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HK1076098B - Aminoindan derivatives - Google Patents

Aminoindan derivatives Download PDF

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Publication number
HK1076098B
HK1076098B HK05110547.2A HK05110547A HK1076098B HK 1076098 B HK1076098 B HK 1076098B HK 05110547 A HK05110547 A HK 05110547A HK 1076098 B HK1076098 B HK 1076098B
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Hong Kong
Prior art keywords
calc
found
aminoindan
compounds
compound
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HK05110547.2A
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German (de)
French (fr)
Chinese (zh)
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HK1076098A1 (en
Inventor
Michel Chorev
Tamar Goren
Yacov Herzig
Jeffrey Sterling
Marta Weinstock-Rosin
Moussa B.H. Youdim
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Yissum Research Development Company Of The Hebrew University Of Jerusalem
Technion Research & Development Foundation Limited
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Priority claimed from IL11985396A external-priority patent/IL119853A0/en
Priority claimed from IL12051097A external-priority patent/IL120510A0/en
Application filed by Yissum Research Development Company Of The Hebrew University Of Jerusalem, Technion Research & Development Foundation Limited filed Critical Yissum Research Development Company Of The Hebrew University Of Jerusalem
Publication of HK1076098A1 publication Critical patent/HK1076098A1/en
Publication of HK1076098B publication Critical patent/HK1076098B/en

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Description

The present invention relates to intermediate compounds, useful for the preparation of novel compounds, pharmaceutical compositions containing said compounds and their use in the treatment of various CNS disorders.
Dementia exists in several forms including static dementia, Alzheimer's-type dementia, senile dementia, presenile dementia and progressive dementia. One of the common pathological features of several types of dementia is the lack of the neurotransmitter acetylcholine. This has led to the development of acetylcholine esterase inhibitors for use in the treatment of dementias such as the compound tacrine. A summary of the different approaches to and progress.made in the treatment of Alzheimer's Disease may be found in Drugs of the Future (1995) 20(11): 1145-1162.
Recently, compounds that in addition to inhibiting acetylcholine esterase, possess inhibitory activity against monoamine oxidase type A (MAO-A) have been developed. The perceived benefit of having the anti-MAO-A activity is stated to be an anti-depressant effect ( European Patent Publication Nos. 614,888 and 664, 291 ).
US Patents Nos. 5,387,133 , 5, 453, 446 , 5, 457, 133 and 5, 519, 061 all disclose that the compound (R)-N-propargyl-1-aminoindan, a highly selective monoamine oxidase type B (MAO-B) inhibitor is effective in the treatment of dementias of the Alzheimer type and memory disorders. There is no indication given therein that the compound might have acetylcholine esterase inhibitory activity. Furthermore, the compound is only very weakly active as a MAO-A inhibitor.
PCT International Publication No. WO95/18617 discloses various aminoindan derivatives that are active in a variety of CNS disorders including dementias of the Alzheimer type. There is no indication given therein that any of the compounds disclosed might have acetylcholine esterase inhibitory activity.
The present specification describes compounds of formula I wherein when a is 0; b is 1 or 2; when a is 1, b is 1; m is from 0 to 3; X is O or S; Y is halogeno; R1 is hydrogen or C1-4 alkyl; R2 is hydrogen, C1-4 alkyl or optionally substituted propargyl; and R3 and R4 are each independently hydrogen , C1-8 alkyl, C6-12 aryl, C6-12 aralkyl or C6-12 cycloalkyl optionally substituted.
The present specification describes the compounds themselves, pharmaceutical compositions containing said compounds and their use in the treatment of depression, Attention Deficit Disorder (ADD), Attention Deficit and Hyperactivity Disorder (ADHD), Tourette's Syndrome, Alzheimer's Disease and other dementias such as senile dementia, presenile dementia, progressive dementia, dementia of the Parkinson's type, vascular dementia and Lewy body dementia.
A further aspect of the present specification describes the use of the compounds of formula I in the treatment of neurotraumatic disorder. As used herein the term "neurotraumatic disorder" is meant to include damage caused to the nervous system (both central and peripheral) by virtue of ischemic damage such as that which occurs in stroke, hypoxia or anoxia, neurodegenerative diseases, Parkinson's Disease, Alzheimer's Disease, Huntington's Disease, neurotoxic injury, head trauma injury, spinal trauma injury, peripheral neuropathy or any form of nerve damage.
An additional aspect of the present specification describes the use of the compounds of formula I in the treatment of memory disorder or depression.
The present specification describes the racemic compounds themselves and optically active enantiomers thereof.
The present invention provides a compound having the structure: wherein R2 is Boc and R3 is H; and wherein R1 is OH or the group and racemic mixtures, enantiomers or salts thereof.
Further embodiments of the present invention are apparent from the dependent claims.
The present specification describes compounds of Formula I: wherein when a is 0, b is 1 or 2; when a is 1, b is l, m is from 0-3, X is O or S; Y is halogeno; R1 is hydrogen or C1-4 alkyl; R2 is hydrogen, C1-4 alkyl, or optionally substituted propargyl and R3 and R4 are each independently hydrogen, C1-4 alkyl, C6-12 aryl, C6-12 aralkyl or C6-12 cycloalkyl each optionally substituted.
In an embodiment, a is 0 and b is 1. In another embodiment, a is 0, b is 1, and X is O.
In an embodiment, X is O. In an additional embodiment, X is S.
In an embodiment, R2 is selected from the group consisting of hydrogen, methyl, ethyl or optionally substituted propargyl.
In another embodiment R1 is propargyl.
In a further embodiment, the compound is selected from the group consisting of: (rac) 6-(N-methyl, N-ethyl-carbamyloxy) -N'-propargyl-1-aminoindan HCl; (rac) 6-(N,N-dimethyl, carbamyloxy)-N'-methyl-N'-propargyl-1-aminoindan HCl; (rac) 6-(N-methyl, N-ethyl-carbamyloxy)-N'-propargyl-1-aminotetralin HCl; (rac)6-(N,N-dimethyl-thiocarbamyloxy)-1-aminoindan HCl; (rac)6-(N-propyl-carbamyloxy)-N'-propargyl-1-aminoindan HCl; (rac)5-chloro-6-(N-methyl, N-propyl-carbamyloxy)-N'-propargyl-1-aminoindan HCl; (S)-6-(N-methyl, N-propyl-carbamyloxy)-N'-propargyl-1-aminoindan HCl; and (R)-6-(N-methyl, N-ethyl-carbamyloxy)-N'-propargyl-1-aminoindan hemi-(L) -tartrate.
In a further embodiment, R1 is hydrogen, methyl or ethyl and R2 is hydrogen, methyl, ethyl or optionally substituted propargyl. In a further embodiment, the propargyl group is substituted with a C1-4 alkyl group on the methylene group (R6 is Scheme I).
The term "halogeno" is used to refer to fluoro, chloro, bromo, or iodo.
In an embodiment, when m is greater than 1 each Y may be the same or different.
In an additional embodiment, the group OC(X)NR3R4 is on the 4, 6 or 7 position of the indan ring counting from the amino substituted carbon.
In another embodiment, at least one of R3 and R4 is methyl and the other is hydrogen, methyl, ethyl, propyl, butyl, hexyl, phenyl, benzyl or cyclohexyl.
In the practice of this invention, pharmaceutically acceptable salts include, but are not limited to, the esylate, mesylate, maleate, fumarate, tartrate, hemi-tartarate, hydrochloride, hydrobromide, p-toluenesulfonate, benzoate, acetate, phosphate and sulfate salts.
The present specification further describes a pharmaceutical composition which comprises a therapeutically effective amount of a compound of formula I or a pharmaceutically acceptable salt thereof and a pharmaceutically acceptable carrier. The "therapeutically effective amount" of a compound of formula I or a pharmaceutically acceptable salt thereof may be determined according to methods well known to those skilled in the art, indications of such amounts are given below.
These compositions may be prepared as medicaments to be administered orally, parenterally, rectally, or transdermally.
Suitable forms for oral administration include tablets, compressed or coated pills, dragees, sachets, hard or soft gelatin capsules, sublingual tablets, syrups and suspensions. In one embodiment, the pharmaceutically acceptable carrier is a solid and the pharmaceutical composition is a tablet. The therapeutically effective amount may be an amount from about 0.5mg to about 2000 mg, preferably from about 1mg to about 1000mg.
In an alternative embodiment, the pharmaceutically acceptable carrier is a liquid and the pharmaceutical composition is an injectable solution. The therapeutically effective amount may be an amount from about 0.5mg to about 2000mg, preferably from about 1mg to about 1000mg. The volume administered may be an amount between 0.5 and 10ml.
In a further alternative embodiment, the carrier is a gel and the pharmaceutical composition is a suppository. For parenteral administration the invention provides ampoules or vials that include an aqueous or non-aqueous solution or emulsion. For rectal administration there are provided suppositories with hydrophilic or hydrophobic vehicles. For topical application as ointments and transdermal delivery there are provided suitable delivery systems as known in the art. For oral or suppository formulations, 0.5-2000 mg per dosage unit and preferably 1-1000 mg per dosage unit.
