Selective cox-2 inhibition from non-edible plant extracts

Abstract

The present invention is directed toward a method for inhibiting COX-2 in an organism. In particular, the method is preferably directed toward selectively inhibiting COX-2 in an organism. The method comprises administering to the organism an organic extract isolated from a non-edible plant wherein such extract inhibits COX-2 . A method to purify a composition that exhibits COX-2 inhibition and COX-2 selective inhibition from the organic extract is also provided. In addition, a method for treating and/or preventing COX-2 mediated inflammation or inflammation-associated disorders in an organism is provided.

Description

FIELD OF THE INVENTION

[0001] The current invention is generally directed toward nutraceuticals that are nonsteroidal anti-inflammatory agents capable of inhibiting cyclooxygenase-2 (COX-2). The present invention relates to a method for inhibition of COX-2, or selective inhibition of COX-2 in an organism by administering to the organism organic extracts isolated from non-edible plants wherein such extracts inhibit COX-2 activity. The present invention also relates to purified compositions of the plant organic extracts. In addition, the current invention is directed toward a method for treating and/or preventing COX-2 mediated inflammation or inflammation-associated disorders in an organism.

BACKGROUND OF THE INVENTION

[0002] The prostaglandins are a potent class of biologically active lipid derivatives that play a crucial role in the inflammatory response. The inflammatory response is a localized tissue response to injury or other trauma characterized by pain, heat, redness and swelling. Prostaglandins mediate this response by inhibiting platelet aggregation, increasing vascular permeability, increasing vascular dilation, inducing smooth-muscle contraction and causing the induction of neutrophil chemotaxis. Because of their central role in mediating the inflammatory response, significant efforts have been directed toward elucidating compositions that are capable of inhibiting the biosynthesis of prostaglandins.

[0003] Toward that end, prostaglandin biosynthesis has been extensively characterized. Prostaglandins are a group of oxygenated fatty acids that are generally derived from arachidonic acid. The biosynthesis of prostaglandins from arachidonic acid occurs in a three step process that includes 1) hydrolysis of arachidonic acid from phospholipid precursors catalyzed by a phospholipase A2; 2) cyclooxygenase (“COX”) catalyzed oxygenation of arachidonic acid to prostaglandin G2 (“PGG2”). This COX catalyzed reaction is the first committed and rate limiting step in prostaglandin synthesis; and 3) conversion of prostaglandin G2 to the biologically active end product, prostaglandin, catalyzed by a series of synthases and reductases. Upon their synthesis, prostaglandins exit the cell and act in a hormone-like manner by effecting the target cell via G protein linked membrane receptors.

[0004] Inactivation of the COX enzyme is a natural target as a means to inhibit prostaglandin production due to this enzyme's pivotal role in the prostaglandin biosynthetic pathway. It is now known that two gene products possessing COX enzyme activity are expressed, termed COX-1 and COX-2. COX-1 was the first discovered isoform and is constitutively expressed in most tissue types. Because it is constitutively expressed, COX-1 is available to participate in activities requiring a rapid physiological response and causes the production of prostaglandins involved in “house-keeping” functions. For example, COX-1 is responsible for acute production of prostaglandins that regulate vascular homeostasis, maintain gastrointestinal integrity, and maintain kidney function. Thus, COX-1 activity is responsible for the synthesis of prostaglandins required for the maintenance of several cell types.

[0005] COX-2, on the other hand, is a recently discovered isoform that is inducibly expressed in response to numerous stimuli such as bacterial lipopolysaccharides, growth factors, cytokines, and phorbol esters. In addition, COX-2 is only expressed in a limited number of cell types including monocytes, macrophages, neutrophils, fibroblasts and endothelial cells. COX-2 expression, but not COX-1 expression, has been shown to increase in rheumatoid synovial tissue. Contrastingly, COX-2 expression is inhibited in response to glucocorticoids and by anti-inflammatory cytokines. Thus, based upon these observations, COX-2 has been shown to be the isoform responsible for mediating the production of prostaglandins that participate in the inflammatory response and inflammatory related disorders. In addition, COX-2 has also been shown to participate in certain cancers, Alzheimer's disease, atherosclerosis, and central nervous system damage resulting from stroke, ischemia and trauma.

[0006] Corticosteroids provide one means to reduce effects associated with the inflammatory response. These potent anti-inflammatory agents exert their effect by causing a reduction in the number and activity of immune system cells via various mechanisms. However, prolonged administration of corticosteroids results in drastic side effects that limit the therapeutic value of this class of anti-inflammatory agent.

[0007] Nonsteroidal anti-inflammatory drugs (NSAIDs) are also utilized as a means to reduce effects associated with the inflammatory response. The principal pharmaceutical effects of NSAIDs are due to their ability to prevent COX activity resulting in the inhibition of prostaglandin synthesis. Inhibition of prostaglandin synthesis by NSAIDs is anti-pyretic, analgesic, anti-inflammatory, and anti-thrombogenic. However, administration of NSAIDs may also result in severe side effects such as gastrointestinal bleeding, ulcers and incidence of renal problems. NSAIDs also inhibit both COX isoforms to varying degrees. For example, the most common NSAID, aspirin (acetylated derivative of salicylic acid), inhibits prostaglandin biosynthesis by irreversibly inactivating both COX-1 and COX-2 via acetylation of a serine residue located in the arachidonic binding domain. While aspirin inactivates both isoforms, it is 10 to 100 times more effective inactivating COX-1 as opposed to COX-2.

[0008] The selective inhibition of COX-2 has been shown to be anti-inflammatory and analgesic without the associated gastric and kidney related toxicity problems. This phenomenon is due to the discovery of NSAIDs that are capable of inhibiting COX-2, which is responsible for the production of prostaglandins that mediate the inflammatory response, without causing the inhibition of COX-1, which is responsible for the production of prostaglandins that maintain both gastrointestinal integrity, and kidney function. Thus, the beneficial effects of NSAIDs are separable from their drastic side effects by the development of COX-2 selective inhibitors.

