AURONES AS SELECTIVE PDE INHIBITORS AND THEIR USE IN NEUROLOGICAL CONDITIONS AND DISORDERS

Information

  • Patent Application
  • 20100267823
  • Publication Number
    20100267823
  • Date Filed
    March 29, 2010
    14 years ago
  • Date Published
    October 21, 2010
    14 years ago
Abstract
The invention relates to aurones and extracts comprising them useful in the prophylactic and/or therapeutic treatment of an animal (including a human) with a phosphodiesterase (PDE) dependent disease or condition of the central nervous system, as well as methods, uses and other inventions related thereto.
Description
FIELD OF THE INVENTION

The invention relates to aurones and extracts comprising them useful in the prophylactic and/or therapeutic treatment of an animal (including a human) with a phosphodiesterase (PDE) dependent disease or condition of the central nervous system, as well as methods, uses and other inventions related thereto as described below and in the claims.


BACKGROUND OF THE INVENTION

Phosphodiesterases are a diverse family of enzymes that hydrolyse cyclic nucleotides and thus play a key role in regulating intracellular levels of the second messengers cAMP and cGMP. Thereby, PDEs are governing a host of cellular functions involved e.g. in neural signal transduction in the CNS, lipid metabolism, cardiovascular health, bronchodilation, and inflammatory cell signalling. Additionally, PDE inhibitors have also been shown to be nootropic agents that enhance cognitive functions. Since 11 isoenzyme families have been discovered so far, the impetus for the development of isoenzyme selective inhibitors for the treatment of various diseases has increased.


While specificity of PDE subtype function is related to tissue specific expression of the different sub-types, there is nevertheless some overlap in the respective therapeutic areas that are assigned to them.


PDE1 inhibitors are recognized as cardioprotective and vasodilatory effectors.


PDE3 inhibitors have been recognized as potential therapeutics for e.g. congestive heart failure. PDE3, in addition, is not only highly expressed in the vasculature but also in the airways. It has high affinity for cAMP but can also hydrolyse cGMP. However, it hydrolyses cAMP at 10 times the rate it hydrolyses cGMP. PDE3 inhibitors have been shown to relax vascular and airway smooth muscle, to inhibit platelet aggregation and to induce lipolysis. The effect of PDE3 inhibitors as positive inotropic agents however, provided a strong rationale for developing such drugs for the treatment of chronic heart disease.


Most prominently PDE4 inhibitors have been described for e.g. inflammatory airways disease (Asthma); depression and memory enhancement. PDE4 is a characterized as cAMP-specific PDE. PDE4 is the predominant isoenzyme in the majority of inflammatory cells, with the exception of platelets, implicated in inflammatory airways disease. It is expressed in the airways smooth muscle, brain and cardiovascular tissues and is the largest PDE subfamily with over 35 different isoforms identified thus far. PDE4 is the most widely characterised PDE isoenzyme.


Phosphodiesterase inhibitors are also described to allow for cognitive enhancement (see e.g. Roe, G. M., et al., Curr. Pharm. Des. 11(26), 3329-34 (2005)).


Inhibitors of PDE3 are especially appropriate for the prophylactic and/or therapeutic treatment of nootropic diseases. Inhibitors of PDE4 are especially appropriate for prophylactic and/or therapeutic nootropic treatment.


Furthermore, PDE inhibitors can be considered for prophylactic treatment to reduce obesity and type 2 diabetes. It has been demonstrated that lipolysis in adipose tissue can be induced by natural products (such as e.g. Flavonoids) mediated by PDE inhibitory effects and antagonism of cAMP degradation.


Hebb A L, Robertson H A., PDEs as drug targets for CNS immune disorders; Curr Opin Investig Drugs. 2008 Jul.; 9(7):744-53.


Victoria Boswell-Smith, Domenico Spina, Clive P. Page, Phosphodiesterase inhibitors; British Journal of Pharmacology (2006) 147, S252-S257 & 2006 Nature Publishing.


Michael R. Peluso, Flavonoids Attenuate Cardiovascular Disease, Inhibit Phosphodiesterase, and Modulate Lipid Homeostasis in Adipose Tissue and Liver; Exp Biol Med 231:1287-1299, 2006.


There remains a need for safe and effective compositions for the treatment of PDE dependent diseases in subjects such as humans. The problem to be solved by the present invention is therefore to find novel compositions or compounds useful in the treatment of PDE dependent diseases.



Smilax is a genus of about 600 species of climbing flowering plants, many of which are woody and/or thorny, in the monocotyledon family Smilacaceae, native throughout the tropical and warm temperate regions of the world. On their own, Smilax plants will grow as a shrub, forming dense impenetrable thickets. They will also grow over trees and other plants up to 10 m high using its hooked thorns to hang on to and scramble over branches. The leaves are heart shaped and vary from 4-30 cm long in different species.


Extracts (predominantly from the roots) of Smilax species have been used to treat for various conditions. Therapeutic properties like anti-inflammatory, antifungal, antipruritic, anti-rheumatic, antiseptic, aphrodisiac, wound healing, stimulant, diuretic, diaphoretic, depurative, sudorific, tonic are attributed to them. Traditional/Ethnobotanical use is described for more then 40 Smilax species (http://www.ars-grin.gov/duke/). For selected Smilax species these are: Smilax aristolochiaefolia (Cancer, Depurative, Dyspepsia, Eczema, Fever, Gonorrhea, Kidney, Leprosy, Rash, Rheumatism, Scrofula, Skin, Sudorific, Syphilis), Smilax aristolochiifolia (Depurative, Diaphoretic, Syphilis, Tonic, Wound), Smilax china L. (Aphrodisiac, Dermatosis, Gonorrhea, Parturition, Rheumatism, Syphilis, Tonic), Smilax china (Abscess, Alexiteric, Antidote, Aphrodisiac, Arthritis, Asthma, Boil, Cancer, Carminative, Cold, Debility, Demulcent, Depurative, Diaphoretic, Diarrhea, Diuretic, Enteritis, Flux, Gout, Gravel, Malaria, Menorrhagia, Refrigerant, Rheumatism, Skin, Stimulant, Sudorific, Syphilis, Tonic, Urogenital, Venereal) Smilax glabra (Abscess, Antidote, Arthritis, Boil, Cystitis, Dysentery, Furuncle, Lymphadenopathy, Rheumatism, Skin, Sore, Syphilis, Venereal), Smilax medica (Antidote, Malignancy, Rheumatism, Scrofula, Skin, Stimulant, Sudorific, Venereal), Smilax ornata (Rheumatism, Scrofula, Skin, Tonic), Smilax scobinicaulis (Arthritis, Rheumatism, Skin, Sore), Smilax sieboldi (Arthritis, Rheumatism, Skin, Sore), Smilax zeylanica (Abscess, Ache(Bones), Anodyne, Cachexia, Cholera, Dysentery, Dysuria, Fever, Gravel, Measles, Ophthalmia, Skin, Smallpox, Sore, Swelling, Syphilis, Venereal)



Smilax myosotiflora is a very damage tolerant thorny plant capable of growing back from its rhizomes after being cut down or burned down by fire. It grows wild in the tropical forest in South East Asia, namely but not limited to Malaysia, Indonesia and Southern Thailand.


In Malaysia, the tuber or rhizome is used as an aphrodisiac and sexual tonic and to treat fevers. It is claimed that it increases the production of testosterone in elderly men, hence, improving sperm production and its viscosity, vitality and sexual strength. It also restores vitality and libido in women, firming the vagina especially after delivery and arresting vaginal discharge. The leaves and fruits are used to treat syphilis.


In traditional preparation, the rhizome is boiled by itself or mixed with Tongkat Ali root, horny goat weed (Epimedium) or Kacip Fatimah, Manjakani, Serapat, and other herbs to enhance the efficacy. The tonic is taken regularly once or twice a day. In modern preparation, phyto-chemicals from the Ubi Jaga rhizome are extracted, frozen or spray-dried. The extracts are similarly mixed with other herb-extracts and formulated separately for men or women. The leaves, fruits and rhizomes of Smilax myosotiflora were used to treat syphilis i.e. a bacterial infection. The rhizome is ingested as an aphrodisiac. The leaves and fruits of are used to relieve fever (http://khenerg.com/faq.html).


There are several registered products on the market containing Smilax myosotiflora (Ubi Jaga) in mixtures with other medicinal plants (Malayan Ministery of Health; http://search.moh.gov.my). Mixtures with e.g. Tongkat Ali (Eurycoma longifolia) are widely promoted on the Internet as to be used as an aphrodisiac. The main use is to increase male sexual power, increase general health and energy, and secondarily to improve nerve system and blood circulation.


Aurones are natural molecules which belong to the family of flavonoids, and which are structurally isomers of flavones (Boumendjel, Current Med. Chem. 2003). Systematically they were named as benzylidenebenzofuran-3(2H)-ones.


Aurones are broadly widespread in the plant kingdom, particularly in fruits and flowers in which they contribute to their coloration. Table 1 below contains a non-exhaustive, exemplary list of natural aurones which are found in plants. According to their substitution pattern, these auronones can be grouped into mono-, di-, tri-, tetra-, penta- and heptahydroxylated representatives which carry partially additional alkyl groups attached to core. The hydroxyl groups are free, methylated or carry sugar moieties.


Table 1 shows some aurone type compounds and their sources. (Dictionary of Natural Products, Chapman & Hall, 2008)











TABLE 1





structure-type
quantity of entries
sources







dihydroxy









 4; R = H  2; R = methyl

Glycine
max (soybean) and LygosraetamPterocarpusmarsupium






trihydroxy









 4; R = H  2; R = prenyl

Bidens
tripartita, Bidenssulphureus, Bidenslaevis, Dahliavariabilis, Baeriachrysostoma, Rhuscotinus, Schinopsis, Amphipterygiumadstringens, Cosmossulphureus, Cosmosmaritima, Viguiera, Zinnia, Coreopsis, Lasthenia, Tithonia, Buteafrondosa, Dipteryxodorata, Broussonetiapapyrifera











 4; R = H      2; R = methyl

Asparagus
gonocladus, Limonium sp., Pterocarpusmarsupium, Pterocarpussantalinus, AsarumlongerhizomatosumPterocarpusmarsupium











 2

Cephalocereus
senilis






tetrahydroxy









 9; R = H                    6; R methyl or prenyl

Oxalis
cernua, Chiritamicromusa, Limoniumbonduellii, Petrocosmeakerrii, Mussaendahirsutissima, Antirrhinummajus, Antirrhinumnuttalianum, Linariamaroccana, Marchantiaberteroana, Marchantiapolymorpha, Conocephalumsupradecompositum, Carrpossphaero- carpus, Mussaendahirsutissima, Pterocarpusmarsupium, Melanorrhoea spp., CyperuscapitatusAntiaristoxicaria, Cyperuscapitatus











13

Coreopsis
maritima, Coreopsisgigantea, Coreopsistinctoria, Baeriachrysostoma, Zinnialinearis, Bidensbipinnata, Bidenspilosa, Microglossapyrifolia, Coreopsisgrandiflora, Vacciniumoxycoccus, Cyperusscariosus











 2

Helianthus
annuus











 1

Picris
echoides











 1

Diospyros
melanoxylon






pentahydroxy









 2

Uvaria
hamiltonii











 6; R = H        2; R = methyl

Antirrhinum
nuttalianum, Linariamaroccana, Helichrysumbracteatum, Antirrhinummajus, Antirrhinumorontium, Linaria sp., AmomumsubulatumPterocarpussantalinus






heptahydroxy












 3

Gomphrena
agrestis










Also known are dimers of aurones, such as disulfuretin and biaureusidin.