These compositions may be used alone to treat the above-listed disorders, or alternatively, for example, in the case of Alzheimer's Disease, they may be used as an adjunct to the conventional treatments such as haloperidol, tacrine or deprenyl.
The invention will be better understood from the Experimental Details which follow. However, one skilled in the art will readily appreciate that the specific methods and results discussed are merely illustrative of the invention as described more fully in the claims which follow thereafter.
Examples:
Compounds of general formula I may be prepared, as shown in Scheme I, from the corresponding carbamoyl derivatives of aminoindan III by reacting the latter with propargyl compounds bearing an appropriate leaving group at the 3-position, e.g. a halide group, mesylate, tosylate, etc., under basic conditions provided by an inorganic base, e.g. K2CO3, NaOH, or an organic base e.g. a tertiary amine, in a polar organic solvent, e.g. CH3CN, DMF, etc., at 15-4°C, preferably at 20-25°C, for a period of time in the range of 5-48 hours, preferably 20-30 hours. The products, obtained after a suitable work-up and purification, are in the form of free bases. Preferably these are converted into their pharmaceutically acceptable salts, e.g. HCl, mesylate, hemi-tartarate, etc.
As shown in Scheme I, compounds of general formula III may be prepared by Boc deprotection of compounds of general formula IV. In turn, compounds of general formula IV may be prepared by carbamylating a compound of general formula V in a conventional manner, e.g. by reacting the compound of formula V with an appropriate carbamoyl halogenide or by an alkylisocyanate. Finally, compounds of general formula V may be prepared by Boc protection of the appropriate hydroxy amines, by methods known to those skilled in the art. N,N-dialkyl aminoindan derivatives may be prepared as shown on in Scheme I by the direct carbamylation of the corresponding N,N-dialkyl-hydroxy-aminoindan or by alkylation of a compound of formula III.
Although Scheme I shows the preparation of carbamoyl derivatives the same process and description above is relevant to the preparation of the thiocarbamates of the present invention.
Starting Materials
6- and 7-Hydroxy-1-aminoindans may be prepared by demethylation of the respective 6- and 7-methoxy-1-aminoindans. The latter may be obtained from the corresponding 1-indanones, either by their conversion to the oximes, followed by reduction1, or by their reductive amination (NaCNBH3 and NH4OAc)2.
6-Hydroxy aminoindan may also be prepared from aminoindan via a regioselective Friedel - Crafts acylation of a suitably N-protected aminoindan, followed by a Baeyer - Williger oxidation and finally hydrolysis5. 6-hydroxy-(R)-1-aminoindan may thus be prepared by the method described in the Example below and Scheme II, wherein "R" is optionally substituted alkyl.
N-Methyl-6-hydroxy-1-aminoindan was prepared by demethylation of 6-methoxy-N-methyl-1-aminoindan, which was prepared from 6-methoxy-1-aminoindan by reductive alkylation (e.g. ethyl formate, followed by LiAlH4 reduction), or alternatively, by seductive amination (MeNH2, HCl,NaCNBH3) of 6-methoxy-1-indanone2. N-ethyl-6-hydroxy-1-aminoindan was obtained by acetylation of 6-hydroxy-1-aminoindan (Ac2O, KOH), followed by reduction (LiAlH4). N,N-Dimethyl-6-hydroxy-1-aminoindan was prepared by demethylation of the corresponding 6-methoxy analogue, which was prepared by reductive alkylation (formaldehyde, formic acid) of 6-methoxy-1-aminoindan. 4-Hydroxy-1-aminoindan may be prepared from 4-hydroxy-indanone by converting the latter to the oxime, followed by reduction1. 4-Hydroxy-indanone may be prepared from dihydrocoumarin.3
7-Hydroxy-1-aminotetralin and 7-hydroxy -2-aminotetralin were prepared by demethylation of the corresponding 7-methoxy analogues. The latter were prepared by reductive amination (as above) of the corresponding 7-methoxy 1- and 2- tetralones.
7-Methoxy-2-tetralone was prepared from 2,7-dimethoxytetralin according to Copinga, et al4.
Preparation of 6-Hydroxy-(R)-1-aminoindan (as shown in Scheme II). N-Trifluoroacetyl-(R)-1-aminoindan
To a cooled (0-5°C) solution of trifluoroacetic anhydride (194.6g, 0.926 mol) in toluene (680 ml) was added dropwise a solution of (R)-1-aminoindan (base) (113.32g 0.85 mol) in toluene (50 ml) and stirred under ice-cooling for 3 1/2 hours. A solution of KOH (67.25g, 1.2 mol) in water (1000ml) was then added, under cooling. The reaction mixture was stirred for further 2 hours at room temperature and filtered. The solid was collected by filtration, washed with water (680ml) and dried in vacuo at 60°C to give 152g (78%) of a white solid, mp:153-154°C. The solution was evaporated in vacuum and the crystals were filtered and washed with water. The solid was dried in vacuo at 60°C. The second crop (25g) was crystallized from a mixture of hexane and ethyl acetate to give 18g (9%) of a white solid, mp:153-154°C. The total yield was 170g (87%).
6-Chloroacetyl-N-trifluoroacetyl-(R)-1-aminoindan
To a suspension of AlCl3 (89.2 g, 0.67 mol) in 1,2-dichloroethane (600 ml) was added chloroacetyl chloride (55.7 ml, 78.9 g, 0.7 mol) dropwise at 0-5°C under nitrogen for 20 minutes and it was then left to warm up to 20-25°C. To this mixture was added N-trifluoroacetyl-(R)-1-aminoindan (34.4. g, 0.15 mol) for 3 hours at 20-25°C. The resulting mixture was then stirred for an additional 30 minutes and poured into a mixture of ice-cold water (1.5 1) and 1,2-dichloroethane (11). The mixture was stirred for 5 minutes and the layers were separated. The aqueous layer was extracted with 1,2-dichloroethane (2x750ml). The combined organic layers were washed with water (2x900 ml) and 5% aqueous NaHCO3 solution (3x900 ml). The organic layer was dried (Na2SO4) and the solvent was removed under reduced pressure to give a solid, which was recrystallized from ethanol to give 15 g (48%) of a white solid mp: 166-167°C.
6-Chloroacetoxyl-N-trifluoroacetyl-(R)-1-aminoindan
6 -Choroacetyl-N-trifluoroacetyl-(R)-1-aminoindan (30.57g, 0.1 mol) was dissolved in anhydrous dichloromethane (210ml) and 3-chloroperoxybenzoic acid (70%, 44.87g, 0.26 mol) was added all at once. The suspension was cooled to 0°C and trifluoroacetic acid (11.4g, 0.1 mol) was added dropwise for 5-10 minutes. The reaction flask was protected from light and the mixture was stirred for 3-5 days at room temperature. The reaction mixture was poured into water (300 ml). The mixture was neutralized with ammonium hydroxide solution. The layers were separated. The aqueous layer was extracted with dichloromethane (200ml). The combined organic layers were dried (Na2SO4) and the solvent was removed under reduced pressure to give a solid, which was recrystallized from ethanol to give 15 g (48%) of a white solid mp: 169-170°C.
6-Hydroxy-(R)-1-aminoindan.
A suspension of6-chloroacetoxy-N-trifluoroacetyl-(R)-1-aminoindan (25.4, 0.11 mol) and K2CO3 (38.0g, 0.275 mol) in a mixture of methanol (275ml) and water (175ml) was stirred at 70°C for 1.5 hours. Methanol was removed in vacuo, and the aqueous phase was neutralized with 10% hydrochloric acid. The mixture was filtered and the solid was washed with water. The mother liquor was evaporated under reduced pressure to a small volume. The suspension was neutralized, filtered and the brown solids were crystallized from methanol (twice) to give 7.0g (43%) of a white solid mp:200-203°C.
Preparation of the corresponding S-enantiomer may be carried out in the same manner using (S)-1-aminoindan as the starting material.
Resolution of Enantiomers:
The R- and S- enantiomers of each compound may be obtained by optical resolution of the corresponding racemic mixtures. Such a resolution can be accomplished by any conventional resolution method well known to a person skilled in the art, such as those described in U.S. Patent No. 4,833,273, issued May 23, 1989 (Goel ) and in J. Jacques, A. Collet and S. Wilen, "Enantiomers, Racemates and Resolutions," Wiley, New York (1981). For example, the resolution may be carried out by preparative chromatography on a chiral column. Another example of a suitable resolution method is the formation of diastereomeric salts with a chiral acid such as tartaric, malic, mandelic acid or N-acetyl derivatives of amino acids, such as N-acetyl leucine, followed by recrystallization to isolate the diastereomeric salt of the desired enantiomer.
Alternatively, selected starting materials, intermediates or end products may be resolved into their respective enantiomers by the method described in PCT International Application Publication No. WO/96US/21640 , wherein the compound to be resolved is first converted into its N-benzyl derivative. The N-benzyl derivative is then resolved using either R or S-mandelic acid. The resolved product is converted to its base and reduced under acidic conditions to provide the desired enantiomer. Preferably, the starting material is resolved prior to Boc protection and carbamylation.
