ulcer, systemic lupus erythematous, myeloma uveitis.

Mw cells and/or its constituents involved in the said invention may also be used in co- therapies, partially or completely, in place of other conventional antiinflammatories, such as together with steroids, Dexamethasone, cyclooxygenase-2 inhibitors, NSAIDs, DMARDS, immunosuppressive agents, 5-lipoxygenase inhibitors, LTB4 antagonists and LTA, hydrolase inhibitors.

In accordance with the invention, Mw cells are used to inhibit p38 mediated conditions, in which Mw cells are prepared by the process comprises the following steps; a. Culturing of Mycobacterium w (Mw), b. Harvesting and concentrating, c. Washing the cells, d. Adding pharmaceutically acceptable carrier, e. Adding preservative, f. Terminal sterilization, g. Quality control, h. Preparing constituents of Mw. The process is further described in detail is as following: A. Culturing of Mw: i. Culturing Mw on solid medium like L J medium or liquid medium like middle brook medium or sauton's liquid medium. For better yield middle brook medium is enriched. It can be preferably enriched by addition of glucose,

bactotryptone, and BSA. They are used in ratio of 20:30:2 preferably. The enrichment medium is added to middle brook medium. It is done preferably in ratio of 15:1 to 25:1 more preferably in a ratio of 20:1. Preparing the culture medium at 37+ 0.5° C temperature and at pH 6.7 to 6.8 initially. ii. Bioreactor operation a) Preparation of vessel: Cleaning the inner contact parts of the vessel (Joints, mechanical seals, o-ring/gasket grooves, etc.) to avoid contamination. Filling the vessel with 0.1 N NaOH and leave for 24 hrs to remove pyrogenic material and other contaminants. Cleaning the vessel with acidified water and then with water. Rinsing the vessel with distilled water. b) Sterilization of bioreactor: Sterilizing the bioreactor containing 9L distilled water with steam. Further sterilizing the bioreactor with Middlebrook medium. Bottles, inlet/outlet air filters etc. are autoclaved (twice) at 121 ⁰ C for 15 minutes. Drying the vessel in oven at 50° C before use. B Harvesting and concentrating: Harvesting the cells under aseptic condition at the end of the 6 ^th day of culturing. Concentrating the cells (palletization) by centrifugation. C. Washing of cells: Washing the pallet with normal saline, preferably with isotonic fluid. D. Addition of pharmaceutically acceptable carrier: Adding pyrogen free normal saline to pallet. Any other pyrogen free isotonic fluid can be used as a pharmaceutical carrier. The carrier is added in amount so as to get desired concentration of active in final form.

E. Addition of preservative: Adding preservative to keep the cell/pellets free from contamination. Preferably thiomerosal is used having concentration of 0.01 % w/v.

F. Terminal Sterilization: Sterilizing the cell/pallet by various physical methods like application of heat or ionizing radiation or sterile filtration. Heat can be in the form of dry heat or moist heat. It can also be in the form of boiling or pasteurization. Ionizing radiation can be ultraviolet or gamma rays or microwave or any other form. G. Quality Control: The cell/pallet passed through number of process to check its quality. i. Evaluating purity and sterility of the cell/pallet, ii. Checking the organisms for acid fastness after gram staining, iii. Performing Inactivation test by culturing the product on L J medium to find out any living organism. iv. Checking pathogenicity and/or contamination of the cell/pallet. The cultured organisms are injected to Balb/c mice. All the mice gained weight and found

healthy. Three is no macroscopic or microscopic lesions seen in liver, lung spleen or any other organs of the mice, v. Biochemical Test: The cell/pallet containing organism is subjected to following biochemical tests: - Urease - Tween 80 hydrolysis

Niacin test - Nitrate reduction test

The organism gives negative results when tested with urease, tween 80 hydrolysis and niacin. It gives positive result with nitrate reduction test. H. Preparation of Mycobacterium w constituents: Mw constituents can be prepared by following methods. i. Cell disruption ii. Solvent extraction iii. Enzymatic extraction.

