WO2009153226A1 - 5-(4-methanesulfonyl-phenyl)-thiazole derivatives for the treatment of acute and chronic inflammatory diseases - Google Patents

5-(4-methanesulfonyl-phenyl)-thiazole derivatives for the treatment of acute and chronic inflammatory diseases Download PDF

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Publication number
WO2009153226A1
WO2009153226A1 PCT/EP2009/057324 EP2009057324W WO2009153226A1 WO 2009153226 A1 WO2009153226 A1 WO 2009153226A1 EP 2009057324 W EP2009057324 W EP 2009057324W WO 2009153226 A1 WO2009153226 A1 WO 2009153226A1
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Prior art keywords
compound
substituted
unsubstituted
tnf
alpha
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PCT/EP2009/057324
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French (fr)
Inventor
Victor Rubio Royo
Antonio de la Hera Martínez
Melchor Álvarez de Mon Soto
Ana Muñoz Muñoz
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Faes Farma, S.A.
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Priority claimed from US12/139,661 external-priority patent/US7781594B2/en
Priority claimed from EP08380177A external-priority patent/EP2135864A1/en
Priority to NZ589894A priority Critical patent/NZ589894A/en
Priority to BRPI0915325A priority patent/BRPI0915325A2/en
Priority to EP09765806A priority patent/EP2313382A1/en
Priority to CN2009801226820A priority patent/CN102083806A/en
Priority to CA2728139A priority patent/CA2728139A1/en
Priority to AU2009259451A priority patent/AU2009259451B2/en
Application filed by Faes Farma, S.A. filed Critical Faes Farma, S.A.
Priority to RU2011101439/04A priority patent/RU2495031C2/en
Priority to JP2011513001A priority patent/JP2011524352A/en
Priority to MX2010013978A priority patent/MX2010013978A/en
Publication of WO2009153226A1 publication Critical patent/WO2009153226A1/en
Priority to IL209801A priority patent/IL209801A0/en
Priority to ZA2010/08877A priority patent/ZA201008877B/en
Priority to MA33516A priority patent/MA32473B1/en

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    • C07D277/22Heterocyclic compounds containing 1,3-thiazole or hydrogenated 1,3-thiazole rings not condensed with other rings having two or three double bonds between ring members or between ring members and non-ring members with only hydrogen atoms, hydrocarbon or substituted hydrocarbon radicals, directly attached to ring carbon atoms
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    • C07D277/32Heterocyclic compounds containing 1,3-thiazole or hydrogenated 1,3-thiazole rings not condensed with other rings having two or three double bonds between ring members or between ring members and non-ring members with hetero atoms or with carbon atoms having three bonds to hetero atoms with at the most one bond to halogen, e.g. ester or nitrile radicals, directly attached to ring carbon atoms
    • C07D277/34Oxygen atoms

Definitions

  • the present invention relates to the use of compounds derived from 5-(4- methanesulfonyl-phenyl)-thiazole in the preparation of a medicinal product for the treatment of acute and chronic inflammatory diseases or conditions, such as rheumatoid arthritis.
  • Immunology is the scientific study of the discrimination between self and non-self. The breakdown of tolerance to self is in the origin of auto-immune diseases. Moreover, other conditions such as transplantation, atherosclerosis, septic and nonseptic acute and chronic inflammatory pathologies and many others diseases, up to now not considered as auto-immune, exhibit immune cell-mediated pathogenic mechanisms. Activation of immune inflammatory effector responses is considered by most authors as being based on two signals:
  • TCR-CD3 T-cell receptor complex clonal antigen's receptor
  • MHC Major Histocompatibility Complex
  • extracellular soluble or membrane-bound antigens cross link the Immunoglobulin CD79 (Ig/CD79) clonal receptor complex to deliver the signal 1 to the antibody-secreting lymphocyte lineage.
  • a second signal in addition to antigen-delivered signal 1 , is required to avoid tolerance by anergy or clonal deletion.
  • Signal 2 is delivered by co-stimulators such as CD86 expressed on the surface of professional antigen-presenting cells (APC), like human monocytes and their differentiation lineage progeny.
  • APC professional antigen-presenting cells
  • PRR signalling pathways such as TLR4 (the receptor for the Gram- negative wall bacteria lipo-polysaccharide or LPS) deliver the expression of high levels of co-stimulatory surface molecules (i.e., CD80 or CD86).
  • co-stimulatory ligands CD80 - CD86 cross link CD28 on the surface of helper T-cells.
  • signal 1 i.e., anti-CD3 antibody cross linking
  • signal 2 i.e., CD28 cross linking by specific antibodies
  • approved immune suppressor drugs have some troubles to inhibit the activation of pro-inflammatory cytokine cascades under conditions of high levels of co-stimulation. The latter occur in auto-immune diseases and many other severe acute and chronic inflammatory conditions.
  • APCs are not only crucial for the acquired immune system to decide the class of immune response since they deeply influence whether there is an effector (i.e. T-cell help, Th, cellular cytoxicity, Th, antibody production, B-cell) responses or a tolerant response (by anergy or apoptosis) mediated by the challenged clon.
  • APCs can also deliver themselves effector immediate immune responses.
  • TNF- alpha Tumour Necrosis Factor Alpha
  • TNF-alpha promotes an augmented response and activation of the vascular endothelium, accompanied with secretion of Interleukin 8 (IL-8) and other pro -inflammatory cytokines as well as pro- coagulant activities.
  • IL-8 Interleukin 8
  • TNF-alpha promotes thrombosis and ischaemia with cancer necrosis, which led to the original definition as cachectin or TNF-alpha.
  • TNF-alpha is a pleiotropic cytokine involved in many other disease conditions.
  • LPS may trigger the secretion of massive amounts of TNF-alpha which strongly contribute to the development of septic shock.
  • TNF-alpha is considered as a therapeutic target in auto- immune inflammatory diseases, such as rheumatoid arthritis, spondiloarthropathies, Crohn's disease, uveitis and psoriasis.
  • auto- immune inflammatory diseases such as rheumatoid arthritis, spondiloarthropathies, Crohn's disease, uveitis and psoriasis.
  • anti-TNF-alpha has currently been broadly considered as a state of the art strategy to deal with those diseases in which the reduction of available levels of bioactive TNF-alpha might contribute to ameliorate the patient's condition.
  • TNF-alpha antagonists is growing rapidly and includes atherosclerosis, metabolic syndrome, encephalitis, viral hepatitis, glomerulonephritis, inadequate inflammatory response to tumours and septic shock as among several others.
  • TNF-alpha production monocytes and T-lymphocytes.
  • APCs In the course of an acquired immune response, exposition of APCs to danger signals under pro -inflammatory instructive scenarios, triggers the secretion of IL-12 p70 (an heterodimer of p35 and p40), being the latter a co-stimulatory molecule that polarizes the cytokine secretion profile of the activated Th-cells towards Th-I type.
  • ThI -cells exhibit a characteristic cytokine profile in which interferon gamma (IFN-gamma) secretion is a bonafide footprint. These cells do secrete high amounts of TNF-alpha too.
  • IFN-gamma interferon gamma
  • IFN-gamma produced by ThI promotes many effects that may be relevant in the understanding of inflammatory diseases. On one hand, it further activates monocytes and increases the level of TNF-alpha secretion by a given stimuli. On the other hand, it promotes a stronger signalling pathway downstream TNF-alpha receptors.
  • IFN-gamma in addition to its own direct effects such as anti- viral activity, increases expression in MHC-II and contributes to inflammation and lesions by increasing the still strong effects of TNF-alpha.
  • IL-8 pro -inflammatory cytokine pathways
  • IL-8 in spite of its original name, was described as a chemokine produced by macrophages and other cell types such as epithelial cells, and it is also synthesized by endothelial cells, and accordingly is also termed CXCL8. While neutrophil granulocytes are the primary target cells of IL-8 there is a relative wide range of cells (endothelial cells, macrophages, mast cells, Keratinocytes) responding to this chemokine, too.
  • IL-8 Primary function of IL-8 is the induction of chemotaxis in its target cells (e.g. neutrophil granulocytes). In neutrophils series of cell-physiological responses required for migration and its target function phagocytosis are also induced like increase of intracellular Ca2+, exocytosis (e.g. histamine release), respiratory burst. IL-8 can be secreted by any cells with TLRs which are involved in the innate immune response. IL-8's primary function is to recruit neutrophils to phagocytose the antigen which trigger the antigen pattern TLRs. By conveying IL-8 target cells to the endothelium and other target tissues IL-8 is thus implicated in the amplification and execution of many of the TNF-alpha pathogenic roles, in addition to its role in the body defence.
  • TLRs which are involved in the innate immune response.
  • IL-8's primary function is to recruit neutrophils to phagocytose the antigen which trigger the antigen pattern T
  • Leucocyte migration and homing are not only regulated by chemokines and their receptors but also by a number of adhesion molecules.
  • the selectin CD62L is acknowledged as a therapeutic target to prevent leucocytes migration to the lymph nodes and thus is evaluated as a parameter to rank the in vitro effects of nonsteroid anti- inflammatory drugs (NSAIDs).
  • NSAIDs nonsteroid anti- inflammatory drugs
  • immune suppressor and anti-TNF-alpha molecules affect the normal immune defence mechanisms because they promote cytotoxic effects upon immune cells or inhibit the proliferative mechanism that underlie under the clonal expansion preceding the successful effector immune responses.
  • TNF-alpha cytoplasmic membrane-inserted or secreted soluble forms
  • many efforts have been displayed to design therapeutic agents that block the interaction of extracellular TNF- alpha with both TNF-receptor I and/or TNF-receptor II.
  • the most relevant approaches have been the use of soluble decoy TNF-receptor that captures TNF-alpha and thanks to the long time of dissociation prevents the pro -inflammatory ligand interaction with the cellular receptors.
  • a second strategy has been to produce humanised anti-human TNF-alpha antibodies either conventional or created as bis-specific single chain molecules that target as well other molecules relevant in a given disease (i.e., anti-VEGF/anti-TNF- alpha in rheumatoid arthritis).
  • the molecules described above are TNF-alpha antagonists, they restrict their mechanism of action to the blockade of extracellular secreted TNF-alpha.
  • a comprehensive and not exhaustive list of targets that drive to TNF-alpha production and secretion might be: a) molecules driving transcriptional expression of TNF-alpha; b) molecules driving TNF-alpha-RNA transport from the nucleus to the cytoplasm and RNA splicing; c) molecules directing TNF-alpha translation; d) molecules regulating TNF-alpha-mRNA stability; e) molecules directing Golgi vesicles to the membrane where the pro-TNF-alpha surface form is anchored; f) molecules such as TNF-alpha-converting enzyme (TACE) implicated in the secretory shedding of TNF- alpha and g) molecules regulating the internalization of the surface form of pro-TNF- alpha and its signaling. All of these refer to cellular targets of TNF-alpha production and secretion.
  • TACE TNF-alpha-converting enzyme
  • compounds of formula (I) have shown a number of highly interesting immune modulating effects potentially useful for the control of the pathogenic mechanisms of acute and chronic inflammatory diseases and therefore, with potential clinical applications.
  • the compounds used in the invention have been able to inhibit TNF-alpha production by peripheral blood mononuclear cells (PBMC) from patients suffering from a chronic inflammatory disease, such as rheumatoid arthritis, as well as to inhibit IFN-gamma secretion by those cells after T-cells stimulation.
  • PBMC peripheral blood mononuclear cells
  • the immune cells are sessile, and enter organs to patrol the body tissues that infiltrate in the inflamed conditions where they concentrate in the lesions distributed according to the disease activity, target organs and extension of damage. Since the compounds used in the invention are expected to modulate some aspect of the patho-physiological process, then imaging studies can be used to characterize the number of receptors, binding efficiency, receptor occupancy and medicament probe concentration. Given the homing properties of leukocytes, the detection of the therapeutic target brings together information about the location of the target cells and the lesion sites.
  • the compounds of formula (I) also exhibit a potential use as imaging biomarkers in drug development, clinical trials and individualized medicine, which allows to provide information not only on pharmacokinetics, distribution and dosing but also relevant data on the individualized response patterns in preclinical and clinical trials.
  • the latter may lead to the definition of validated, reliable, individualized surrogate biomarkers of clinical endpoints administering to a patient who needs such prognostic and individualized evaluation of effective amount of a compound of formula (I) or a pharmaceutical composition thereof optimized for the distinct bio-imaging technology known by persons skilled in the art.
  • the present invention relates to the use of a compound of formula (I):
  • Ri is selected from hydrogen, substituted or unsubstituted Ci-C 6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl;
  • R 2 is selected from hydrogen, substituted or unsubstituted Ci-C 6 alkyl, substituted or unsubstituted cycloalkyl, and N(R'R") wherein R' and R" are independently hydrogen or Ci-C 6 alkyl; and
  • R3 is a Ci-C 6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof, in the preparation of a medicament for the treatment of an acute or chronic inflammatory disease, by inhibiting the production of at least one pro-inflammatory cytokine selected from TNF- alpha and IFN-gamma, or by inmunomodulating the IL-8 chemokine and/or the IL-IO regulatory cytokine.
  • the acute or chronic inflammatory disease is selected from acute and chronic seropositive or seronegative olygo arthritis and polyarthritis, spondiloarthropathies, glomerulonephritis, colagenopathies, tubulo- interstitial nephritis, metabolic syndrome, atherosclerosis, osteoarthritis, asthma, chronic obstructive pulmonary disease, interstitial lung disease, multiple sclerosis, demyelinating diseases, meningitis, encephalitis, meningoencephalitis, inflammatory radiculopathies and peripheral neuropathies, inflammatory bowel disease, cirrhosis, hepatitis, heart failure, ischemic disease, renal failure, inflammatory cystitis, benign prostatic hyperplasia, prostatitis, myocarditis, pericarditis, uveitis, atopic dermatitis, eccema, urticaria, psoriasis, rosacea, allergic rhin
  • These therapeutic indications are the consequence of at least an abnormal immune-response, an immune-disregulation, an immune-disturbance, an immune- pathogenesis, an immune-therapy, an immune-suppression or an immune-modulating biological response.
  • Ri is selected from hydrogen, substituted or unsubstituted Ci-C 6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl;
  • R3 is a Ci-C 6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
  • the invention is aimed at a pharmaceutical composition
  • a pharmaceutical composition comprising a compound of formula (F) as defined above, or a pharmaceutically acceptable salt, prodrug or solvate thereof, and at least one pharmaceutically acceptable carrier, adjuvant and/or vehicle.
  • Another aspect of the present invention relates to a compound of formula (F) as defined above, for its use as a medicament.
  • Another aspect of the invention refers to the use of a compound of formula (I) as defined above as an imaging biomarker in imaging and pharmaco- imaging technologies, for finding immunological lesions, target cells and target molecules.
  • FIG. 1 Different fluorescent features of selected microparticles for the development of Cytometric Bead Array (CBA).
  • Figure 12 Effect of compound 12 on the shedding of CD62L in lymphocytes (a) and monocytes (b) of PBMC from healthy volunteers.
  • Ci_6 alkyl refers to a linear or branched hydrocarbon chain radical consisting of carbon and hydrogen atoms, containing no insaturation, having one to six carbon atoms, and which is attached to the rest of the molecule by a single bond, e. g., methyl, ethyl, n-propyl, i-propyl, n-butyl, t-butyl, n-pentyl, etc.
  • Ci_6 alkyl radicals may be optionally substituted by one or more substituents such as cycloalkyl, aryl, heterocyclyl, halo, hydroxy, alkoxy, cyano, amino, nitro or alkylthio.