The R and S enantiomers of the starting materials may also be prepared from R and S enantiomers of aminoindan via a regioselective Friedel - Crafts acylation of a suitably N-protected optical isomer of aminoindan, followed by a Baeyer-Williger oxidation and finally hydrolysis5, thus obviating the need for optical resolution.
References
  1. 1. Y. Oshiro, et al, J. Med. Chem. 34: 2004 (1991);
  2. 2. R.F. Borch, et al, J. Am. Chem. Soc. 93: , 2897 (1971);
  3. 3. J.G. Cannon, et al, J. Med. Chem. 28: 515 (1985);
  4. 4. S.C.Copinga, et al, J. Med. Chem. 36: 2891 (1993); and
  5. 5. K. Teranishi et al, Synthesis 1018 (1994).
Preparation of Compounds of the Invention as shown in Scheme I A: Boc - protection and carbamylation 1. Boc Protection 6-hydroxy N-Boc aminoindan
A solution of 6-hydroxy aminoindan (16 g, 107 mmol), di-t-butyl dicarbonate (23.8 g, 109.2 mmol) and Et3N (16.74 ml, 120 mmol) in THF (375 ml) was stirred at room temperature (RT) for 20 hrs. The reaction mixture was evaporated to dryness under reduced pressure, and the residue was dissolved in CH2Cl2 (200 ml), washed with water (200 ml), dried over Na2SO4 and evaporated to dryness under reduced pressure. The crude product was purified by column chromatography (hexane/EtOAc 2:1) to give 23 g of a solid (86%).
2. Carbamylation 6-(N-Me, N-Et carbamyloxy) N-Boc aminoindan
To a stirred and ice-cooled solution of N-Boc 6-hydroxy aminoindan (7.5 g, 30 mmol) in acetonitrile (75 ml) was added N-Me,N-Et carbamoyl chloride (6.3 g, 51.8 mmol), followed by a dropwise addition of NaH (60% in oil, 1.56 g, 39 mmol). The reaction mixture was stirred for 2 hrs at RT under argon. After evaporation of the solvent in-vacuo, water (100 ml) was added, and extracted with ether (3x100 ml). The organic phase was washed with dilute NaOH (pH 10-11), dried and evaporated to dryness in-vacuo. Purification by column chromatography (hexane:EtOAc 2:1) afforded 7.8 g (77 %) of an oil.
In this manner the intermediates in Tables 1 and 2 were prepared. In Table 1 and all further Tables the heading "position" refers to the ring position of the carbamyl group unless otherwise indicate
position Y R1 R3 R4 yield (%)
6- H H Me Me 92
6- H H Me Pr 95
6- H H Me Et 77
7- H H Me Me 92
7- H H Me Et 83
7- H H Me Pr 95
6- H Et Me Me 76
6- H Me Me Me 92
7- H Me Me Me 78
6- H Me Me Pr 80
6- H H Me n-hexyl 98
4- H H Me Me 85
4- H H Me Et 87
6- H H Me Et 89
6- H H Me cyclohexyl 98
6- H H Me p-OMe-phenyl 97
6- H H Me phenyl 93
6- H H Me 83
6- 5-Cl H Me Et 88
6- 5-Cl H Me Pr 97
6- H H Me Bu 99
6- H H Et Bu 93
6- H H Et cyclohexyl 94
position of amine R1 R3 R4 yield (%)
2- H Me Me 85
2- H Me Et 79
1- H Me Me 85
1- H Me Et 98
B: Boc - Deprotection 6-(N-Me,N-Et Carbamyloxy) aminoindan HCl (Compound 3)
6-(N-Me, N-Et Carbamyloxy) N-Boc aminoindan (7.8 g, 23.3 mmol) was dissolved in dioxane (80 ml), and a 20% solution of gas. HCl in dioxane (80 ml) was added. After 2 hr stirring at RT the solvent was evaporated in-vacuo and the residue was treated with dry ether (200 ml) and the mixture stirred at RT for 4 hrs and filtered, to give 6.15 g (.7 mmol, 97%) of 6-(N-Me, N-Et carbamyloxy) aminoindan hydrochloride.
In this manner the following compounds of general formula I as shown in Tables 3, 3a and 4 were prepared. Spectral data relating to these compounds is given in Tables 7 , 7a and 8.
# position R1,R2 R3 R4 cryst/slurry solvent mp(°C) yield (%)
1 6- H,H Me Me 156-8 93
2 6- H,H Me Pr 165-7 27
3 6- H,H Me Et 150-2 50
4 7- H,H Me Me 156-60 93
5 7- H,H Me Et 185-7 55
6 7- H,H Me Pr 153-5 33
7 6- H,Et Me Me 172-4 91
8 6- H,Me Me Me 178-80 88
9 7- H,Me Me Me dioxane 169-71 98
10 6- H,Me Me Et 172-4 87
11 6- H,Me Me Pr 165-7 98
12 6- Me,Me Me Me 164-6 62
13 4- H,H Me Me 198-200 90
14 4- H,H Me Et 183-5 92
15 6- H,H Me n-hexyl dioxane 111-12 78
16* 6- H,H Me Et 197-8 89
17 6- H,H Me cyclohexyl 207-8 86
18** 6- H,H Me Et 202-4 84
48 6- H,H H Et MeOH/EtOAc 191-2 74
49 6- H,H H Pr MeOH/EtOAc 171-3 67
50 6- H,H Me p-OMe-Phenyl iPrOH 225-7 92
51 6- H,H Me 78
52* 6- H,H Me Me 83
53** 6- H,H Me Me 81
88 6- H,H Me Ph 96
66*** 6- H,H Me Et 116-9 92
67*** 6- H,H Me Pr 181-3 86
80 6- H,H Me Bu 54
84 6- H,H Et cyclohexyl 196-8 89
*R-enantiomer **S-enantiomer ***5-chloro
# position R1,R2 R3 R4 cryst/slurry solvent mp(°C) yield (%)
44 6- H,H Me Me MeOH/EtO 244-5 55
45 6- H,H Me Et MeOH/EtOAc 236-8 58
# position of amine R1 R3 R4 cryst/slurry solvent mp(°C) yield (%)
19 2- H Me Me ether 96
20 2- H Me Et ether 98
21 1- H Me Me ether 196-8 99
22 1- H Me Et ether 166-8 85
a): wide melting range; compound is a hemi-hydrate
C: Propargylation and salt formation
The compounds prepared in Step B may be optionally propargylated to provide further compounds of general formula I.
6-(N-Me, N-Et carbamyloxy) N-propargyl aminoindan. HCl (Compound 25)
To a stirred mixture of 6-(N-Me, N-Et carbamyloxy) aminoindan, HCl (5.2 g, 19.2 mmol), potassium carbonate (5.31 g, 38.4 mmol) in acetonitrile (250 ml), was added a solution of propargyl bromide (2.06 g, 17.28 mmol) in acetonitrile (10 ml). The reaction mixture was stirred at RT under nitrogen for 25 hrs, and filtered. The filtrate was evaporated to dryness in-vacuo and the residue was purified by column chromatography (EtOAc) to give 3.6 g (13.2 mmol, 69%) of the free base as a yellow oil.
The free base was dissolved in dry ether (150 ml) and HCl/ether (15 ml) was added. The mixture was stirred at RT for 1 hr, filtered and the solid was recrystallized from iPrOH/ether to give 3.5 g (11.3 mmol, 59%) of the title compound as a white solid.
6-(N,N-Dimethylcarbamyloxy)-N-propargyl aminoindan mesylate (Compound 24)
To a stirred mixture of 6-(N,N-dimethylcarbamyloxy) aminoindan HCl (1.88 g, 7.33 mmol), K2CO3 (2.03 g, 14.66 mmol) and acetonitrile (70 ml) was added a solution of propargyl bromide (0.79 g, 6.6 mmol) in CH3CN (5 ml) dropwise over 5 min, under nitrogen. The mixture was stirred under N2 for 24 hrs, filtered and the solvent was removed at reduced pressure. The residue was taken up into water (150 ml) and toluene (150 ml). This mixture was stirred while adjusting the pH of the aqueous layer to 3.75 by the addition of 20% aq. HCl. The aqueous layer was separated and extracted with toluene (2x100 ml) and brought carefully to pH 7.5 by the addition of 10% aq. NaOH solution. It was then extracted with toluene (100 ml + 4x70 ml). The combined toluene layers were dried (Na2SO4), filtered and the solvent was removed under reduced pressure to give 1.06 g (62%) of a yellow oil.
To a stirred solution of the free base (1.65 g, 6.4 mmol) in anh. ether (60 ml) was added dropwise a solution of methanesulfonic acid (0.7 g, 7.29 mmol) in ether (10 ml). The resulting suspension was stirred at 25° C for 30 min and then allowed to settle for an additional 30 min. The ether was then decanted off, and the residue was dried under vacuum. It was then recrystallized from iPrOH/ether to give 2.05 g of a white solid (90.3%).