[0009] Toward that end, several drugs that are COX-2 selective inhibitors of prostaglandin synthesis have been developed. The most extensively characterized class of COX-2 selective inhibitor is diarylheterocycles, which include the recently approved drugs celecoxib and rofecoxib. However, other classes include, but are not limited to, acidic sulfonamides, indomethacin analogs, zomepirac analogs, chromene analogs, and di-t-butylphenols. For example, U.S. Pat. No. 5,380,738 describes oxazoles which selectively inhibit COX-2, U.S. Pat. No. 5,344,991 describes cyclopentenes which selectively inhibit COX-2, U.S. Pat. No. 5,393,790 describes spiro compounds which selectively inhibit COX-2, WO94/15932 describes thiophene and furan derivatives which selectively inhibit COX-2, and WO95/15316 describes pyrazolyl sulfonamide derivatives which selectively inhibit COX-2.

[0010] In order to afford an alternative to drug-based selective COX-2 therapy, it would be highly beneficial to provide nutraceuticals that inhibit COX-2, or even more preferably that selectively inhibit COX-2. A nutraceutical, in this context, is a composition that is a naturally occurring product that can safely be consumed and that exhibits COX-2 inhibitory activity. In particular, it would be highly beneficial to obtain the nutraceutical composition or extract from a plant source due to the ability to derive a large quantity of the nutraceutical from a plant at a relatively affordable cost. These nutraceutical compositions could be utilized in the diet in a preventative manner to maintain a “healthy” physiological state. The nutraceutical compositions could also be used as a means to treat, cure or mitigate an existing inflammatory-related ailment either alone or in combination with another compound as a part of combination therapy.

SUMMARY OF THE INVENTION

[0011] Among the several aspects of the invention therefore, is provided a method for inhibiting the activity of COX-2 in an organism, the method comprising the step of administering to the organism a therapeutically or prophylactically effective amount of an organic extract of a non-edible plant, wherein the plant is selected from the order consisting of Arales, Asterales, Coniferales, Equisetales, Euphorbiales, Geraniales, Lamiales, Lillales, Pteridophyta, Ranales, Rhamnales, Rutales, Scrophulariales, Umbellales, and Urticales.

[0012] Another aspect of the invention is a method for inhibiting the activity of COX-2 in an organism, the method comprising the step of administering to the organism a therapeutically or prophylactically effective amount of an organic extract of a plant, wherein the plant is selected from the order consisting of Arales, Asterales, Coniferales, Equisetales, Euphorbiales, Geraniales, Lamiales, Lillales, Pteridophyta, Ranales, Rhamnales, Rutales, Scrophulariales, Umbellales, and Urticales, wherein the organic extract is a purified composition obtained by a method comprising contacting the plant with an organic solvent to remove an extract from the plant wherein the extract inhibits COX-2 activity and then isolating the extract with COX-2 inhibitory activity.

[0013] Still another aspect provides a method of treating or preventing COX-2 mediated inflammation or an inflammation-associated disorder in an organism, the method comprising administering to the organism a therapeutically or prophylactically effective amount of the purified composition of an organic plant extract wherein the purified composition is obtained by a method comprising contacting the plant with an organic solvent to remove an extract from the plant wherein the extract inhibits COX-2 activity and then isolating the extract with COX-2 inhibitory activity.

[0014] Other features of the present invention will be in part apparent to those skilled in the art and in part pointed out in the detailed description provided below.

BRIEF DESCRIPTION OF THE DRAWINGS

[0015] These and other features, aspects, and advantages of the present invention will become better understood with regard to the following description, appended claims and accompanying figures where:

[0016] FIG. 1 depicts COX-2>COX-1 inhibition by an extract isolated from Arisaema heterophyllum.

[0017] FIG. 2 depicts COX-2>COX-1 inhibition by an extract isolated from Mohonia fortunei.

[0018] FIG. 3 depicts COX-2>COX-1 inhibition by an extract isolated from Hydrastis canadensis.

ABBREVIATIONS AND DEFINITIONS

[0019] To facilitate understanding of the invention, a number of terms and abbreviations as used herein are defined below:

[0020] “Purified” means partially purified and/or completely purified. Thus, a “purified composition” may be either partially purified or completely purified.

[0021] “Extract” means crude extract, purified extract, and purified composition obtained by purification of the extract.

[0022] “COX activity” means the ability of either COX isoform, COX-1 or COX-2, to catalyze the oxygenation reaction of arachidonic acid to PGG2.

[0023] “COX inhibitor or COX inhibition” means a composition, agent or extract, purified or otherwise, that prevents either COX isoform, COX-1 or COX-2, from catalyzing the oxygenation reaction of arachidonic acid to PGG2 either in whole or in part.

[0024] “Selective inhibition of COX-2” means a composition, agent, or extract, purified or otherwise, which selectively inhibits COX-2 activity over COX-1 activity as determined by the ratio of the percentage of COX-2 inhibition divided by the percentage of COX-1 inhibition, unless otherwise indicated herein.

[0025] “IC50” means the concentration (in mol L−1) that reduces a specified response to 50% of its former value. As used herein this value measures the amount of composition, agent or extract (ug extract/ml solvent) causing 50% inhibition of PGE2 production. The IC50 value may be used to determine COX-2 selectivity as specifically set-forth herein.

[0026] “Plant or parts thereof” means either the whole plant, or any part of the plant such as an aerial part, fruit, leaf, stem, or root and any combination thereof.

[0027] “Order”, as utilized herein, is a taxonomic category of related organisms with a category consisting of a number of similar families.

[0028] “Family”, as utilized herein, is a taxonomic category of related organisms ranking below the order and above the genus.

[0029] “Species”, as utilized herein, is a fundamental taxonomic category ranking below a genus and consisting of a group of closely related individuals.

[0030] COX=the enzyme cyclooxygenase

[0031] COX-1=the isoform cyclooxygenase-1

[0032] COX-2=the isoform cyclooxygenase-2

[0033] NSAIDs=nonsteroidal anti-inflammatory drugs

[0034] PGE2=prostaglandin E2

DESCRIPTION OF THE PREFERRED EMBODIMENT

[0035] Applicants have discovered that organic extracts of certain non-edible plants or parts therefrom inhibit COX-2 activity. Applicants have also discovered that organic extracts of certain non-edible plants or parts therefrom selectively inhibit COX-2 activity. The inhibitory effect is selective because inhibition of COX-2 is greater than inhibition of COX-1. Consequently, organic extracts of such plants or parts therefrom may be used to selectively inhibit the activity of COX-2 in an organism without causing an equivalent inhibition of COX-1 activity. Advantageously, these organic extracts are nutraceuticals that may be safely consumed and provide an alternative to traditional drug-based therapy for COX-2 inhibition.