  • cycloalkyl refers to a stable 3-to 8-membered ring radical which is saturated or partially saturated, and which consists solely of carbon and hydrogen atoms, such as cyclohexyl or cyclopentyl. Unless otherwise stated specifically in the specification, the term “cycloalkyl” is meant to include cycloalkyl radicals which are optionally substituted by at least one substituent independently selected from the group consisting of hydrogen, Ci_6 alkyl radical, halo, hydroxyl, -N(Rs)(R 4 ), wherein R3 and R 4 are independently selected from hydrogen and linear or branched Ci_ 6 alkyl radical.
  • aryl refers to a stable 5- to 8-membered aromatic ring radical, and which consists solely of carbon and hydrogen atoms, such as phenyl or cyclooctatetraene. Unless otherwise stated specifically in the specification, the term
  • aryl is meant to include aryl radicals which are optionally substituted by at least one substituent independently selected from the group consisting of hydrogen, Ci_ 6 alkyl radical, halo, hydroxyl, -N(R 3 )(R 4 ), wherein R 3 and R 4 are independently selected from hydrogen and linear or branched Ci_6 alkyl radical.
  • Heterocyclyl refers to a stable 3-to 8 membered ring radical which consists of carbon atoms and from one to five heteroatoms selected from the group consisting of nitrogen, oxygen, and sulphur.
  • the heterocycle may be partially or fully saturated or aromatic. Examples of such heterocycles include, but are not limited to pyrrolidine, pyridine, thiophene, furan, etc.
  • heterocyclyl is meant to include heterocyclyl radicals which are optionally substituted by at least one substituent independently selected from the group consisting of hydrogen, Ci_6 alkyl radical, halo, hydroxyl, - N(R 3 )(R 4 ), wherein R 3 and R 4 are independently selected from hydrogen and linear or branched Ci_6 alkyl radical.
  • halo refers to bromo, chloro, iodo or fluoro.
  • acute and chronic seropositive or seronegative olygo arthritis and polyarthritis refers to diseases with synovitis involving one or several dyarthrodial joints, with either positive or negative rheumatoid factor, including rheumatoid arthritis and both primary and secondary Sjogren syndrome.
  • pondiloarthropahies refers to immune pathogenically HLA-B27- associated inflammatory diseases with involvement of sacro-ileal joints and/or spinal and/or peripheral joints, also including uveitis.
  • glomerulonephritis refers to inflammatory lesions of the renal glomerulus.
  • tubulo-interstitial nephritis refers to inflammatory diseases involving tubules and renal interstitium.
  • colagenopathies refers to systemic inflammatory diseases with pathogenic immune mechanism including systemic lupus erythematosus (SLE), dermatomyositis and sclerodermia.
  • inflammatory bowel disease refers to inflammatory diseases of the gastrointestinal tract with pathogenic immune mechanism, either with or without systemic features, including Crohn's disease and ulcerative colitis.
  • obstructive pulmonary disease refers to bronchial diseases with either reversible or irreversible decrease of the flow expiratory volume (FEV), including asthma and chronic obstructive pulmonary disease.
  • FEV flow expiratory volume
  • interstitial lung disease refers to inflammatory diseases involving lung interstitium.
  • demyelinating diseases refers to inflammatory diseases of the central nervous system with an immune pathogenic mechanism provoking myelin lysis, including multiple sclerosis and optical neuritis.
  • meningitis, encephalitis and meningoencephalitis refers to inflammatory diseases of the meninges and/or other structures of the central nervous system.
  • inflammatory radiculopathies and peripheral neuropathies refers to inflammatory diseases of the peripheral nervous system.
  • inflammatory cystitis refers to inflammatory diseases of the bladder.
  • benign prostatic hyperplasia refers to non-malignant hyperthrophy and/or hyperplasia of the prostate.
  • atopic dermatitis, eccema and urticaria refers to allergic skin diseases with immune pathogenic mechanism with or without involvement of IgE.
  • psoriasis refers to hyperkeratosic and erythematous skin reaction with an immune system pathogenic mechanism.
  • rosacea refers to common inflammatory condition of the skin characterised by erythema (flushing and redness) on the central face and across the cheeks, nose or forehead also can also less commonly affect the neck and chest.
  • allergic rhinitis refers to intermittent (also called seasonal) or persistent (also called perennial) inflammatory nose mucosa diseases of immune hipersenivity pathogenic mechanism.
  • spontaneous shock refers to systemic inflammatory diseases mediated by an abnormal immune response to microbial agents and other ethio logical factors.
  • sarcoidosis and amyloidosis refers to idiopathic immunological diseases with organ and/or systemic involvement and no well defined ethiology in which an abnormal immune response can be observed.
  • organ specific auto-immune diseases refers to immune system- mediated lesion of organs with no defined ethio logical factors, including myastenia gravis, tyroiditis, hypophysitis, adrenalitis and others.
  • organ transplantation refers to prevention and treatment of rejection of transplanted cells, tissues and organs.
  • infection and tumour-induced inflammation refers to abnormal immune responses secondary to microbial agents or cancer stimuli.
  • TNF-alpha dependent cellular degeneration, apoptosis or necrosis refers to tissue degeneration or death induced by TNF-alpha.
  • graft versus host disease refers to inflammatory immune responses induced by graft cells.
  • caquexia refers to systemic anorexia or malnutrition and weight loss induced by inflammatory or neoplasic diseases.
  • atherosclerosis refers to any hardening of arteries secondary to atheroma or accumulation in the arthery walls that is made up of inflammatory cells (mostly macrophage cells) and cell debris, that contain lipids.
  • ischemic diseases refers to lesion of organs secondary to reduced tissue oxigenation and/or blood flow including heart and cerebrovascular ischaemia.
  • autocrine and paracrine pathological cell growth refers to malignant or benign diseases with cell use of TNF-alpha as a cytokine regulating activation and proliferation factor for the cells.
  • the compounds used in the invention are intended to include compounds that only differ in the presence of one or more isotopically enriched atoms.
  • compounds having the present structures except for the substitution of an hydrogen with deuterium or tritium, or the substitution of a carbon with a 13 C- or
  • salts, prodrugs and derivatives can be prepared by means of methods known in the state of the art.
  • “Pharmaceutically acceptable” preferably relates to molecular entities and compositions which are physiologically tolerable and do not typically cause an allergic reaction or a similar unfavorable reaction, such as gastric disorders, dizziness and the like, when administered to a human or animal.
  • pharmaceutically acceptable means that it is approved by a regulatory agency of a federal or state government or is included in the US pharmacopoeia or another generally recognized pharmacopoeia for use in animals, and more particularly in humans.
  • the pharmaceutically acceptable salts of the compounds described previously herein are synthesized from the previously described compound containing a basic or acidic unit by means of conventional chemical methods.
  • Such salts are generally prepared, for example, by reacting the free acidic or basic forms of these compounds with a stoichiometric amount of the suitable base or acid in water or in an organic solvent or in a mixture of both.
  • Non-aqueous media such as ether, ethyl acetate, ethanol, isopropanol or acetonitrile, are generally preferred.
  • acid addition salts include mineral acid addition salts such as hydrochloride, hydrobromide, hydroiodide, sulfate, nitrate, phosphate, for example, and organic acid addition salts such as acetate, maleate, fumarate, citrate, oxalate, succinate, tartrate, malate, mandelate, methanesulfonate and p-toluenesulfonate, for example.
  • alkaline addition salts include inorganic salts such as sodium, potassium, calcium, ammonium, magnesium, aluminium and lithium, for example, and organic alkaline salts such as ethylenediamine, ethanolamine, N,N-dialkylenethanolamine, glucamine and basic amino acid salts for example.
  • prodrug is defined herein as a chemical compound which has undergone a chemical derivation such as a substitution or addition of an additional chemical group in order to change (for pharmaceutical use) some of its physical chemistry properties, such as solubility or bioavailability, for example an ester or ether derived from an active compound giving an active compound per se after the administration to a subject.
  • chemical derivation such as a substitution or addition of an additional chemical group in order to change (for pharmaceutical use) some of its physical chemistry properties, such as solubility or bioavailability, for example an ester or ether derived from an active compound giving an active compound per se after the administration to a subject.
  • solubility or bioavailability for example an ester or ether derived from an active compound giving an active compound per se after the administration to a subject.
  • solvate is understood to mean any form of a compound of the invention having another molecule (most likely a polar solvent) bound to it through a non-covalent bond.
  • solvates include hydrates and alcoholates, for example methanolate.
  • Particularly preferred prodrugs are those increasing the bioavailability of the compounds of this invention when such compounds are administered to a patient (allowing an orally administered compound to be more quickly absorbed into the blood, for example) or those increasing the distribution of the original compound to a biological compartment (the brain or the lymphatic system, for example) with respect to the original species.
  • the compounds used in the invention may be in crystalline form, i.e. as polymorphs, either as free compounds or as solvates (hydrates, for example) and it is understood that both forms are within the scope of the present invention.
  • Solvation methods are generally known in the art. Suitable solvates are pharmaceutically acceptable solvates. In a particular embodiment, the solvate is a hydrate.
  • Salts, solvates and prodrugs can be prepared by means of methods known in the state of the art. It will be observed that pharmaceutically unacceptable salts, solvates or prodrugs are also included within the scope of the invention because they can be useful in the preparation of pharmaceutically acceptable salts, solvates or prodrugs.
  • the compounds of formula (I) or their salts or solvates are preferably in pharmaceutically acceptable form or in substantially pure form.
  • a pharmaceutically acceptable form is understood, inter alia, as having a pharmaceutically acceptable purity level, excluding normal pharmaceutical additives such as diluents and excipients, and without including any material considered to be toxic at normal dosage levels.
  • the purity levels for the drug are preferably above 50%, more preferably above 70%, and still more preferably above 90%. In a preferred embodiment, it is above 95% of the compound of formula (I), or of its salts, solvates or prodrugs.
  • the compounds used in the invention shown by the formula (I) described above can include enantiomers depending on the presence of chiral centers or isomers depending on the presence of multiple bonds (for example, Z, E).
  • the individual isomers, enantiomers, diastereoisomers and mixtures thereof are within the scope of the present invention.
  • the compound of formula (I) may be labeled with fluorescent or luminiscent tags or flags, introducing the markers by any method known by a skilled person in the art.
  • Ri is a substituted or unsubstituted Ci-C 6 alkyl.
  • Ri is methyl.
  • R 2 is hydrogen, substituted or unsubstituted Ci-C 6 alkyl, substituted or unsubstituted cycloalkyl.
  • R 2 is a substituted or unsubstituted cycloalkyl. More preferably, R 2 is cyclopentyl.
  • R 3 is methyl.
  • the compound of formula (I) used in the present invention is selected from the following compounds:
  • the compounds of formula (I) used in the present invention can be obtained by available synthetic procedures. For example, they can be prepared by a process which is summarised in the following scheme:
  • This process firstly comprises an esterification reaction of the compound 4-R 3 - thiophenylacetic acid to render the methyl ester derivative.
  • Said reaction can be carried out using a methylating agent, such as MeI, in the presence of a salt, such as NaHCO 3 , or using MeOH as methylating agent in the presence of an acidic medium.
  • the methyl ester derivative is oxidized at the sulphur atom using an oxidizing agent, for instance, oxone, thus obtaining the sulfone compound from the thioether group.
  • an oxidizing agent for instance, oxone
  • Said thioamides include compounds wherein Ri is selected from hydrogen, substituted or unsubstituted Ci-C 6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl as defined above.
  • R 2 radical through the hydro xyl group
  • the hydroxyl group is reacted with an halide of formula R 2 -HaI, preferably R 2 -Br, to provide the compound of formula (I).
  • the present invention provides a compound of formula (F):
  • Ri is selected from hydrogen, substituted or unsubstituted Ci-C 6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclic and R 3 is a Ci-C 6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
  • Ri is a substituted or unsubstituted Ci-C 6 alkyl.
  • Ri is methyl
  • R 3 is methyl.
  • the compound of formula (F) of the invention is selected from the following: or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
  • the present invention further provides pharmaceutical compositions comprising the novel compound of formula (F) of the present invention, or pharmaceutically acceptable salts, solvates or prodrugs thereof and at least one pharmaceutically acceptable carrier, adjuvant and/or vehicle, for the administration to a patient.
  • the compounds of formula (I), their pharmaceutically acceptable salts, prodrugs and/or solvates will be formulated in a suitable pharmaceutical composition, in the therapeutically effective amount, together with one or more pharmaceutically acceptable carriers, adjuvants, and/or vehicles.
  • carrier, adjuvant and/or vehicle relates to molecular entities or substances with which the active ingredient is administered.
  • Such pharmaceutical carriers, adjuvants or vehicles can be sterile liquids, such as waters and oils, including those of petroleum or with an animal, plant or synthetic origin, such as peanut oil, soybean oil, mineral oil, sesame oil and the like, excipients, disintegrants, wetting agents or diluents.
  • Suitable pharmaceutical carriers are described in "Remington's Pharmaceutical Sciences” by E.W. Martin.
  • compositions can be administered by any suitable method of administration, for example, oral, parenteral (for example, subcutaneous, intraperitoneal, intravenous, intramuscular, etc.), rectal administration, etc., typically orally due to the chronic nature of the disease to be treated.
  • parenteral for example, subcutaneous, intraperitoneal, intravenous, intramuscular, etc.
  • rectal administration etc., typically orally due to the chronic nature of the disease to be treated.
  • said pharmaceutical compositions can be in an oral administration pharmaceutical form, either in solid or liquid form.
  • oral administration pharmaceutical forms include tablets, capsules, granulates, solutions, suspensions, etc., and can contain conventional excipients such as binders, diluents, disintegrants, lubricating agents, wetting agents, etc., and can be prepared by conventional methods.
  • the pharmaceutical compositions can also be adapted for their parenteral administration, in the form of, for example, sterile, lyophilized products, suspensions or solutions in the suitable dosage form; in this case, said pharmaceutical compositions will include suitable excipients, such as buffers, surfactants, etc. In any case, the excipients will be chosen according to the selected administration pharmaceutical form.
  • the compound of formula (I) will preferably be found in a pharmaceutically acceptable or substantially pure pharmaceutical form, i.e. the compound of formula (I) has a pharmaceutically acceptable purity level excluding pharmaceutically acceptable excipients and does not include material considered to be toxic at normal dosage levels.
  • the purity levels for a compound of formula (I) are preferably greater than 50%, more preferably greater than 70%, more preferably greater than 90%. In a preferred embodiment, they are greater than 95%.
  • the therapeutically effective amount of the compound of formula (I) to be administered will generally depend, among other factors, on the individual to be treated, on the severity of the disease suffered by said individual, on the chosen method of administration, etc. For this reason, the doses mentioned in this invention must only be considered as guidelines for the person skilled in the art, and the latter must adjust the doses according to the aforementioned variables. Nevertheless, a compound of formula (I) can be administered once or more times a day, for example, 1, 2, 3 or 4 times a day, in a typical total daily amount comprised between 0.1 and 1000 mg/kg of body mass/day, preferably 10 mg/kg of body mass/day.
  • the compound of formula (I), its pharmaceutically acceptable salts, prodrugs and/or solvates, as well as the pharmaceutical compositions containing them can be used together with other additional drugs useful for treating acute and chronic inflammatory diseases.