In this manner the following compounds of general formula I as shown in Tables 5, 5a and 6 were prepared. Analytical data relating to these compounds is given in Tables 9, 9a and 10.
# X position R1 R3 R4 cryst/slurry solvent mp (°C) yield (%)
23 Cl 6- H Me Me 180-2 52
24 mesylate 6- H Me Me 147-9 60
25 Cl 6- H Me Et 194-6 59
26 Cl 6- H Me Pr 183-5 46
27 Cl 7- H Me Me 219-20 65
28 Cl 7- H Me Pr 185-6 53
29 Cl 6- Me Me Me 199-201 55
30 Cl 6- Me Me Et 196-8 47
31 Cl 6- Et Me Me 212-3 71
32 Cl 7- Me Me Me 169-71 63
33 Cl 7- H Me Et 208-9 64
34 Cl 4- H Me Me 196-8 85
35 Cl 4- H Me Et 183-5 85
36 Cl 6- H Me n-hexyl 106-8 53
37* Cl 6- H Me Et 159-60 88
38 Cl 6- H Me cyclohexyl 174-5 55
39** Cl 6- H Me Et 160-2 61
54* mesylate 6- H Me Me 139-41 54
55** mesylate 6- H Me Me 138-40 52
56 Cl 6- H H Et 175-7 38
57 Cl 6- H H Pr 165-7 48
58* mesylate 6- H Me Et 92-4 64
59** mesylate 6- H Me Et 72
60 mesylate 6- H Me Et 121-3 87
61 Cl 6- H Me p-OMe-Ph 172-4 84
62 Cl 6- H Me Ph 182-4 61
63 Cl 6- H Me 188-90 58
64*** Cl 6- H Me Me 195-7 55
65*** Cl 6- H Me Et 188-90 51
68**** fumarate 6- H Me Et iPrOH 146-8 48
69* fumarate 6- H Me Et iPrOH 115-7 35
70 esylate 6- H Me Et EtOAc 109-11 60
71**** Cl 6- H Me Et 161-3 55
72**** Cl 6- H Me Pr 164-6 58
73** fumarate 6- H Me Et iPrOH 114-6 81
74" esylate 6- H Me Et EtOAc 95-7 82
75** 1/2 D-tartrate 6- H Me Et iPrOH 143-5 44
76* 1/2 L-tartrate 6- H Me Et iPrOH 143-5 41
77* esylate 6- H Me Et EtOAc 106-8 93
78* Cl 6- H Me Pr 126-8 89
79* Cl 6- H Me Pr 135-7 33
81 Cl 6- H Me Bu 168-70 63
83 Cl 6- H Et Bu 148-50 42
85 Cl 6- H Et cyclohexyl 178-80 56
86* Cl 6- H Me Bu 86-8 51
87** Cl 6- H Me Bu 88-9 52
Table 5a Thiocarbamyloxy-N-propargyl aminoindans
 Table 5a Thiocarbamyloxy-N-propargyl aminoindans
# X position R1 R3 R4 cryst/slurry solvent mp (°C) yield (%)
46 Cl 6- H Me Me 152-4 53
47 Cl 6- H Me Et 193-5 54
# position of amine R1 R3 R4 cryst/slurry solvent mp (°C) yield (%)
40 2- H Me Me 206-8 66
41 2- H Me Et 208-9 65
42 1- H Me Me ether 207-9 57
43 1- H Me Et ether 201-3 42
aryl indan R1, R2 R3, R4
1 7.38,7.20 4.85,3.10 3.10,2.96 3446,2943 221 calc.: 56.14,6.62,10.90
7.10 2.96,2.63 1711,1487 found: 55.90,6.67,10.89
2.14 1393,1240
2 7.40,7.21 9.80,3.10 3.43,3.27 2970,2863 249 calc.: 59.05,7.38,9.84
7.10 2.95,2.65 3.10,2.95 1735,1608 found: 58.75,7.33,9.86
2.15 1.70,1.63 0.94,0.90 1396,1241
2a calc.: 57.23,7.55,9.54
- " - - " - - " - - " - found: 57.54.7.29.9.45
4 7.47,7.36 4.91,3.25 3.18,3.03 2950,1701
7.09 3.07,2.60 1504,1396
2.25 1234,1177
5 7.44,7.29 4.88,3.20 3.55,3.39 3446,2920 235 calc.: 57.70,7.25,10.35
7.02 3.14,2.55 3.14,2.99 1710,1472 found: 57.38,6.97,10.32
2.23 1.26,1.18 1403,1235
6 7.45,7.30 4.86,3.20 3.50,3.32 3448,2923 249 calc.: 59.05,7.43,9.84
7.02 3.04,2.55 3.13,2.99 1710,1485 found: 58.78,7.47,9.91
2.23 1.70,1.63 1226,1154
0.94,0.90
7 7.45,7.29 4.83,3.17 3.20,1.33 3.15,3.0 2948,2766 249 calc.: 59.05,7.38,9.84
7.17 3.02,2.65 2680,1725 found: 57.75,7.40,9.65
1485,1386
8 7.43,7.27 4.75,3.14 2.73 3.13,2.97 2950,2722 235 calc.: 57.70,7.02,10.35
7.17 3.03,2.60 1720,1390 found: 56.83,7.09,10.27
2.30 1160
9 7.52,7.37 4.83.3.27 2.74 3.19,3.04 2963,2710 235 calc.: 57.70,7.02,10.35
7.10 3.10,2.55 1715,1579 found: 57.46,6.73,10.36
2.38 1472,1389
10 7.44,7.25 4.80,3.15 2.74 3.35,3.35 2950,2705 calc.: 59.08,7.38,9.84
7.15 3.03,2.62 3.12,2.98 1720,1450 found: 58.74,7.51,9.72
2.30 1.25,1.18 1402
11 7.42,7.25 4.75,3.15 2.72 3.45,3.30 2963,2723 calc.: 60.33,7.70,9.38
7.14 3.10,2.60 3.10,2.95 1715,1465 found: 60.32,7.75,9.42
2.28 1.65,0.94 1404,1234
0.88
12 7.43,7.27 4.96,3.12 2.75 3.10,2.96 3480,1718 249 calc.: 59.05,7.38,9.84
7.17 3.05,2.55 1475,1390 found: 58.75,7.41,9.84
2.42 1237,1174
7.53,7.29 4.71,2.95, 8.75 3.04,2.9 221
7.08 2.74,2.43,
2.0
7.53,7.3, 4.71,2.95, 8.7 3.41,3.3, 235
7.08 2.73,2.48, 3/01,2.89,
2.0 1.18,1.07
15 3.1,3.06 2930,1720 291 calc.: 62.47,8.33,8.37
7.35,7.23 4.83,3.3 2.95,2.91 1471,1405 found: 62.54,8.30,8.61
7.01 2.6.2.16 1.6,1.29 1248
0.85
16 7.42,7.22 4.87,3.16 3.53,3.39 235
7.12 3.01,2.65 3.92,2.99
2.17 1.26, 1.17
17 7.42, 7.22 4.87,3.15 4.10,3.85 289 calc.: 62.85,7.76,8.63
7.11 2.95,2.6 3.00,2.85 found: 62.35,7.81,8.33
2.19 1.90-1.40
1.34,1.13
3 7.43, 7.20 4.86,3.15 3.51,3.38 235 calc.: 55.70,7.25,10.35
7.12 3.02, 2.64 3.10,2.95 found: 57.44,7.06,10.38
2.18 1.23,1.15
18 7.43, 7.20 4.86.3.15 3.51,3.38 235 calc.: 55.70,7.25,10.35
7.12 3.02,2.64 3.10,2.95 found: 57.44,7.06,10.38
2.18 1.25,1.15
48 7.41,7.24 4.87,3.13 3.23,1.17 221 calc.: 56.13,6.68,10.91
7.13 3.0.2.65 found: 36.00,6.66,10.81
2.17
49 7.41,7.24 4.87.3.12 3.17,1.56 235 calc.: 57.67,7.07,10.35
7.13 2.98,2.65 0.94 found: 57.32,7.13,10.31.
2.17
50 7.37,7.16 4.80, 3.10 7.40-7.0 calc.: 61.98,6.02,8.03
7.03 2.96, 2.61 3.82, 3.43 found: 61:16,6.07,7.77
2.15 3.29
66 7.57,7.39 4.91,3.18 3.61,3.43 269 calc.: 50.41,6.02,9.05
3.05,2.71, 3.20,3.03 271 found: 50.46.6.11,8.77
2.25 1.33,1.23
67 7.55,7.36 4.89,3.14 3.52,3.36 283 calc.: 52.67,6.32,8.78
3.02,2.68 3.18,3.02 285 found: 52.67,6.28,8.48
2.20 1.77,1.67
0.99,093
Table 7a
Table 7a
aryl Indan R1, R2 R3, R4
7.45,7.20, 4.87,3.15. 3.44,3.36 2833,1714, calc.: 52.83,618,10.21,11.75 found: 51.11,6.48,10.23,12.16
44 7.11 3.05,2.65, 1599,1536,
2.20 1488,1392
7.45,7.20, 4.75,3.10, 3,88.3.79, 2934,1719. calc.: 51.22,6.94,9.19,10.52 found: 51.04,7.30,9.31,11.24
45 7.11 2.97,2.85, 3.39,3.32. 1594,1622.