[0036] Accordingly, the extracts of the present invention preferably inhibit COX-2 activity more than COX-1 activity. Preferably, the inhibitory effect of the plant extract on COX-2 is at least about two times greater than its inhibitory effect on COX-1. More preferably, the inhibitory effect on COX-2 is at least about 10 times greater than the inhibitory effect on COX-1. COX enzyme inhibition and selectivity may be determined in accordance with any method generally known to those of ordinary skill in the field, as set forth in more detail below.

[0037] In addition to inhibiting COX-2, the organic extracts of the present invention are preferably isolated from a non-edible plant. In general, plants are classified as non-edible if they are utilized for a purpose other than nourishment. For example, medicinal plants are considered non-edible because they are consumed for the purpose of correcting symptoms of illness and are considered too potent to be consumed on a daily basis. Classification of plants as edible versus non-edible may be accomplished utilizing references commonly known to those skilled in the art for example, such references include, NAPRALERT; Tyozaburo Tanaka, (Edited by Sasuke Nakoa) Tanaka's Cyclopedia of Edible Plants of the World, Keigaku Publishing Co., Tokyo, Japan, 1976; Stephen Facciola, Cornucopia II: A Source Book of Edible Plants, Kampong Publications, Vista, Calif., 1998; James A. Duke, Database of Phytochemical constituents of GRAS Herbs and Other Economic Plants, CRC Press, Boca Raton, Fla., 1992; and George Macdonald Hocking, Dictionary of Natural Products, Plexus Publishing, Inc., Medford, N.J., 1997. The contents of these references are hereby incorporated in their entirety.

[0038] In a particularly preferred embodiment, organic extracts are isolated from non-edible plants of the following plant orders: Arales, Asterales, Coniferales, Equisetales, Euphorbiales, Geraniales, Lamiales, Lillales, Pteridophyta, Ranales, Rhamnales, Rutales, Scrophulariales, Umbellales, and Urticales. The ability of extracts isolated from non-edible plants of these particular orders to inhibit COX-2, selectively inhibit COX-2 and their use as non-edible plants are set-forth below in Tables 1-5 and FIGS. 1-3.

[0039] In order to prepare the extracts of the invention, a non-edible plant or parts thereof is ground into a fine powder, the resultant powder is extracted with a solvent, and the extraction solvent is removed from the extract. The whole plant may be used or parts of the plant including an aerial part, fruit, leaf, stem, or root and any combination thereof may be used. If desired, the resultant extract may be further purified to yield a purified extract or one or more purified compositions. The grinding step may be accomplished by any commonly known method for grinding a plant substance. For example, the plant or parts thereof may be passed through a grinder to obtain a fine powder.

[0040] After the plant or parts thereof have been ground into a fine powder, they are combined with an extraction solvent. The solution is then stirred at a temperature, and for a period of time, that is effective to obtain an extract with the desired inhibitory effects on the activity of COX-2. The solution is preferably not overheated, as this may result in degradation and/or denaturation of proteins in the extract. The solution may be stirred at a temperature between about room temperature (25° C.) and the boiling point of the extraction solvent. Preferably, the solution is stirred at about room temperature.

[0041] The length of time during which the plant powder is exposed to the extraction solvent is not critical. Up to a point, the longer the plant powder is exposed to the extraction solvent, the greater is the amount of extract that may be recovered. Preferably, the solution is stirred for at least 1 minute, more preferably for at least 15 minutes, and most preferably for at least 60 minutes.

[0042] The extraction process of the present invention is desirably carried out using an organic solvent or a mixture of organic solvents. Organic solvents which may be used in the extraction process of the present invention, include but are not limited to hydrocarbon solvents, ether solvents, chlorinated solvents, acetone, ethyl acetate, butanol, ethanol, methanol, isopropyl alcohol and mixtures thereof. Hydrocarbon solvents which may be used in the present invention include heptane, hexane and pentane. Ether solvents which may be used in the present invention include diethyl ether. Chlorinated solvents which may be used in the present invention include dichloromethane and chloroform. Preferably, the solvent utilized for such extraction is a nonpolar organic solvent, such as dichloromethane or hexane.

[0043] The relative amount of solvent used in the extraction process may vary considerably, depending upon the particular solvent employed. Typically, for each 100 grams of plant powder to be extracted, about 500 ml of extraction solvent would be used. The organic solvent may be removed from the extract by any method known in the field of chemistry for removing organic solvents from a desired product, including, for example, rotary evaporation.

[0044] It is believed that the inhibitory effect of the plant extract of this invention on the activity of COX-2 is due to the presence of one or more compounds in the extract. Compounds present in the extract which inhibit the activity of COX-2 may be isolated and purified by those of ordinary skill in the art employing methods known in the art. For example, column chromatography and fractional distillation may be used to obtain pure compounds from the plant extract of this invention.

[0045] The isolation and purification of particular compounds from the organic plant extracts of this invention may be performed as described in Resch, et al., J. Nat. Prod., 61, 347-350 (1998), the entire contents of which are incorporated by reference herein. The methods disclosed therein may be used to isolate and purify compositions which inhibit COX-2.

[0046] The ability of a particular organic extract to inhibit COX-1 or COX-2 is preferably determined by performing COX activity assays utilizing recombinant COX-1 and COX-2. The COX-1 and COX-2 genes may be subcloned from a variety of organisms, however in a preferred embodiment such genes are isolated from human or murine sources, using a variety of procedures known to those skilled in the art and detailed in, for example, Sambrook et al., Molecular Cloning, A Laboratory Manual, 2nd ed., Cold Spring Harbor Laboratory Press, (1989) and Ausabel et al., Short Protocols in Molecular Biology, 3rd. ed., John Wiley & Sons (1995). Additionally, the subcloned portion of the particular COX gene may be inserted into a vector by a variety of methods. In a preferred method, the sequence is inserted into an appropriate restriction endonuclease site(s) in a baculovirus transfer vector pVL1393 utilizing procedures known to those skilled in the art and detailed in, for example, Sambrook et al., Molecular Cloning, A Laboratory Manual, 2nd ed., Cold Spring Harbor Laboratory Press, (1989) and Ausubel et al., Short Protocols in Molecular Biology, 3rd ed., John Wiley & Sons (1995).