One Aurone is known to be isolated out of Smilax bracteata (Zhang 2008).







Nevertheless, till now no secondary metabolites of this class have been described with chemical structure for Smilax myosotiflora.


Aurones are biochemically and structurally related to flavons. The flavons are widely present in aromatic, medicinal and edible plants, and also in fruits and vegetables. In general they exist as aglycones or glycosylated at various hydroxyl groups.


Recent advances were made to evaluate the therapeutical potential of aurones in different pharmacological areas like:

    • Use in cancer chemotherapy (modulators of P-glycoprote in-mediated MDR; inhibition of cyclin-dependent kinases; interactions with adenosine receptors; effects through DNA scission and telomerase Inhibition)
    • Use in treating parasitic infections
    • Use in treating microbial infections
    • Antihormonal activity of aurones
    • Aurones as antidiabetics.


DETAILED DESCRIPTION OF THE INVENTION

The present invention relates to a compound of the formula I,







wherein each of R1 to R9 is, independently of the others, H, hydroxy, fluoro, chloro, bromo, iodo, C1-C8-alkyl, C2-C8-alkenyl, C2-C8-alkynyl, C3-C10-cycloalkyl, phenyloxy, C1-C8-alkoxy, C1-C9-alkanoyloxy, benzoyl or the radical of a C5-C12-carbohydrate bound via one of its oxygen atoms, where alkyl, alkenyl, alkynyl, cycloalkyl, phenyl, alkoxy, alkanoyloxy and benzoyl can be unsubstituted or substituted by one, two or three substituents selected independently of each other from the group consisting of —F, —Cl, —Br, —I, —OH, —OCH3, —OCH2CH3, —OCOCH3, —CH3, —CHO, and —CO2H, or the radical of a C5-C12-carbohydrate bound via one of its oxygen atoms, preferably with the proviso that if R1, R3 and R7 each are bound via an oxygen, R2, R4, R5 and R9 each are hydrogen and one of R6 and R8 is bound via an oxygen, then the other of R6 and R8 has one of the meanings mentioned above other than H;


where one of R1 to R9 may, in addition, be a substitutent of the subformula IA







wherein one of R1′ to R9′ forms the bond to the rest of the molecule in formula I, while the others are, independently of each other, H, hydroxy, fluoro, chloro, bromo, iodo, C1-C8-alkyl, C2-C8-alkenyl, C2-C8-alkynyl, C3-C10-cycloalkyl, phenyloxy, C1-C8-alkoxy, C1-C9-alkanoyloxy, benzoyl or the radical of a C5-C12-carbohydrate bound via one of its oxygen atoms, where alkyl, alkenyl, alkynyl, cycloalkyl, phenyl, alkoxy, alkanoyloxy and benzoyl can be unsubstituted or substituted by one, two or three substituents selected independently of each other from the group consisting of —F, —Cl, —Br, —I, —OH, —OCH3, —OCH2CH3, —OCOCH3, —CHO, and —CO2H;


or two adjacent moieties of R1 to R9 and of R1′ to R9′ together form a —O—CH2—O— or a —O—CH2—CH2—O— bridge, thus forming with the two atoms to which they are bound a ring, while the other moieties are independently selected from those mentioned above;


in formula I either bond a and bond c each are a double bond, or bonds b and bond d each are a double bond, respectively;


and, if present, in subformula IA either bond a′ and bond c′ each are a double bond, or bonds b′ and bond d′ each are a double bond, respectively;


where the double bonds in formula I and, if present, subformula IA, may also be in tautomeric equilibrium (of a beta di-keto system);


X is hydrogen, oxo, hydroxy, C1-C8-alkoxy, especially methoxy, C1-C8-alkanoyloxy, especially acetyloxy, benzoyloxy or 3,4,5-trihydroxybenzoyloxy, or, if bonds a and c are double bonds in formula I and Y is oxo, can also be a moiety of the subformula IB,







wherein the waved line indicates the end of the bond where said moiety of the subformula IB is bound to the rest of the molecule of formula I and wherein

    • Y* is oxo and
    • R1* to R9* are, independently of each other, H, hydroxy, fluoro, chloro, bromo, iodo, C1-C8-alkyl, phenyloxy, C1-C8alkoxy, C1-C9-alkanoyloxy, benzoyl or the radical of a C5-C12-carbohydrate bound via one of its oxygen atoms;


      and Y is oxo, hydroxy or C1-C8-alkoxy, preferably oxo;


      a mixture of two or more compounds of the formula I, and/or an extract comprising one or more compounds of the formula I, for use in the prophylactic and/or therapeutic treatment of an animal with a (at least preferably) phosphodiesterase (PDE) dependent disease or condition of the central nervous system;


      where the compounds of the formula I may be present in free form, in the form of a pharmaceutically and/or nutraceutically acceptable salt, in the form of a tautomer, in the form of an ester and/or in the form of a solvate.


Surprisingly aurones of the formula I are found to inhibit phosphodiesterases PDE 1, PDE 3 and PDE 4, preferred compounds even being capable to inhibit them selectively (especially over other PDEs such as PDE 2, PDE5 and PDE6).


Surprisingly in the roots of Smilax myosotiflora (traditionally named as Ubi Jaga) Aurones were found in a remarkable amount. Some of these compounds were isolated and structurally characterised as shown below. This result is surprisingly new for nearly all species of the genus of Smilax, especially for those naturally grown in South East Asia.


The present invention therefore, in one embodiment, also relates to an extract, especially an extract from Smilax myosotiflora, especially its roots, comprising one or more compounds of the formula I, e.g. in an amount of 10 or more % by weight, e.g. 30 or more % by weight, such as 50 or more % by weight, for example 80 to 100% by weight.


The general expressions, within the present disclosure, preferably have the following or precedingly mentioned meanings, where in each embodiment on, more than one or all more general expressions may, independently of each other, be replaced with the more specific definitions, thus forming preferred embodiments of the invention, respectively.


Where “a compound of the formula I” or “compounds of the formula I” or the like is mentioned, this is intended to include a single compound, a mixture of two or more compounds of the formula I, and/or an extract comprising one or more compounds of the formula I, where the compounds of the formula I may be present in free form, in the form of a pharmaceutically and/or nutraceutically acceptable salt, in the form of a tautomer, in the form of an ester and/or in the form of a solvate.


Among the diseases and conditions of the nervous system to be treated prophylactically or therapeutically, neurodegenerative disorders, such as Parkinson's disease, Alzheimer's disease, age related dementia or dementia in general, neurological trauma including brain or central nervous system trauma and/or recovery therefrom, depression, anxiety, psychosis, cognitive dysfunction, mental dysfuntion, learning and memory disorders, and ischemia of the central and/or peripheral nervous systems may be mentioned. In other embodiments, the disclosed methods are used to improve cognitive outcomes and mood disorders. In one aspect, methods of modulating, such as by stimulating or increasing, neurogenesis are disclosed. In some embodiments, neurogenesis is stimulated or increased in a neural cell or tissue, such as that of the central or peripheral nervous system of an animal or human being. In cases of an animal or human, the methods may be practiced in connection with one or more disease, disorder, or condition of the nervous system as present in the animal or human subject. Thus, embodiments disclosed herein include methods of treating a disease, disorder, or condition by administering at least one neurogenesis modulating, nootropic agent of the formula I, hereinafter referred to as a “nootropic agent”. A nootropic agent may be formulated or used alone, or in combination with one or more additional neurogenic agents. Among the treatment goals are also improvement and (eg. prophylactic) support of cognitive function as well as neuroprotection in diseases states (such as Parkinson's Disease, Alzheimer's Disease, dementia).


Preferably, X is hydrogen and Y is oxo, and if present X′ is hydrogen and Y′ is oxo.


Preferably, bonds a and c in formula I are double bonds, bonds b and d single bonds, respectively, and, if present, also bonds a′ and c′ are double bonds, bonds b′ and d′ are single bonds.


Among the various possible forms of a compound of the formula I, the free form, the pharmaceutically acceptable salt form and/or the tautomer form are especially preferred. Tautomers may e.g. be represented by the formulae:







with the meanings as given in claim 1 as appropriate.


“Carbohydrate” refers to a mono or disaccharide consisting of one or two pentoses and/or hexoses optionally in their desoxy forms connected via a glycosidic bond unsubstituted or substituted with one, two, three, four or five substituents independently selected from the group consisting of methyl, ethyl, acetyl, benzoyl or 3,4,5-trihydroxybenzoyl. Examples of preferred pentoses are xylose, arabinose, and either in case when possible in the pyranosidic or furanosidic form. Examples of preferred hexoses are glucose, 6-deoxyglucose, rhamnose, and either in case when possible in the pyranosidic of furanosidic form. Examples of preferred glycosidic connections are 1→4 and 1→6.


Where salt-forming groups (e.g. acidic groups, such as phenolic OH groups) are present within them, a compound of the formula I may be in the free form or in the form of a salt. The term “salt(s)”, as employed herein, denotes basic salts formed with inorganic and/or organic bases. Pharmaceutically (or nutraceutically) acceptable (i.e., non-toxic, physiologically acceptable) salts are preferred, although other salts are also useful, e.g., in isolation or purification steps which may be employed during preparation. Salts of a compound of the formula I may be formed, for example, by reacting a compound of the formula I with an amount of base, such as an equivalent amount, in a medium such as one in which the salt precipitates or in an aqueous medium followed by lyophilization. Also ion exchangers can be used to form salts from free forms or free forms from salts of a compound of the formula I. A compound of the formula I which contain an acidic moiety may form salts with a variety of organic and inorganic bases. Exemplary basic salts include ammonium salts, alkali metal salts such as sodium, lithium, and potassium salts, alkaline earth metal salts such as calcium and magnesium salts, salts with organic bases (for example, organic amines) such as benzathines, dicyclohexylamines, N-methyl-D-glucamines, N-methyl-D-glucamides, t-butyl amines, and salts with amino acids such as arginine, lysine and the like. Also salts with salt-forming pharmaceutical and/or nutraceutical carrier materials are possible and encompassed by the invention.