  • Said additional drugs can form part of the same pharmaceutical composition or alternatively, can be provided in the form of a separate composition for its simultaneous or non-simultaneous administration with the pharmaceutical composition comprising a compound of formula (I), or a pharmaceutically acceptable salt, prodrug or solvate thereof.
  • the expression "acute and chronic inflammatory disease” relates to any disease, disorder or condition which results from the activation and pathogenic involvement of inflammatory/immune cells and inflammatory cytokine cascade under condition in which abnormal co-stimulation is a pathogenic mechanism.
  • the predominant cells involved are inflammatory/immune cells such as monocytes, macrophages, APC, T, B and Natural Killer (NK) cells, plasma cells, granulocytes and mast cells, or combinations of the above cell subpopulations implicated in the diseases proposed for treatment.
  • cytokine refers to a secreted protein that affects the functions of other cells, particularly as it relates to the modulation of interactions between cells of the immune system or cells involved in the inflammatory response.
  • cytokines are TNF-alpha (tumor necrosis factor- ⁇ ), IFN-gamma (inter feron- ⁇ ), the IL-8 (interleukin- 8) chemokine, and the regulatory cytokine IL-IO (interleukin-10).
  • IL-IO production is induced by high TNF-alpha levels and promotes a negative feed-back upon TNF-alpha production, upon blockade of pro-inflammatory cytokine transcription.
  • the acute or chronic inflammatory disease is selected from acute and chronic seropositive or seronegative olygo arthritis and polyarthritis, spondiloarthropathies, glomerulonephritis, colagenopathies, tubulo- interstitial nephritis, metabolic syndrome, atherosclerosis, osteoarthritis, asthma, chronic obstructive pulmonary disease, interstitial lung disease, multiple sclerosis, demyelinating diseases, meningitis, encephalitis, meningoencephalitis, inflammatory radiculopathies and peripheral neuropathies, inflammatory bowel disease, cirrhosis, hepatitis, heart failure, ischemic disease, renal failure, inflammatory cystitis, benign prostatic hyperplasia, prostatitis, myocarditis, pericarditis, uveitis, atopic dermatitis, eccema, urticaria, psoriasis, rosacea, allergic rhin
  • the acute or chronic inflammatory disease is seropositive or seronegative chronic polyarthritis, more preferably is rheumatoid arthritis.
  • Another aspect of the present invention is a method for treating an acute or chronic inflammatory disease, which comprises administering to a patient who needs such treatment a therapeutically effective amount of a compound of formula (I) as defined above or a pharmaceutical composition thereof.
  • treatment means the administration of a compound with a formulation according to the invention for preventing, alleviating or eliminating the disease or one or more symptoms associated to said disease.
  • Treatment also includes preventing, alleviating or eliminating the physiological sequel of the disease.
  • Another aspect of the invention refers to the use of a compound of formula (I) as defined above as an imaging biomarker in imaging and pharmaco -imaging technologies, for finding immunological lesions, target cells and target molecules.
  • the pharmaco-imaging technology extends the scope of biomarkers obtained by the rapidly growing combination of adequate preclinical (molecular, cellular, organ and whole animal tracking and study of proof of concept and mechanisms, efficacy assessment, etc) and clinical (human medical) in vivo imaging technologies, to those valuable information data generated by compounds described herein and used as medicines.
  • NMR 1 H (CDCl 3 ), ⁇ : 7.9 (d, 2 H), 7.75 (d, 2H), 5.4 (s, IH), 3.8 (s, 3H), 3,1 (s, 3H).
  • the degree of disease activity was defined as follows: a) DAS28 > 3,2 and/or b) 6 or more swollen articulations and 6 or more painful articulations.
  • exclusion criteria were considered the following: a) to suffer from active infectious diseases in the inclusion visit; b) to suffer from oncological diseases prior the inclusion; 3) to suffer from another systemic or organ specific auto-immune disease which had not entered into a complete remission at least one year prior the inclusion visit; d) to suffer from a severe renal, cardiac or hepatic condition not related with the changes at those levels induced by the rheumatoid arthritis as main disease; e) to suffer a severe deterioration of the general status due to a condition not related with the main disease; f) to have received treatment with corticosteroids, immunosuppresors, cytostatic or any other drugs with known activity on the immune system during the year prior the inclusion visit with the exception of the indicated doses of Methrotexate; 7) to be pregnant or within the puerperium in the inclusion visit.
  • Herasafe HS 12 Heraeus, Germany.
  • FCS Phoetal bovine serum
  • PHA Phytohaemaglutinin M
  • - Antibiotic mixture A mixture of Sodium Ampycilline 10 mg/ml (Britapen, Beecham A., Toledo, Spain), Gentamycin sulphate 1.6 mg/ml (Tamadit Lab., Dr. Esteve SA., Madrid, Spain) and Amphotherycine B 0.5 ⁇ g/ml (Fungizona, Squibb, Esplugues, Barcelona, Spain) was added to the culture medium.
  • - Anti-CD3 monoclonal antibody Orthoclone OKT3, Orthopharmaceutical Corporation, Raritan, NJ, USA).
  • Venous blood Mononuclear cells were obtained from venous blood as collected by antecubital venous punction. Fifty ml of blood were extracted and stored in lithium heparin tubes (Venojet), further diluted with saline 1/1 (vol/vol) being all performed under sterile conditions. b) Human Cell subsets harvesting. For isolating PBMC, the remaining blood components were separated by a density gradient on Ficoll. This method is based on the differences on density of blood cells. In a 50 ml centrifuge tube containing the diluted and heparinized blood, 15 ml Ficoll-Hipaque (density 1.077 g/ml) was carefully placed on.
  • PBMC erythrocytes, Ficoll and plasma
  • PBMC erythrocytes, Ficoll and plasma
  • the extracted blood was stored in tubes both with and without anti-coagulant (collected by antecubital venopunction and arterial catheter, respectively). Blood was allowed to coagulate at room temperature in the laboratory, further separating the serum by centrifugation (600xg during 20 minutes). Supernatant were collected, filtered, divided in aliquotes and stored at -7O 0 C. Concentration assays for different cytokines were performed by using the commercial kits described in Table 2.
  • PE phycoerythrin-labeled
  • FACSCalibur flow cytometer equipped with argon laser tuned at 488 nm was used in order to induce phycoerythrin fluorescence.
  • study cells with no labelling and other irrelevant labelled with monoclonal antibodies of equal isotypes than the ones used in the study (IgGl-FITC, PE y TC, IgG2a FITC, PE, TC), were used.
  • lymphocytes Faced against a mitogen stimulation, lymphocytes suffer a blastogenesis and cellular differentiation process.
  • the method used to quantify the cellular proliferation was the assay of the incorporation of 3 [H] -Thymidine to the DNA de novo synthesized, and the emission of betha-radiation from the cellular cultures dried extracts (to which the tritiated base was added) was detected before its ending and harvesting.
  • the purified cellular preparations were incubated in 96 microwells plain bottom plates at concentrations of 5 x 10 4 cells/well (200 ⁇ l final volume), in the presence of different concentrations of various mitogens with triplicate repetitions and along 4 days of culture. The response to a specific stimuli depended on the density and cell type studied, as well as of the culture time and of the mitogenic agent concentration.
  • DNA synthesis was expressed in counts per minute (c.p.m.). Each assay was performed in triplicate, rejecting those data with a variability higher than 10 % in the mean of the triplicate as they might indicate a technical error or a contamination of the culture. Cultures were performed with a constant amount of cells per well as well as with a constant volume of 200 ⁇ l. All mitogens and cytokines were first tested by carrying out dose-response curves and time-response.
  • the experimental protocol consisted of a plate pre-washing out with Wash Buffer. After decantation, the mixture of capture microparticles was re-suspended in the vortex. Standards and samples were added in the adequate dilution. After permanent stirring incubation during 1 h, the PE detection reagent was added and incubated again during 2h at room temperature. After a washing-out, the acquisition was performed in the flow cytometer. Table 3. -Kit CBA Human Soluble Protein Multiplex Flex Set System.
  • PBMC peripheral blood mononuclear cells
  • PBMC TNF-alpha production by PBMC of healthy volunteers in the presence or in the absence of LPS were first investigated.
  • PBMC PBMC (5 x 10 4 cells/well, 200 ⁇ l) from 10 healthy volunteers were cultured in parallel in duplicate in tissue culture plates, 96 well, flat-bottom with low evaporation lid (353072 Falcon, Becton Dickinson labware, Franklin Lakes, USA, 07417-1886 NJ) in complete medium (RPMI-1640 with glutamine Cat BE-12-70F, Cambrex Biosciences, B4880 Verviers, Belgium), supplemented with phoetal bovine serum (origin USA, Gibco ref.
  • Immune modulator effects of compound 12 were further characterised on the production of a cytokine panel by PBMC either after monocyte stimulation with either LPS or lymphocyte activation with a combination of monoclonal antibodies anti-CD3 and anti-CD28. This study was performed in the presence or absence of titrated doses of compound 12 in cultures of PBMC obtained from healthy volunteers and patients with rheumatoid arthritis.
  • PBMC peripheral blood mononuclear cells
  • CBA Flex Multiplex Set (BDTM Cytometric Bead Array, CBA: IL-8, IL-IO, TNF-alpha and IFN-gamma Becton Dickinson Biosciences Pharmingen, San Diego CA 92121).
  • PBMC peripheral blood mononuclear cells
  • Example 7 Effects of compound 12 on the production of IFN-gamma.
  • PBMC peripheral blood mononuclear cells
  • Compound 12 at a concentration of 10 "6 M significantly inhibited the production of IFN-gamma by PBMC from healthy volunteers either LPS-stimulated or stimulated with monoclonal antibodies anti-CD3 and anti-CD28 (p ⁇ 0.05) (Figure 5).
  • PBMC peripheral blood mononuclear cells
  • PBMC peripheral blood mononuclear cells
  • Example 8 Effects of compound 12 on Interleukin 8 (IL-8) production.
  • the effect of compound 12 on the IL-8 production by the PBMC from healthy volunteers was further investigated, both in the presence and absence of LPS stimuli and monoclonal antibodies anti-CD3 and anti-CD28.
  • PBMC (5 x 10 4 cells/well) from 13 healthy volunteers were cultured in duplicate in 200 ⁇ l of complete medium supplemented with the highest solvent concentration (10 ⁇ 6 M), and 10 "6 M, 10 "7 M and 10 "8 M of compound 12, in the presence and absence of either LPS (10 ⁇ g/ml) or anti- CD3 (12.5 ng/ml) + anti-CD28 (l/3xl ⁇ 5 ), during 24 hours.
  • PBMC peripheral blood mononuclear cells
  • PBMC peripheral blood mononuclear cells
  • 10 "6 M, 10 "7 M and 10 "8 M of compound 12 were cultured in duplicate in 200 ⁇ l of complete medium supplemented with the highest solvent concentration (10 ⁇ 6 M), and 10 "6 M, 10 "7 M and 10 "8 M of compound 12, in the presence and in the absence of either LPS (10 ⁇ g/ml) or anti-CD3 (12.5 ng/ml) + anti-CD28 (l/3xl ⁇ 5 ), during 24 hours.
  • Culture supernatants were frozen at -2O 0 C and IL-8 concentration was quantified by BD FACS Array Bioanalyser by using CBA Flex
  • Example 9 Effects of compound 12 on Interleukin 10 (IL-IO) production.
  • PBMC (5 x 10 4 cells per well) from 13 healthy volunteers were cultured in duplicate 200 ⁇ l of complete medium supplemented with the highest solvent concentration (10 ⁇ 6 M), and 10 "6 M, 10 "7 M and 10 "8 M of compound 12, in the presence and absence of either LPS (10 ⁇ g/ml) or anti-CD3 (12.5 ng/ml), + anti-CD28 (l/3xl ⁇ 5 ), during 24 hours.
  • PBMC peripheral blood mononuclear cells
  • PBMC peripheral blood mononuclear cells
  • 10 "6 M, 10 "7 M and 10 "8 M of compound 12 in the presence and absence of either LPS (10 ⁇ g/ml) or anti-CD3 (12.5 ng/ml), + anti-CD28 (l/3xl ⁇ 5 ), during 24 hours.
  • Culture supernatants were frozen at -2O 0 C and IL-10 concentration was assayed by BD FACS Array Bioanalyser by using CBA Flex Set, specific to determine IL-10 concentration, following the manufacturer instructions.
  • Compound 12 showed no effects on the IL-10 production by PBMC from healthy volunteers in the presence and in the absence of both studied stimuli ( Figures 9). However, the presence of compound 12 in the culture, at a concentration of 10 "8 , significantly upmodulated IL-10 production after stimulation of PBMC from patients with rheumatoid arthritis with LPS (p ⁇ 0.05). Compound 12 induced no significant effects neither on the spontaneous production of IL-10 nor after the stimulation with monoclonal antibodies anti-CD3 and anti-CD28 by PBMC from patients with rheumatoid arthritis ( Figure 10).
  • Example 10 Effect of compound 12 on the proliferative response of PBMC.
  • PBMC peripheral blood mononuclear cells
  • Culture stimulation conditions were the absence or presence or phytohaemaglutinin (PHA Sigma Ref #L-8902, Madrid, Spain), 10 ⁇ g/ml; PHA 2 ⁇ g/ml with exogenous IL-2 supplementation (25 IU/ml, Human recombinant IL-2, Macrolin, Chiron Iberica, batch #SA753228/4, Madrid, Spain) and monoclonal antibodies anti-CD3 (12.5 ng/ml) + anti-CD28 (1 :320.000).
  • Methyl- 3 H- Thymidine was added (American Radiochemical 60 Ci/mmol methyl- 3 H-Thymidine, ITISA, Madrid, Spain) during the last 8 hours of culture.
  • Example 11 Effect of compound 12 on the shedding of CD62L by PBMC
  • CD62L shedding CD62L -Phycoerithryn (PE), clon BD SKI l Cat No. 341012, BD Biosciences
  • MFI geometric mean fluorescence intensity

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Abstract

The invention relates to the use of a compound of formula (I) or a pharmaceutically acceptable salt, prodrug and/or solvate thereof, in the preparation of a medicament for the treatment of an acute or chronic inflammatory disease, by inhibiting the production of at least one pro-inflammatory cytokine selected from TNF-alpha and IFN-gamma, or by inmunomodulating the IL-8 chemokine and/or the IL-10 regulatory cytokine. The invention also relates to novel compounds of formula (I') or a pharmaceutically acceptable salt, prodrug and/or solvate thereof, as well as a pharmaceutical composition comprising said compound.

Description

5-(4-METHANESULFONYL-PHENYL)-THIAZOLE DERIVATIVES FOR THE TREATMENT OF ACUTE AND CHRONIC INFLAMMATORY DISEASES
FIELD OF THE INVENTION The present invention relates to the use of compounds derived from 5-(4- methanesulfonyl-phenyl)-thiazole in the preparation of a medicinal product for the treatment of acute and chronic inflammatory diseases or conditions, such as rheumatoid arthritis.
STATE OF THE ART
Immunology is the scientific study of the discrimination between self and non-self. The breakdown of tolerance to self is in the origin of auto-immune diseases. Moreover, other conditions such as transplantation, atherosclerosis, septic and nonseptic acute and chronic inflammatory pathologies and many others diseases, up to now not considered as auto-immune, exhibit immune cell-mediated pathogenic mechanisms. Activation of immune inflammatory effector responses is considered by most authors as being based on two signals:
- Signal 1 implies the triggering of the clonal antigen's receptor (TCR-CD3 T-cell receptor complex), that recognize the cognate antigen embedded in the Major Histocompatibility Complex (MHC) molecules. In B-cells, extracellular soluble or membrane-bound antigens cross link the Immunoglobulin CD79 (Ig/CD79) clonal receptor complex to deliver the signal 1 to the antibody-secreting lymphocyte lineage.