[0047] The recombinant baculoviruses may be isolated by transfecting an appropriate amount of baculovirus transfer vector DNA into a sufficient quantity of SF9 insect cells along with linearized baculovirus plasmid DNA by the calcium phosphate method or any other method generally know to those skilled in the art. (See M. D. Summers and G. E. Smith, A Manual of Methods for Baculovirus Vectors and Insect Cell Culture Procedures, Texas Agric. Exp. Station Bull. 1555 (1987)). Recombinant viruses may be purified by three rounds of plaque purification and high titer (107-108 pfu/ml) stocks of virus may be prepared.

[0048] Preferably, for large scale production, cells may be infected in approximately 10 liter fermentors (0.5×106/ml) with the recombinant virus stock such that the multiplicity of infection is greater than about 0.1. After several hours the cells are centrifuged and the cell pellet is homogenized in an appropriate buffer such as Tris/sucrose (50 mM/25%, pH 8.0). The homogenate may then be centrifuged at an appropriate speed and for an appropriate time (such as 10,000×G for 30 minutes) so as to cause the homogenate to separate into a pellet and supernatant fraction. The resultant supernatant fraction will contain the desired product and may be stored at −80° C. until use.

[0049] In order to test organic extracts for COX-2 inhibition and selectivity, standard COX-1 and COX-2 assays may be performed by employing ELISA procedures generally known to those skilled in the art. In such procedures, COX-1 and COX-2 activities are assayed as PGE2 formed/mg protein/time using ELISA to detect the amount of PGE2 synthesized from arachindonic acid. PGE2 formation may be measured using PGE2 specific antibody. Indomethacin, a non-selective COX-2/COX-1 inhibitor, may be employed as a positive control. The relative ability of various organic extracts to inhibit COX-1 or COX-2 at a particular concentration may be determined by comparing the IC50 value expressed as mg extract/ml solvent resulting in a 50% inhibition of PGE2 production. Selective inhibition of COX-2 may then be determined by the IC50 ratio of COX-1/COX-2. Additionally, any other means to determine COX inhibition known to those generally skilled in the art may be employed.

[0050] The extracts of this invention may be used to manage, prevent and/or treat an organism having, or at risk for developing, a condition which is mediated in whole or in part by COX-2. Accordingly, conditions which may be benefited by inhibition of COX-2 or selective inhibition of COX-2 include, but are not limited to, the treatment of inflammation in an organism, and for treatment of other inflammation-associated disorders, such as, an analgesic in the treatment of pain and headaches, or as an antipyretic for the treatment of fever. For example, extracts of the invention would be useful to treat arthritis, including but not limited to rheumatoid arthritis, spondyloarthopathies, gouty arthritis, osteoarthritis, systemic lupus erythematosus and juvenile arthritis. Such extracts of the invention would be useful in the treatment of asthma, bronchitis, menstrual cramps, tendinitis, bursitis, skin-related conditions such as psoriasis, eczema, burns and dermatitis, and from post-operative inflammation including ophthalmic surgery such as cataract surgery and refractive surgery. Extracts of the invention also would be useful to treat gastrointestinal conditions such as inflammatory bowel disease, Crohn's disease, gastritis, irritable bowel syndrome and ulcerative colitis, and treatment of cancer, including but not limited to the following types of cancer: colon, breast, prostate, bladder, or lung. In yet another preferred use, the extracts of the present invention may also be utilized as chemopreventive agents. Extracts of the invention would be useful in treating inflammation in such diseases as vascular diseases, migraine headaches, periarteritis nodosa, thyroiditis, aplastic anemia, Hodgkin's disease, sclerodoma, rheumatic fever, type I diabetes, neuromuscular junction disease including myasthenia gravis, white matter disease including multiple sclerosis, sarcoidosis, nephrotic syndrome, Behcet's syndrome, polymyositis, gingivitis, nephritis, hypersensitivity, swelling occurring after injury, myocardial ischemia, and the like. The extracts would also be useful in the treatment of ophthalmic diseases, such as retinitis, retinopathies, uveitis, ocular photophobia, and of acute injury to the eye tissue. The extracts would also be useful in the treatment of pulmonary inflammation, such as that associated with viral infections and cystic fibrosis. Additionally, the extracts would be beneficial for the treatment of certain central nervous system disorders such as cortical dementias including Alzheimer's disease. The extracts of the invention are useful as anti-inflammatory agents, such as for the treatment of arthritis, with the additional benefit of having significantly less harmful side effects. These extracts would also be beneficial in the treatment of allergic rhinitis, respiratory distress syndrome, endotoxin shock syndrome, atherosclerosis and central nervous system damage resulting from stroke, ischemia and trauma. Additionally, the extracts would be useful in the treatment of pain, including but not limited to postoperative pain, dental pain, muscular pain, and pain resulting from cancer.

[0051] The present extracts may also be employed either alone or in combination with other compounds as a part of combination therapy, partially or completely, in place of other conventional anti-inflammatory agents. For example, such as together with steroids, NSAIDs, 5-lipoxygenase inhibitors, leukotriene receptor antagonists, LTA4 hydrolase inhibitors, and LTC4 synthase inhibitors. Preferably, with combination therapy one will typically combine a drug or drugs and a nutraceutical, such as a plant extract of the current invention, in a manner such that the drug and the nutraceutical have different mechanisms of action, but yet target the same disease. For example, in a typical selection of agents for use in combination therapy to treat arthritis, one could utilize a plant extract of the present invention, which exhibits selective COX-2 inhibition with another agent known to attenuate inflammation associated with arthritis via an independent mechanism.

[0052] Those of ordinary skill in the art of preparing pharmaceutical formulations can readily formulate pharmaceutical compositions having plant extracts using known excipients (e.g., saline, glucose, starch, etc.). Similarly, those of ordinary skill in the art of preparing nutritional formulations can readily formulate nutritional compositions having plant extracts. And those of ordinary skill in the art of preparing food or food ingredient formulations can readily formulate food compositions or food ingredient compositions having plant extracts.