Further, a compound of the formula I (in free form or as salt) may be in the form of a solvate, such as a hydrate.


Where ratios of components are given in %, this means weight %, if not indicated otherwise. By the term “extract”, either a direct extract (in liquid or preferably dried form), e.g. obtained as described below, or preferably a further enriched extract (obtainable e.g. by one or more further purification steps after extraction, e.g. chromatography, for example as described below) containing one or more, preferably two or more compounds of the formula I is meant.


Preferably, the total weight share of the compound or compounds of the formula I in an extract or mixture of compounds of the formula I or a purified compound of the formula I that is useful according to the invention in the final extract, mixture or compound (direct or further enriched) is in the range from 0.01 to 100% by weight, more preferably from 0.02 to 95%, most preferably 0.05 to 95%, from 0.05 to 50% or e.g. from 0.1 to 90%.


The extracts or compounds according to the invention may be used as such, in the form or pharmaceutical or nutraceutical formulations (the latter term including food additives) or in the form of functional food.


Where a compound or mixture of compounds of the formula I, especially extracts comprising one or more compounds of the formula I, are used as supplement, this means that the compound(s), extract or a pharmaceutical or nutraceutical formulation comprising it or them can be added to any other nutrient or pharmaceutical or nutraceutical, preferably other than (exclude especially mixtures known). Thus they can especially serve as food supplement. However, the compound(s), extract or formulations may also be administered as such. “Nutraceuticals”, “Functional Food”, or “Functional Food products” (sometimes also called “Foodsceuticals”, “Medicinal Food” or “Designer Food”) for USE according to the present invention are defined as food products (including beverages) suitable for human consumption—the expression comprises any fresh or processed food having a health-promoting and/or disease-preventing property beyond the basic nutritional function of supplying nutrients, including food made from functional food ingredients or fortified with health-promoting additives, especially with effects in the prophylaxis or treatment of a disease or disorder as mentioned herein, that is, a compound of the formula I is used as an ingredient (especially additive) as health benefit agent, especially in an effective amount.


“Comprising” or “including” or “having” wherever used herein is meant not to be limiting to any elements stated subsequently to such term but rather to encompass one or more further elements not specifically mentioned with or without functional importance, that is, the listed steps, elements or options need not be exhaustive. In contrast, “containing” would be used where the elements are limited to those specifically after “containing”.


Where “about” is used or a specific numerical value is given without explicitly mentioning “about”, this preferably means that a given value may deviate to a certain extent from the value given, e.g. preferably by ±20% of the given numerical value, more preferably by ±10%, e.g. in one embodiment ±5%. Where numerical ranges are given, also where it is not mentioned “about” is present before any numbers.


The functional food products or pharmaceutical products may be manufactured according to any suitable process, preferably comprising extraction of one or more compounds of the formula I and admixing to a functional food product or at least one nutraceutically or pharmaceutically acceptable carrier.


Preferably, a functional food or a pharmaceutical or nutraceutical formulation comprising a compound, more preferably a compound mixture, useful according to the present invention, can be obtained by


(a) extraction of one or more compounds and/or mixture of compounds of the formula I from one or more plants of the genera mentioned below, especially from Smilax myosotiflora (and there especially from the roots); and


(b) mixing the resulting one or more compounds and/or mixtures of compounds as active ingredient in the preparation of the functional food product with the other constituents thereof or in order to obtain a pharmaceutical or nutraceutical formulation with one or more carrier materials or with a solvent, e.g. water or an aqueous solvent (e.g. to give a juice or dispersion or solution).


Further processing steps may precede and/or follow, such as drying (e.g. freeze-drying, spray-drying and evaporation), granulation, agglomeration, concentrating (e.g. to syrups, formed via concentration and/or with the aid of thickeners), pasteurizing, sterilizing, freezing, dissolving, dispersing, filtering, centrifuging, confectioning, and the like.


When one or more compounds and/or a compound mixture or an extract according to the invention are added to a food product or pharmaceutical or nutraceutical, this also results in a functional food product or pharmaceutical or nutraceutical formulation according to the invention.


Preferably, a functional food product according to the invention comprises 0.01 to 30, e.g. 0.02 to 20, such as preferably 0.05 to 5, weight-% of a compound or mixture of compounds of the formula I or of an (especially further enriched) extract according to the invention, the rest being food and/or nutraceutically acceptable carriers and/or customary additives. Further additives may be included, such as vitamins, minerals, e.g. in the form of mineral salts, unsaturated fatty acids or oils or fats comprising them, other extracts, or the like. The functional food products according to the invention may be of any food type. They may comprise one or more common food ingredients in addition to the food product, such as flavours, fragrances, sugars, fruit, minerals, vitamins, stabilisers, thickeners, dietary fibers, protein, amino acids or the like in appropriate amounts, or mixtures of two or more thereof, in accordance with the desired type of food product.


Examples of basic food products and thus of functional food products according to the invention are fruit or juice products, such as orange and grapefruit, tropical fruits, banana, apple, peach, blackberry, cranberry, plum, prune, apricot, cherry, peer, strawberry, marionberry, black currant, red currant, tomato, vegetable, e.g. carrot, or blueberry juice, soy-based beverages, or concentrates thereof, respectively; lemonades; extracts, e.g. coffee, tea, green tea; dairy type products, such as milk, dairy spreads, quark, cheese, cream cheese, custards, puddings, mousses, milk type drinks and yoghurt; frozen confectionary products, such as ice-cream, frozen yoghurt, sorbet, ice milk, frozen custard, water-ices, granitas and frozen fruit purees; baked goods, such as bread, cakes, biscuits, cookies or crackers; spreads, e.g. margarine, butter, peanut butter honey; snacks, e.g. chocolate bars, muesli bars; pasta products or other cereal products, such as muesli; ready-to-serve-dishes; frozen food; tinned food; syrups; oils, such as salad oil; sauces, such as salad dressings, mayonnaise; fillings; dips; chewing gums; sherbet; spices; cooking salt; instant drink powders, such as instant coffee, instant tee or instant cocoa powder; instant powders e.g. for pudding or other desserts; or the like.


One or more other customary additives may be present, such as flavour, fragrances or other additives, such as one or more selected from stabilizers, e.g. thickeners; colouring agents, such as edible pigments or food dyes; bulking agents, such as fruit pulp, e.g. in dried form; polyols, such as xylitol, mannitol, maltitol or the like; preservatives, such as sodium or potassium benzoate, sodium or calcium carbonate or other food grade preservatives; antioxidants, such as ascorbic acid, carotionoids, tocopherols or polyphenols; mono-, oligo- or polysaccharides, such as glucose, fructose, sucrose, soy-oligosaccharides, xylo-oligosaccharides, galacto-oligosacharides; other artificial or natural non- or low-caloric sweeteners, such as aspartame or acesulfame; bitterness blockers; acidifiers in the form of edible acids, such as citric acids, acetic acid, lactic acid, adipic acid; flavours, e.g. artificial or natural (e.g. botanical flavours); emulsifiers; thiols, e.g. allylic thiols; diluents, e.g. maltodextrose; wetting agents, e.g. glycerol; stabilizers; coatings; isotonic agents; absorption promoting or delaying agents; and/or the like.


The one or more compounds of the formula I or compound mixtures thereof or extracts comprising them according to the invention can also be comprised in confectioned formulations to be added to foods including beverages, e.g. in the form of powders or granules, e.g. freeze-dried or spray-dried, concentrates, solutions, dispersions or other instant form, or the like.


The pharmaceutical or nutraceutical formulation (=compositions) according to the present invention can be prepared in various forms, such as granules, tablets, pills, syrups, solutions, dispersions, suppositories, capsules, suspensions, salves, lotions and the like. Pharmaceutical grade or food grade organic or inorganic carriers and/or diluents suitable for oral and topical use can be used to formulate compositions containing the therapeutically-active compounds. Diluents known in the art include aqueous media, vegetable and animal oils and fats. Stabilizing agents, wetting and emulsifying agents, salts for varying the osmotic pressure or buffers for securing an adequate pH value, and skin penetration enhancers can be used as auxiliary agents. The compositions may also include one or more of the following: carrier proteins such as serum albumin; buffers; fillers such as microcrystalline cellulose, lactose, corn and other starches; binding agents; sweeteners and other flavouring or fragrancing agents; coloring agents; and polyethylene glycol. Those additives are well known in the art, and are used in a variety of formulations.


By “administered” herein is meant administration of a prophylactically and/or therapeutically effective dose of a compound of the formula I or a mixture of compounds of the formula I, or an extract comprising one or more of them, to an animal, especially a patient. By “therapeutically effective dose” herein is meant a dose that produces the effects for which it is administered, especially an ameliorative or therapeutic effect on PDE dependent diseases or conditions of the central nervous system, more especially on Parkinson's Disease, Alzheimer's Disease and dementia.


The pharmaceutical composition or a nutraceutical according to the present invention is suitable for administration intravenously, intraperitoneally, subcutaneously, intramuscularly, intrathecally, orally, rectally, topically, or by inhalation.


An animal or human, especially being a “patient” or “subject” for the purposes of the present invention, includes especially humans and further other (especially warm-blooded) animals. Thus, the compound of the formula I or a mixture of compounds of the formula I, or an extract comprising one or more of them, are applicable to both humans and animals. In the preferred embodiment the patient is a human. The patients will be treated either in a prophylactic or therapeutic intention.


Typically, the compound of the formula I or a mixture of compounds of the formula I, or an extract comprising one or more of them, having therapeutical activity mentioned hereinbefore may be administered with at least one physiologically (=pharmaceutically or nutraceutically) acceptable carrier to a patient, as described herein. The total concentration of therapeutically active compound of the formula I or a mixture of compounds of the formula I or extracts comprising them in the formulation may vary from about 0.001-100 wt %, e.g. from 0.1 to 50% by weight, the rest being the carrier material(s) and/or customary additives.


The compound of the formula I or a mixture of compounds of the formula I or extracts comprising them may be administered alone or in combination with other treatments, i.e., other nootropic agents.


Combination does not necessarily mean a fixed combination but may also mean that the compound(s) of the formula I or the extract comprising it or them may be administered in a chronically staggered manner with the combination partner(s), e.g. in the form of a kit of parts (which also is an embodiment of the invention) with other combination partners, other than those excluded hereinbefore. Preferably, the chronically staggered administration takes place such that the combination partners mutually influence, especially intensify (e.g. by way of an additive or preferably synergistic effect) their therapeutic efficiency.