- A second signal, in addition to antigen-delivered signal 1 , is required to avoid tolerance by anergy or clonal deletion. Signal 2 is delivered by co-stimulators such as CD86 expressed on the surface of professional antigen-presenting cells (APC), like human monocytes and their differentiation lineage progeny.
In innate immune inflammatory responses, danger signals are promoted by microbial and self-modified antigens or mitogens that trigger Pattern Recognition Receptors (PRR). PRR signalling pathways, such as TLR4 (the receptor for the Gram- negative wall bacteria lipo-polysaccharide or LPS) deliver the expression of high levels of co-stimulatory surface molecules (i.e., CD80 or CD86). In turn, co-stimulatory ligands CD80 - CD86 cross link CD28 on the surface of helper T-cells. The combination of signal 1 (i.e., anti-CD3 antibody cross linking) plus signal 2 (i.e., CD28 cross linking by specific antibodies) experimentally mimics the natural conditions of an efficient inflammatory effector immune response. Notably, approved immune suppressor drugs have some troubles to inhibit the activation of pro-inflammatory cytokine cascades under conditions of high levels of co-stimulation. The latter occur in auto-immune diseases and many other severe acute and chronic inflammatory conditions.
APCs are not only crucial for the acquired immune system to decide the class of immune response since they deeply influence whether there is an effector (i.e. T-cell help, Th, cellular cytoxicity, Th, antibody production, B-cell) responses or a tolerant response (by anergy or apoptosis) mediated by the challenged clon. APCs can also deliver themselves effector immediate immune responses. A well documented example is the production and release of high amounts of Tumour Necrosis Factor Alpha (TNF- alpha) by monocytes in cancer patients. In these patients, TNF-alpha promotes an augmented response and activation of the vascular endothelium, accompanied with secretion of Interleukin 8 (IL-8) and other pro -inflammatory cytokines as well as pro- coagulant activities. Altogether, TNF-alpha promotes thrombosis and ischaemia with cancer necrosis, which led to the original definition as cachectin or TNF-alpha. However, TNF-alpha is a pleiotropic cytokine involved in many other disease conditions. There is long-standing evidence that, upon monocytes, LPS may trigger the secretion of massive amounts of TNF-alpha which strongly contribute to the development of septic shock. More recently, the production and secretion of inadequately high amounts of TNF-alpha is considered as a therapeutic target in auto- immune inflammatory diseases, such as rheumatoid arthritis, spondiloarthropathies, Crohn's disease, uveitis and psoriasis. Thus, the use of anti-TNF-alpha has currently been broadly considered as a state of the art strategy to deal with those diseases in which the reduction of available levels of bioactive TNF-alpha might contribute to ameliorate the patient's condition. In this regard, the number of diseases which might benefit from the treatment with
TNF-alpha antagonists is growing rapidly and includes atherosclerosis, metabolic syndrome, encephalitis, viral hepatitis, glomerulonephritis, inadequate inflammatory response to tumours and septic shock as among several others.
In addition to that produced by some somatic cells, there are two major sources of
TNF-alpha production, monocytes and T-lymphocytes. In the course of an acquired immune response, exposition of APCs to danger signals under pro -inflammatory instructive scenarios, triggers the secretion of IL-12 p70 (an heterodimer of p35 and p40), being the latter a co-stimulatory molecule that polarizes the cytokine secretion profile of the activated Th-cells towards Th-I type. ThI -cells exhibit a characteristic cytokine profile in which interferon gamma (IFN-gamma) secretion is a bonafide footprint. These cells do secrete high amounts of TNF-alpha too.
IFN-gamma produced by ThI promotes many effects that may be relevant in the understanding of inflammatory diseases. On one hand, it further activates monocytes and increases the level of TNF-alpha secretion by a given stimuli. On the other hand, it promotes a stronger signalling pathway downstream TNF-alpha receptors. Altogether, IFN-gamma in addition to its own direct effects such as anti- viral activity, increases expression in MHC-II and contributes to inflammation and lesions by increasing the still strong effects of TNF-alpha.
The pro -inflammatory cascade initiated by the production of TNF-alpha in monocytes or IFN-gamma and TNF-alpha in ThI -cells, becomes amplified through other pro -inflammatory cytokine pathways such as IL-8. IL-8, in spite of its original name, was described as a chemokine produced by macrophages and other cell types such as epithelial cells, and it is also synthesized by endothelial cells, and accordingly is also termed CXCL8. While neutrophil granulocytes are the primary target cells of IL-8 there is a relative wide range of cells (endothelial cells, macrophages, mast cells, Keratinocytes) responding to this chemokine, too. Primary function of IL-8 is the induction of chemotaxis in its target cells (e.g. neutrophil granulocytes). In neutrophils series of cell-physiological responses required for migration and its target function phagocytosis are also induced like increase of intracellular Ca2+, exocytosis (e.g. histamine release), respiratory burst. IL-8 can be secreted by any cells with TLRs which are involved in the innate immune response. IL-8's primary function is to recruit neutrophils to phagocytose the antigen which trigger the antigen pattern TLRs. By conveying IL-8 target cells to the endothelium and other target tissues IL-8 is thus implicated in the amplification and execution of many of the TNF-alpha pathogenic roles, in addition to its role in the body defence.
Leucocyte migration and homing are not only regulated by chemokines and their receptors but also by a number of adhesion molecules. Among them, the selectin CD62L is acknowledged as a therapeutic target to prevent leucocytes migration to the lymph nodes and thus is evaluated as a parameter to rank the in vitro effects of nonsteroid anti- inflammatory drugs (NSAIDs).
Many immune suppressor and anti-TNF-alpha molecules affect the normal immune defence mechanisms because they promote cytotoxic effects upon immune cells or inhibit the proliferative mechanism that underlie under the clonal expansion preceding the successful effector immune responses.
Given the importance of the extracellular space secreted TNF-alpha (either cytoplasmic membrane-inserted or secreted soluble forms), many efforts have been displayed to design therapeutic agents that block the interaction of extracellular TNF- alpha with both TNF-receptor I and/or TNF-receptor II. The most relevant approaches have been the use of soluble decoy TNF-receptor that captures TNF-alpha and thanks to the long time of dissociation prevents the pro -inflammatory ligand interaction with the cellular receptors.
A second strategy has been to produce humanised anti-human TNF-alpha antibodies either conventional or created as bis-specific single chain molecules that target as well other molecules relevant in a given disease (i.e., anti-VEGF/anti-TNF- alpha in rheumatoid arthritis). Whereas the molecules described above are TNF-alpha antagonists, they restrict their mechanism of action to the blockade of extracellular secreted TNF-alpha. A comprehensive and not exhaustive list of targets that drive to TNF-alpha production and secretion might be: a) molecules driving transcriptional expression of TNF-alpha; b) molecules driving TNF-alpha-RNA transport from the nucleus to the cytoplasm and RNA splicing; c) molecules directing TNF-alpha translation; d) molecules regulating TNF-alpha-mRNA stability; e) molecules directing Golgi vesicles to the membrane where the pro-TNF-alpha surface form is anchored; f) molecules such as TNF-alpha-converting enzyme (TACE) implicated in the secretory shedding of TNF- alpha and g) molecules regulating the internalization of the surface form of pro-TNF- alpha and its signaling. All of these refer to cellular targets of TNF-alpha production and secretion.
In spite of the different approaches to design therapeutic agents that block the production of TNF-alpha, it would be highly desirable to find new drugs which selectively blocker not only the TNF-alpha production but also the production of another key pro-inflammatory cytokines, as IFN-gamma.
SUMMARY OF THE INVENTION
The authors of the present invention have surprisingly found that compounds of formula (I) have shown a number of highly interesting immune modulating effects potentially useful for the control of the pathogenic mechanisms of acute and chronic inflammatory diseases and therefore, with potential clinical applications. In particular, the compounds used in the invention have been able to inhibit TNF-alpha production by peripheral blood mononuclear cells (PBMC) from patients suffering from a chronic inflammatory disease, such as rheumatoid arthritis, as well as to inhibit IFN-gamma secretion by those cells after T-cells stimulation. Additionally, compounds of formula
(I) have been able to modulate the biological response profiles of secretion of chemokines (i.e. IL-8) and regulatory cytokines (i.e. IL-IO), and do it in a differential way in health and disease. This whole of immune modulating effects of compounds of formula (I) was not associated to any toxic effect on mononuclear cells from peripheral blood and, moreover, the activation and proliferative response after mitogenic stimuli was not modified by these compounds.
The combination, in only one small molecule, of inhibitory effects on several pro-inflammatory cytokines as TNF-alpha and IFN-gamma, and the potential to modulate IL-8 chemokine and/or IL-IO regulatory cytokine, since all of them are of crucial importance in the pathophysiology of systemic and organ-specific autoimmune disorders, transplantation, acute and chronic inflammatory diseases, some metabolic and degenerative diseases and atherosclerosis, allows compounds of formula (I) to belong to a new category of immune modulators for targeting the cascade of pro- inflammatory/regulatory cytokines and chemokines at various potentially re- programming levels of clinical and therapeutic relevance.
Notably the immune cells are sessile, and enter organs to patrol the body tissues that infiltrate in the inflamed conditions where they concentrate in the lesions distributed according to the disease activity, target organs and extension of damage. Since the compounds used in the invention are expected to modulate some aspect of the patho-physiological process, then imaging studies can be used to characterize the number of receptors, binding efficiency, receptor occupancy and medicament probe concentration. Given the homing properties of leukocytes, the detection of the therapeutic target brings together information about the location of the target cells and the lesion sites.
Therefore, the compounds of formula (I) also exhibit a potential use as imaging biomarkers in drug development, clinical trials and individualized medicine, which allows to provide information not only on pharmacokinetics, distribution and dosing but also relevant data on the individualized response patterns in preclinical and clinical trials. The latter may lead to the definition of validated, reliable, individualized surrogate biomarkers of clinical endpoints administering to a patient who needs such prognostic and individualized evaluation of effective amount of a compound of formula (I) or a pharmaceutical composition thereof optimized for the distinct bio-imaging technology known by persons skilled in the art.
According to a first aspect, the present invention relates to the use of a compound of formula (I):
Figure imgf000008_0001
(I) wherein:
Ri is selected from hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl;
R2 is selected from hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, and N(R'R") wherein R' and R" are independently hydrogen or Ci-C6 alkyl; and
R3 is a Ci-C6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof, in the preparation of a medicament for the treatment of an acute or chronic inflammatory disease, by inhibiting the production of at least one pro-inflammatory cytokine selected from TNF- alpha and IFN-gamma, or by inmunomodulating the IL-8 chemokine and/or the IL-IO regulatory cytokine.
In a particular aspect of the invention, the acute or chronic inflammatory disease is selected from acute and chronic seropositive or seronegative olygo arthritis and polyarthritis, spondiloarthropathies, glomerulonephritis, colagenopathies, tubulo- interstitial nephritis, metabolic syndrome, atherosclerosis, osteoarthritis, asthma, chronic obstructive pulmonary disease, interstitial lung disease, multiple sclerosis, demyelinating diseases, meningitis, encephalitis, meningoencephalitis, inflammatory radiculopathies and peripheral neuropathies, inflammatory bowel disease, cirrhosis, hepatitis, heart failure, ischemic disease, renal failure, inflammatory cystitis, benign prostatic hyperplasia, prostatitis, myocarditis, pericarditis, uveitis, atopic dermatitis, eccema, urticaria, psoriasis, rosacea, allergic rhinitis, sepsis, septic shock, multiorganic failure, systemic autoimmune diseases such as systemic lupus erythematosus, vasculitis, dermatomyositis, amyloidosis or sarcoidosis, organ specific autoimmune diseases such as myasthenia gravis, thyroiditis or insulinitis, organ transplantation, infectious ant tumor induced inflammation, TNF-alpha dependent cellular degeneration, necrosis, apoptosis, graft versus host disease, cachexia and autocrine and paracrine pathological cell growth.
These therapeutic indications are the consequence of at least an abnormal immune-response, an immune-disregulation, an immune-disturbance, an immune- pathogenesis, an immune-therapy, an immune-suppression or an immune-modulating biological response.
In another aspect the present invention relates to a compound of formula (F):
Figure imgf000010_0001
(T) wherein:
Ri is selected from hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl; and
R3 is a Ci-C6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
In a third aspect, the invention is aimed at a pharmaceutical composition comprising a compound of formula (F) as defined above, or a pharmaceutically acceptable salt, prodrug or solvate thereof, and at least one pharmaceutically acceptable carrier, adjuvant and/or vehicle.
Another aspect of the present invention relates to a compound of formula (F) as defined above, for its use as a medicament.
Finally, another aspect of the invention refers to the use of a compound of formula (I) as defined above as an imaging biomarker in imaging and pharmaco- imaging technologies, for finding immunological lesions, target cells and target molecules.
BRIEF DESCRIPTION OF THE FIGURES
Figure 1 : Different fluorescent features of selected microparticles for the development of Cytometric Bead Array (CBA).
Figure 2: Influence on TNF-alpha production in LPS-stimulated PBMC from healthy volunteers (n=10) by compound 12. Columns represent the median and standard error of the duplicate cultures performed in each sample in the different experimental conditions. Asterisks represent statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for each experimental condition.
Figure 3: Influence on TNF-alpha production in LPS- or TCR/CD3+CD28-stimulated PBMC from healthy volunteers (n=13) by compound 12. Columns represent the mean and standard error of the duplicate cultures performed in the samples in the different experimental conditions. Asterisks represent statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for each of the different experimental conditions. Figure 4: Influence on TNF-alpha production in PBMC from patients with rheumatoid arthritis (n=7) by compound 12. Columns represent the mean and standard error of the duplicate cultures performed in each sample in the different experimental conditions. Asterisks represent statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for each different experimental condition. Figure 5: Influence on IFN-gamma production in PBMC from healthy volunteers (n=13) by compound 12. Columns represented the mean and standard error of the duplicate cultures performed in each sample in the different experimental conditions. The asterisk represented the statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for the indicated experimental condition. Figure 6: Influence on IFN-gamma production in PBMC from patients with rheumatoid arthritis (n=8) by compound 12. Columns represent the mean and standard error of the duplicate cultures performed in each sample in the different experimental conditions. Asterisks represent statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for each of the different experimental conditions. Figure 7: Influence on IL-8 production in PBMC from healthy volunteers (n=13) by compound 12. Columns represent the mean and standard error of the duplicate cultures performed in each sample under the different experimental conditions. Asterisks represent statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for each experimental condition. Figure 8: Influence on IL-8 production in PBMC from patients with rheumatoid arthritis (n=8) by compound 12. Columns represent the mean and standard error of the duplicate cultures in each sample in the different experimental conditions. Asterisks represent statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle for each experimental condition.
Figure 9: Influence on IL-IO production in PBMC from healthy volunteers (n=13) by compound 12. Columns represent the mean and the standard error of the duplicate cultures performed in each sample in the different experimental conditions. No statistical differences were found.
Figure 10: Influence on IL-10 production in PBMC from patients with rheumatoid arthritis (n=8) by compound 12. Columns represent the mean and standard error of the duplicate cultures performed in each sample in the different experimental conditions. The asterisk represents the statistically significant differences (p < 0.05) of the corresponding data with respect to the vehicle.