[0053] In addition, those of ordinary skill in the art can readily determine appropriate dosages that are necessary to achieve the desired therapeutic or prophylactic effect upon oral, parenteral, rectal and other administration forms. Typically, in vivo models (i.e., laboratory mammals) are used to determine the appropriate plasma concentrations necessary to achieve a desired mitigation of inflammation related conditions.

[0054] The extracts of the present invention may be employed for the treatment and/or prevention of inflammation-related disorders, as identified above, in a number of organisms. Besides being useful for human treatment, these extracts are also useful for veterinary treatment of companion animals, exotic animals and farm animals, including mammals, rodents, avians, and the like. More preferred animals include horses, dogs, cats, sheep, and pigs.

[0055] The detailed description set-forth above is provided to aid those skilled in the art in practicing the present invention. Even so, this detailed description should not be construed to unduly limit the present invention as modifications and variation in the embodiments discussed herein can be made by those of ordinary skill in the art without departing from the spirit or scope of the present inventive discovery.

[0056] All publications, patents, patent applications and other references cited in this application are herein incorporated by reference in their entirety as if each individual publication, patent, patent application or other reference were specifically and individually indicated to be incorporated by reference.

[0057] Without further elaboration, it is believed that one skilled in the art can, using the preceding description, utilize the present invention to its fullest extent. The following preferred specific embodiments are, therefore, to be construed as merely illustrative, and not limitative of the remainder of the disclosure in any way whatsoever.

EXAMPLES

Sample Preparation

[0058] Plants or parts thereof were dried and sliced (“sample”). Samples of organic extracts were prepared from the non-edible plants listed in Table 1. The plant order and families that the various samples were prepared from are also set-forth in Table 1. In addition, details regarding the use of these some of these plants as medicinals is set-forth in Table 2. The particular sample was then ground into a fine powder using a coffee grinder. Approximately 100 grams of the resulting powder were added to approximately 500 ml of dichloromethane and stirred at room temperature for about 1 hour. The solvent was then removed by rotary evaporation, leaving several grams of the particular extract.

Inhibitory Effect of Various Plant Organic Extracts on COX-1 and COX-2 Activity

[0059] The particular extracts resulting from the sample preparation procedure detailed above were each evaluated for inhibition of COX-1 and COX-2. The COX-1 and COX-2 inhibition activities were determined in vitro according to the method of Gierse et al., J. Biochem., 305, 479-484 (1995). This method is summarized below.

Preparation of Recombinant COX Baculoviruses

[0060] Recombinant COX-1 was prepared by cloning a 2.0 kb fragment containing the coding region of human or murine COX-1 into a BamH1 site of the baculovirus transfer vector pVL1393 (Invitrogen) to generate the baculovirus transfer vectors for COX-1 according to the method of D. R. O'Reilly et al., Baculovirus Expression Vectors: A Laboratory Manual (1992).

[0061] Recombinant baculoviruses were then isolated by transfecting 4 mg of baculovirus transfer vector DNA into (2×108) SF9 insect cells along with 200 mg of linearized baculovirus plasmid DNA by the calcium phosphate method. (See M. D. Summers and G. E. Smith, A Manual of Methods for Baculovirus Vectors and Insect Cell Culture Procedures, Texas Agric. Exp. Station Bull. 1555 (1987)). Recombinant viruses were purified by three rounds of plaque purification and high titer (107-108 pfu/ml) stocks of virus were prepared.

[0062] For large scale production, SF9 insect cells were infected in 10 liter fermentors (0.5×106/ml) with the recombinant baculovirus stock such that the multiplicity of infection was 0.1. After 72 hours the cells were centrifuged and the cell pellet was homogenized in Tris/sucrose (50 mM/25%, pH 8.0) containing 1% of 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS). The homogenate was then centrifuged at 10,000×G for 30 minutes, and the resultant supernatant was stored at −80° C. until use.

[0063] Recombinant COX-2 was prepared by cloning a 2.0 kb fragment containing the coding region of human or murine COX-2 in accordance with the same method described above for COX-1.

Assay for COX-1 and COX-2 Activities

[0064] COX-1 and COX-2 activities were assayed as prostaglandin E2 (PGE2) formed/mg protein/time using ELISA to detect PGE2 synthesized from arachindonic acid. CHAPS-solubilized insect cell membranes containing recombinant COX-1 or COX-2 enzyme were incubated in a potassium phosphate buffer (50 mM, pH 8.0) containing epinephrine, phenol, and heme. Compounds or were pre-incubated with the appropriate enzyme or plant extract for approximately 10-20 minutes. Arachidonic acid (10 mM) was then added to the mixture and the reaction was permitted to occur for ten minutes at room temperature (25° C.).

[0065] Any reaction between the arachidonic acid and the enzyme was stopped after ten minutes by transferring 40 ml of reaction mixture into 160 ml ELISA buffer and 25 mM indomethacin. Indomethacin, a non-selective COX-2/COX-1 inhibitor, was utilized as a positive control. The PGE2 formed was measured by standard ELISA technology utilizing a PGE2 specific antibody (Cayman Chemical).

[0066] Approximately 200 mg of each extract obtained from the sample preparation procedure set-forth above were each individually dissolved in 2 ml of dimethyl sulfoxide (DMSO) for bioassay testing to determine the COX-1 and COX-2 inhibitory effects of each particular extract. Potency was determined by the IC50 value expressed as mg extract/ml solvent resulting in a 50% inhibition of PGE2 production. Selective inhibition of COX-2 was determined by the IC50 ratio of COX-1/COX-2. The results of these bioassays performed utilizing extract isolated from the plant family indicated are reported in Tables 1-5 and FIGS. 1-3 delineated below.