Other helpful drugs or active agents may be administered, e.g. psychoactive agents, agents that help in the treatment of addictive behaviour, e.g. nicotine addiction, or the like, especially in so far as they help to support the prophylaxis or treatment according to the invention intended.


The dosage in both nutraceutical or pharmaceutical use typically is such that the amount of the compound(s) of the formula I administered to a patient is such that it is effective in inhibition of PDE, or preferably a daily dose of about 0.2 to 1000 g, e.g. 0.5 to 5 g is administered to a person with a weight of 70 kg per day in one or more, e.g. 1 to 3, dosages (children or persons with differing weights receive a correspondingly modified dosage).


Extracts comprising one or more compounds of the formula I can be prepared from plants as mentioned above or below or plant parts.


The following list provides possible sources without being limited to this list of compounds of the formula I or extracts comprising among others:


1. List of all Smilax:


S. aberrans, S. acanthophylla, S. aculeata, S. aculeatissima, S. acuminata, S. acutifolia, S. adhaerens, S. aequatorialis, S. alba, S. alpini, S. altissima, S. amaurophlebia, S. amblyobasis, S. ampla, S. anamitica, S. anceps, S. anguina, S. angustifolia, S. annamensis, S. annua, S. argyraea, S. argyrea, S. arisanensis, S. aristolochiaefolia, S. aristolochiifolia, S. asparagoides, S. aspera, S. aspero-variabilis, S. astrosperma, S. auraimensis, S. auriculata, S. australis, S. austrosinensis, S. austrozhejiangensis, S. balansaeana, S. balbisiana, S. balearica, S. banglaoensis, S. bapouensis, S. barbata, S. barbillana, S. basilata, S. bauhinioides, S. bella, S. benthamiana, S. bermudensis, S. bernhardi, S. berteroi, S. beyrichii, S. biflora, S. biltmoreana, S. biumbellata, S. blancoi, S. blinii, S. blumei, S. bockii, S. bodinieri, S. bona-nox, S. bonii, S. boninensis, S. borbonica, S. borneensis, S. botteri, S. botterii, S. brasiliensis, S. brevipes, S. caduca, S. calaris, S. califormica, S. calocardia, S. calophylla, S. cambodiana, S. campestris, S. canaliculata, S. canariensis, S. candelariae, S. canellaefolia, S. capitata, S. castaneiflora, S. catalonica, S. caudata, S. cavaleriei, S. celebica, S. cercidifolia, S. ceylanica, S. chapaensis, S. chiapensis, S. chimantensis, S. china, S. chingii, S. chiriquensis, S. ciliata, S. cinerea, S. cinnamomes, S. cinnamomifolia, S. cinnamomiifolia, S. cinnamommea, S. cissoides, S. cocculoides, S. cognata, S. collina, S. colossea, S. colubrina, S. columnifera, S. compressa, S. conchipes, S. conferta, S. corbularia, S. corcovadensis, S. cordato-ovata, S. cordifolia, S. coriacea, S. coriifolia, S. cumanensis, S. cuspidata, S. cyclophylla, S. cynanchifolia, S. cynodon, S. darrisii, S. davidiana, S. decipiens, S. deltifolia, S. densibarbata, S. densiflora, S. dentata, S. dilatata, S. discolor, S. discotis, S. divaricata, S. diversifolia, S. domingensis, S. dominguensis, S. duidae, S. dulcis, S. dunniana, S. ecirrata, S. ecirrhata, S. ehrenbergiana, S. elastica, S. elegans, S. elegantissima, S. elliptica, S. elmeri, S. elongato-reticulata, S. elongato-umbellata, S. emeiensis, S. engelmanniana, S. engleriana, S. erythrocarpa, S. eucalyptifolia, S. excelsa, S. extensa, S. farinosa, S. febrifuga, S. ferox, S. ficifolia, S. fistulosa, S. flaccida, S. flavescens, S. flavicaulis, S. flexuosa, S. floribunda, S. fluminensis, S. fokiensis, S. fooningensis, S. formosana, S. fulgens, S. gagnepainii, S. gaudichaudiana, S. gaultheriifolia, S. gaumeri, S. gaumerii, S. gemina, S. gentlei, S. gigantocarpa, S. gilva, S. glabra, S. glauca, S. glaucocarpos, S. glaucochina, S. glauco-china, S. glaucophylla, S. globifera, S. globulifera, S. glyciphylla, S. glycyphylla, S. goetzeana, S. goudotiana, S. goyazana, S. graciliflora, S. gracillima, S. grand flora, S. grandifolia, S. grandis, S. griffithii, S. guianensis, S. guiyangensis, S. gymnopoda, S. hastata, S. havanensis, S. hawaiensis, S. hayatae, S. hederaefolia, S. helferi, S. hemsleyana, S. herbacea, S. heterophylla, S. higoensis, S. hilariana, S. hirsutior, S. hohenackeri, S. hongkongensis, S. hookeri, S. horrida, S. horridiramula, S. hostmanniana, S. hugeri, S. humilis, S. hypoglauca, S. ilicifolia, S. illinoensis, S. immersa, S. impressinervia, S. incerta, S. indica, S. indosinica, S. inermis, S. insignis, S. intricatissima, S. invenusta, S. inversa, S. iriomotensis, S. irrogata, S. irrorata, S. jacquini, S. jacquinii, S. jalapensis, S. jamesii, S. japicanga, S. japonica, S. jauaensis, S. javensis, S. jiankunii, S. kainantensis, S. kaniensis, S. kerberi, S. keyensis, S. klotzschii, S. korthalsii, S. kraussiana, S. krukovii, S. kunthii, S. kwangsiensis, S. labidurommae, S. labordei, S. laevis, S. lamarensis, S. lancaefolia, S. lanceaefolia, S. lanceifolia, S. lancifolia, S. lappacea, S. larvata, S. lasioneura, S. lasioneuron, S. lasseriana, S. law, S. latifolia, S. latipes, S. laurifolia, S. laurina, S. lebrunii, S. lessertiana, S. leucocarpa, S. leucophylla, S. ligustrifolia, S. liukiuensis, S. loheri, S. lomoplis, S. longebracteolata, S. longifolia, S. longipedunculata, S. longipes, S. loupouensis, S. luculenta, S. lundellii, S. lunglingensis, S. lushuiensis, S. luteocaulis, S. lutescens, S. luzonensis, S. macabucha, S. macalucha, S. maclurei, S. macrocarpa, S. macrophylla, S. macropoda, S. maculata, S. magnifolia, S. mairei, S. malipoensis, S. marginata, S. marginulata, S. maritima, S. martini, S. mauritanica, S. maximowiczii, S. maypurensis, S. mazatlanensis, S. mcclurei, S. medica, S. medicinalis, S. megacarpa, S. megalantha, S. megalophylla, S. melanocarpa, S. melastomifolia, S. membranacea, S. mengmaensis, S. menispermoidea, S. mexicana, S. micro-china, S. microphylla, S. micropoda, S. microscola, S. milleri, S. minarum, S. minutiflora, S. modesta, S. mollis, S. montana, S. montevidensis, S. moranensis, S. morongii, S. morsaniana, S. mossambicensis, S. multiflora, S. munda, S. munita, S. muricata, S. muscosa, S. myosotiflora, S. myrtillus, S. nageliana, S. nana, S. nantoensis, S. narcotica, S. nebelii, S. neocaledonica, S. neo-calcdonica, S. nervo-marginata, S. nigra, S. nigrescans, S. nipponica, S. nitida, S. nova-guineensis, S. obliqua, S. obliquata, S. oblonga, S. oblongata, S. oblongifolia, S. obtusa, S. occidentalis, S. ocreata, S. odontolama, S. odontoloma, S. odoratissima, S. officinalis, S. oldhami, S. oldhamii, S. opaca, S. orbiculata, S. ornata, S. orthoptera, S. osmastonii, S. outanscianensis, S. ovalifolia, S. ovata, S. ovatolanceolata, S. ovato-rotunda, S. oxycarpa, S. oxyphylla, S. pachysandroides, S. pallescens, S. panamensis, S. pandurata, S. panduriformis, S. paniculata, S. papuana, S. papyracea, S. parviflora, S. parvifolia, S. pavoniana, S. peduncularis, S. peguana, S. pekingensis, S. pendulina, S. perfoliata, S. pertenuis, S. perulata, S. petelotii, S. petiolatumida, S. phyllantha, S. phyllobola, S. picta, S. pilcomayensis, S. pilosa, S. pinfaensis, S. pirarensis, S. pittieriana, S. plani-peduncula, S. planipes, S. platoplis, S. platycentron, S. platyphylla, S. plurifurcata, S. poeppigii, S. pohliana, S. poilanei, S. poiretii, S. polyantha, S. polycephala, S. polycolea, S. populnea, S. pottingeri, S. pringlei, S. procera, S. prolifera, S. pruinosa, S. pseudochina, S. pseudo-china, S. pseudo-sarsa, S. pseudosyphilitica, S. pseudo-syphilitica, S. pteropus, S. pubens, S. pubera, S. puberula, S. pulverulenta, S. pumila, S. purampui, S. purhampuy, S. purpurata, S. purpusii, S. purtrampui, S. pygmaea, S. quadrangularis, S. quadrangulata, S. quadrata, S. quadrumbellata, S. quinquenervia, S. ramiflora, S. ramonensis, S. randaiensis, S. regelii, S. remotinervis, S. renifolia, S. reniformis, S. reticulata, S. retroflexa, S. rettiana, S. retusa, S. rhombifolia, S. riedeliana, S. rigida, S. riparia, S. ripogonum, S. ripponica, S. robert-kingii, S. robusta, S. rotundiflora, S. rotundifolia, S. roxburghiana, S. roxburghii, S. rubiginosa, S. rubra, S. rubriflora, S. rubromarginata, S. rufa, S. rufescens, S. ruizana, S. ruiziana, S. sadoensis, S. sagittaefolia, S. sagittata, S. sagittifera, S. sagittifolia, S. salicifolia, S. salutaris, S. sanguinea, S. santaremensis, S. sarsaparilla, S. sarumame, S. saulensis, S. saxicola, S. scabriuscula, S. scalaris, S. schaffneriana, S. schafneriana, S. schiedeana, S. schlechtendalii, S. schombiurgkiana, S. schomburgkiana, S. scobinicaulis, S. sebeana, S. selloana, S. semiamplexicaulis, S. sempervirens, S. senticosa, S. setiramula, S. setosa, S. shuttleworthii, S. siamensis, S. siderophylla, S. sieboldi, S. sieboldii, S. simadai, S. simulans, S. sinclairi, S. singaporensis, S. siphilitica, S. smalli, S. smallii, S. solanifolia, S. spicata, S. spinescens, S. spinosa, S. spinulosa, S. spissa, S. sprengelii, S. spruceana, S. staminea, S. standleyi, S. stans, S. stemonifolia, S. stenophylla, S. stipulacea, S. subaculeata, S. subarmata, S. subpubescens, S. subsessiliflora, S. surinamensis, S. sylvatica, S. synandra, S. syphilitica, S. syringoides, S. taiheiensis, S. takaoensis, S. talbotiana, S. tamnoides, S. taquetii, S. telfaireana, S. tenuis, S. tenuissima, S. tetragona, S. tetraptera, S. thomsoniana, S. tijucensis, S. timorensis, S. tomentosa, S. tonduzii, S. tongaensis, S. tortopetiolata, S. tortuosa, S. trachyclada, S. trachypoda, S. trifurcata, S. trigona, S. trinervula, S. trukensis, S. tsaii, S. tsinchengshanensis, S. tuberculata, S. turbans, S. umbellata, S. umbellifera, S. umbrosa, S. undulata, S. uruapensis, S. utilis, S. vaga, S. vaginata, S. vanchingshanensis, S. vanilliodora, S. variabilis, S. variegata, S. velutina, S. venosa, S. verticalis, S. vicaria, S. villandia, S. viminea, S. virginiana, S. viscifolia, S. vitiensis, S. wagneriana, S. wallichii, S. walteri, S. watsonii, S. wightii, S. williamsi, S. williamsii, S. willkommii, S. woodii, S. xalapensis, S. yai, S. yui, S. yunnanensis, S. zeylanica, S. zollingeri, S. polyacantha, S. gigantea, S. kingii.