2.20 1.28,1.25 1497,1402
Table 8
Table 8
aryl cyclohex. R1, R2 R3, R4
19 7.22,6.95 3.69,3.22 3.12,2.97 3484,2930 calc: 55.81,7.20,10.02 found: 55.29,6.93,9.71
2.93.2.97 2362,1699 235
2.22.1.92 1612, 1500 1391
20 7.20,6.94 3.70,3.19 3.48,3.35 calc: 37.23,7.55,9.54 found : 57.0,7.53.9.54
2.90,2.23 3.08,2.94 249
1.90 1.20,1.12
21 7.28,7.11, 4.56,2.87 3.10,2.96 235 calc: 57.70,7.02,10.35 found: 56.97,6.93,10.06
7.06 2.77,2.16
2.05,1.88
22 7.29,7.13 4.57,2.88 3.52,3.37 249 calc: 59.05,7.38,9.84 found: 58.91,7.18,9.99
7.07 2.79,2.15 3.10,2.97
2.05,1.90 1.25,1.17
Table 8
Table 9
Table 9
aryl indan R1 proparg R3,R4
23 7.46.7.30 5.01,3.20 4.0,3:16 3.15,3.0 239 calc.: 61.12,6.50,9.51
7.18 3.15,2.65 found: 60.93,6.38,9,47
2.36
24 7.46,7.30 5.01,3.20 4.0,3.16 3.15,3.0 1711,1482, 259 calc.: 54.22,616,7.91
7.18 3.15,2.65 1439,1394, found: 53.92,6.28,7.84
2.36 1192,1170
25 7.42, 7.27 4.97,3.16, 3.97,3.02 3.52,3.36 1728,1435, 273 calc. 62.23,6.86,9.37
7.15 3.0,2.62, 3.10,2.97, 1403, 1242, found: 62.42,6.84,8.94
2.32 1.24,1.15 1166
7.50,1.32 4.78,3.10 3.91,3.74 3.43,3.32 273
7.10 2.85,2.45 3.03,2.90 -"- -"-
2.28 1.20,1.10
26 7.45,7.30 5.0.3.16 4.0,3.03 3.48,3.32 1725,1465, 287 calc.: 63.25,7,18,8.68
7.17 3.04,2.65 3.12,2.98 1429,1403, found: 63.13,7.28,8.93
2.33 1.72,1.63 0.96,0.92 1232,1165
27 7.52,7.38 5.05,3.26 3.99,3.21 3.12,3.03 3200,1722, 259, calc.: 61.12,6.50,9.51
7.10 3.07.2.56 1567,1434, found:61.01,6.46,9.64
2.40 1408,1238
28 7.52,7.37 5.02,3.27 3.98,3.10 3.65,3.42 3200,1727, 287 calc.: 63.25,7.18,8.68
7.07 3.09,2.55 3.18,3.02 1566,1468, found: 63.06,7.30,8.37
2.38 1.75,0.98 1438,1406,
0.93 1222
29 7.44,7.30 5.20,3.15 2.80 4.01,3.13 3.12,2.97 1729,1388, 273 calc.: 62.33,6.80,9.07
7.19 3.03,2.57. 1234,1165 found:61.97,6.80,8.78
2.44
31 7.48,7.30 5.34,3.20 3.36, 4.05,3,12 3.16,3.01 3180,1723, 287 calc.: 63.25,7.18,8.68
7.23 3.08,2.65 1.37 1490,1440, found :63.42,7.09,8.71
2.50 1389,1230,
1160
32 7.56,7.39 5.30,3.28 2.78 4.12,3.23 3.20,3.02 1712,1472, 273 calc.: 62.23,6.86,9.07
7.15 3.09,2.55 1392,1238, found :62.05,6.81,8.87
1171
33 7.46,7.32, 4.96,2.50 3.92,3.04 3.13,2.96 1719,1426, 273 calc.:62.23,6.86,9.07
7.03 2.33 1.24,1.15 1404,1233, found:62.19,6.77,9.08
1154
34 7.48,7.23 5.07,3.08 4.05,3.07 3.29,3.03 3238,2907 calc.:
2.95,2.65 2769,2635 259 found:
2.35 1714,1470
1392,1240
35 7.48,7.23 5.07,3.08 4.05,3.07 3.56,3.41 3197,2934 calc.:
2.95,2.65 3.15,3.01 2363,2431 273 found:
2.35 1.29,1.21 1707,1445
1403,1236
36 7.45,7.28 7.15 4.98,3.16 3.98,3.04 3.49,3.35 calc.: 65.83,8.01.7,68
3.03,2.63 3.11,2.97 found: 65.65,8.11,7.82
2.33 1.66,1.33
0.88
37 7.44,7.29 4.98,3.15 3.98,3.03 3.53,3.38 3275,2754 273 calc.: 62.23,6.86,9.07
7.18 3.01,2.63 3.12,2.98 1719,1445 found: 62.30,6.94,9.09
2.31 1.25,1.16 1393,1303
38 7.44,7.27 4.98,3.14 3.98,3.04 4.09,3.85 3227,2936 327 calc.: 66.19,7.50,7.72
7.16 3.00,2.64 3.01,2.88 2612,2128, found: 65.90,7.63,7.55
2.33 1.90-1.45 1711,1584
1.35,1.14 1440, 1401
39 7.46,7.30 4.97,3.17 3.97,3.03 3.54,3.39 3275,2933 273 calc. 62.23,6.86,9.07
7.19 3.04,2.64 3.13,3.0 2758,1720 found: 62.27,6.95,9.03
2.32 1.27,1.19 1445,1396
1303
54 7.46,7.30 5.00,3.17 3.99,3.05 3.15,3.0 1711,1482 259 calc.: 54.17,6.20,7.90
7.19 3.05,2.64 1438,1395 found:54.18,6.27,7.78
2.33 1192,1169
55 7.46,7.30 5.00,3.17 3.99,3.05 3.15,3.0 1711,1482 259 calc.: 54.17,6.20,7.90
7.19 3.05,2.64 1438,1395 found: 54.07,6.25,7.88
2.33 1192,1169
56 7.46,7.32 4.99,3.17 3.99,3.05 3.27,1.20 259 calc.: 61.12,6.50,9.51
7.20 304,2.65 found: 60.87,6.47,9.34
2.33
57 7.47,7.32 4.99,3.18 3.99,3.06 3.20,1.61 273 calc.: 61.23,6.86,9.07
7.20 3.05,2.65 0.98 found: 61.60,6.93,9.04
2.34
58 7.47,7.32 5.01,3.20 4.01,3.07 3.56,3.41 273 calc.: 55.43,6.52,7.60
7.22 3.08,2.67 3.14,3.01 found:55.08,6.52,7.31
2.36 1.29,1.21
59 7.47,7.32 5.01,3.20 4.01,3.07 3.56,3.41 273 calc.:
7.22 3.08,2.67 3.14,3.01 found:
2.36 1.29,1.21
60 7.47,7.32 5.01,3.20 4.01,3.07 3.56,3.41 273 calc.: 55.43,6.52,7.60
7.22 3.08.2.67 3.14,3.01 found: 55.21,6.64,7.40
2.36 1.29,1.21
61 7.40-7.0 4.96,3.10 3.96,3.90 7.40-7.0 351 calc.: 6.5.20,5.95,7.24
2.97,2.57 3.03 3.81 found:64.72,6.04,6.81
2.30
62 7.60-7.10 4.96,3.15 3.98,3.07 7.60-7.10 321 calc.: 67.32,5.89,7.85
3.00,2.61 3.42 found: 67.22,6,00,7.54
2.34
63 7.55-7.10 4.97,3.17, 3.99,3.07 7.55-7.10 335 cale.: 67.47,6.20,7.55
3.00,2.64, 4.73,4.59 found:67.75,6.32,7.47
2.36,2.36 3.14,3.05
64 7.48,7.35 5.16,5.12 4.44,4.27 3.17,3.03 273 calc. 62.23,6.86,9.07
7.21 3.20,3.05 3.17,1.68 found: 62.12,6.86,8.96
2.70,2.35 1.63
65 7.44,7.36, 5.15,5.09 4.43,4.25 3.35,3.39 calc.: 63.25,7.18,8.68
7.27,7.19 3.20.3.02 3.25,3.17 3.13,3.00 found: 63.15.7.15,8.31
2.65,2.32 1.67,1.61 1.27,1.19
71 7.60,7.44 5.02,3.20. 4.02,3.07 3.60,3.43. 307 calc.: 55.98, 5.87, 8.16
3.06,2.68, 3.20,3.02, 309 found: 55.72,5.88,8.11
2.36 1.33, 1.23
72 7.59,7.44 5.01,3.20, 4.03,3.07 3.53, 3.36, 321 calc.:57.15,6.21,7.84
3.06, 2.68, 3.20,3.02. 323 found:57.05.6.21.7,81
2.38 1.79,1.68,
1.01,0.95
76 7.47,7.31, 5.00,3.20, 4.00,3.07 3.56,3.40, 3286, 2972, 273 calc.: 62.17,6.62,8.05
7.20 3,06,2,66, 3.16,3.00, 1724,1637, found: 62.31,6.66,7.94
2.35 1.28,1.20 1400,1308, 1233
81 7.48,7.31, 5.00,3.20. 4.01,3.07 3.53,3.38, calc.: 64.19,7.42,8.32
7.20 3.07, 2.66, 3.14,3.01, found: 63.99,7.42,8.04
2.35 1.65,1.39, 0.97
83 7.47,7.31, 5.00,3.19, 4.01,3.07 3.52,3.38, 315 calc.: 65.04,7.70.7.99
7.19 3.04,2.66. 1.68,1.40, found: 64.75,7.72,7.94
2.34 1.29,1.22, 0.98
85 7.47,7.31, 5.00,3.19, 4.01,3.07, 3.84,3.42 341 calc.: 66.33, 7.70, 7.43
7.19 3.02,2.63, 1.85,1.66, found: 66.75,7.69,7.36
2.34 1.23
Table 9
Table 9a
Table 9a
aryl indan propargyl R3, R4
46 7.48,7.29, 5.02,3.19, 4.0,3.07 3.48,3.41 calc.: 57.97,6.11,9.01,10.30 found: 58.07,6.06,8.85,10.23
7.18 3.05,2.67,
2.37
47 7.50,7.31 5.04,3.21. 4.20,3.09 3.95,3.87 calc.: 59.16,6.47,8.62,9.86 found: 59.23,6.39,8.52,9.76