[0067] Table 1 below sets forth results of screening extracts of plants isolated from the orders, families, genera, and species indicated. A primary screen (indicated as 1° assay in Table 1) was performed in order to identify particular extracts that inhibited COX-2 at a concentration of 10 ug/ml. The extracts were then subjected to a confirmation screen to determine the extent of COX-2 inhibition at three different concentrations (10 ug/ml, 3.3 ug/ml and 1.1 ug/ml). The extracts were then tested for their ability to inhibit COX-1 at a concentration of 10 ug/ml. The percentage of COX inhibition is indicated as a percentage in each column, with a higher percentage indicating a greater degree of COX inhibition. In addition, the IC50 value for COX-1 and COX-2 was also determined for certain extracts as indicated in Table 1. The selectivity for these extracts was then determined by the IC50 ratio of COX-1/COX-2, as set-forth above. The COX-2 selectivity of extracts whose IC50 value was not determined may be calculated by dividing the percentage of COX-2 inhibition (at a concentration of 10 ug/ml) by the percentage of COX-1 inhibition (at a concentration of 10 ug/ml).

TABLE 1

Extracts from Non-Edible Plants that Inhibit COX-2

1* assay

Confirmation assay

COX-1

IC50

IC50

Selectivity

COX-2 (% Inhib.)

COX-2 (% Inhib.)

(% Inhib.)

(ug/ml)

(ug/ml)

COX-2/

Order

Family

Genus

Species

Common name

Part

10 ug/ml

10 ug/ml

3.3 ug/ml

1.1 ug/ml

10 ug/ml

COX-2

COX-1

COX-1

Arales9

Araceae

Arisaema

heterophylium

79%

87%

**

.0.2

−46%

2

25

12.5

Asterales

Asteraceae

Artemisia

anomola

herba artemisiae

PL

76%

71%

30%

27%

15%

***

***

***

Asterales

Asteraceae

Microglossa

angolensis

86%

66%

**

27%

−100%

***

***

***

Asterales

Asteraceae

Senecio

discifolius

ragwort

75%

76%

41%

32%

18%

***

***

***

Asterales

Asteraceae

Sigesbeckia

orientalis

St. Paul's wort

84%

67%

47%

20%

14%

***

***

***

Asterales

Asteraceae

Spilanthes

mauritiana

isisilili (Africa)

83%

81%

63%

26%

37%

***

***

***

Coniferales

Cupressaceae

Biota

orientalis

SD

78%

79%

67%

73%

62%

***

***

***

Equisetales

Equisetaceae

Equisetum

hyemale

ST

75%

88%

**

30%

−32%

***

***

***

Euphorbiales

Euphorbiaceae

Acalypha

ornata

78%

40%

19%

21%

−6%

***

***

***

Euphorbiales

Euphorbiaceae

Phyllanthus

guineensis

Guinea spurge

81%

75%

39%

37%

26%

***

***

***

Geraniales

Geraniaceae

Geranium

carolinianum

Carolina geranium

79%

100%

**

22%

35%

***

***

***

Lamiales

Lamiaceae4

Salvia

miltorrhiza

radix salviae miltorrhizac; sage

RT

86%

93%

**

49%

27%

***

***

***

Lamiales

Lamiaceae4

Solenostemon

latifolius

inuka; nidayana

79%

68%

40%

27%

12%

***

***

***

Liliales

Liliacese

Paris

chinensis

rhizome of Chinese paris

RT

75%

71%

40%

12%

25%

***

***

***

Pteridophyta

Polypodiaceae11

Platycerium

elephantotis

93%

61%

31%

34%

4%

***

***

***

Ranales

Berberidacea

Mahonia

fortunei

shi da gong lao ye (China)

81%

100%

**

25%

11%

0.8

7

8.8

Ranales

Ranunculaceae

Clematis

hirsuta

bisinda (Africa)

80%

57%

**

25%

17%

***

***

***

Ranales

Ranunculaceae

Hydrastis

canadensis

golden seal

86%

93%

**

25%

22%

3.5

15

4.3

Ranales

Ranunculaceae

Ranunculus

multifidus

wild buttercup

89%

98%

**

35%

36%

***

***

***

Rhamnales

Rhamnaceae

Rhamnus

purshiana

cascara sagrada

BK

80%

95%

**

74%

69%

***

***

***

Rhamnales

Vitaceae

Cyphostemma

adenocaule

iwengere

82%

58%

43%

16%

11%

***

***

***

Rutales1

Rutaceae

Zanthoxylum

americanum

prickly ash

79%

79%

47%

20%

60%

***

***

***

Scrophulariales

Acanihaceae

Justicia

secunda

Saint John's bush

76%

80%

**

18%

−58%

***

***

***

Umbellales

Apiaceae5

Angelica

dahurica

pai-chi

RT

76%

71%

38%

20%

39%

***

***

***

Urticales

Urticaceae

Fleurya

ovalifolia

stinging nettle

83%

47%

26%

23%

−20%

***

***

***

*Primary screen performed at three concentrations. Samples were not repeated in a COX-2 confirmation assay.

** No data due to assay error.

*** Not tested.

1Brassicales also classified as Sapindales or Rulales

4Lamiaceae also classifled as Labialae

5Apiaceae also classified as Umbelliferae

9Pandanales also classified as Arales or Alismatales

11Polypodiaceae also classified as Pteridophyta

[0068] The order, family, genus, and species of each plant whose extract was tested for COX-2 and COX-1 inhibitory activities are shown.

[0069] Table 2 below provides a description detailing the medicinal use of some of the plant extracts tested for COX-2 inhibition as set-forth in Table 1. In addition, a comprehensive listing of references known to those generally skilled in the art is provided detailing plant uses.