The cell disruption is done by sonication or using of high pressure fractionometer or applying osmotic pressure.

The solvent extraction is done by any organic solvent like chloroform, ethanol, methanol, acetone, phenol, isopropyl alcohol, acetic acid, urea, hexane etc.

The enzymatic extraction is done by proteolytic enzymes which can digest cell wall/membranes. Liticase and pronase are the preferred enzymes. Mw cell constituents can be used in place of Mw. Addition of Mw cell constituents results in improved efficacy of the product. Cell/pallet containing Mw so prepared is further evaluated for its p38 inhibiting activity.

In accordance with this invention, Mw cell prepared by the aforementioned process is used in the preparation of pharmaceutical compositions. A. Each dose of 0.1 ml of therapeutic agent contains:

Mycobacterium w., (heat killed) 0.50 x 10 ⁹

Sodium Chloride I. P. 0.90% w/v

Tween 80 0.1% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative) Water for injection I. P. q. s. to 0.1 ml

B. Each dose of 0.1 ml of therapeutic agent contains: Mycobacterium w., (heat killed) 0.50 x 10 ⁹ Sodium Chloride I. P. 0.90% w/v Triton x 100 0.1% w/v Thiomerosal I. P. 0.01% w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml

C. Each dose of 0.1 ml of therapeutic agent contains:

Mycobacterium w., (heat killed) 0.50 x 10 ⁹ Sodium Chloride I. P 0.90% w/v Thiomerosal I. P. 0.01% w/v (As a Preservative) Water for injection I. P. q. s. to 0.1 ml D. Each dose of 0.1 ml of therapeutic agent contains

Extract of Mycobacterium w after sonication from 1x10 ¹⁰ Mycobacterium w Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml E. Each dose of 0.1 ml of therapeutic agent contains

Methanol Extract of 1x10 ¹⁰ Mycobacterium w Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml F. Each dose of 0.1 ml of therapeutic agent contains:

Chloroform Extract of 1x10 ¹⁰ Mycobacterium w Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01 % w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml G. Each dose of 0.1 ml of therapeutic agent contains

Acetone Extract of 1x10 ¹⁰ Mycobacterium w Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml H. Each dose of 0.1 ml of therapeutic agent contains

Ethanol Extract of 1x10 ¹⁰ Mycobacterium w Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml I. Each dose of 0.1 ml of therapeutic agent contains

Liticase Extract of 1x10 ^1c 'Mycobacterium w Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative)

Water for injection I. P. q. s. to 0.1 ml J. Each dose of 0.1 ml of therapeutic agent contains

Mycobacterium w (heat killed) 0.5x10 ⁷

Extract of Mycobacterium w obtained 1x10 ³ Mycobacterium w by disruption, solvent extraction or enzymatic extraction. Sodium Chloride I. P. 0.90% w/v

Thiomerosal I. P. 0.01% w/v (As a Preservative) Water for injection I. P. q. s. to 0.1 ml

The amount of Mw cell that may be combined with the carrier materials to produce a single dosage form will vary depending upon the host treated and the particular mode of administration. The route of administration can be injection intraderamal, intra venous, intra vesicle, intra peritoneal, intra articular, intra cerebral, intramuscular, sub cutaneous or any other route known in art for the particular treatment. For transdermal administration, the pharmaceutical composition may be given in the form of a transdermal patch, such as a transdermal iontophoretic patch. The pharmaceutical compositions so manufactured are surprisingly found to have following properties. They include p38 inhibitors, TNF-α inhibitor, suppression of cytokinese and death of transformed cells.

The concentration at which death of transformed cell take place is safe for normal cells like splenocytes, PBMC, bone marrow cell, fiber blass, macro phages, etc The invention is further illustrated with the following examples which do not limit to the scope of the invention.