Including plants named with their traditional name as:


Sarsaparilla, Greenbriar, Catbriar, Horsebriar, Bullbirar, Ubi Jaga, Ubi Besi, Akar Ali, Akar Ding, Akar Tanding, Akar Restong, Kerating, Manto.
2. List of Smilax in SE Asia:


S. blumei, S. calophylla, S. china, S. corbularia, S. extensa, S. gigantea, S. glabra, S. helferi, S. kingii, S. laevis, S. lanceifolia, S. leucophylla, S. luzonensis, S. macrocarpa, S. megacarpa, S. myosotiflora, S. polyacantha, S. verticalis, S. walteri, S. woodii, S. zeylanica


Ubi Jaga, Ubi Besi, Akar Ali, Akar Ding, Akar Tanding, Akar Restong, Kerating, Manto, (which are all synonyms for Smilax myosotiflora), Akar dawai, dawai dawai, sedawai, akar kancil(which are all synonyms for Smilax calophylla), Radix Chinae, China Root, Gadong China, Gadong Saberang, Akar Restong, Ubat Raja, Akar Resting, Chinese Sarsaparilla, Peundang (which are all synonyms for Smilax china and Smilax ferox), Ubi Danau or Danai, Akar Banar, Channar Bokor, Sarsaparillang-Puti, Banag, Kaguno, Wanabekira (which are all synonyms for Smilax leucophylla), Akar Banar, Banar Babi, Chanar Babi, Akar Kelona Betina, Semenjoh, Akar Gadong Tikus, Gadong Jantan (which are all synonyms for Smilax helferi and Smilax luzonensis), Akar Kelona, Akar Banar, Akar Rebanar, Akar Beruboh, Akar Lampu Bukit, Chanar Bokor, Chanar Gede, Chanar Gengge, Chanar Minyak (which are all synonyms for Smilax megacarpa), Canar Bokor, Canar Gede, Canar Minyak (which are all synonyms for Smilax macrocarpa), Koh Kong, Xieng Khouang, Hua Khaao-yen wok (which are all synonyms for Smilax carbularia), Koh Kong, Yaa Hua (which are all synonyms for Smilax glabra), Dao, Naam Dao, Thao Yang Dong, Kim Cang (which are all synonyms for Smilax lanceifolia), Akar Banar, Akar Gadung Tikus, Banar Babi, Khueang, Yaan That, Faa Laep (which are all synonyms for Smilax luzonensis), Akar Ali, Akar Tanding, Akar Dedingin, Akar Restong, Itah Besi, Ubi Besi, Keleh, Ali Bertinggong, Manto (which are all synonyms for Smilax myosotiflora), Voe Me, Khrua Daao, Kim Chang (which are all synonyms for Smilax verticalis and Smilax simulans), Kayu Cina Utan, Saihe Maruani, Asaihe Tuni (which are all synonyms for Smilax zeylanica).


3. Smilax myosotiflora or Ubi Jaga (especially preferred).


Plant parts are, e.g., leaves, bark, flowers, buds, fruits, stems, shoots, roots, tubers or other parts of plants, and they or the plants can be complete, hackled, crushed, chopped up, broken up, homogenized, dried, fermented or treated otherwise. Roots are especially preferred.


A compound the formula I or a mixture of compounds of the formula I, or an extract comprising one or more of them, of the present invention can be prepared by extracting and preferably enriching up to isolating them from the plants or parts of plants. Auxiliary means such as (especially ultrasonic) sonication, heating (e.g. to temperatures from room temperature to 50° C.), stirring, re-extraction, evaporation or the like, may be used to allow for appropriate extraction.


Extraction preferably takes place with a non polar or more preferably a polar solvent or solvent mixture, e.g. water and/or an alcohol, such as ethanol, and/or with a liquid gas, especially superfluid CO2.


Preferably, the extracts can subsequently be further enriched by one or more additional purification steps, such as distribution (especially into an apolar solvent, such as an alkane and/or an ester, e.g. n-heptane and ethyl acetate), precipitation (e.g. crystallisation) or chromatography, by which it is possible to obtain further enriched extracts or isolated compounds of the formula I.


In order to optimize the production of the compound of the formula I, e.g. aurones, after one or more extraction steps, a liquid-liquid extraction procedure can be employed. Liquid-liquid extraction, also known as solvent extraction or solvent partitioning, is a method to separate compounds based on their relative solubilities in two different immiscible liquids, preferably not or only partially miscible, usually water and an organic solvent. This way a desired substance or substance mixture can be extracted from one first liquid phase into another liquid phase or remain in the first phase, while less desired substances remain in the other phase, respectively. It is also possible to influence the distribution by establishing specific conditions in the solvents used for partition, such as acidic, neutral or basis conditions. Thus, e.g., less polar molecules or polar neutralized acids or basis can be induced to distribute into the less polar solvent, charged or otherwise polar molecules, such as the dissociated acids or bases preferably can be directed into the more polar solvent. Liquid-liquid extraction is a basic technique in chemical laboratories, where it is preferably performed using a separatory funnel.


For the enrichment of phytochemicals from a crude plant extract, usually the concentrated extract, is partly dissolved in water or solvent-containing water (solvents here are co-solvents, for example methanol, ethanol, propanol, isopropanol, acetone, acetonitrile or other water-miscible solvents) and extracted once or successively with identical or different water-immiscible solvents or solvent mixtures, preferably not or only partially miscible, in the case of successively used different water-immiscible or partially water-miscible solvents, successively using solvents of e.g. increasing polarity (for example, without that this is intended to exclude other alternatives known to the person skilled in the art, in the order of; 1. heptane, hexane, pentane, cyclohexane, petroleum ether; 2. diethyl ether, toluene, benzene, t-butyl methyl ether, chloroform, dichloromethane, ethyl methyl ketone, dioxane, tetrahydrofuran; 3. ethyl acetate).


Further, surprisingly it could be shown that an improved yield can be obtained when an extraction and purification process is used that avoids strongly alkaline (e.g. pH 9 or larger) and strongly acidic conditions (e.g. pH 1.8 or lower) conditions—without being bound to this theory, a possible explanation may be that the compounds of the formula I might be prone to degradation, such as hydrolysis under too alkaline conditions.


Therefore a preferred procedure for the extract production has been found that, in particular, addresses various specific aspects:

    • a) the extraction yield of the aurones is strongly dependent on the pH conditions adjusted in the water phase(s) in the extraction process. This is especially important and thus preferred in a first liquid/liquid separation step;
    • b) with a second liquid/liquid separation step, which preferably again comprises a specific pH adjustment, “undesired compounds”, such as homopanthothenic acid, are eliminated to a wide extent, e.g. in the case of homopanthothenic acid even quantitatively. This allows to reduce or eliminate undesired components and thus to diminish e.g. the risk of undesired side effects or toxic components.
    • c) Parallel to the elimination of undesired material found after the first and the second extraction step, a further enrichment of the compounds of the formula I (and thus aurones) has been achieved.


Especially the adjustment of the pH at which the initial extraction and the following first liquid/liquid separation step has surprisingly been found to be of high importance for the overall yield of the compounds of the formula I (aurones). In a series of experiments, the pH of the added water (added to the ethanol) has been adjusted to various pH values, e.g. to pH 1, pH 2, pH 3 and pH 4.5. The optimum yield was achieved at about pH 2 followed by about pH 3 (similar yield), followed by about pH 4.5 (50% decrease of yield). In parallel the absolute content of the aurones in the ethyl acetate phases of the first liquid/liquid separation step was found to be highest at about pH 2. At pH 1 respectively, no yield or content could be determined, presumably and according to analytical results since virtually complete decomposition of the aurones took place.


The compounds of the formula I, e.g. Aurones therefore preferably are extracted from the plant material (e.g. S. myosotiflora) and subjected to a first liquid/liquid extraction under acidic conditions, respectively, which is what a preferred embodiment of the extraction and purification process according to the invention comprises. The preferred pH is in the range of about 2 to about 4.5, more preferred pH is about 2 to about 3, and the most preferred pH is about 2. The aurones/compounds of the formula I are here enriched preferably in the less polar solvent phase.


The pH conditions in a subsequent second liquid/liquid separation step have also been varied to provide opportunity to eliminate “undesired compounds” (such as homopanthothenic acid), and the pH value of the water phase in the liquid/liquid separation system has been found to be preferably about neutral to slightly alkaline, e.g. about 7 or larger. A preferred pH range is about 7 to about 9, and a most preferred pH is 7.4 to 7.6. The aurones/compounds of the formula I are here enriched preferably in the less polar solvent phase.


Thus, in one aspect the present invention also relates to an extraction and purification (or at least enrichment) process comprising an extraction step from a plant or plant parts and a first liquid/liquid separation step under acidic conditions, respectively, as described above or below, and a subsequent second liquid/liquid extraction of the material found in the less polar phase of the first extraction step, preferably under neutral to slightly alkaline conditions mentioned above or e.g. in the examples, in particular as mentioned to be preferred, yielding a purified product from the less polar phase also in the second extraction step. Further liquid/liquid partition or other purification may follow and can lead to yet more pure product. Alternatively, further purification to yield enriched mixtures of few compounds of the formula I or pure compounds of the formula I is added, e.g. by chromatographic methods, e.g. as shown in the Examples.