TABLE 2
MEDICINAL USES OF PLANT EXTRACTS
Scientific	Common Name	Isolate/	Sample	Extract
Name	or Comment	Chemical ID	ID	#	Reference
Acalypha ornata	Used in	78459	914108		5
	scabies,
	leprosy
Angelica	Pai-chi	78957	914526		5
dahurica
Arisaema	No common	76943	912370		5
heterophyllum	name available
Artemesia	Herba	79489	914823		5
anomola	Artemisiae
Biota orientalis	Species not	79560	914894		1
	found, but
	others
	medicinal
Clematis hirsuta	bisinda	78472	914121		6
	(Africa)
Cyphostemma	iwengere	78480	914128		2
adenocaule
Equisetum	Species not	79032	914601		5
hyemale	found, but
	others are
	medicinal.
Fleurya	Stinging	78460	914109		5
ovalifolia	nettle
Geranium	Carolina	76818	912282		5
carolinianum	geranium
Hydrastis	golden seal	79476	914810		2
canadensis	tea
Justicia	Saint John	77160	912439		5
secunda	bush
Mahonia fortunei	shi da gong	76787	912259		5
	lao ye (China)
Microglossa	Species not	78453	914102		5
angolensis	found, but
	other species
	medicinal.
Paris chinensis	Rhizome of	79044	914613		1
	Chinese Paris
Phyllanthus	Guinea spurge	78449	914099		5
guineensis
Platycerium	Species not	78461	914110		5
elephantotis	found. A
	genus of
	medicinal
	ferns.
Ranunculus	wild buttercup	78455	914104		5
multifidus
Rhamnus	cascara	79373	914707
purshiana	sagrada
Salvia	Radix salviae	79324	914658
miltorrhiza	miltorrhizae
Senecio	Ragwort	78479	914127		5
discifolius
Sigesbeckia	St. Paul's	78452	914101		5
orientalis	wort
Solenostemon	inuka,	78476	914124		5
latifolius	nidayana
Spilanthes	isisilili	78465	914114		5
mauritiana	(African)
Zanthoxylum	prickly ash	80396	922769		5
americanum	bark

References

[0070] 1. NAPRALERT (NATural Products ALERT), which currently contains the extracted information from over 116,000 scientific research articles and books from 1650 A.D. to the present. The NAPRALERT database is housed and maintained by the Program for Collaborative Research in the Pharmaceutical Sciences (PCRPS), within the Department of Medicinal Chemistry and Pharmacognosy, in the College of Pharmacy of the University of Illinois at Chicago, 833 South Wood Street (M/C 877), Chicago, Ill. 60612, U.S.A.

[0071] 2. Tyozaburo Tanaka, (Edited by Sasuke Nakao) Tanaka's Cyclopedia of Edible Plants of the World, Keigaku Publishing Co., Tokyo, Japan, 1976.

[0072] This is a compendium of about 11,000 species of plants, including the essential wild species of the world. This book is considered to be one of the principle references on the world's edible plants.

[0073] 3. Stephen Facciola, Cornucopia II: A Source Book of Edible Plants, Kampong Publications, Vista, Calif., 1998.

[0074] This book records the more than 3,000 species available in the U.S. and abroad.

[0075] 4. James A. Duke, Database of Phytochemical Constituents of GRAS Herbs and Other Economic Plants, CRC Press, Boca Raton, Fla., 1992.

[0076] A database of approximately 1000 plants and 3000 compounds.

[0077] 5. George Macdonald Hocking, Dictionary of Natural Products, Plexus Publishing, Inc., Medford, N.J., 1997.

[0078] “Terms in the field of Pharmacognosy relating to natural medicinal and pharmaceutical materials and the plants, animals and minerals from which they are derived.” The work contains over 18,000 entries.

[0079] 6. Enrique Sanchez-Monge, Flora Agricola: Taxonomia de las Magnoliofitas (Angiospermas) de interes agricola, con excepcion de las de aprovechamiento exclusivamente ornamental o forestall, Ministerio de Agriculture, Pesca y Alimentacion, Madrid, Spain, (date unknown).

[0080] An excellent reference work in Spanish with descriptions of plants, common names in many languages and commercial use of agricultural organisms of the world.

[0081] 7. Anthony R. Torkelson, The Cross Name Index to Medicinal Plants, Volumes !-IV, CRC Press, Boca Raton, Fla., (1998-1999).

[0082] 8. Umberto Quattrocchi, CRC World Dictionary of Plant Names: Common Names, Scientific Names, Eponyms, Synonyms, and Etymology (Volumes 1-4), CRC Press, Boca Raton, Fla. (2000).

[0083] 9. W3TROPICOS, a web site providing access to the Missouri Botanical Garden's VAST (VAScular Tropicos) nomenclatural database and associated authority files.

[0084] 10. Webster's Ninth New Collegiate Dictionary, Merriam-Webster Inc., Springfield, Mass., (1983).

[0085] Tables 3-5 further illustrate the ability of certain extracts isolated from the families identified in Table 1 to selectively inhibit COX-2. A total of 6 different concentrations of the various extracts were tested for their ability to inhibit both COX-1 and COX-2. The IC50 value for COX-1 and COX-2 was also determined and a selectivity ratio was then calculated as set forth above. FIGS. 1-3 are graphs that depict the data shown in Tables 3-5 as indicated.

TABLE 3
Extract isolated from Arisaema heterophyllum
	COX-1	COX-2
Amount of	Activity	Activity
Extract	Relative	Relative
(mg/ml)	to Control	to Control
100	17%	4%
33.3	42%	8%
11.1	68%	16%
3.70	90%	37%
1.23	105%	59%
0.41	129%	78%
IC50	IC50	COX-2
(mg/ml)	(up/ml)	Selectivity
COX-1	COX-2	Ratio
25	2	12.5

[0086]

TABLE 4
Extract isolated from Mahonia fortunei
	COX-1	COX-2
Amount of	Activity	Activity
Extract	Relative	Relative
(mg/ml)	to Control	to Control
100	10%	1%
33.3	27%	6%
11.1	41%	9%
3.70	64%	22%
1.23	85%	36%
0.41	118%	74%
IC50	IC50	COX-2
(mg/ml)	(mg/ml)	Selectivity
COX-1	COX-2	Ratio
7	0.8	8.8

[0087]

TABLE 5
Extract isolated from Hydrastis canadensis
	COX-1	COX-2
Amount of	Activity	Activity
Extract	Relative	Relative
(mg/ml)	to Control	to Controll
100	5%	5%
33.3	24%	10%
11.1	59%	20%
3.70	70%	46%
1.23	84%	79%
0.41	90%	94%
IC50	IC50	COX-2
(mg/ml)	(mg/ml)	Selectivity
COX-1	COX-2	Ratio
15	3.5	4.3

[0088] As illustrated by these data, the organic extracts isolated from the indicated plant families inhibit COX-2. In fact, one of the extracts selectively inhibits COX-2 over COX-1 by greater than 10 fold. In view of the above, it will be seen that the several objectives of the invention are achieved and other advantageous results attained.