Figure 11 : Effect of compound 12 (a) and vehicle (b) on the proliferative response of PBMC from healthy volunteers (n=8) in the presence and in the absence of stimulation with either PHA, PHA plus IL-2, or a combination of monoclonal antibodies anti-CD3 (T3) and anti-CD28.
Figure 12: Effect of compound 12 on the shedding of CD62L in lymphocytes (a) and monocytes (b) of PBMC from healthy volunteers.
DETAILED DESCRIPTION OF THE INVENTION
In the context of the present invention, the following terms have the meaning detailed below:
The term "Ci_6 alkyl" refers to a linear or branched hydrocarbon chain radical consisting of carbon and hydrogen atoms, containing no insaturation, having one to six carbon atoms, and which is attached to the rest of the molecule by a single bond, e. g., methyl, ethyl, n-propyl, i-propyl, n-butyl, t-butyl, n-pentyl, etc. Ci_6 alkyl radicals may be optionally substituted by one or more substituents such as cycloalkyl, aryl, heterocyclyl, halo, hydroxy, alkoxy, cyano, amino, nitro or alkylthio.
The term "cycloalkyl" refers to a stable 3-to 8-membered ring radical which is saturated or partially saturated, and which consists solely of carbon and hydrogen atoms, such as cyclohexyl or cyclopentyl. Unless otherwise stated specifically in the specification, the term "cycloalkyl" is meant to include cycloalkyl radicals which are optionally substituted by at least one substituent independently selected from the group consisting of hydrogen, Ci_6 alkyl radical, halo, hydroxyl, -N(Rs)(R4), wherein R3 and R4 are independently selected from hydrogen and linear or branched Ci_6 alkyl radical.
The term "aryl" refers to a stable 5- to 8-membered aromatic ring radical, and which consists solely of carbon and hydrogen atoms, such as phenyl or cyclooctatetraene. Unless otherwise stated specifically in the specification, the term
"aryl" is meant to include aryl radicals which are optionally substituted by at least one substituent independently selected from the group consisting of hydrogen, Ci_6 alkyl radical, halo, hydroxyl, -N(R3)(R4), wherein R3 and R4 are independently selected from hydrogen and linear or branched Ci_6 alkyl radical.
"Heterocyclyl" refers to a stable 3-to 8 membered ring radical which consists of carbon atoms and from one to five heteroatoms selected from the group consisting of nitrogen, oxygen, and sulphur. For the purposes of this invention, the heterocycle may be partially or fully saturated or aromatic. Examples of such heterocycles include, but are not limited to pyrrolidine, pyridine, thiophene, furan, etc. Unless otherwise stated specifically in the specification, the term "heterocyclyl" is meant to include heterocyclyl radicals which are optionally substituted by at least one substituent independently selected from the group consisting of hydrogen, Ci_6 alkyl radical, halo, hydroxyl, - N(R3)(R4), wherein R3 and R4 are independently selected from hydrogen and linear or branched Ci_6 alkyl radical.
The term "halo" refers to bromo, chloro, iodo or fluoro.
The term "acute and chronic seropositive or seronegative olygo arthritis and polyarthritis" refers to diseases with synovitis involving one or several dyarthrodial joints, with either positive or negative rheumatoid factor, including rheumatoid arthritis and both primary and secondary Sjogren syndrome.
The term "spondiloarthropahies" refers to immune pathogenically HLA-B27- associated inflammatory diseases with involvement of sacro-ileal joints and/or spinal and/or peripheral joints, also including uveitis.
The term "glomerulonephritis" refers to inflammatory lesions of the renal glomerulus.
The term "tubulo-interstitial nephritis" refers to inflammatory diseases involving tubules and renal interstitium. The term "colagenopathies" refers to systemic inflammatory diseases with pathogenic immune mechanism including systemic lupus erythematosus (SLE), dermatomyositis and sclerodermia.
The term "inflammatory bowel disease" refers to inflammatory diseases of the gastrointestinal tract with pathogenic immune mechanism, either with or without systemic features, including Crohn's disease and ulcerative colitis.
The term "obstructive pulmonary disease" refers to bronchial diseases with either reversible or irreversible decrease of the flow expiratory volume (FEV), including asthma and chronic obstructive pulmonary disease. The term "interstitial lung disease" refers to inflammatory diseases involving lung interstitium.
The term "demyelinating diseases" refers to inflammatory diseases of the central nervous system with an immune pathogenic mechanism provoking myelin lysis, including multiple sclerosis and optical neuritis. The term "meningitis, encephalitis and meningoencephalitis" refers to inflammatory diseases of the meninges and/or other structures of the central nervous system.
The term "inflammatory radiculopathies and peripheral neuropathies" refers to inflammatory diseases of the peripheral nervous system. The term "inflammatory cystitis" refers to inflammatory diseases of the bladder.
The term "benign prostatic hyperplasia" refers to non-malignant hyperthrophy and/or hyperplasia of the prostate.
The term "atopic dermatitis, eccema and urticaria" refers to allergic skin diseases with immune pathogenic mechanism with or without involvement of IgE. The term "psoriasis" refers to hyperkeratosic and erythematous skin reaction with an immune system pathogenic mechanism.
The term "rosacea" refers to common inflammatory condition of the skin characterised by erythema (flushing and redness) on the central face and across the cheeks, nose or forehead also can also less commonly affect the neck and chest. The term "allergic rhinitis" refers to intermittent (also called seasonal) or persistent (also called perennial) inflammatory nose mucosa diseases of immune hipersenivity pathogenic mechanism.
The term "sepsis, septic shock and multiorganic failure" refers to systemic inflammatory diseases mediated by an abnormal immune response to microbial agents and other ethio logical factors.
The term "sarcoidosis and amyloidosis" refers to idiopathic immunological diseases with organ and/or systemic involvement and no well defined ethiology in which an abnormal immune response can be observed.
The term "organ specific auto-immune diseases" refers to immune system- mediated lesion of organs with no defined ethio logical factors, including myastenia gravis, tyroiditis, hypophysitis, adrenalitis and others.
The term "organ transplantation" refers to prevention and treatment of rejection of transplanted cells, tissues and organs.
The term "infection and tumour-induced inflammation" refers to abnormal immune responses secondary to microbial agents or cancer stimuli.
The term "TNF-alpha dependent cellular degeneration, apoptosis or necrosis" refers to tissue degeneration or death induced by TNF-alpha. The term "graft versus host disease" refers to inflammatory immune responses induced by graft cells.
The term "caquexia" refers to systemic anorexia or malnutrition and weight loss induced by inflammatory or neoplasic diseases.
The term "atherosclerosis" refers to any hardening of arteries secondary to atheroma or accumulation in the arthery walls that is made up of inflammatory cells (mostly macrophage cells) and cell debris, that contain lipids.
The term "ischemic diseases" refers to lesion of organs secondary to reduced tissue oxigenation and/or blood flow including heart and cerebrovascular ischaemia.
The term "autocrine and paracrine pathological cell growth" refers to malignant or benign diseases with cell use of TNF-alpha as a cytokine regulating activation and proliferation factor for the cells.
Unless otherwise indicated, the compounds used in the invention are intended to include compounds that only differ in the presence of one or more isotopically enriched atoms. For example, compounds having the present structures except for the substitution of an hydrogen with deuterium or tritium, or the substitution of a carbon with a 13C- or
14C-enriched carbon or a 15N-enriched nitrogen are within the scope of this invention.
The term "pharmaceutically acceptable salts, solvates or prodrugs thereof relates to salts, solvates or prodrugs which, when administered to the recipient, can provide (directly or indirectly) a compound such as the one described herein. Nevertheless, it will be observed that pharmaceutically unacceptable salts are also within the scope of the invention because they can be useful for preparing pharmaceutically acceptable salts. Salts, prodrugs and derivatives can be prepared by means of methods known in the state of the art. "Pharmaceutically acceptable" preferably relates to molecular entities and compositions which are physiologically tolerable and do not typically cause an allergic reaction or a similar unfavorable reaction, such as gastric disorders, dizziness and the like, when administered to a human or animal. The term "pharmaceutically acceptable" means that it is approved by a regulatory agency of a federal or state government or is included in the US pharmacopoeia or another generally recognized pharmacopoeia for use in animals, and more particularly in humans.
For example, the pharmaceutically acceptable salts of the compounds described previously herein are synthesized from the previously described compound containing a basic or acidic unit by means of conventional chemical methods. Such salts are generally prepared, for example, by reacting the free acidic or basic forms of these compounds with a stoichiometric amount of the suitable base or acid in water or in an organic solvent or in a mixture of both. Non-aqueous media, such as ether, ethyl acetate, ethanol, isopropanol or acetonitrile, are generally preferred. Examples of acid addition salts include mineral acid addition salts such as hydrochloride, hydrobromide, hydroiodide, sulfate, nitrate, phosphate, for example, and organic acid addition salts such as acetate, maleate, fumarate, citrate, oxalate, succinate, tartrate, malate, mandelate, methanesulfonate and p-toluenesulfonate, for example. Examples of alkaline addition salts include inorganic salts such as sodium, potassium, calcium, ammonium, magnesium, aluminium and lithium, for example, and organic alkaline salts such as ethylenediamine, ethanolamine, N,N-dialkylenethanolamine, glucamine and basic amino acid salts for example.
The term "prodrug" is defined herein as a chemical compound which has undergone a chemical derivation such as a substitution or addition of an additional chemical group in order to change (for pharmaceutical use) some of its physical chemistry properties, such as solubility or bioavailability, for example an ester or ether derived from an active compound giving an active compound per se after the administration to a subject. Examples of well known methods for producing a prodrug from a given active compound are known by persons skilled in the art and can be found in Krogsgaard-Larsen et al, Textbook of Drug Design and Discovery, Taylor & Francis (April 2002), for example. According to this invention, the term "solvate" is understood to mean any form of a compound of the invention having another molecule (most likely a polar solvent) bound to it through a non-covalent bond. Examples of solvates include hydrates and alcoholates, for example methanolate.
Particularly preferred prodrugs are those increasing the bioavailability of the compounds of this invention when such compounds are administered to a patient (allowing an orally administered compound to be more quickly absorbed into the blood, for example) or those increasing the distribution of the original compound to a biological compartment (the brain or the lymphatic system, for example) with respect to the original species.
The compounds used in the invention may be in crystalline form, i.e. as polymorphs, either as free compounds or as solvates (hydrates, for example) and it is understood that both forms are within the scope of the present invention. Solvation methods are generally known in the art. Suitable solvates are pharmaceutically acceptable solvates. In a particular embodiment, the solvate is a hydrate.
Salts, solvates and prodrugs can be prepared by means of methods known in the state of the art. It will be observed that pharmaceutically unacceptable salts, solvates or prodrugs are also included within the scope of the invention because they can be useful in the preparation of pharmaceutically acceptable salts, solvates or prodrugs.
The compounds of formula (I) or their salts or solvates are preferably in pharmaceutically acceptable form or in substantially pure form. A pharmaceutically acceptable form is understood, inter alia, as having a pharmaceutically acceptable purity level, excluding normal pharmaceutical additives such as diluents and excipients, and without including any material considered to be toxic at normal dosage levels. The purity levels for the drug are preferably above 50%, more preferably above 70%, and still more preferably above 90%. In a preferred embodiment, it is above 95% of the compound of formula (I), or of its salts, solvates or prodrugs. The compounds used in the invention shown by the formula (I) described above can include enantiomers depending on the presence of chiral centers or isomers depending on the presence of multiple bonds (for example, Z, E). The individual isomers, enantiomers, diastereoisomers and mixtures thereof are within the scope of the present invention.
In a particular embodiment, for its use in imaging and pharmaco-imaging technologies, or their displacement as biomarkers in drug development, clinical trials, and individualized medicine, the compound of formula (I) may be labeled with fluorescent or luminiscent tags or flags, introducing the markers by any method known by a skilled person in the art.
In a particular embodiment of the invention, Ri is a substituted or unsubstituted Ci-C6 alkyl. Preferably Ri is methyl.
In another particular embodiment, R2 is hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl. Preferably, R2 is a substituted or unsubstituted cycloalkyl. More preferably, R2 is cyclopentyl. In a still another particular embodiment, R3 is methyl.
In another still more particular embodiment, the compound of formula (I) used in the present invention is selected from the following compounds:
Figure imgf000018_0001
Figure imgf000019_0001
Figure imgf000020_0001
or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
The compounds of formula (I) used in the present invention can be obtained by available synthetic procedures. For example, they can be prepared by a process which is summarised in the following scheme:
"COOCH3
Figure imgf000020_0003
Figure imgf000020_0002
Figure imgf000020_0004
This process firstly comprises an esterification reaction of the compound 4-R3- thiophenylacetic acid to render the methyl ester derivative. Said reaction can be carried out using a methylating agent, such as MeI, in the presence of a salt, such as NaHCO3, or using MeOH as methylating agent in the presence of an acidic medium.
In the following step, the methyl ester derivative, optionally without any purification, is oxidized at the sulphur atom using an oxidizing agent, for instance, oxone, thus obtaining the sulfone compound from the thioether group.
Subsequent halogenation with an agent such as NBS, leads to the formation of the halide at the α-position of the ester group. The cycloaddition of this compound with different thioamides under heating yields Ri -substituted 5-(4-R3-sulfonyl-phenyl)- thiazol-4-ol with a high degree of purity. Thioamides used for the cycloaddition are obtained from the amides corresponding to Lawesson reagent as described in J. Med. Chem (34) 2158-2165, 1991 and J. Org. Chem. (65), 13, 3973, 2000. Said thioamides include compounds wherein Ri is selected from hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl as defined above.
The introduction of the R2 radical through the hydro xyl group can be carried out by any method known by a skilled person to render the compound of formula (I) used in the present invention. In a particular embodiment, the hydroxyl group is reacted with an halide of formula R2-HaI, preferably R2-Br, to provide the compound of formula (I).
All reactants used in the mentioned reactions are commercially available.
In an additional aspect, the present invention provides a compound of formula (F):
Figure imgf000021_0001
(T) wherein:
Ri is selected from hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclic and R3 is a Ci-C6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
In a particular embodiment, Ri is a substituted or unsubstituted Ci-C6 alkyl.
Preferably, Ri is methyl.
In another particular embodiment, R3 is methyl. In another particular embodiment, the compound of formula (F) of the invention is selected from the following:
Figure imgf000022_0001
or a pharmaceutically acceptable salt, prodrug and/or solvate thereof. The present invention further provides pharmaceutical compositions comprising the novel compound of formula (F) of the present invention, or pharmaceutically acceptable salts, solvates or prodrugs thereof and at least one pharmaceutically acceptable carrier, adjuvant and/or vehicle, for the administration to a patient.
In a particular embodiment, for its administration in the prevention and/or treatment of acute or chronic inflammatory diseases, the compounds of formula (I), their pharmaceutically acceptable salts, prodrugs and/or solvates will be formulated in a suitable pharmaceutical composition, in the therapeutically effective amount, together with one or more pharmaceutically acceptable carriers, adjuvants, and/or vehicles.
The term "carrier, adjuvant and/or vehicle" relates to molecular entities or substances with which the active ingredient is administered. Such pharmaceutical carriers, adjuvants or vehicles can be sterile liquids, such as waters and oils, including those of petroleum or with an animal, plant or synthetic origin, such as peanut oil, soybean oil, mineral oil, sesame oil and the like, excipients, disintegrants, wetting agents or diluents. Suitable pharmaceutical carriers are described in "Remington's Pharmaceutical Sciences" by E.W. Martin.