7.19 3.07,2.70, 3.45,3.38
2.38 1.35,1.32
Table 10
Table 10
aryl cyclohex. R1 proparg R3,R4
40 calc :
found:
41 7.22,6.95 3.79,3.26 4.06,3.01 3.50,3.36 3227,2938 calc: 63.25,7.18,8.68
2.95,2.32 3.09,2.96 2768,1713 287 found: 63.16,6.93,8.69
1.91 1.24,1.16 1587,1474
1394,1301
42 7.21,7.03 4.60,2.81 3.88.2.95 3.01,2.87 3234,2936 calc: 62.23,6.80,9.07
2 72,2.15 2774,2130 273 found: 62.20,7.01,9.3
2.02,1.84 1732,1497
1.80 1390
43 7.32,7.12 4.65,2.88 3.99,3.04 3.51,3.37 3216,2933 calc : 63.06,7.41,8.65
2.80,2.20 3.10,2.96 2768,2663 287 found: 63.2,7.14,8.81
2.12,1.94 1.23,1.16 2129,1723
1.85 1425,1399
Table 10
Biological Examples Example 1 Acetylcholinesterase Inhibition in Mice 1.1 In vitro measurement of Acetylcholinesterase (AChE) Inhibition
Human erythrocyte acetylcholinesterase (type XIII, Sigma Israel), was prepared in a stock solution of 10/ml, containing Triton (1%) and bovine serum albumin (0.05%) in phosphate buffer (pH 8). The enzyme (0.05U) was incubated with 3-5 different concentrations of test compound (in triplicate) for periods of from 15 to 60 minutes at 37°C. The substrate acetylthiocholine (0.075M) and 5,5'-dithiobis-(2-nitrobenzoic acid) (DTNB, 0.01M) were then added and the rate of hydrolysis of the substrate which yields a yellow product monitored spectrophotomerically at 412nM (Ellman et al., Biochem Pharmacol. (1961) 7: 88-95). The percentage inhibition of AChE by each concentration of drug is calculated by comparison with that of enzyme, in the absence of drug. The concentration of each drug that inhibits AChE by 50% (IC50) at the time of peak activity was calculated and is given in Table 11 below.
1.2 Ex vivo measurement of Acetylcholinesterase (AChE) Inhibition
Test drugs or saline were administered sub-cutaneously to male mice (Sabra strain, 28-35g). At least 4-5 mice were used per dose and a minimum of 3 doses per drug were tested. The mice were sacrificed 15, 30, 60, 70, 90, 120 or 180 minutes after drug administration, the brains rapidly removed (minus cerebellum), weighed and homogenized in 0.1M phosphate buffer, pH 8.0, containing Triton (lmg/100g tissue) and centrifuged to remove cell debris. Aliquots (25 µl) of the supernatant were then incubated with acetylthiocholine and DTNB. AChE activity measured as described above. The % inhibition of whole brain AChE by each dose of drug was calculated by comparison with enzyme activity from 3 saline treated control mice run at the same time. The dose of each drug that inhibits AChE by 50% at the peak of activity (ED50) was calculated and is given in Table 11.
1.3 Acute Toxicity in Mice
Drugs were administered sub-cutaneously in at least 3 doses, to a minimum of 10 mice per dose. The dose that was lethal to 50% of the mice (LD50) within 6 hours after administration was calculated for each drug and is given in Table 11. Therapeutic Ratio was calculated as LD50 divided by ED50 of ex vivo acetylcholine esterase inhibition.
Example 2 2.1 Inhibition of MAO activity in vitro
The MAO enzyme source was a homogenate of rat brain in 0.3M sucrose, which was centrifuged at 600g for 15 minutes. The supernatant was diluted appropriately in 0.05M phosphate buffer, and pre-incubated with serial dilutions of test compounds for 20 minutes at 37°C. 14C-Labeled substrates (2-phenylethylamine, hereinafter PEA; 5-hydroxytryptamine, hereinafter 5-HT) were then added, and the incubation continued for a further 20 minutes (PEA), or 30-45 minutes (5-HT). Substrate concentrations used were 50 µM. (PEA) and 1mM (5-HT). In the case of PEA, enzyme concentration was chosen so that not more than 10% of the substrate was metabolized during the course of the reaction. Deaminated products were extracted into toluene-ethyl acetate (1:1 v/v) containing 0.6% (w/v) 2,5-diphenyloxazole (ppo) prior to determination by liquid scintillation counting. Radioactivity in the eluate indicates the production of neutral and acidic metabolites formed as a result of MAO activity. Activity of MAO in the sample was expressed as a percentage of control activity in the absence of inhibitors after subtraction of appropriate blank values. The activity determined using PEA as substrate is referred to as MAO-B, and that determined using 5-HT as MAO-A.
Concentrations of inhibitor producing 50% inhibition of substrate metabolism (IC50) were calculated from the inhibition curves, and are shown in Table 11.
2.2 Inhibition of MAO activity ex vivo
Male Sabra mice, weighing 45-50g were injected with test compound solutions (prepared in 0.9% saline). Each dose was administered to two or three mice. The mice were sacrificed two hours after drug administration or at a time corresponding to the peak AChE inhibition time (see Table 11). The brain and liver were rapidly dissected and stored in appropriate vials on ice. The tissues were weighed, diluted to 1/20 in sucrose 0.3M and stored at -20°C before performance of the MAO assay described above. The results given in Table 11 relate to measurements made on brain tissue only.
2.3 Inhibition of MAO activity following sub-acute administration to rats
Experiments were done in Sprague Dawley male rats. Procedures were repeated as described in Examples 2.1 and 2.2, but drug administration was continued daily for 14 days. At the end of this period animals were sacrificed and MAO levels determined in the brain, liver and intestines. Compounds 24, 25, 37 and 39 were administered sub-cutaneously and/or per os at a dose of 6mg/kg(sc) and 10mg/kg(po) (compound 24), 25 and 50mg/kg (compound 25), 45mg/kg (compound 37) and 40mg/kg (compound 39). The results are shown in Table 11a from which it can be seen that these compounds displayed selectivity in inhibiting MAO enzyme sub-types in the brain in preference to the periphery.