Claims

1. A method for inhibiting the activity of COX-2 in an organism, the method comprising the step of administering to the organism a composition comprising a therapeutically or prophylactically effective amount of an organic extract of a non-edible plant, wherein the plant is selected from the order consisting of Arales, Asterales, Coniferales, Equisetales, Euphorbiales, Geraniales, Lamiales, Lillales, Pteridophyta, Ranales, Rhamnales, Rutales, Scrophulariales, Umbellales, and Urticales.

2. The method of claim 1 wherein the inhibitory effect of the extract on COX-2 activity is greater than or equal to about 2 times greater than the inhibitory effect of the extract on COX-1 activity.

3. The method of claim 1 wherein the inhibitory effect of the extract on COX-2 activity is greater than or equal to about 10 times greater than the inhibitory effect of the extract on COX-1 activity.

4. The method of claim 1 wherein the organic extract of the Arales order is selected from the plant family Araceae.

5. The method of claim 4 wherein the organic extract of the Araceae family is from the genus Arisaema.

6. The method of claim 1 wherein the organic extract of the Asterales order is selected from the plant family Asteraceae.

7. The method of claim 6 wherein the organic extract of the Asteraceae family is selected from the genera consisting of Artemisia, Microglossa, Senecio, Sigesbeckia, and Spilanthes.

8. The method of claim 1 wherein the organic extract of the Coniferales order is selected from the plant family Cupressaceae.

9. The method of claim 8 wherein the organic extract of the Cupressaceae family is selected from the genus Biota.

10. The method of claim 1 wherein the organic extract of the Equisetales order is selected from the plant family Equisetaceae.

11. The method of claim 10 wherein the organic extract of the Equisetaceae family is selected from the genus Equisetum.

12. The method of claim 1 wherein the organic extract of the Euphorbiales order is selected from the plant family Euphorbiaceae.

13. The method of claim 12 wherein the organic extract of the Euphorbiaceae family is from the genera consisting of Acalypha and Phyllanthus.

14. The method of claim 1 wherein the organic extract of the Geraniales order is selected from the plant family Geraniaceae.

15. The method of claim 14 wherein the organic extract of the Geraniaceae family is from the genus Geranium.

16. The method of claim 1 wherein the organic extract of the Lamiales order is selected from the plant family Lamiaceae.

17. The method of claim 16 wherein the organic extract of the Lamiaceae family is selected from the genera consisting of Salvia and Solenostemon.

18. The method of claim 1 wherein the organic extract of the Lilales order is selected from the plant family Liliaceae.

19. The method of claim 18 wherein the organic extract of the Liliaceae family is from the genus Paris.

20. The method of claim 1 wherein the organic extract of the Pteridophyta order is selected from the plant family Polypodiaceae.

21. The method of claim 20 wherein the organic extract of the Polypodiaceae family is from the genus Platycerium.

22. The method of claim 1 wherein the organic extract of the Ranales order is selected from the plant families consisting of Berberidaceae and Ranunculaceae.

23. The method of claim 22 wherein the organic extract of the Berberidaceae family is from the genus Mahonia.

24. The method of claim 22 wherein the organic extract of the Ranunculaceae family is selected from the genera consisting of Clematis, Hydrastis, and Ranunculus.

25. The method of claim 1 wherein the organic extract of the Rhamnales order is selected from the plant families consisting of Rhamnaceae and Vitaceae.

26. The method of claim 25 wherein the organic extract of the Rhamnaceae family is from the genus Rhamnus.

27. The method of claim 25 wherein the organic extract of the Vitaceae family is from the genus Cyphostemma.

28. The method of claim 1 wherein the organic extract of the Rutales order is from the plant family Rutaceae.

29. The method of claim 28 wherein the organic extract of the Rutaceae family is from the genus Zanthoxylum.

30. The method of claim 1 wherein the organic extract of the Scrophulariales order is from the plant family Acanthaceae.

31. The method of claim 30 wherein the organic extract of the Acanthaceae family is from the genus Justicia.

32. The method of claim 1 wherein the organic extract of the Umbellales order is selected from the plant family Apiaceae.

33. The method of claim 32 wherein the organic extract of the Apiaceae family is from the genus Angelica.

34. The method of claim 1 wherein the organic extract of the Urticales order is from the plant family Urticaceae.

35. The method of claim 34 wherein the organic extract of the Urticaceae family is from the genus Fleurya.

36. The method of claim 1 wherein the organic extract is a purified composition obtained by a method comprising: (a) contacting the plant with an organic solvent to remove an extract from the plant wherein the extract inhibits COX-2 activity; and (b) isolating the extract with COX-2 inhibitory activity.

37. The method of claim 36 wherein the extract selectively inhibits COX-2 activity.

38. The method of claim 36 wherein step (a) further comprises mixing the plant with the organic solvent and stirring the resulting mixture at a temperature between about 25° C. and the boiling point of said solvent for at least one minute.

39. The method of claim 36 wherein the organic solvent is selected from the group consisting of hydrocarbon solvents, ethers, chlorinated solvents, acetone, ethyl acetate, butanol, ethanol, methanol, isopropyl alcohol and mixtures thereof.

40. The method of claim 36 wherein the organic solvent is non-polar.

41. The method of claim 40 wherein the non-polar organic solvent is dichloromethane or hexane.

42. The method of claim 36 wherein step (b) further comprises separating the solvent from the organic extract by evaporating the solvent.

43. A method of treating or preventing COX-2 mediated inflammation or an inflammation-associated disorder in an organism, the method comprising administering to the organism a composition comprising a therapeutically or prophylactically effective amount of the purified composition according to claim 36.

44. The method of claim 43 wherein the inflammation-associated disorder is arthritis.

45. The method of claim 43 wherein the inflammation-associated disorder is pain.

46. The method of claim 43 wherein the inflammation-associated disorder is fever.

47. The method of claim 43 for use in the treatment or prevention of cancer.

48. The method of claim 47 wherein the cancer is epithelial cell cancer.

49. The method of claim 48 wherein the epithelial cell cancer is colon, breast, prostate, bladder, or lung cancer.

50. The method of claim 43 for use in the treatment or prevention of central nervous system disorders.

51. The method of claim 50 wherein the central nervous system disorder is Alzheimer's Disease.