Example 1 : In vivo p38 inhibition by Mw by intra dermal route:

Naive Balb/C mice were divided in two randomized groups. All mice received intradermal injections. The first group received 100 mcL of PBS, second group received 100 mcL of Mw (10 ^λ 8 cells). On eighth day mice were sacrificed and spleens were isolated from all animals. The Splenocytes were isolated from each group and cultured in RPMI 1640 media with 10% Fetal Bovine Serum (FBS) and 1% antibiotics in microtitre plate. After 48 hrs of culture the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D

Systems.

The result depicted in Table 1 show significant inhibition of p38 MAPK following intradermal administration of pharmaceutical composition of present invention.

Table: 1 p38 MAPK inhibition in vivo by Mycobacterium w in normal cells

Example 2: In vivo p38 inhibition by Mw with intra venous route:

Naive Balb/C mice were divided in two randomized groups. All mice received intravenous injection of a PBS (Placebo) of Mw. The first group received 100 mcL of PBS, second group received 100 mcL of Mw (10 ^λ 8 cells). On eighth day mice were sacrificed and spleens were isolated from all animals. The Splenocytes were isolated from each group and cultured in RPMI 1640 media with 10% Fetal Bovine Serum (FBS) and 1 % antibiotics in microtitre plate. After 48 hrs of culture the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result depicted in Table 1 show significant inhibition of p38 following administration of Mw by intra venous route.

Example 3: In vitro inhibition of p38 by Mw :

Naϊve Balb/C mice were sacrificed and spleens were isolated. The Splenocytes were isolated and cultured in RPMI 1640 media with 10%FBS and 1% antibiotics in microtitre plate. The number of wells were divided into two sets one was stimulated with 100 mcL of Mw (10 ^λ 8 cells) and second set was stimulated with 100 mcL placebo (PBS). After 48 hrs of incubation the cells were harvested and the. cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result depicted in Table 2 shows down regulation of p38 MAPK significantly when in vitro incubation of mice splenocytes with Mw. Table 2 Inhibition of p38 MAPK by in vitro stimulation with Mycobacterium w in normal and transformed cells

Example 4: p38 inhibition in NFS-60 cells by Mw:

NFS 60 cells were cultured in Dubalco's Minimul Eagle's Media (DMEM) with 10% FBS, 1 % antibiotics and IL-3 10 nG/mL. The cells were plated in microtiter wells at concentration of 1x 10 ^λ 5 cells. The numbers of wells were divided in to two sets. Set one

was stimulated with PBS as control and set two with 4 X 10 ^λ 6 Mw cells. At 24 hrs of culture the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result depicted in Table 2 shows down regulated level of p38 levels in Mw stimulated cells compared to control (non stimulated cells) at 24th hrs. At all the concentration above 4x 10 ^λ 6 Mw cells, cell death was observed at 48 hrs Cell death seen was due to apoptosis.

Example 5: p38 inhibition in Mia-pa- ca 2 cells by Mw: Mai-pa-ca 2 cells (pancreatic cancer cell line) were obtained from ATCC and were cultured in DMEM media with 10% FBS, 1% antibiotics. The cells were plated in microtiter wells at concentration of 1x 10 ^λ 5 cells. The numbers of wells were divided in to two sets. Set one was stimulated with PBS as control and set two with 2 X 10 ^λ 6 M w cells At 48 hrs of culture the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result depicted in Table 2 shows down regulated level of p38 levels in Mw stimulated cells compared to control (non stimulated cells) at 48th hrs. At a concentration of Mw above 10 ⁷ Mia-pa-ca 2 cells found to undergo apoptotic cell death. Example 6: Inhibition of p38 MAPK with single injection compared to seven injection of Mycobacterium w administrating intradermally.

Naϊve Balb/C mice were divided in three randomized groups. All mice received drugs intradermally. The first group received 100 mcL of PBS, second group received 100 mcL of Mw (10 ^λ 8 cells) once only, while third group was immunized with 100 mcL of Mw (10 ^λ 8 cells) every day for seven days. On eighth day after first immunization, mice were sacrificed and spleens were isolated for all three groups. The Splenocytes were isolated from each group and cultured in RPMI 1640 media with 10%FBS and 1 % antibiotics in microtitre plate.