AChE inhibition Time MAO-B Inhibition MAO-A Inhibition Acute Toxicity
In vitro Ex vivo to peak activity to return to 50% of peak In vitro Ex vivo In vitro Ex vivo
IC50 µM ED50 µmoles/kg (AC) 1 (min) 1(min) IC50 µM ED50 µM µmoles/kg IC50 µm ED50 µmoles/kg LD50 µmoles/kg (LD) Therapeutic Ratio LD/AC
1 0.6 5.0 30 >120 >1000 >>80 75 >>80 83.8 16.8
23 3.5 22.4 15 70 600 100 800 >120 255 11.4
2 7.3 NT >1000 32
3 20.0 46.3 60-90 >180 >1000 12.6 950 20.6
25 53.0 140.0 60 >180 >1000 200 270 >>350 1400 10.8
26 17.0 120 30-60 264 333 114 >>440 1200 9
27 5.72 30 15 >60 >1000 >>160 >1000 >>160 300 10
28 100.0 NT
5 11.5 85.0 60 >120 >>277 >>277 840 9.9
7 32.0 NT >1000 600
8 1.0 10.0 15-30 >60 >1000 >>50 50 >>50 87 8.7
9 0.18 1.9 15 93 4.9
29 8.5 53.3 15 >60 40 30 40 50 500 9.3
10 38.0 34.7 60-90 >180 >1000 >175 22 >175 740 21.3
30 1300.0 NT
31 10.0 110 >1000 >100 >1000 >100
32 3.7 7.8 15 500 >>20 190 >>20 68 9.0
12 2.0 8.0 15 >1000 130 <20 <2.5
33 540.0 NT >1000 1000 >1000 >>1200
34 0046 0.65 30 100 0.5 3.7 5.7
35 2.2 10 60 100 <1 33 3.3
37 51 125 500 200 750 >200 1700 13.6
39 36 80 30-60 >180 1000 >>200 550 >>200 1150 14.4
24 3 16.6 15 750 100 850 >120 179 10.8
60 42
58 51 >1000 300
54 1.8 >100 >100
55 2 >100 >100
56 11.5 180
57 2.4 70 25 69
48 10
49 2
17 4
16 9
50 0.26
61 0.75 47 500 >100 700 >100
64 1.9 13.2 >1000 >120 1000 >120 150 11.4
38 33 >1000 10 >400 170 >400
36 15 >400 >1000 >100 >1000 >100 >1000
62 0.57 290 60 100 >>200 80 >>200
63 2.5 140 60-90 120 >300 40 >300 1300 9.3
71 29 >100 130 >100
72 38 >200 >100 >100
78 10 101 60-90 >120 450 >>450 1300 12.9
79 9.4 94 90 >180 >>450 >>450 1000 10.6
81 11.5 40 90 >120 >>100 >>100 920 23
83 80
86 10.5
87 9.1
85 17 >100
Table 11a.
%MAO-A inhibition %MAO-B inhibition
Compound 24 25 37 39 24 25 37 39
Dose (mg/kg) 6(sc) 10(po) 25 50 45 40 25 25 50 45 40
Brain sc 30 53 75 78 17 50 61 45 87 27
po 0 0 70 67 20 80 82
Intestine sc 0 30 0 0 0 29 45 26 40
po 30 25 0 20 30 21
Liver sc 0 0 10 0 0 0 14 40 29 0
po 10 25 28 0 35 28
Example 3 Effect of drug treatment following closed head injury (CHI) in mice
The procedure for closed head injury followed was as described for rats in Shohami, et al. (J Neurotrauma (1993) 10(2): 109-119) with changes as described.
Animals: Male Sabra mice (Hebrew University strain) weighing 34-40g were used. They were housed in groups of 10 per cage, in a 12hr:12hr light:dark cycle. Food and water were provided ad libitium.
Trauma was induced under ether anesthesia. A longitudinal incision was performed in the skin covering the skull and the skin retracted to expose the skull. The head was fixed manually at the lower plane of the impact apparatus. A weight of 333g was delivered by an electric device from a distance of 3cm to the left hemisphere, 1-2mm lateral to the midline in the midcoronal plane. Test compounds were injected sub-cutaneously at a dosage corresponding to the ED50 acetylcholinesterase, once 15 min. after CHI.
3.1 Assessment of Motor Function.
Motor function and reflexes were evaluated in the injured mice at different times after closed head injury (CHI) using a neurological severity score (NSS) as shown in Table 12 below, which is modified from that described for rats (Shohami, et al. supra.). One point was awarded for the lack of a tested reflex or for the inability to perform the tasks outline in the Table. The maximal score that can be reached at 1 hour post-CHI is 25 points and 21 at later times. The difference in NSS at 1hr and at any other time reflects the recovery, and is referred to as ΔNSS. An NSS score of 15-19 at 1hr denotes severe injury, 11-14 moderate injury and less than 10 mild injury. The NSS recorded after treatment with test compound or control is shown in Table 13. Table 12
Parameter Points at 1 hour Points at any other time
Inability to exit from a circle (30cm diameter) when left in its center
for 30min 1
for 60 min 1
for >60 min 1 1
Loss of righting reflex
for 10 second 1
for 20 seconds 1
for >30 seconds 1 1
Hemiplegia inability of mouse to resist forced changes in position 1 1
Flexion of hind limb when lifted by tail 1 1
Inability to walk straight when placed on the floor 1 1
Reflexes
Pinna reflex 1 1
Corneal reflex 1 1
Startle reflex 1 1
Clinical grade
Loss of seeking behaviour 1 1
Proscanon 1 1
Loss of reflexes
Left forelimb 1 1
Right forelimb 1 1
Left hindlimb 1 1
Right hindlimb 1 1
Functional test
Failure in beam balancing task (0.5cm wide) 1 1
for 20 seconds 1 1
for 40 seconds 1 1
for > 60 seconds
Failure in round stick balancing task (0.5cm in diameter
for 10 seconds 1 1
3cm wide 1 1
2cm wide 1 1
1cm wide 1 1
Maximum Points 25 21
Results Assessment of Motor Function.
Table 13.
Drug/dose N ΔNSS, 24 hr post-CHI ΔNSS, 7 days post-HCI ΔNSS, 14 days post-CHI
Saline, 1ml/kg 51 4.75±0.17 3.83±0.36 5.96±0.4
1 (1.3mg/kg) 10 5.50±0.34* 7.31±0.42* 9.21±0.47
24 (6.5mg/kg) 12 6.11±0.23* 8.67±0.41* 9.67±0.66*
25(46mg/kg) 10 5.00±0.42 7.42±0.62* 9.01±0.69*
10 4.90±0.43 7.70±0.33* 8.80±0.33*
10 (15mg/kg) 11 5.36±039 6.64±0.41* 6.73±0.52
37 (30mg/kg) 12 5.50±0.26 6.92±0.38 8.25±0.62
39 (30mg/kg) 14 5.36±0.25 6.71±0.45 7.64±0.48
Table 13.
1. administered 60min before CHI *significantly different from saline control (p<0.05)
3.2 Assesement of Reference Memory
Morris Water Maze Test: the water maze consists of a circular aluminium pool, 1m in diameter and 60cm in depth, filled with water to a depth of 17.5cm. The hidden goal platform is a glass vessel (15cm diameter x 16.5cm height) placed upside down at' a fixed location in the pool, 1cm below the surface of the water. The water temperature is maintained at 24°C and the pool is always placed in the same position in the room to provide the same extra-maze cues. Prior to CHI (as described in Example 3 above), mice were given 3 trials per day for 5 consecutive days to establish a baseline performance - measured as the latency to find the platform from the same start location. Commencing 24hr after CHI, mice were retested daily for 2 weeks in 3 trials per day.
Figures 1, 2 and 3 show the reduction in latency for mice treated with compounds 24 (6.5mg/kg), 25 (46mg/kg), 1 (1.3mg/kg), 10 (15mg/kg), 37 (30mg/kg) or 39 (30mg/kg) compared to saline treated controls after CHI. It appears that immediately post-CHI mice forget the location of the goal Memory is enhanced following treatment with test compounds, as compared to saline treated mice. In the Figures the arrow shows the time of CHI:
Example 4: Effect On Mice Having Experienced A Hypobaric Hypoxic Episode
The hypobaric hypoxic model is a well accepted model for assessing the activity of compounds believed to possess neuroprotective activity. The model is based on that described in Nakanishi, M., et al. Life Sci. (1973) 13: 467, Oshiro, et al. , J. Med. Chem. (1991) 34: 2004-2013 and US Patent 4,788,130 .
A 12 liter desiccator (desiccator A) and a 2.5 liter desiccator (desiccator B) were separately connected to a vacuum pump. Desiccator B was disconnected and allowed to equilibrate with room air whilst desiccator A was evacuated to a pressure of 100mmHg. Four male ICR albino mice (22-28g) were placed in desiccator B. Desiccator B was then closed to room air and connected to desiccator A. The pressure inside desiccator B was monitored using a mercury manometer and at the point were the pressure in desiccator B reached 200mmHg (usually within 14 seconds), the two desiccators were disconnected from the vacuum pump and the pump switched off. The survival time from the moment of induction of hypoxia to the time of cessation of respiration was recorded for each mouse for a maximum of 15 minutes after which time room air was reintroduced to desiccator B. Survivors were monitored for signs of lethargy or vitality.
Effect of drug treatment was assessed as the percent of the survival time of the drug-treated group with respect to the saline injected or vehicle injected control group. Control groups were run twice, before and after each experimental group and consisted of 8 mice in groups of 4 mice to ensure a constant residual volume of oxygen in all tests. The effect of each dose of test drug was determined in duplicate i.e. two groups of 4 mice. The range of survival times of control mice was from 108-180 seconds.
Positive reference drugs were sodium pentobarbital at a dose of 40 mg/kg, and diazepam 10 mg/kg given 0.5h prior to hypoxia, physostigmine 0.2 and 0.4 mg/kg and neostigmine 0.2 mg/kg given sc 30 min before hypoxia. Methyl atropine 1 mg/kg was given sc. 10 min. before physostigmine.
Test drugs were dissolved in 0.9% saline, and injected sc. in the nip of the neck at a dose in accordance with body weight, 60-90 min. before hypoxia. The volume of injection was 0.2-0.3 mL per mouse (10 mL/kg). The initial dose was about one third of the reported LD50 for acetylcholine esterase inhibition. If no protection could be obtained, the dose was further increased to the nearest non-toxic dose. In case of protection, the dose was further reduced in an attempt to locate the "protective" dose range. .