The pharmaceutical compositions can be administered by any suitable method of administration, for example, oral, parenteral (for example, subcutaneous, intraperitoneal, intravenous, intramuscular, etc.), rectal administration, etc., typically orally due to the chronic nature of the disease to be treated.
In a particular embodiment, said pharmaceutical compositions can be in an oral administration pharmaceutical form, either in solid or liquid form. Illustrative examples of oral administration pharmaceutical forms include tablets, capsules, granulates, solutions, suspensions, etc., and can contain conventional excipients such as binders, diluents, disintegrants, lubricating agents, wetting agents, etc., and can be prepared by conventional methods. The pharmaceutical compositions can also be adapted for their parenteral administration, in the form of, for example, sterile, lyophilized products, suspensions or solutions in the suitable dosage form; in this case, said pharmaceutical compositions will include suitable excipients, such as buffers, surfactants, etc. In any case, the excipients will be chosen according to the selected administration pharmaceutical form. A review of the different pharmaceutical forms for administering drugs and of their preparation can be found in "Tratado de F armada Galέnica", by C. Fauli i Trillo, 10th Edition, 1993, Luzan 5, S.A. de Ediciones.
For its application in therapy, the compound of formula (I) will preferably be found in a pharmaceutically acceptable or substantially pure pharmaceutical form, i.e. the compound of formula (I) has a pharmaceutically acceptable purity level excluding pharmaceutically acceptable excipients and does not include material considered to be toxic at normal dosage levels. The purity levels for a compound of formula (I) are preferably greater than 50%, more preferably greater than 70%, more preferably greater than 90%. In a preferred embodiment, they are greater than 95%.
The therapeutically effective amount of the compound of formula (I) to be administered will generally depend, among other factors, on the individual to be treated, on the severity of the disease suffered by said individual, on the chosen method of administration, etc. For this reason, the doses mentioned in this invention must only be considered as guidelines for the person skilled in the art, and the latter must adjust the doses according to the aforementioned variables. Nevertheless, a compound of formula (I) can be administered once or more times a day, for example, 1, 2, 3 or 4 times a day, in a typical total daily amount comprised between 0.1 and 1000 mg/kg of body mass/day, preferably 10 mg/kg of body mass/day.
The compound of formula (I), its pharmaceutically acceptable salts, prodrugs and/or solvates, as well as the pharmaceutical compositions containing them can be used together with other additional drugs useful for treating acute and chronic inflammatory diseases. Said additional drugs can form part of the same pharmaceutical composition or alternatively, can be provided in the form of a separate composition for its simultaneous or non-simultaneous administration with the pharmaceutical composition comprising a compound of formula (I), or a pharmaceutically acceptable salt, prodrug or solvate thereof.
Within the scope of the present invention, the expression "acute and chronic inflammatory disease" relates to any disease, disorder or condition which results from the activation and pathogenic involvement of inflammatory/immune cells and inflammatory cytokine cascade under condition in which abnormal co-stimulation is a pathogenic mechanism. The predominant cells involved are inflammatory/immune cells such as monocytes, macrophages, APC, T, B and Natural Killer (NK) cells, plasma cells, granulocytes and mast cells, or combinations of the above cell subpopulations implicated in the diseases proposed for treatment. The term "cytokine" refers to a secreted protein that affects the functions of other cells, particularly as it relates to the modulation of interactions between cells of the immune system or cells involved in the inflammatory response. Said cytokines are TNF-alpha (tumor necrosis factor-α), IFN-gamma (inter feron-γ), the IL-8 (interleukin- 8) chemokine, and the regulatory cytokine IL-IO (interleukin-10). IL-IO production is induced by high TNF-alpha levels and promotes a negative feed-back upon TNF-alpha production, upon blockade of pro-inflammatory cytokine transcription.
In a particular aspect of the invention, the acute or chronic inflammatory disease is selected from acute and chronic seropositive or seronegative olygo arthritis and polyarthritis, spondiloarthropathies, glomerulonephritis, colagenopathies, tubulo- interstitial nephritis, metabolic syndrome, atherosclerosis, osteoarthritis, asthma, chronic obstructive pulmonary disease, interstitial lung disease, multiple sclerosis, demyelinating diseases, meningitis, encephalitis, meningoencephalitis, inflammatory radiculopathies and peripheral neuropathies, inflammatory bowel disease, cirrhosis, hepatitis, heart failure, ischemic disease, renal failure, inflammatory cystitis, benign prostatic hyperplasia, prostatitis, myocarditis, pericarditis, uveitis, atopic dermatitis, eccema, urticaria, psoriasis, rosacea, allergic rhinitis, sepsis, septic shock, multiorganic failure, systemic autoimmune diseases such as systemic lupus erythematosus, vasculitis, dermatomyositis, amyloidosis or sarcoidosis, organ specific autoimmune diseases such as myasthenia gravis, thyroiditis or insulinitis, organ transplantation, infectious ant tumor induced inflammation, TNF-alpha dependent cellular degeneration, necrosis, apoptosis, graft versus host disease, cachexia and autocrine and paracrine pathological cell growth.
In a preferred embodiment, the acute or chronic inflammatory disease is seropositive or seronegative chronic polyarthritis, more preferably is rheumatoid arthritis.
Another aspect of the present invention is a method for treating an acute or chronic inflammatory disease, which comprises administering to a patient who needs such treatment a therapeutically effective amount of a compound of formula (I) as defined above or a pharmaceutical composition thereof.
The term "treatment" or "treat" in the context of this specification means the administration of a compound with a formulation according to the invention for preventing, alleviating or eliminating the disease or one or more symptoms associated to said disease. "Treatment" also includes preventing, alleviating or eliminating the physiological sequel of the disease.
The term "alleviate" in the context of this invention is understood to mean any improvement of the situation of the treated patient- both subjectively (the feelings of or about the patient) and objectively (measured parameters).
Another aspect of the invention refers to the use of a compound of formula (I) as defined above as an imaging biomarker in imaging and pharmaco -imaging technologies, for finding immunological lesions, target cells and target molecules. The pharmaco-imaging technology extends the scope of biomarkers obtained by the rapidly growing combination of adequate preclinical (molecular, cellular, organ and whole animal tracking and study of proof of concept and mechanisms, efficacy assessment, etc) and clinical (human medical) in vivo imaging technologies, to those valuable information data generated by compounds described herein and used as medicines.
The present invention is additionally explained below by means of examples. This explanation must by no means be interpreted as a limitation of the scope of the invention as it is defined in the claims.
Examples Synthesis
Example 1. Synthesis of (4-methylthiophenyD-acetic acid methyl ester
Figure imgf000026_0001
1.82 g (10 mmol) of the 4-methylthiophenylacetic acid were dissolved in 30 mL of DMF and 1.34 g (16 mmol) of NaHCCh are then added; the agitation mixture is stirred for 15min approx. Next, 1.9 mL of ICH3 are added while keeping agitation at room temperature for 24h. Once this time elapsed the mixture is poured on water/ice. As no precipitation occurs ether is added and extracted. The organic phase is washed with water and after drying on sodium sulfate anhydride, the organic phase is concentrated in a rotary evaporator getting 1.92 g (9.7 mmol, 97% yield) of colorless oil which spectroscopic data confirm the expected structure. This product will be used in the next step of the synthesis process without purification as it provides a single stain in TLC (eluting dichloromethane/methanol 9/1). RMN 1H (CDCl3): 7.2 (s, 4H) 3.7 (s, 3H) 3.5 (s, 2H) 2.4 (s, 3H CH3S) RMN 13C (CDCl3): 171.5 136.9 130.4 129.4 126.4 51.6 40.2 15.5
Example 2. Synthesis of (4-methylsulfonyl-phenyl)-acetic acid methyl ester
Figure imgf000027_0001
A solution of oxone 30.7 g (50 mmol) was added drop by drop in 80 mL of water to a solution of 3.4 g (17.3 mmol) of the compound obtained in example 1 in 100 mL of methanol keeping the reaction in a water/ice bath. Once added, agitation continues for 5h, allowing temperature to get room level. Then, part of the solvent is concentrated at reduced pressure and the precipitated solid is filtered washing with water repeatedly. After drying, this solid weighs 3 g. Waters from filtering are extracted with dichloromethane, the organic phase is washed with water, dried on sodium sulfate anhydride and concentrated in a rotary evaporator obtaining 1 more g of product than expected, yield 4 g (17 mmol, 100% yield). This solid melts with decomposition at 570C and its purity is 99% by HPLC. Spectroscopic data confirm the expected structure:
RMN 1H (CDCl3): 7.9 (d, 2H), 7.5 (d, 2H), 3.7 (s,s 3+2H), 3.1 (s, 3H)
RMN 13C (CDCl3): 170.80 140.13 139 130.33 127.63 52.31 44.49 40.82
Example 3. Synthesis of bromo-(4-methylsulfonyl-phenyl)-acetic acid methyl ester
Figure imgf000028_0001
20 g (87.62 mmol) of the ester were dissolved in 300 mL of carbon tetrachloride; 19 g (105 mmol) of N-bromosuccinimide, 2 g (12.18 mmol) of azobisisobutyronitrile and 0.1 mL of bromine were added in portions. The reaction mixture was heated at 8O0C for 3 hours and, then cooled, filtered off and washed with dichloromethane. The filtrate was washed with water and then with brine. The solution was dried over anhydrous sodium sulfate and concentrated under vacuum to yield 28 g of an oil, which was purified by flash chromatography using heptane/ethyl acetate (1/1) as eluent. Concentration of the purer fractions yielded 19.63 g (72.94% of yield) of the bromo derivative compound.
mp: 81.8 - 83.30C
NMR 1H (CDCl3), δ: 7.9 (d, 2 H), 7.75 (d, 2H), 5.4 (s, IH), 3.8 (s, 3H), 3,1 (s, 3H). NMR 13C(CDCl3), δ,: 168.0 ( C); 141.6 ( C); 141.1 ( C); 129.8 (CH); 127.8 (CH); 53.7 (CH); 44.7 (CH3) and 44.2 (CH3) ppm.
Example 4. Synthesis of 2-methyl-5-(4-methylsulfonyl-phenyl)-thiazol-4-ol
Figure imgf000028_0002
16.7 g (54.3 mmol) of the ester obtained in example 3 were dissolved in 400 mL of toluene, 19 mL of pyridine and 4.08 g (54.34 mmol) of the thioamide were then added. The reaction mixture is heated at 8O0C (bath temperature) with agitation for 2h. Next, the mixture was left to cool and the precipitate solid was filtered, washed with water (2 x 50 mL) and then with ether (2 x 30 mL). The product was dried under vacuum to yield 7 g (26 mmol, 47.86% yield) of a cream solid melting at 216-2260C.
Spectroscopic data confirm the structure of the expected product. RMN 1H (d6DMSO) δ: 11.8 (s, IH) 7.8 (m, 4H) 3.1 (s, 3H) 2.6 (s, 3H) ppm
RMN 13C (d6DMSO): 162.9 (C); 159.4 (C); 146.2 (C); 143.0 (C); 128.0 (CH); 126.1 (CH); 104.4 (C); 44.2 (CH3); 19.9 (CH3) ppm.
Example 5. Synthesis of 4-cyclopentyloxy-5-(4-methylsulfonyl-phenyl)-2-methyl- thiazole.
Figure imgf000029_0001
7.0 g (26 mmol) of the hydro xythiazo Ie obtained in example 4 and 8.8 g (63.67 mmol) of potassium carbonate were dissolved in 200 mL of DMF. Cyclopentylbromide, 14 mL (130 mmol), were added dropwise. The reaction mixture was heated at 8O0C for 3 hours and then cooled, poured over a mixture of ice/water and extracted with ethyl acetate. The organic phase was washed with water (3 X 100 mL), dried over anhydrous sodium sulfate and concentrated to give 12 g of a crude material which crystallized from heptane/ether (1/1). Purification of the product by flash chromatography using heptane/ethyl acetate (2/1) as eluent yielded 6.7 g (19.85 mmol, 76.39% of yield) of compound 12.
mp: 124.6 - 125.20C
NMR 1H (CDCl3), δ: 7.9 (dd, 4H), 5.4, (m, IH), 3.0, (s, 3H), 2.6, (s, 3H), 1.7-2.0 (m, 8H) ppm NMR 13C(CDCl3), δ: 162.6 (C); 159.5 (C); 138.3 (C); 137.1 (C); 128.1 (CH); 126.8 (CH); 109.1 (C); 83.7 (CH); 45.0 (CH3); 33.5 (CH2); 24.1 (CH2); 20.4 (CH3) ppm
Biological assays
Material and methods
1. Subjects The study was performed on heparinized peripheral blood obtained by venopunction from healthy volunteers and from patients with rheumatoid arthritis.
Healthy volunteers were blood-donors under routine control within the hospital practice. Patients with rheumatoid arthritis included in this study complied with the diagnosis criteria of the American College of Rheumatology and exhibited a clinically active disease by the time of the inclusion visit having been treated for at least 6 months with 20mg/week oral Methrotexate. The degree of disease activity was defined as follows: a) DAS28 > 3,2 and/or b) 6 or more swollen articulations and 6 or more painful articulations. As exclusion criteria were considered the following: a) to suffer from active infectious diseases in the inclusion visit; b) to suffer from oncological diseases prior the inclusion; 3) to suffer from another systemic or organ specific auto-immune disease which had not entered into a complete remission at least one year prior the inclusion visit; d) to suffer from a severe renal, cardiac or hepatic condition not related with the changes at those levels induced by the rheumatoid arthritis as main disease; e) to suffer a severe deterioration of the general status due to a condition not related with the main disease; f) to have received treatment with corticosteroids, immunosuppresors, cytostatic or any other drugs with known activity on the immune system during the year prior the inclusion visit with the exception of the indicated doses of Methrotexate; 7) to be pregnant or within the puerperium in the inclusion visit.
The study was approved by the Investigational Committee of the Alcala University, Madrid, Spain.
2. Materials - Tissue culture plates, 96 wells flat bottom with low evaporation lid, 353073 Falcon, Becton Dickinson Labware, Franlklin Lakes, 07417-1886, NJ, USA).
- Non sterile plates, 96 wells V bottom (Greiner, Soria Greiner, Madrid, Espaiia).
- Disposable Pipettes Pasteur (Brand, Alemania).
- Adjustable volume Pipettes Pipetman P de 20, 200, 1000 and 5000 μl (Gilson, Francia). - Eppendorf multipipette 4780 (Hamburg, Germany).
- Sterile tips Eppendorf (Hamburg, Germany).
- Virgin propilen sterile tips (Daslab, Madrid, Spain).
- Sterile plastic tubes 5 and 10 ml (Daslab, Madrid, Spain). - Sterile centrifuge tubes 15 and 50 ml (BD Falcon, Franklin Lakes, USA).
- Cytometer polyestirene tubes 5 ml (BD Falcon, Franklin Lakes, USA).
- Blood extraction tubes with heparin 10 ml (Venojet, Terumo Europe, Belgium)
- Plasma extraction tubes 10 ml (BD Vacutainer, Plymouth, UK)
- Pipet filler, Pipetboy plus (Flow Lab., Germany). - Sterile filtres 22 μm Millex-GS (Millipore, Molshein, France).
- Crystal slide covers (Hirschman, Germany).
- Count chamber Neubauer (Saaringia, Germany).
- Vertical laminar flux chamber Herasafe HS 12 (Heraeus, Germany).