After 48 hrs of culture the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869- 5) from R & D Systems

The results shows administration of single injection of Mw inhibits p38 MAPK by 20%, while seven injections inhibits of p38 levels by 25% compared to control.

Example 7: Duration of p38 inhibition by Mw: Naϊve Balb/C mice were randomized in six groups and were administered intravenously 1 mL of PBS in group one while group two to six received 1 ml. Mw (10 ^λ 9 cells). The group 1 and 2 were sacrificed on day 1 , while group three on 7day, group four on

14day, group five on 21day, group six on 28day and spleens were isolated. The Splenocyte were isolated and cultured in RPMI 1640 media with 10%FBS and 1% antibiotics in microtitre plate. After 48 hrs cells were harvested and the MAPK ELISA were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result depicted in Table 3 shows p38 level down regulated when immunization with Mw cells from 24 hrs to 28 ^th day (17.4% and 17.3%). The maximum inhibition of p38 occurs on 14 ^th day (25.1 %). p38 level remains inhibited for the entire period of study (i.e. 28 days).

Table 3 Inhibition of p38 MAPK by in vivo stimulation with Mycobacterium w intravenous immunization in mice

Example 8: Inhibition of p38 MAPK by Mw : Dose dependent effect.

Naive Balb/C mice were sacrificed and spleens were isolated. The Splenocytes were isolated and cultured in RPMI 1640 media with 10%FBS and 1% antibiotics in microtitre plate. The number of wells were divided into three sets one was stimulated with 100 mcL placebo (PBS). The second set was stimulated with 100 mcL of Mw (10 ^λ 8 cells). The third set was stimulated with 100 mcL of Mw (10 ^λ 6 cells).After 48 hrs of incubation the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result shows that in vitro incubation of splenocytes with Mw 10 ^λ 8 cells down regulate p38 MAPK by 46% while 10 ^λ 6 Mw cells have 5% inhibitory effect.

Example 9: p38 MAPK inhibition in NFS-60 cells by Mw in dose dependent manner

NFS 60 cells were cultured in DMEM media with 10% FBS, 1 % antibiotics and IL-3 10 nG/mL. The cells were plated in microtiter wells at concentration of 1x 10 ^λ 5 cells. The numbers of wells were divided in to five sets. Set one was stimulated with PBS as control, set two with 6 X 10 ^λ 7 Mw cells, set three with 3 X 10 ^λ 7 Mw cells, set four with 7 X 10 ^λ 6 Mw cells, set five with 4 X 10 ^λ 6 Mw cells. At 24 hrs of culture the cells were harvested and the cell signaling assays were performed as per manufacturers instructions, using the commercial kits (Cat no # DYC869-5) from R & D Systems.

The result depicted in Table 4 shows, alteration in p38 levels in Mw compared to control at 24 ^th hrs it is down regulated. The dose dependency is in inverse relation to the Mw concentration The maximum inhibition was observed with 4X 10 ^λ 6 Mw cells. At all the concentration above 4x 10 ^λ 6 Mw cells use for the stimulation, NFS 60 cells do not live for more than 48 hrs. The cells are found to undergo cell death by apoptosis. Table 4 Inhibition of p38 MAPK in transformed cells

Example 10: TNF alfa inhibition by Mw:

Naive Balb/C mice were randomized in two groups. The group 1 and 2 were sacrificed and spleens were isolated. The Splenocytes were isolated and cultured in RPMI 1640 media with 10%FBS and 1% antibiotics in microtitre plate. Group 1 was incubated with PBS while group 2 was incubated with 10 ^λ 8 Mw cells.After 48 hrs the cell supernatant was separated and the levels of TNF alfa were checked using commercial kit from R & D systems (Cat # MTAOO).