Per cent survival times as compared to saline treated control is shown in Table 14. Table 14.
Compound Dose mg/kg Time of dose (min before hypoxia) Protection (% of control) p
Control (saline) 100
Nembutal 40 30 253±200 <0.005
Diazepam 10 30 316±78 <0.003
Neostigmine 0.2 30 141±32 <0.01
Physostigmine 0.2 30 453±222 <0.001
0.4 30 552±210 <0.001
Physostigmine and Atropine methyl nitrate 0.4 30 296±193 <0.05
1.0 40
1 8 60 637±116 0.007
4 60 470±200 0.001
2 60 120±51 NS
24 50 60 738±00 <0.001
21 60 269±166 <0.02
25 100 60 761±91 0.001
75 60 559±225 0.001
50 60 380±231 0.01
25 60 84±35 NS
27 50 60 455±23 <0.001
3 60 287±119 <0.001
15 60 143±56 <0.05
8 60 119±45 NS
29 77 60 508±206 <0.001
51 60 638±10 <0.001
25 60 131±56 NS
25 30 273±183 <0.02
10 50 90 705±101 0.001
25 90 700±201 0.001
10 90 304±129 0.001
12 20 60 725±129 <0.001
15 60 649±221 <0.001
10 60 386±238 <0.01
7 60 248±97 <0.001
Example 5 Neurological score and brain infarct size in male Wistar rate after middle cerebral arrery occlusion (MCA-O)
A modification of the procedure described by Tamura, et al was used (Tamura A, Graham Dl, McCulloch J, Teasdale GH (1981) J. Cereb. Blood Flow and Metab. 1: 53-60). Male Wistar rats (Olac England-Jerusalem) 300-400g each were anesthetized with a solution of Equitesine administered i.p. at a dose of 3 ml/kg. Equitesine consists of 13.5 ml sodium pentothal solution (60 mg/ml), 3.5 g chloral hydrate, 1.75 g MgSO4, 33 ml propylene glycol, 8.3 ml absolute alcohol, made up to 83 ml with distilled water.
Surgery was performed with the use of a high magnification operating microscope, model SMZ-2B, type 102 (Nikon, Japan) In order to expose the left middle cerebral artery, a cut was made in the temporal muscle. The tip of the coronoid process of mandible was excised as well and removed with a fine rongeur. Craniectomy was made with a dental drill at the junction between the median wall and the roof of the inferotemporal fossa.
The dura matter was opened carefully using a 27 gauge needle. The MCA was permanently occluded by microbipolar coagulation at low power setting, beginning 2-3 mm medial to the olfactory tract between its cortical branch to the rhinal cortex and the laterate striate arteries. After coagulation, the MCA was severed with microscissors and divided to ensure complete occlusion. Following this, the temporalis muscle was sutured and laid over the craniectomy site. The skin was closed with a running 3-0 silk suture. A sham craniectomy operation was performed on a parallel group of rats, but without cauterization of the MCA.
During the entire surgical operation (20-25 min) in either group, body temperature was maintained at 37 to 38°C by means of a body-temperature regulator (Kyoristsu, Japan) consisting of a self-regulating heating pad connected to a rectal thermistor. At 24 and 48 hours post surgery a neurological score was taken in order to assess the severity of the injury in the drug-treated rats with respect to their untreated controls.
Drugs were administered as an s.c. injection, according to the following schedule :
  • Compound 24: 7.8mg/kg 15 minutes prior to MCA-O and 6.5mg/kg 2 hours post MCA-O.
  • Compound 25: 43mg/kg 90 minutes prior to MCA-O and 30mg/kg 3 hours post MCA-O.
After 48 hours of ischemia induced by permanent occlusion morphometric, the animals were anesthetized with Equitesine and measurement of infarct volume was performed as follows by TTC (2,3,5-triphenyl tetrazolium chloride) staining. TTC 1% in saline was prepared immediately before use and protected from exposure to light by aluminum foil wrap. MCA-O rats were deeply anesthetized and a 23-gauge butterfly needle with an extended tubing and a 20 ml syringe was inserted into the ventricle via thoracotomy. The right atrium was incised to allow outflow of saline. Heparine 50 i.u. in saline was delivered until the perfusate was bloodless. A 30-ml TTC-filled syringe was exchanged for the saline syringe and TTC was injected into the left ventricle at a rate of 5 ml/min. Both perfusate solutions were administered at 37.5°C. The brains were removed and immersed into 20 ml of 1% TTC contained in tightly closed glass vials. These were further placed for 2 hours in a water bath maintained at 37°C. The TTC solution was decanted, the brains removed, wiped dry and placed into 10% buffered formalin solution for 3 days. Six coronal slices each 2 mm thick, 3,5,7,9,11 and 13mm distal from the frontal pole were obtained with a brain matrix (Harvard Apparatus, South Natick, MA). Infarction areas were measured with a video imaging and analyzer from both sides of the coronal slices and expressed in mm2. The volume of the infarcted region in mm2 was calculated by taking the sum of the ischemic areas in all six slices.The volume of infarcted region for the saline control and compounds 24 or 25 are given in Table 15a.
Neurological score
The neurological score was measured in a manner slightly different from that given in Example 3. This method consists of the sum total of a series of ratings assigned to the performance of specific locomotor activities in a given rat. The scale runs from 0 (fully normal rats) to 13 (fully incapacitated rats). Most parameters are rated as either 0 (normal), or 1 (incapacitated) others are graded. The following tests were used in the present study:
  • General observation tests: hypoactivity, sedation, piloerection.
  • Motor reflex. Rats were lifted by the tail about 15 cm above the floor. Normal rats assume a posture in which they extend both forelimbs towards the floor and spread that hind limbs to the sides in a trapeze-like manner. MCAO, when severe, causes consistent flexion of the contralateral limb.
  • Motor ability. This is seen as the ability to grasp a rod 1 cm in diameter by the contralareral limb for 5-15 sec when the rat is left hanging on the rod through the arm pit.
  • Motor coordination. Normal rats are able to walk up and down a beam, 5 cm wide placed at a moderate slant. Failure to walk the beam in either direction reveals some motor incoordination, lack of balance and limb weakness.
  • Gait. Ability to restore normal position to either hind contralateral or fore contralateral limb when intentionally displaced while on a narrow beam.
  • Balance. Ability to grasp and balance on a narrow beam 2 cm wide.
  • Locomotor activity. Total movements over a period of 15 min in an automated activity cage.
Ratings assigned to each of the above parameters are given in Table 15. Table 15.
Parameter Score
a. Activity in home cage normal=0 hypoactive=1
b. Sedation none=0 marked=1
c. Piloerection none=0 marked=1
d. Extension of contralateral forelimb towards floor when lifted by tail good=0 flexed limb=1
e. Spread of contralateral hind limb when lifted by tails (trapezoid posture) good=0 flexed limb=1
f. Grasp rod with contralateral limb for 5-15 sec. when suspended by armpit good=0 poor=1
g. Walk on beam 5cm wide good=0 poor=1
h. Resoration of contralateral hind and/or forelimb to original position when intentionally displaced good=0 poor=1 (one limb)
2 (two limbs)
i. Grasping & balance on beam 2cm wide good=0 poor= 1
j. Motor activity with respect to control (15min in activity cage) 0-25% of control=3
26-50% of control=2
51-75% of control=1
76-100% of contol=0
k. Tendency to lean on contralateral side 1
l. Contralateral circling when pulled by tail 1
m. Contralateral circling spontaneous. 1
Table 15a shows the effect of compounds 24 and 25 in this model, comparing the change in NSS measured in 24 and 48 hours post injury. .Table
Saline 0.745 211±75
24 1.625 152±45
25 1.78 189±54
.Table
*Difference in ΔNSS measured at 24 hours and 48 hours, from this it can be seen that compounds 24 and 25 have a longer lasting effect than the saline treated control.

Claims (5)

  1. A compound having the structure: wherein R2 is Boc and R3 is H; and wherein R1 is OH or the group and racemic mixtures, enantiomers or salts thereof.
  2. The compound of claim 1 comprising 6-hydroxy-1-N-Boc-aminoindan and racemic mixtures or enantiomers thereof.
  3. The compound of claim 1 having the structure: and racemic mixtures, enantiomers or salts thereof.
  4. The compound of any one of claims 1-3, wherein the enantiomer is the R enantiomer.
  5. The compound of any one of claims 1-3, wherein the enantiomer is the S enantiomer.
HK05110547.2A 1996-12-18 2005-11-22 Aminoindan derivatives HK1076098B (en)

Applications Claiming Priority (4)

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IL11985396 1996-12-18
IL11985396A IL119853A0 (en) 1996-12-18 1996-12-18 Aminoindan derivatives
IL12051097A IL120510A0 (en) 1997-03-24 1997-03-24 Phenylethylamine derivatives
IL12051097 1997-03-24

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HK1076098B true HK1076098B (en) 2008-05-30

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