Where “useful” is mentioned, this especially refers to one or more of the following embodiments of the invention which can be inserted wherever “useful” is mentioned:


(1) A compound of the formula I, or a mixture of compounds of the formula I, or especially a (preferably further enriched) extract comprising one or more compounds of the formula I, for use in therapeutic (including prophylactic) treatment of an animal, preferably a mammal, especially a human, for the treatment of a phosphodiesterase (PDE) dependent disease or condition of the central nervous system, especially a disease mentioned as preferred;


(2) A pharmaceutical or nutraceutical composition comprising a compound of the formula I, or a mixture of compounds of the formula I, or especially a (preferably further enriched) extract comprising one or more compounds of the formula I, as active ingredient together with a pharmaceutically acceptable diluent or carrier, especially for use in the therapeutic and/or prophylactic treatment mentioned under (1).


(2′) A pharmaceutical or nutraceutical composition for the treatment as mentioned under (1) comprising a compound of the formula I, or a mixture of compounds of the formula I, or especially a (preferably further enriched) extract comprising one or more compounds of the formula I, and a pharmaceutically acceptable diluent or carrier, as active ingredient supplement to a food.


(3) A functional food comprising a compound of the formula I, or a mixture of compounds of the formula I, or especially a (preferably further enriched) extract, as active ingredient for the treatment as mentioned under (1).


(4) A method for the treatment as mentioned under (1), in a subject in need of such treatment, comprising administering a pharmaceutically or nutraceutically effective amount of a compound of the formula I, a mixture of compounds of the formula I, or a (preferably further enriched) extract comprising one or more compounds of the formula I, as active ingredient.


(5) The use of a compound of the formula I, or a mixture of compounds of the formula I, or a (preferably further enriched) extract comprising one or more compounds of the formula I, as active ingredient for the manufacture of a medicament or nutraceutical or food supplement for the treatment mentioned under (1).


(6) A method or use as defined under (4), comprising co-administration, e.g. concomitantly or in sequence, of a therapeutically effective amount of compound of the formula I, or a mixture of compounds of the formula I, or a (preferably further enriched) extract comprising one or more compounds of the formula I, as active ingredient and a different pharmaceutically active compound and/or a pharmaceutically acceptable salt thereof, said different pharmaceutically active compound and/or salt thereof being especially for use in the treatment as mentioned under (1).


(7) A combination product comprising a therapeutically effective amount of a compound of the formula I, or a mixture of compounds of the formula I, or a (preferably further enriched) extract comprising one or more compounds of the formula I, as active ingredient, and a different pharmaceutically active compound and/or a pharmaceutically acceptable salt thereof, said second pharmaceutically active compound being especially for use or of use in the treatment mentioned under (1).


For any of the uses, the use is such that the compound(s) of formula I or the extract comprising such compound(s) of the formula I are the active ingredient, that is, they are already alone capable of achieving the intended effect.


By “administering” herein is especially meant administration of a therapeutically effective dose of a compound of the formula I, or a mixture of compounds of the formula I, to a cell either in cell culture or especially to an animal, especially a human patient. By “therapeutically effective dose” herein is preferably meant a dose that produces the effects for which it is administered.


The pharmaceutical or nutraceutical preparations may be sterilized and/or may contain carrier materials or adjuvants such as preservatives, stabilizers, binders, disintegrants, wetting agents, skin or mucuous membrane penetration enhancers, emulsifiers, salts for varying the osmotic pressure and/or buffers, or other ingredients, excipients or carrier materials known in the art.





BRIEF DESCRIPTION OF THE FIGURES


FIG. 1: workflow diagram, isolation procedure.



FIG. 2: HPLC-UV-MS-ELSD analysis of an Ethyl acetate extract of Smilax myosotifolia.



FIG. 3: Typical UV spectrum of an aurone.



FIG. 4: 1H NMR spectrum of SM 29 (3) (DMSO-d6, 500 MHz).



FIG. 5: 1H NMR spectrum of SM 30 (3) (DMSO-d6, 500 MHz).





PREFERRED EMBODIMENTS

A compound of the formula I, e.g. the compound, compound mixture or an extract comprising one or more compounds of the formula I is preferably useful in the treatment of a disease as mentioned that depends on the activity of any one or more of PDE1, PDE3 and PDE4.


Whether a compound is effective here is defined as follows: It shows PDE inhibition in at least one of the assays as shown below in the Examples. “Dependent on PDE” thus means that PDE inhibition contributes to amelioration or even cures regarding the symptoms of the disease, thus preferably meaning “responding” to PDE inhibition.


Preferably a compound of the formula I is useful in the treatment of neurodegenerative disorders, such as Parkinson's disease, Alzheimer's disease, age related dementia or dementia in general.


Alternatively, a compound of the formula I is preferably useful in the treatment of neurological trauma including brain or central nervous system trauma and/or recovery therefrom, and/or ischemia of the central and/or peripheral nervous systems.


Yet alternatively, a compound of the formula I is preferably useful in the treatment of depression, anxiety, psychosis, cognitive dysfunction, mental dysfuntion, learning and memory disorders.


Yet alternatively, a compound of the formula I is preferably useful to improve cognitive outcomes and mood disorders.


Yet alternatively, a compound of the formula is preferably useful for modulating, such as stimulating or increasing, neurogenesis and glial function, e.g. in a neural cell or tissue, such as that of the central or peripheral nervous system of an animal or human being. Additionally a compound of the formula I is preferably useful for modulating, such as protecting of stabilizing, neuronal and glial function and CNS homeostasis.


In yet another alternative, a compound of the formula I is preferably useful as a “nootropic agent”.


A compound of the formula I may be used alone, or in combination with one or more additional neurogenic agents. Among the treatment goals are also improvement and (eg. prophylactic) support of cognitive function as well as neuroprotection in diseases states (such as Parkinson's Disease, Alzheimer's Disease, dementia).


Preferably, a compound of the formula I is a natural compound, that is, a compound that is present in and can be isolated or extracted from natural sources (especially those mentioned in detail) without chemical synthesis steps (though it may also be prepared by chemical synthesis), and not a derivative only obtainable by chemical synthesis.


Preferred are also the embodiments of the invention given in the claims, which are incorporated into the present description by reference, and especially in the examples.


In yet another alternative, the present invention relates to an extract from Smilax myosotiflora, especially from its roots, comprising a compound of the formula I described above withouth the proviso, and embodiments claiming a usefulness as described above. In a more preferred embodiment, also the proviso given under formula I may be present in the embodiments of the last paragraph that if R1, R3 and R7 each are hydroxyl, R2, R4, R5 and R9 each are hydrogen and one of R6 and R8 is bound via an oxygen, then the other of R6 and R8 has one of the meanings mentioned above other than H.


The present invention preferably does not relate to the use of compounds of the formula







as defined in WO 2001/055218 as antioxidant, radical scavenging, immunoprotective, protecting Langerhans cells, protecting DNA and RNA inhibitors of histidine decarboxylase, protein kinases, elastase, aldose reductase or hyaluronidase, where the disease is not PDE dependent, or more preferably of said diseases in general with said compounds.


Patent applications and other references, where mentioned, are included herein by reference, especially regarding the passages defining compounds and/or uses.


The mentioning or published documents does not constitute an admission that these are prior art.


The present invention especially does not relate to a disease which is not PDE dependent (meaning that PDE activity is at least contributing to the disease, e.g. to the symptoms) in the prophylactic and/or therapeutic treatment.


The following examples illustrate the invention without limiting its scope.


EXAMPLES
Example 1
Preparation of Crude Extracts

1960 g of Smilax myosotiflora roots (SM) were ground into a powder using a lab mill and afterwards extracted at room temperature with 4000 ml 95% Ethanol twice by using ultrasonic. The solution was separated from the remaining material and concentrated under reduced pressure. The remaining water phase was added with water to a final volume of 400 ml and subsequently extracted with n-heptane and Ethyl acetate by liquid/liquid separation. The n-heptane extract (SM 1 (1) was dried (Na2SO4) and the solvent evaporated under reduced pressure. The remaining water phase was extracted with Ethyl acetate for three times. The three Ethyl acetate extracts were combined (SM 1 (2)), dried (Na2SO4) and the solvent evaporated under reduced pressure. The remaining water phase (SM 1 (3)) was also evaporated under reduced pressure and the amounts for the three crude extracts were determined:


















Plant
SM-No
Phases
Amount










S. myosotiflora

SM 1 (1)
n-Heptane
4.8 g




S. myosotiflora

SM 1 (2)
Ethyl acetate
8.0 g




S. myosotiflora

SM 1 (3)
Water
28.2 g 










SM 1 (2) was selected as starting material for isolation of pure compounds.


Example 2
Preparation of Pure Compounds

The initial separation steps were performed as MPLC (procedure 3, 9 and 10) separations on reverse phase material (Macherey & Nagel, Dueren, Germany). For the separation of the single compounds in preparative scale a HPLC-setup was used comprising reverse phase separation columns (all provided by Macherey & Nagel, Dueren, Germany). The gradients for elution were chosen according to the separation problem. Generally the systems were based on Water/Acetonitrile mixtures. UV-Signals were detected at 210 nm & 254 nm. Every fraction was dried by using a vacuum concentrator and the yield was determined.


For the control of every single fractionation step the resulting fractions were analysed by HPLC-UV-ELSD.