- Cell culture stove with CO2 regulation Heracell 150 (Heraeus, Germany). - Refrigerated centrifuge Beckman. Multifuge 3SR (Heraeus, Germany).
- Freezer -7O0C (Selecta, Tarrasa, Spain).
- Mycroscope Olympus CHS-2 (Olympus, Tokyo, Japan).
- Flow Cytometer FACScalibur (Becton Dickinson, Mountain View USA), with software and analyser BD Cellquest Pro v. 5.5.1. - BD FACS Arrray Bioanalyser.
- Enzyme-immunoanalysis reader (Titertek Multiscan Plus, Flow laboratories).
- Radioactivity beta counter Beckman
3. Reagents used in the separation and identification of cell subsets - Simple Chloride Saline (SSF) Apiroserum (Ibys, Madrid, Spain).
- Lymphoprep (Ficoll-Hypaque, Nyegaard Co, Oslo, Norway). - Blue Trypan (Flucke AG., Buchs SG., Germany).
- PBS FACS FLOW (Becton Dickinson).
- HEPES buffer (Reactivos de Sigma y Panreac)
- Methyl- H tymydine (3[H]-T). Specific activity 60 Ci/mmol (American Radiochemicals, ITISA, Madrid, Spain).
- Monoclonal antibodies used in the immunofluorescence and flux cytometry studies: Table 1
Table 1. Monoclonal antibodies used in the study:
CD* Ac Mo Cell subset Subclass Fluorochrome
62L SKl 1 Leucocytes. L-Selectin IgG2a Phycoerythrine (PE)
* Defined in the "7th Workshop on Human Leucocyte Differentiation Antigens".
4. Reagents used in the cell cultures
- Complete Medium made of RPMI- 1640 (Cambrex BioSciences B4800 Verviers, Belgium) supplemented with 1 % L-Glutamine 200 mM y 25 mM Hepes (Flow Lab., Irvine, California, USA).
- Phoetal bovine serum (FCS) (Gibco, Grand Island, NY, USA).
- Culture medium: complete medium was used by adding 10 % FCS. Complement was eliminated from all serum by heating to 570C during 45 minutes.
- Phytohaemaglutinin M (PHA) (Sigma Ref #L-8902, Lot#115K4132, Sigma, Madrid, Spain).
- LPS (E. co Ii 0111 : B4 strain, InvivoGene, San Diego CA92121, USA).
- Antibiotic mixture. A mixture of Sodium Ampycilline 10 mg/ml (Britapen, Beecham A., Toledo, Spain), Gentamycin sulphate 1.6 mg/ml (Tamadit Lab., Dr. Esteve SA., Madrid, Spain) and Amphotherycine B 0.5 μg/ml (Fungizona, Squibb, Esplugues, Barcelona, Spain) was added to the culture medium. - Anti-CD3 monoclonal antibody (Orthoclone OKT3, Orthopharmaceutical Corporation, Raritan, NJ, USA).
- Anti-CD28 monoclonal antibody (Clon 15E8, Menarini, Madrid, Spain).
5. Obtention of biological samples a) Venous blood: Mononuclear cells were obtained from venous blood as collected by antecubital venous punction. Fifty ml of blood were extracted and stored in lithium heparin tubes (Venojet), further diluted with saline 1/1 (vol/vol) being all performed under sterile conditions. b) Human Cell subsets harvesting. For isolating PBMC, the remaining blood components were separated by a density gradient on Ficoll. This method is based on the differences on density of blood cells. In a 50 ml centrifuge tube containing the diluted and heparinized blood, 15 ml Ficoll-Hipaque (density 1.077 g/ml) was carefully placed on. After 45 minutes centrifugation (400xg), three strati were obtained (erythrocytes, Ficoll and plasma), separated by two interfaces: PBMC are contained in the one located between the diluted plasma and the Ficoll. It can be collected by aspirating with a Pasteur pipette. Cells so obtained are re-suspended in SSF and centrifugated (300xg during 10 minutes); supernatant is thrown out (washing out process) and the cellular pellet is re-suspended in RPMI 1640 medium with 10 % of PBS.
6. Count and viability study
In all cell suspensions the cell concentration and viabilities were determined with a 0.1 % dilution of Blue Trypan and Neubauer chamber my croscope counting. The percentage of living cells was established by the ability of dyeing exclusion. The experiment only continued when the cell viability was above 95 %.
7. Serum cytokines quantification by ELISA
In order to quantify the serum cytokines concentration, the extracted blood was stored in tubes both with and without anti-coagulant (collected by antecubital venopunction and arterial catheter, respectively). Blood was allowed to coagulate at room temperature in the laboratory, further separating the serum by centrifugation (600xg during 20 minutes). Supernatant were collected, filtered, divided in aliquotes and stored at -7O0C. Concentration assays for different cytokines were performed by using the commercial kits described in Table 2.
Table 2.- Commercial ELISA kits used in this study
Cytokine Quantification PM Company sensibility in (KDa) supernatants (pg/ml) TNF-alpha 3.83 pg/ml 17 Bender
Supernatants were unfrozen up to the room temperature and faced against the respective anti-cytokine by fixing them in the plate bottom and incubating them during a variable time. Subsequently, wash-outs were carried out and the substances recommended by the corresponding company were added in order to allow a colorimetric reaction, in a proportional manner to the amount of cytokine present in the supernatant. The results were assessed with the enzymo-immunoanalysis reader Multititer Plus (Tiertek Multiscan Plus, Flow Laboratories). These results were compared with a standard curve obtained from known concentrations of each cytokine as provided by the company.
The analysis of the standard curves and subsequent interpolation was performed with the software Delta Soft II version 4.1 (Biometallics, Inc.) in an Apple Macintosh computer. Cytokine concentrations were converted to molar in order to calculate the molecular ratios of each case and the number of soluble molecules.
8. Immuno-phenotype assays
Direct immuno-fluorescence techniques of one colour with monoclonal antibodies phycoerythrin-labeled (PE) was used. PE is a fluorescent substance excitable with a 488 nm laser, which emits at 570 nm, and it is detectable and easily distinguishable by a flow cytometer. By using the antibody described in Table 1, a direct labelling was performed: PBMC labelling: the process consisted in a labelling using 96 well V bottom plates. In each well, 5 x 104 cells are located, and afterwards centrifugated at 400 xg during 5 minutes. After washing-out, cells are re-suspended and 5 μl of the corresponding monoclonal antibody are added. Cells are again re-suspended and the plate is incubated in darkness, during 20 minutes, at 40C. Subsequently, 150 μl PBS are added and two washouts are performed. Finally, it is re-suspended in 150 μl PBS and collected in a cytometer tube, adding PBS up to a final volume of 0.3 ml.
For the counting, a FACSCalibur flow cytometer equipped with argon laser tuned at 488 nm was used in order to induce phycoerythrin fluorescence. The equipment, apart from the fluorescence channels, also provided information about the size (FSC) and cellular complexity (SSC).
As negative controls, the study cells with no labelling and other irrelevant labelled with monoclonal antibodies of equal isotypes than the ones used in the study (IgGl-FITC, PE y TC, IgG2a FITC, PE, TC), were used.
9. Cellular cultures and functional studies
General conditions of the culture: all cellular cultures were performed under sterile conditions within a vertical laminar flux chamber, using either sterile disposable materials or sterilized by ethylene oxide or sterilizer apparatus. Cultures were kept in a stove at 370C under 5 % CO2 and 95% relative humidity.
10. Proliferation study with 3 [H] -Thymidine
Faced against a mitogen stimulation, lymphocytes suffer a blastogenesis and cellular differentiation process. The method used to quantify the cellular proliferation was the assay of the incorporation of 3 [H] -Thymidine to the DNA de novo synthesized, and the emission of betha-radiation from the cellular cultures dried extracts (to which the tritiated base was added) was detected before its ending and harvesting. In the different experiments performed to study the proliferation, the purified cellular preparations were incubated in 96 microwells plain bottom plates at concentrations of 5 x 104 cells/well (200 μl final volume), in the presence of different concentrations of various mitogens with triplicate repetitions and along 4 days of culture. The response to a specific stimuli depended on the density and cell type studied, as well as of the culture time and of the mitogenic agent concentration.
Twenty to twenty four hours before finishing the cellular culture, 1 microCi 3 [H] -Thymidine was added to each well; cultures were harvested by aspiration through a glass filter by using a specific culture harvester.
DNA synthesis was expressed in counts per minute (c.p.m.). Each assay was performed in triplicate, rejecting those data with a variability higher than 10 % in the mean of the triplicate as they might indicate a technical error or a contamination of the culture. Cultures were performed with a constant amount of cells per well as well as with a constant volume of 200 μl. All mitogens and cytokines were first tested by carrying out dose-response curves and time-response.
11. Assays for analytical determination by quantitative multiparametric flow citometry (BD™ Cytometric Bead Array o CBA) CBA protocol was followed according to the manufacturer's instructions. The election of microparticles was performed following the summary of Figure 1. Those which showed a little risk of spectral overlapping were finally selected.
The catalogue number and batch of each reagent used for this experimental development is shown in Tables 3 and 4. The acquisition on samples was performed with the BD FACS Array Bioanalyser System (FACSArray, Becton Dickinson, San
Jose, CA, USA) and the analysis of the results was completed with the software FCAP
Array (Becton Dickinson) in a PC computer.
Briefly, the experimental protocol consisted of a plate pre-washing out with Wash Buffer. After decantation, the mixture of capture microparticles was re-suspended in the vortex. Standards and samples were added in the adequate dilution. After permanent stirring incubation during 1 h, the PE detection reagent was added and incubated again during 2h at room temperature. After a washing-out, the acquisition was performed in the flow cytometer. Table 3. -Kit CBA Human Soluble Protein Multiplex Flex Set System.
N0
Reagent Batch catalogue
Master buffer kit 500 test 558265 95098
51-
Assay Diluent 86192 90003992
51-
Capture Bead Diluent 90262 90003804
51-
Detection Reagent Diluent 95811 90003993
51-
Wash Buffer 85964 90003798
51-
Instrument Setup Bead Al 87987 90003855
51-
Instrument Setup Bead A9 95933 90003858
51-
Instrument Setup Bead Fl 89231 90003851
51-
Instrument Setup Bead F9 94229 90003854
51-
PE Instrument Setup Bead Fl 94498 9005038
51-
PE Positive Control Detector 92154 9005065
CBA Flex Set Kits Sensitivity
IL-8 (A9) 558277 85109 1.2 pg/ml
IL-IO (B7) 558274 97196 0.13 pg/ml
TNF-α (D9) 558273 85106 0.7 pg/ml
IFN-γ (E7) 558269 81562 1.8 pg/ml Table 4. -Batches of reagents included in the design of the Kit CBA Flex Set.
Capture Fluorescent reagent
Reagent Standard microparticles (PE)
IL-8 (A9) 84854 87670 77948
IL-IO (B7) 70333 96280 95934
TNF-α (D9) 65908 87667 77294
IFN-γ (E7) 80390 87664 77136
STATISTICAL ANALYSIS Results of the experimental tests were presented as means and standard and estimate errors of the mean, according to the type of distribution.
For the statistical analysis, the nature of the distributions was firstly analysed by using the contrast of normality of Shapiro-Whilk. The non- parametric contrast of Mann- Whitney U was used to establish comparisons. In all cases, lower than 5 % signification levels were valued (p< 0.05).
The statistical analysis was performed with the software S P S S 1 1 .0 ( S P S S Inc . Headquarters, 233 S. Wacker Drive, 1 lth floor. Chicago, Illinois 60606)
Results of the studies on the immune modulator effects of compound 12
Immune modulator effects of compound 12 on the production of TNF-alpha, IFN- gamma and other cytokines by the peripheral blood mononuclear cells (PBMC) on healthy volunteers and patients with rheumatoid arthritis.
Example 6. Effects of compound 12 on TNF-alpha production
Effects of compound 12 on TNF-alpha production by PBMC of healthy volunteers in the presence or in the absence of LPS were first investigated. PBMC (5 x 104 cells/well, 200 μl) from 10 healthy volunteers were cultured in parallel in duplicate in tissue culture plates, 96 well, flat-bottom with low evaporation lid (353072 Falcon, Becton Dickinson labware, Franklin Lakes, USA, 07417-1886 NJ) in complete medium (RPMI-1640 with glutamine Cat BE-12-70F, Cambrex Biosciences, B4880 Verviers, Belgium), supplemented with phoetal bovine serum (origin USA, Gibco ref. 26140-079) and a solvent concentration of 10"6 M alone or supplemented with 10"6 M or 10"7 M of compound 12, in the presence and in the absence of LPS (lOmicrog/ml; E. coli LPS 0111 :B4 strain InvivoGene, San Diego CA92121 USA) during 24 hours. Supernatant of cultures were frozen at -2O0C and the concentration of TNF-alpha was quantified with ELISA species-specific (enzyme- linked immunosorbent assay for quantitative detection of tumour necrosis factor- alpha: human TNF-alpha ELISA BM S223/4TEUCE, Bender Med System Inc, Burlinghane CA 94010). Figure 2 shows that the presence of compound 12 in the culture, at concentrations of
10"6 M and 10"7 M diminished in a statistically significant manner the TNF-alpha concentration as quantified in the supernatant of the culture of LPS-stimulated PBMC (p<0.05). Moreover, compound 12, at 10"6 M also lowered the spontaneous TNF-alpha production by PBMC. Table 5. -TNF-alpha production by healthy volunteers. Results are indicated as median ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000039_0001
Immune modulator effects of compound 12 were further characterised on the production of a cytokine panel by PBMC either after monocyte stimulation with either LPS or lymphocyte activation with a combination of monoclonal antibodies anti-CD3 and anti-CD28. This study was performed in the presence or absence of titrated doses of compound 12 in cultures of PBMC obtained from healthy volunteers and patients with rheumatoid arthritis.
PBMC (5 x 104 cells/well) from 13 healthy volunteers were cultured in duplicate in 200 μl of complete medium supplemented with the highest solvent concentration (10~6 M), or 10"6 M and 10"7 M compound 12 and in the presence and in the absence of LPS (lOμg/ml) during 24 hours. Supernatant of cultures were frozen at -2O0C and quantification was carried out by BD FACS Array Bioanayliser (BD Biosciences Cat No. 340128, San Diego CA 92121) by using specific reagents for the simultaneous assay of the indicated cytokines concentration (CBA Flex Multiplex Set (BD™ Cytometric Bead Array, CBA: IL-8, IL-IO, TNF-alpha and IFN-gamma Becton Dickinson Biosciences Pharmingen, San Diego CA 92121).
The presence of compound 12 in the culture, at concentrations 10"6 M and 10"7 M diminished TNF-alpha production by the PBMC of healthy volunteers stimulated with LPS in a statistically significant manner (p<0.05) (Figure 3). On the contrary, neither TNF-alpha secretion by PBMC stimulated with monoclonal antibodies anti-CD3 and anti-CD28 nor spontaneous one (as observed in the absence of exogenous stimuli) was modified by compound 12.