The result depicted in Table 5 shows incubated of TNF- alfa in group stimulated with Mw. Surprisingly it is observed that TNF-alfa inhibition is around 74%while p38 inhibition is only around 47%

Table 5: Inhibition of TNF-alfa production by Mycobacterium w

TNF alfa Inhibition b Mw

Thus TNF-mediated disease or condition that can be treated according to present invention, but are not limited to includes, rheumatoid arthritis, Crohn's disease, ankylosing spondylitis, ulcerative colitis, apthous ulcer, systemic lupus erythematous, myeloma uveitis and said management of mediated disorders comprises treating a subject having or susceptible to such disorder with a therapeutically-effective amount of a Mw and/or Mw constituents.

Example 11 : Cytokine suppression by Mw:

Naive Balb/C mice were randomized in two groups. The group 1 and 2 were sacrificed and spleens were isolated. The Splenocytes were isolated and cultured in RPMI incubated 1640 media with 10%FBS and 1% antibiotics in microtitre plate. Group 1 was

incubated with PBS while group 2 was incubated with 10 ^λ 8 Mw cells After 48 hrs the cell supernatant was separated and the levels of cytokines were checked using commercial kit from R & D systems (Cat # M2000, Cat # M4000B, Cat # M1240).

The result depicted in Table 6 shows inhibited of cytokine IL-2, IL-4, IL-5 and IL-12 p40 in group two incubated with Mw.

Surprisingly it is observed that all types of cytokines are inhibited. The effect is significantly more than amount of p38 inhibition (64% for IL-12p40 to 95% for IL-4 with a p38 inhibitory activity of around 47%).

Table 6: Inhibition of cytokine production by Mycobacterium w

Example 12: Comparison with Dexamethasone for cytokine supression

Naive Balb/C mice were sacrificed and spleens were isolated for all five groups. The splenocytes were isolated from each group and cultured in RPMI 1640 media with 10% antibiotics in microtitre plate. The cells were plated in micro titer plate. The wells were divided into five sets. Set was control, set two was stimulated with Mw, set three with 10 mM of Dexamethasone set four with 10 mcM (micro mole) of Dexamethasone and set five with 1 mcM of dexammethasone. After 48 hrs of culture the cells were harvested and the cytokine assays were performed using commercial kits from R & D systems. (Cat #M5000, Cat #M4000B, Cat #M2000, Cat #M 1240)

The result depicted in Table 7 reveals that Mw is effective in suppression of all cytokines like Dexamethasone. The suppressive effect seen is identical to the one observed with 1OmM Dexamethasone. This concentration of Dexamethasone is typically seen as Cmax after administration of 200 mg of Dexamethasone intravenously. 200 mg of Dexamethasone is used in very severe inflammatory conditions as a pulse therapy. Generally it is used at a significantly lower dose as an oral dosage. Generally adults receive 4.0 to 8.0 mg of Dexamethasone per day by oral or parenteral route.

Table 7: Cytokine suppression by Mycobacterium w and dexamethasone

Glucocorticoids like dexamethasone are known anti-inflammatory compounds. The commonly used glucocorticoids include hydrocortisone, prednisolene, betamethasone, dexamethasone, triaminolone, methyl prednisolene, prednisone. They suppress antiinflammatory as well as proinflammatory cytokines. They are used in management of wide range of diseases which include rheumatoid arthritis, rheumatoid spondylitis, asthma, atopic dermatitis, drug hypersensitivity reactions, perennial or seasonal allergic rhinitis, serum sickness, bullous dermatitis herpetiformis, exfoliative erythroderma, mycosis fungoids, pemphigus, severe erythema multiforme (Stevenes), ulcerative colitis, idiopathic thrombocytopenic purpura, pure red cell aplasia, temporal arthritis, uvetitis, proteinuria in idiopathic nephritis, idiopathic eosinophilic pneumonias, symptomatic sarcoidosis, acute gouty arthritis, ankylosing spondylitis, dermatomyositis, polymyositis, systemic lupus, refractory multiple myeloma, myelodysplastic syndromes, severe COPD, chronic granulomatous disease, angiogenesis, sarcoidosis. Thus all the disease/ disease condition including the up-regulation of cytokines, interleukins and chemokines can be treated with Mycobacterium w and/ or its constituents with more effective suppression of the said inflammatory and anti-inflammatory cytokine suppression.