FIG. 1: isolation procedure









TABLE 2







History of isolation













Conditions of separation

retention time


Procedure
Starting
Solvent A: H2O + 0.1% TFA
Product of
period [min],


number
Fraction(s)
Solvent B: Acetonitrile + 0.1% TFA
separation step
yields [mg]














3
SM 1 (2)
Nucleodur 100-20 C18ec, 130 × 40 mm,
SM 3 (7 + 8)
51-54




Flow: 20 ml/min

433




Nucleodur 100-20 C18ec, 130 × 40 mm,
SM 3 (9)
55-57




Flow: 20 ml/min

228




Nucleodur 100-20 C18ec, 130 × 40 mm,
SM 3 (10)
58-67




Flow: 20 ml/min

1004 


9
SM 3 (7 + 8)
Nucleodur 100-20 C18ec, 130 × 40 mm,
SM 9 (3)
32-67




20 ml/min

117


10
SM 3 (9)
Nucleosil 100-7 C8ec, 250 × 20 mm,
SM 10 (2)
5-6




20 ml/min

 30


11
SM 3 (10)
Nucleodur 100-20 C18ec, 130 × 40 mm,
SM 11 (3)
38-44




20 ml/min

202


20
SM 9 (3)
Nucleodur 100-5 C18ec, 250 × 20 mm,
SM 20 (4)
18-19




20 ml/min

 26


21
SM 10 (2)
Nucleosil 100-7 C18, 250 × 10 mm,
SM 21 (4)
27-29




8 ml/min

 10


23
SM 11 (3)
Nucleodur 100-5 C18ec, 250 × 20 mm,
SM 23 (4)
17.5-18.5




20 ml/min

 35


29
SM 20 (4) +
Nucleosil 100-7 C18, 250 × 10 mm,
SM 29 (3)
17.0-17.5



SM 21 (4)
8 ml/min

 7


30
SM 23 (4)
Nucleosil 100-7 C18, 250 × 10 mm,
SM 30 (3)
18.5-19.5




8 ml/min

 13









Identification Characterisation of the Pure Compounds SM 29 (3) and SM 30 (3):

LC-MS analyses are performed using an Agilent HP1100 (Agilent, Waldbronn, Germany) liquid chromatograph coupled with a LCQ™ Deca XPplus mass spectrometer (Thermo Fisher Scientific, Waltham, Mass., USA) in the positive and negative electrospray ionisation (ESI) mode. A Waters symmetry column is used as stationary phase. Mobile phase A: 0.1% Formic acid in water, mobile phase B: 0.1% Formic acid in acetonitrile; gradient: 0-1 min. 98% A, from 1-21 min. to 100% B, from 21-27 min 100% B. LC-MS spectra are recorded in the range of molecular weights between 160 and 1.600 U.


HR-ESIMS data were obtained on a Bruker MicroTOF instrument, coupled with an HPLC system as described before and using sodium formiate as internal reference.


















Molecular





Retention
formula





time [min]
MW [g/mol]
HRMS [m/z]
Name









10.07
C15H10O6 286.24
obtained: m/z 287.05587 calculated: m/z 287.0550 [C15H11O6]+, Δ 3.0 ppm
2′,4,4′,6- Tetrahydroxy- aurone










10.73
C15H10O5 270.24
n.d.
4,4′,6-Trihydroxy- aurone









NMR Spectroscopic Data:

NMR spectra were recorded in DMSO-d6 on a Bruker DRX500 spectrometer at 293 K, operating at 500.13 MHz proton frequency and 125.76 MHz carbon frequency. The solvent peak was used as internal reference (δH 2.50, δC 39.5). Scalar coupling constants J are given in Hertz. 1H NMR spectra are shown in FIGS. 4 and 5


Structure elucidations and peak assignments are based on thorough analysis of two-dimensional 1H, 1H-gCOSY, 1H, 13C-gHSQC, and 1H, 13C-gHMBC spectra as well as chemical shift interpretation. Furthermore, HPLC-MS data including extracted UV as well as positive and negative mode ESI spectra were used. The molecular formula and elemental composition of novel congener SM 29 (3) was confirmed by high resolution ESIMS experiments (see above). Numbering of the aurone skeleton was done in agreement with the scientific literature (e.g., Jang D S et al., J. Nat. Prod. 2003, 66, 583-587).















SM 29 (3)
SM 30 (3)



























Atom

13C


1H (J in Hz)


13C *)


1H (J in Hz)






 1






 2
145.4

146.5



 3
179.1

179.5



 4
158.0

157.8



 5
 97.5
 6.04, d (1.9)
 97.5
 6.06, d (1.8)


 6
166.7

167.1



 7
 90.4
 6.18, d (1.8)
 90.5
 6.20, d (1.8)


 8
167.4

167.0



 9
103.0

103.3



10
103.6
 6.87, s
109.3
 6.54, s


 1′
110.8

123.8



 2′
158.6

132.8
 7.75, d (7.9)


 3′
102.3
 6.39, m
115.9
 6.86, d (7.9)


 4′
160.3

159.3



 5′
108.1
 6.38, m
115.9
 6.86, d (7.9)


 6′
132.0
 7.88, d (8.7)
132.8
 7.75, d (7.9)


 2′-OH

10.17, s




 4-OH

10.79, s

10.05, br s


 4′-OH

 9.92, s

10.89, br s


 6-OH

10.76, s

10.86, br s





*) Carbon chemical shifts of SM 30 (3) were obtained from 2-dimensional HSQC and HMBC experiments.






Example 3
Preparation of Enriched Extracts

20 g of Smilax myosotiflora (SM) were ground into a powder using a lab mill (Retsch ZM200, Haan, Germany) and afterwards extracted for 45 min at 40° C. with 50 ml of 75% ethanol in water (v/v) using ultrasonic treatment. Before the water was mixed with the ethanol for the extraction process, the pH value of the water was adjusted to pH 2 by addition of 2M hydro-chloric acid. The final pH was checked either with indicator paper (strips: Fisherbrand pH 0-14) and with a pH-meter (WTW pH330).


The extract solution was separated from the remaining material by filtration and the filtrate was concentrated under reduced pressure using a rotary evaporator (max. 40° C. bath temperature; max. 15 mbar; Büchi, Essen, Germany) in order to remove the organic solvent. For enrichment of aurones, the remaining water phase was subjected to further liquid/liquid separation steps.


First Liquid/Liquid Enrichment Step:

Subsequently the remaining water phase was filled up with water to a final volume of 50 ml and extracted in a first liquid/liquid separation twice with 50 ml ethyl acetate. The two ethyl acetate extract phases were combined (called SM 31(1)), dried (Na2 SO4) and the solvent was evaporated under reduced pressure. The remaining water phase (called SM 31(2)) was also evaporated to dryness. The yields for the dried samples were determined.


Second Liquid/Liquid Enrichment Step:

In a subsequent second liquid/liquid separation step, further enrichment of the aurones was achieved by re-dissolving 45 mg SM 31(1) in a mixture of 25 ml ethyl acetate and 25 ml PBS (30 mM phosphate buffered saline) at pH 7.4 followed by extraction. The extraction with 25 ml ethyl acetate was repeated. The two ethyl acetate extract phases were combined to yield a product named SM 31(3) and dried (Na2 SO4) and the solvent was evaporated under reduced pressure. The remaining water phase (called SM 31(4)) was also evaporated to dryness. The yields of the dried samples were determined.


Yields:


















Plant
SM No.
Phase
Amount










S. myosotiflora

SM 31 (1)
Ethyl acetate
49 mg




S. myosotiflora

SM 31 (2)
Water
227 mg 




S. myosotiflora

SM 31 (3)
Ethyl acetate
30 mg




S. myosotiflora

SM 31 (4)
Water
15 mg










Since aurones remain throughout the two liquid/liquid separation processes in the ethyl acetate phases, an enrichment of factor 5.6 in the first step and additional enrichment of factor 1.5 is achieved.


Example 4
Social Recognition Test (SRT), In Vivo

Using the material obtained according to the preceding procedure (e.g. here dried SM 31(3)) a social recognition test was performed.


An unfamiliar juvenile rat was introduced into the individual home cage of a matured adult rat for 5 minutes. Following this first contact (C1), the juvenile was returned to its isolation cage, until a second contact of 5 minutes with the same mature adult rat (C2), 120 minutes later was allowed.


The time the adult rat spends investigating (sniffing, grooming, licking, closely following) the juvenile at each contact was recorded. A recognition index (═C2/C1) was calculated. Under such conditions, a mature adult rat fails to recognize the juvenile as familiar, as indicated by an absence of reduction in the duration of social investigatory behaviour at C2.


Three sub-experiments in groups of 4 animals were tested and their behaviour monitored in comparison to a vehicle control group.


An extract prepared according to Example 3 (SM 31(3) in dried form) (dispersed in 4% Cremophor E1, (polyoxyethylated castor oil, BASF, Ludwigshafen, Germany) in physiological saline), when administered p.o. immediately after the first contact (i.e. 120 minutes before the second contact), significantly decreased the duration of investigation of the juvenile at the second contact at a dosage of 1000 mg/kg, as compared with the first contact. In addition, the recognition index was significantly decreased, as compared with vehicle controls.


Example 5
Object Recognition Test (ORT), In Vivo

Rats (300-400 g) were first habituated to the experimental enclosure, a grey plastic arena (65×34×45 cm) illuminated from above. Approximately after 24 hours, rats were individually repositioned in the enclosure for 5 minutes in the presence of two identical objects (sample object) placed approximately 19 cm apart. Following this first exposure (E1), each rat was then returned to its home cage. After 48 hours, the rat was again placed in the enclosure for 3 minutes (E2) in the presence of a third copy of the sample object (familiar) and a novel object. The behaviour of the rat was monitored by video.


The time spent investigating the 2 sample objects during E1 and both the novel object (E2N) and the familiar object (E2F) during E2 was recorded on videotape. A recognition index (RI=E2N−E2F/E2N+E2F) was then calculated.


Under such conditions, a rat does not show a preference for investigation of the novel object during E2, suggesting that it fails to recognize the sample object as familiar.


An extract prepared according to example 3 (SM 31(3) in dried form) (dispersed in 4% Cremophor E1 in physiological saline), administered p.o. significantly decreased the duration of investigation of the familiar object, as compared with the novel object during the second exposure at a dosage of 1000 mg/kg.


Example 6
PDE 1

PDE1 protein isolated from bovine brain (MDS Pharma Services: cat. No. 146000) was pre-incubated with the respective test compound dissolved in 1% DMSO aqueous solution for 15 minutes at 25° C. in an incubation buffer (50 mM Tris-HCl, pH 7.5, 5 mM MgCl2, 2 mM CaCl2, 100 U/ml Calmodulin). After pre-incubation phase 1.01 μM [3H]cAMP+cAMP where added as substrate to the buffer and the mixture was incubated for additional 20 minutes (25° C.).


At the end of incubation phase [3H] Adenosine concentrations were quantified. The final concentration of the test compound is 10 μM.


With compound SM 29 (3), 52% inhibition compared with the control were found in this assay, with compound SM 30(3) 52% inhibition.


Example 7
PDE 3

PDE3 protein isolated from human platelets (MDS Pharma Services: cat. No. 152000) was pre-incubated with the respective test compound dissolved in 1% DMSO aqueous solution for 15 minutes at 25° C. in an incubation buffer (50 mM Tris-HCl, pH 7.5, 5 mM MgCl2, 5 mM MgCl2). After pre-incubation phase 1.01 μM [3H]cAMP+cAMP where added as substrate to the buffer and the mixture was incubated for additional 20 minutes (25° C.). At the end of incubation phase [3H] Adenosine concentrations were quantified. Stimulating or inhibiting effects equal or larger than 50% in comparison to vehicle (1% DMSO) control were considered as significant effects.