Table 6. -TNF-alpha production by healthy volunteers. Results are indicated as mean ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000040_0001
In another experiment, PBMC (5 x 104 cells per well) from 7 patients with rheumatoid arthritis were cultured in duplicate in 200 μl of complete medium supplemented with the highest solvent (10~6 M), and 10"6 M, 10"7 M and 10"8 M compound 12 and in the presence and absence of either LPS (10 μg/ml), or anti-CD3 (12.5ng/ml) (Orthoclone OKT3, Ortho Pharmaceutical Corporation, Raritan NJ, USA) + anti-CD28 (l/3xlθ5) (Clon 15E8, Menarini, Madrid, Spain), during 24 hours. Culture supernatants were frozen at -2O0C and the concentration of TNF-alpha quantified by BD FACS Array Bioanalyser by using CBA Flex Set (Becton Dickinson), specific for determining the concentration of that cytokine, following the manufacturer instructions. In LPS-stimulated PBMC from patients with rheumatoid arthritis, the production of TNF-alpha was significantly inhibited by compound 12 at a concentration of 10~6 M (p<0.05) (Figure 4). The presence of compound 12 in the culture neither inhibited the spontaneous TNF-alpha production nor the one obtained after stimulation with monoclonal antibodies anti-CD3 and anti-CD28 in PBMC from patients with rheumatoid arthritis.
Table 7. -TNF-alpha production by patients with rheumatoid arthritis. Results are indicated as mean ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000041_0001
Example 7. Effects of compound 12 on the production of IFN-gamma.
PBMC (5 x 104 cells per well) from 13 healthy volunteers were cultured in duplicate in 200 μl of complete medium supplemented with the highest solvent concentration (10" 6 M), and 10"6 M, 10"7 M and 10"8 M of compound 12 in the presence or absence, either of LPS (10 μg/ml), or anti-CD3 (12.5 ng/ml) + anti-CD28 (l/3xlθ5), during 24 hours. Culture supernatants were frozen at -2O0C and the concentration of IFN-gamma was quantified by BD FACS Array Bioanalyser by using CBA Flex Set (Becton Dickinson), specific to determine the concentration of IFN-gamma, following the manufacturer instructions.
Compound 12, at a concentration of 10"6 M significantly inhibited the production of IFN-gamma by PBMC from healthy volunteers either LPS-stimulated or stimulated with monoclonal antibodies anti-CD3 and anti-CD28 (p<0.05) (Figure 5).
Table 8. -IFN-gamma production by healthy volunteers. Results are indicated as mean ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000042_0001
The spontaneous secretion of IFN-gamma by PBMC from healthy volunteers was not modified by compound 12.
PBMC (5 x 104 cells/well) from 8 patients with rheumatoid arthritis were cultured in duplicate 200 μl of complete medium supplement with the highest solvent concentration 0 (10~6 M), and 10"6 M, 10"7 M and 10"8 M of compound 12, in the presence and absence either of LPS (10 μg/ml), or anti-CD3 (12.5 ng/ml) + anti-CD28 (l/3xlθ5), during 24 hours. Culture supernatants were frozen at -2O0C and IFN-gamma concentration was assessed by BD FACS Array Bioanalyser by using CBA Flex Set, specific to determine IFN-gamma concentration, following the manufacturer instructions. 5 The presence of compound 12, at concentrations of 10"6 M, 10"7 M and 10"8 M, significantly lowered the production of IFN-gamma by PBMC from patients with rheumatoid arthritis when induced by the stimulation with monoclonal antibodies anti- CD3 and anti-CD28 (p<0.05) (Figure 6). Compound 12 modified neither the spontaneous IFN-gamma secretion nor the LPS-induced by the PBMC from healthy 0 volunteers.
Table 9. -TNF-alpha production by patients with rheumatoid arthritis. Results are indicated as mean ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each 5 experimental condition) included in parenthesis.
0
Figure imgf000043_0001
Example 8. Effects of compound 12 on Interleukin 8 (IL-8) production. The effect of compound 12 on the IL-8 production by the PBMC from healthy volunteers was further investigated, both in the presence and absence of LPS stimuli and monoclonal antibodies anti-CD3 and anti-CD28. PBMC (5 x 104 cells/well) from 13 healthy volunteers were cultured in duplicate in 200 μl of complete medium supplemented with the highest solvent concentration (10~6 M), and 10"6 M, 10"7 M and 10"8 M of compound 12, in the presence and absence of either LPS (10 μg/ml) or anti- CD3 (12.5 ng/ml) + anti-CD28 (l/3xlθ5), during 24 hours. Culture supernatants were frozen at -2O0C and IL-8 concentration was quantified by BD FACS Array Bioanalyser by using CBA Flex Set, specific to determine the IL-8 concentration, following the manufacturer instructions. At concentrations of 10 6 M, 10"7 M and 10"8, the compound 12 significantly inhibited the spontaneous production of IL-8 (p< 0.05) (Figure 7). A significant inhibition of the IL-8 production induced by monoclonal antibodies anti-CD3 and anti- CD28 was observed with compound 12 at concentrations of 10"7 and 10"8 M. Nevertheless, no effects were observed on the IL-8 production under the LPS stimulation of PBMC.
Table 10. -IL-8 production by healthy volunteers. Results are indicated as mean ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000044_0001
The effect on IL-8 production by PBMC from patients with rheumatoid arthritis was also studied. PBMC (5 x 104 cells per well) from 8 patients with rheumatoid arthritis 5 were cultured in duplicate in 200 μl of complete medium supplemented with the highest solvent concentration (10~6 M), and 10"6 M, 10"7 M and 10"8 M of compound 12, in the presence and in the absence of either LPS (10 μg/ml) or anti-CD3 (12.5 ng/ml) + anti-CD28 (l/3xlθ5), during 24 hours. Culture supernatants were frozen at -2O0C and IL-8 concentration was quantified by BD FACS Array Bioanalyser by using CBA Flex
10 Set, specific to determine IL-8 concentration, following the manufacturer instructions.
The presence of compound 12 in the culture, at concentrations of 10"6 M and 10"8 M, significantly modulated the LPS-induced production of IL-8 in PBMC from patients with rheumatoid arthritis whereas neither modified the spontaneous IL-8 production nor that induced by the combination of monoclonal antibodies anti-CD3 and anti-CD28
15 (Figure 8). Altogether the results indicate that IL-8 modulation by compound 12 might interestingly show distinct modulation patterns under distinct conditions of health and defined diseases.
Table 11. -IL-8 production by patients with rheumatoid arthritis. Results are indicated as mean ± 0 standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000044_0002
Example 9. Effects of compound 12 on Interleukin 10 (IL-IO) production. The effects of compound 12 on IL-IO production by the PBMC from healthy volunteers and patients with rheumatoid arthritis were investigated in the presence and absence of LPS stimulation and with the combination of monoclonal antibodies anti- CD3 and anti-CD28. PBMC (5 x 104 cells per well) from 13 healthy volunteers were cultured in duplicate 200 μl of complete medium supplemented with the highest solvent concentration (10~6 M), and 10"6 M, 10"7 M and 10"8 M of compound 12, in the presence and absence of either LPS (10 μg/ml) or anti-CD3 (12.5 ng/ml), + anti-CD28 (l/3xlθ5), during 24 hours.
On the other hand, PBMC (5 x 104 cells per well) from 8 patients with rheumatoid arthritis were cultured in duplicate in 200 μl of complete medium supplemented with the highest solvent concentration (10~6 M), and 10"6 M, 10"7 M and 10"8 M of compound 12 in the presence and absence of either LPS (10 μg/ml) or anti-CD3 (12.5 ng/ml), + anti-CD28 (l/3xlθ5), during 24 hours. Culture supernatants were frozen at -2O0C and IL-10 concentration was assayed by BD FACS Array Bioanalyser by using CBA Flex Set, specific to determine IL-10 concentration, following the manufacturer instructions. Compound 12 showed no effects on the IL-10 production by PBMC from healthy volunteers in the presence and in the absence of both studied stimuli (Figures 9). However, the presence of compound 12 in the culture, at a concentration of 10"8, significantly upmodulated IL-10 production after stimulation of PBMC from patients with rheumatoid arthritis with LPS (p < 0.05). Compound 12 induced no significant effects neither on the spontaneous production of IL-10 nor after the stimulation with monoclonal antibodies anti-CD3 and anti-CD28 by PBMC from patients with rheumatoid arthritis (Figure 10).
Table 12. -IL-10 production by healthy volunteers. Results are indicated as mean ± standard error values of the secreted cytokine. The corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000046_0001
Table 13. -IL-10 production by patients with rheumatoid arthritis. Results are indicated as mean ± standard error values of the secreted cytokine. Statistically significant results are indicated in bold, with their corresponding p values (data with respect to the vehicle for each experimental condition) included in parenthesis.
Figure imgf000046_0002
Other effects of compound 12 on immune system cells.
Example 10. Effect of compound 12 on the proliferative response of PBMC.
The effect of compound 12 on the proliferative response of PBMC from healthy volunteers (n=8) was investigated in the presence and in the absence of stimulation with phytohaemaglutinin (PHA) 10 μg/ml; PHA 2 μg/ml plus exogenous IL-2 supplementation (25 IU/ml), and a combination of monoclonal antibodies anti-CD3 (12.5 ng/ml) and anti-CD28 (1 :320.000).
PBMC was cultured during 4 days (50.000 cells per well) at 370C and 5 % CO2 atmosphere (Cell incubator HERA Cell 150, Thermoscientifϊc, Thermoelectron, 63505 Lagenselbold, GE) in complete culture medium. Culture stimulation conditions were the absence or presence or phytohaemaglutinin (PHA Sigma Ref #L-8902, Madrid, Spain), 10 μg/ml; PHA 2 μg/ml with exogenous IL-2 supplementation (25 IU/ml, Human recombinant IL-2, Macrolin, Chiron Iberica, batch #SA753228/4, Madrid, Spain) and monoclonal antibodies anti-CD3 (12.5 ng/ml) + anti-CD28 (1 :320.000). Methyl-3H- Thymidine was added (American Radiochemical 60 Ci/mmol methyl-3H-Thymidine, ITISA, Madrid, Spain) during the last 8 hours of culture. Cells were harvested in glass fibre membranes and embebed in scintillation medium (1450-441 Meltilex A, de Wallac Oy, Ref# 1450-441). The DNA-incorporated radioactive was quantified by using a betha particles counter Wallac Oy. As a control of the cellular viability of the cultures, these were observed at the microscope (Zeiss Axiovert 40CFL, Karl Zeiss Microimagen GmbH, Gόttingen, Germany) regarding the density and morphology of the cell cultures in the presence of medium, with no other signals, in order to detect and quantify possible mitogenic direct actions of the study molecules on the PBMC, and the cellular viability after incubation was assessed.
The presence of compound 12 in the culture did not significantly modify the proliferative response of the PBMC from healthy volunteers in the absence and in the presence of the various mitogenic stimuli studied (Figures l la and 1 Ib).
Example 11. Effect of compound 12 on the shedding of CD62L by PBMC
The effect of compound 12 on the shedding of CD62L in lymphocytes and monocytes of PBMC from healthy volunteers was investigated.
In the presence of compound 12 at a concentration of 10"6 M, the CD62L shedding (CD62L -Phycoerithryn (PE), clon BD SKI l Cat No. 341012, BD Biosciences) increases significantly (p< 0.05). Notably, this decrease in the geometric mean fluorescence intensity (MFI) of CD62L-PE labelling detected after the shedding of CD62L selectively occurred in lymphocytes but significant differences were not observed in monocytes (Figures 12a and 12b).
Table 14. -Mean fluorescence intensity of surface CD62L expression in lymphocytes, p values correspond to data with respect to the vehicle for each experimental condition.
Figure imgf000047_0001
Table 15. -Mean fluorescence intensity of surface CD62L expression in monocytes, p values correspond to data with respect to the vehicle for each experimental condition.
Figure imgf000048_0001

Claims

1. Use of a compound of formula (I) :
Figure imgf000049_0001
(I) wherein:
Ri is selected from substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclyl; R2 is selected from hydrogen, substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, and N(R'R") wherein R' and R" are independently hydrogen or Ci-C6 alkyl; and
R3 is a Ci_6 alkyl radical, or a pharmaceutically acceptable salt, prodrug and/or solvate thereof, in the preparation of a medicament for the treatment of an acute or chronic inflammatory disease, by inhibiting the production of at least one pro -inflammatory cytokine selected from TNF-alpha and IFN-gamma, or by inmunomodulating the IL-8 chemokine and/or the IL-IO regulatory cytokine.
2. The use according to claim 1, wherein the acute or chronic inflammatory disease is selected from acute and chronic seropositive or seronegative olygoarthritis and polyarthritis, spondiloarthropathies, glomerulonephritis, colagenopathies, tubulo- interstitial nephritis, metabolic syndrome, atherosclerosis, osteoarthritis, asthma, chronic obstructive pulmonary disease, interstitial lung disease, multiple sclerosis, demyelinating diseases, meningitis, encephalitis, meningoencephalitis, inflammatory radiculopathies and peripheral neuropathies, inflammatory bowel disease, cirrhosis, hepatitis, heart failure, ischemic disease, renal failure, inflammatory cystitis, benign prostatic hyperplasia, prostatitis, myocarditis, pericarditis, uveitis, atopic dermatitis, eccema, urticaria, psoriasis, rosacea, allergic rhinitis, sepsis, septic shock, multiorganic failure, systemic autoimmune diseases such as systemic lupus erythematosus, vasculitis, dermatomyositis, amyloidosis or sarcoidosis, organ specific autoimmune diseases such as myasthenia gravis, thyroiditis or insulinitis, organ transplantation, infectious ant tumor induced inflammation, TNF-alpha dependent cellular degeneration, necrosis, apoptosis, graft versus host disease, cachexia and autocrine and paracrine pathological cell growth.
3. The use according to claim 2 wherein the chronic inflammatory disease is seropositive or seronegative chronic polyarthritis.
4. The use according to claim 3 wherein the chronic polyarthritis is rheumatoid arthritis.
5. The use according to any of claims 1 to 4, wherein Ri is a substituted or unsubstituted Ci-C6 alkyl.
6. The use according to claim 5 wherein Ri is methyl.
7. The use according to any of claims 1 to 6, wherein R2 is a substituted or unsubstituted cycloalkyl.
8. The use according to claim 7, wherein R2 is cyclopentyl.
9. The use according to any of claims 1 to 8 wherein R3 is methyl.
10. The use according to any of claims 1 to 4 wherein the compound of formula (I) is selected from the following compounds:
Figure imgf000050_0001
Figure imgf000051_0001
Figure imgf000052_0001
or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
11. A compound of formula (F) which is:
Figure imgf000052_0002
(I') wherein:
Ri is selected from substituted or unsubstituted Ci-C6 alkyl, substituted or unsubstituted cycloalkyl, substituted or unsubstituted aryl and substituted or unsubstituted heterocyclic
R3 is a Ci-C6 alkyl radical; or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
12. The compound according to claim 11 wherein Ri is a substituted or unsubstituted Ci-C6 alkyl.
13. The compound according to claim 12 wherein Ri is methyl.
14. The compound according to claim 11 which is selected from the following:
Figure imgf000053_0001
Figure imgf000054_0001
or a pharmaceutically acceptable salt, prodrug and/or solvate thereof.
15. A pharmaceutical composition comprising a compound of formula (F) as defined in any of claims 11 to 14, or a pharmaceutically acceptable salt, prodrug or solvate thereof, and at least one pharmaceutically acceptable carrier, adjuvant and/or vehicle.
16. A compound of formula (F) as defined in any of claims 11 to 14, for its use as a medicament.
17. Use of a compound of formula (I) as defined in claim 1, as an imaging biomarker in imaging and pharmaco-imaging technologies, for finding immunological lesions, target cells and target molecules.
PCT/EP2009/057324 2008-06-16 2009-06-15 5-(4-methanesulfonyl-phenyl)-thiazole derivatives for the treatment of acute and chronic inflammatory diseases WO2009153226A1 (en)

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