At the end of incubation phase [3H] Adenosine concentrations were quantified. The final concentration of the test compound is 10 μM.


With compound SM 29 (3), 39% inhibition compared with the control were found in this assay, with compound SM 30(3) 74% inhibition.


Example 8
PDE 4

PDE4 protein from human leukemic monocyte lymphoma cell line (U937, for example abcam ab3959) (MDS Pharma Services: cat. No. 152000) was pre-incubated with the respective test compound dissolved in 1% DMSO aqueous solution for 15 minutes at 25° C. in an incubation buffer (50 mM Tris-HCl, pH 7.5, 5 mM MgCl2, 2 mM CaCl2, 100 U/ml Calmodulin). After pre-incubation phase 1.01 μM [3H]cAMP+cAMP where added as substrate to the buffer and the mixture was incubated for additional 20 minutes (25° C.). At the end of incubation phase [3H] Adenosine concentrations were quantified.


At the end of incubation phase [3H] Adenosine concentrations were quantified. The final concentration of the test compound is 10 μM.


With compound SM 29 (3), 29% inhibition compared with the control were found in this assay, with compound SM 30(3) 41% inhibition.


The assays from the examples 3, 4 and 5 were conducted by MDS,


Thus the compounds are active as PDE 1, PDE 3 and PDE 4 inhibitors. In contrast, they show only no or less than 17% inhibition with PDE2, PDE5 and PDE6 and are thus selective, which allows to assume that compounds of formula I in general are especially active as selective inhibitors of any one or more of PDE 1, PDE 3 and PDE 4.

Claims
  • 1. A compound of the formula I,
  • 2. A compound for use of the formula I, mixture of compounds of the formula I or extract of the formula I according to claim 1, wherein Y is oxo,X is H, hydroxy, methoxy, acetoxy, benzoyloxy or 3,4,5-trihydroxybenzoyloxy,the bonds a and c are double bonds, respectively, the bonds b and d are single bonds, respectively,where the compounds of the formula I may be present in free form, in the form of a pharmaceutically and/or nutraceutically acceptable salt, in the form of a tautomer, in the form of an ester and/or in the form of a solvate.
  • 3. A compound for use of the formula I, mixture of compounds of the formula I or extract of the formula I according to claim 1, wherein each of R1 to R9 is, independently of the others, H, hydroxy, chloro, C1-C8-alkyl, C1-C8-alkoxy, C1-C9-alkanoyloxy or benzoyl with the proviso that if R1, R3 and R7 each are hydroxyl, R2, R4, R5 and R9 each are hydrogen and one of R6 and R8 is hydroxy, then the other of R6 and R8 has one of the meanings mentioned above other than H;Y is oxo, andX is H, hydroxy, methoxy, acetoxy, benzoyloxy or 3,4,5-trihydroxybenzoyloxy,the bonds a and c are double bonds, respectively, the bonds b and d are single bonds,where the compounds of the formula I may be present in free form, in the form of a pharmaceutically and/or nutraceutically acceptable salt, in the form of a tautomer, in the form of an ester and/or in the form of a solvate.
  • 4. A compound of the formula I, mixture of compounds of the formula I and/or extract of the formula I for use according to claim 1, where the compound(s) of the formula I is or are selected from the group consisting of:
  • 5. An extract comprising one or more compounds of the formula I in free or any other form mentioned for use according to claim 1 which is obtained from Smilax myosotiflora, especially from the roots.
  • 6. An extraction and purification or at least enrichment process for obtaining a compounds or an extract according to claim 1, comprising an extraction step from a plant or plant parts, where the plant is of the Genus Smilax, anda first liquid/liquid separation step under acidic conditions, followed bya subsequent second liquid/liquid extraction of the material found in the less polar phase of the first extraction step, preferably under neutral to slightly alkaline conditions,where preferablysaid extraction and said first liquid/liquid separation step takes place under acidic conditions at a pH of about 2 to about 4.5, more preferably about 2 to about 3, most preferably at a pH of about 2a followed by said second liquid/liquid extraction step performed at a pH of about 7 or larger, preferably about 7 to about 9, and a most preferably a pH of 7.4 to 7.6.
  • 7. A compound of the formula I, mixture of compounds of the formula I and/or extract for use obtainable according to the process according to claim 6, wherein the compound or compounds according to formula I are present in an amount of 10 or more % by weight.
  • 8. A compound of the formula I, mixture of compounds of the formula I and/or extract for use obtainable according to the process according to claim 6, wherein the compound or compounds according to formula I are present in an amount of 30 or more % by weight.
  • 9. A compound of the formula I, mixture of compounds of the formula I and/or extract for use obtainable according to the process according to claim 6, wherein the compound or compounds according to formula I are present in an amount of 50% or more by weight.
  • 10. A compound of the formula I, mixture of compounds of the formula I and/or extract for use obtainable according to the process according to claim 6, wherein the compound or compounds according to formula I are present in an amount of 80 to 100% by weight.
  • 11. An extract from plants of the genus Smilax obtainable according to the method of claim 6, comprising a compound of the formula I
  • 12. A compound of the formula I, mixture of compounds of the formula I or extract according to claim 11, wherein Y is oxo,X is H, hydroxy, methoxy, acetoxy, benzoyloxy or 3,4,5-trihydroxybenzoyloxy,the bonds a and c are double bonds, respectively, the bonds b and d are single bonds, respectively, where the compounds of the formula I may be present in free form, in the form of a pharmaceutically and/or nutraceutically acceptable salt, in the form of a tautomer, in the form of an ester and/or in the form of a solvate.
  • 13. A compound of the formula I, mixture of compounds of the formula I or extract according to claim 11, wherein each of R1 to R9 is, independently of the others, H, hydroxy, chloro, C1-C8-alkyl, C1-C8-alkoxy, C1-C9-alkanoyloxy or benzoyl with the proviso that if R1, R3 and R7 each are hydroxyl, R2, R4, R5 and R9 each are hydrogen and one of R6 and R8 is hydroxy, then the other of R6 and R8 has one of the meanings mentioned above other than H;Y is oxo, andX is H, hydroxy, methoxy, acetoxy, benzoyloxy or 3,4,5-trihydroxybenzoyloxy,the bonds a and c are double bonds, respectively, the bonds b and d are single bonds,where the compounds of the formula I may be present in free form, in the form of a pharmaceutically and/or nutraceutically acceptable salt, in the form of a tautomer, in the form of an ester and/or in the form of a solvate.
  • 14. The extract of claim 11, obtained from Smilax myosotiflora.
  • 15. A pharmaceutical or nutraceutical composition, comprising an extract according to claim 11 and at least one pharmaceutically or nutraceutically acceptable carrier material.
  • 16. The use of an extract according to claim 11 for the manufacture of a medicament for the prophylactic and/or therapeutic treatment of a PDE dependent disease or condition of the central nervous system.
  • 17. A method of prophylactically and/or therapeutically treating an animal, especially a human in need of such treatment, of using a compound of the formula I, presumed to suffer in future or suffering from a phosphodiesterase (PDE) dependent disease or condition of the central nervous system, comprising administering to said animal or human an effective amount of an extract according to claim 11.
  • 18. A pharmaceutical composition or a nutraceutical comprising a compound of the formula I, a mixture of compounds of the formula I or an extract according to claim 1 for use in the prophylactic and/or therapeutic treatment of an animal with a phosphodiesterase (PDE) dependent symptom or condition of the central nervous system, together with at least one pharmaceutically or nutraceutically acceptable carrier material.
  • 19. The composition according to claim 18, where the compound(s) of formula I are present in an amount of 0.001 to 100% by weight. e.g. from 0.1 to 50% by weight.
  • 20. The composition according to claim 18, where the compound(s) of formula I are present in an amount of 0.1 to 50% by weight.
  • 21. A method of prophylactically and/or therapeutically treating an animal, especially a human in need of such treatment, of using a compound of the formula I, presumed to suffer in future or suffering from a phosphodiesterase (PDE) dependent disease or condition of the central nervous system, comprising administering to said animal or human an effective amount of a compound of the formula I, a compound mixture or an extract according to claim 1 in free or other forms mentioned therein.
  • 22. The use of a compound of the formula I, or a mixture of compounds of the formula I, or an extract comprising one or more compounds of the formula I, as defined in claim 1 in free or other forms mentioned therein, as active ingredient for the manufacture of a medicament or nutraceutical or food supplement for the treatment of a PDE dependent disease or condition of the central nervous system.
  • 23. The use of a compound of the formula I, or a mixture of compounds of the formula I, or an extract comprising one or more compounds of the formula I, as defined in claim 1 in free or other forms mentioned therein, as active ingredient in the treatment of a PDE dependent disease or condition of the central nervous system.
  • 24. The compound, compound mixture or extract in free or any other form mentioned according to claim 1, where the PDE dependent disease or condition of the central nervous system is a neurodegenerative disease.
  • 25. The compound, compound mixture or extract in free or any other form mentioned according to claim 1 where the PDE dependent disease or condition of the central nervous system is Parkinson's disease, Alzheimer's disease, age related dementia or dementia in general.
  • 26. The compound, compound mixture or extract in free or any other form mentioned according to claim 1 where the PDE dependent disease or condition of the central nervous system is neurological trauma including brain or central nervous system trauma and/or recovery therefrom, and/or ischemia of the central and/or peripheral nervous systems.
  • 27. The compound, compound mixture or extract in free or any other form mentioned according to claim 1, where the PDE dependent disease or condition of the central nervous system is depression, anxiety, psychosis, cognitive dysfunction, mental dysfuntion, a learning disorder, and memory disorder.
  • 28. The compound, compound mixture or extract in free or any other form mentioned according to claim 1, where the PDE dependent disease or condition of the central nervous system is one that requires improvement of cognitive outcomes and mood disorders.
  • 29. The compound, compound mixture or extract in free or any other form mentioned according to claim 1, where the PDE dependent disease or condition of the central nervous system is one that requires enhancement of cognition.
  • 30. The pharmaceutical composition or a nutraceutical comprising a compound of the formula I, a mixture of compounds of the formula I or an extract according to claim 1 for wherein the composition is suitable for administration intravenously, intraperitoneally, subcutaneously, intramuscularly, intrathecally, orally, rectally, topically, or by inhalation.
  • 31. The compound, compound mixture or extract in free or any other form mentioned according to claim 1 where the PDE dependent disease of condition of the central nervous system is one that requires modulating, such as protecting or stabilizing, neuronal and glial function and CNS homeostasis.
RELATED APPLICATIONS

The present application claims benefit of U.S. Provisional Application No. 61/164,052 filed Mar. 27, 2009, which is incorporated herein in its entirety by reference.

Provisional Applications (1)
Number Date Country
61164052 Mar 2009 US