Huperzine A derivatives, their preparation and their use

Description

This application is the national phase of PCT/CN95/00100, filed Dec. 26, 1995, published as WO96/20176 on Jul. 4, 1996.

The present invention relates to semi-synthesis of natural product, and particularly to alkaloid and analogues thereof.

In the past ten years a lot of researches have been made in foreign countries about application of choline esterase inhibitor to enhance the function of the intracerebral cholinergic system for the treatment of presenile dementia. Although delightful results of research have been obtained, there still exist some defects; at the time of producing the treatment effect, there occurs a relatively serious toxic side reaction; and the duration of the effect is relatively short.

In recent years China has isolated from a Chinese herb Lycopodium serratum Thunb., a new alkaloid huperzine A (5R, 9R, 11E)-5-amino-11-ethylidene-5,6,9,10-tetrahydro-7-methyl-5,9-methylene cycloocta [b] pyridyl-2(1H)-one having the formula (I)

Upon a pharmacological study it is proved that it exhibits highly effective reversible anticholinesterase activity, and has selective inhibitory effect on intracerebral acetylcholinesterase (U.S. Pat. No. 5,177,082). In foreign countries modification of the structure of huperzine A has been carried out and analogues of huperzine A have been synthesized in hopes of discovering therefrom compounds having anticholinesterase activity [J. Org. Chem. 56, 1991(4636-4645)] and finding a method of synthesizing huperzine A [U.S. Pat. No. 4,929,731]. However, neither a good method nor an analogue having a better effect has been found so far.

The present invention has made use of the excellent resources of Chinese herbs in China to design a semi-synthesis starting from huperzine A, in the hope of finding among a great variety of huperzine A derivatives compounds having better treatment effect and lower toxicity than the existing huperzine A.

The present invention is carried out through the following steps:

1. Using alcohols such as ethanol as extraction solvent, from the plant Lycopodium serratum Thunb., the residue obtained is concentrated, and then treated with an inorganic acid (such as hydrochloric acid). The aqueous layer is neutralized with alkali (such as ammonia water, NaOH), after which an organic solvent (such as chloroform) is used to extract the total alkaloid. After the treatment, separation by layer chromatography is carried out to produce the compound of the formula (I).

2. After condensation is carried out between the compound of the formula (I), and the corresponding substituted aldehyde or the corresponding substituted acyl chloride or acid anhydride in anhydrous solvent, a compound of the formula (II) is obtained.

When Y is —C═O or —R″, Y is ═CH, R is C

1

-C

5

lower alkyl;

n=0,1, X is hydrogen, C

1

-C

5

lower alkyl, C

1

-C

5

lower alkyloxy, nitro, halogen, carboxy, alkyloxycarbonyl, hydroxymethyl, hydroxy, amino substituted by bis-C

1

-C

5

lower alkyl; —(CH

2

)

m

COOZ group, m=0-5, Z is hydrogen or C

1

-C

5

lower alkyl; —CH═CH—G group, G is phenyl, furanyl, carboxy, alkyloxycarbonyl; dihydro or tetrahydropyridyl substituted by C

1

-C

5

lower alkyl at the nitrogen atom;

R′ is hydrogen, C

1

-C

5

lower alkyl, pyridoyl, benzoyl substituted by C

1

-C

5

lower alkyloxy;

R″ is hydrogen and C

1

-C

5

lower alkyl.

When Y is C═O, R is C

1

-C

5

lower alkyl,

n=0,1, X is hydrogen, C

1

-C

5

lower alkyloxy, carboxy, alkyloxycarbonyl, pyridyl, dihydro or tetrahydropyridyl substituted by C

1

-C

5

lower alkyl at the nitrogen atom; —(CH

2

)

m

COOZ group, m=0-5, Z is hydrogen or C

1

-C

5

lower alkyl; —CH═CH—G group, G is phenyl, furanyl, carboxy, alkyloxycarbonyl;

R′ is hydrogen, C

1

-C

5

lower alkyl, pyridoyl, benzoyl substituted by C

1

-C

5

lower alkyloxy;

R″ is hydrogen and C

1

-

5

lower alkyl.

When R″, Y are ═CH, R is

n=0, X is hydrogen, C

1

-C

5

lower alkyl, C

1

-C

5

lower alkyloxy, nitro, halogen, hydroxy, hydroxymethyl, amino substituted by bis-C

1

-C

5

lower alkyl; —CH═CH—G group, G is phenyl, furanyl;

R′ is hydrogen and C

1

-C

5

lower alkyl.

Huperzine A derivatives:

No.

Y

R

R′

R″

No. 1

C═O

HOOC—CH

2

CH

2

—

H

H

No. 2

C═O

C

6

H

5

CH

2

—

H

H

No. 3

C═O

CH

3

CH

3

═

No. 4

C═O

H

H

═

No. 5

C═O

H

═

═

No. 6

C═O

H

H

═

No. 7

C═O

4-CH

3

OC

6

H

4

—

H

H

No. 8

C—O

2,3,4-(CH

3

O)

3

C

6

H

2

—

H

H

No. 9

C═O

2,3,4-(CH

3

O)

3

C

6

H

2

—

H

—

No. 10

C═O

(CH

3

)

2

CH—

H

H

No. 11

C═O

C

6

H

5

—

H

H

No. 12

C═O

2-py

H

H

No. 13

C═O

3-py

3-py-CO—

H

No. 14

C═O

4-py

H

H

No. 15

C═O

2-HOOC—C

6

H

4

—

H

H

No. 16

C═O

trans-HOOCCH

2

CH═CH—

H

H

No. 17

CH

H

—

No. 18

CH

H

—

No. 19

CH

H

—

No. 20

CH

H

—

No. 21

CH

H

—

No. 22

CH

H

—

No. 23

CH

H

—

No. 24

CH

H

—

No. 25

CH

H

—

No. 26

CH

H

—

No. 27

CH

H

—

No. 28

CH

H

—

No. 29

CH

H

—

No. 30

CH

H

—

No. 31

CH

H

—

No. 32

CH

H

—

No. 33

CH

H

—

No. 34

CH

H

—

No. 35

CH

H

—

No. 36

CH

H

—

No. 37

CH

H

—

No. 38

CH

H

—

Pharmacological effect of huperzine A derivatives:

In the present invention a calorimetric method reported by Ellman was used to determine the effect of inhibition of the pharmaceutical on enzyme activity. The total volume of the solution of the enzyme activity reaction was 4 ml, which contained 0.3 mmol/L of acetylcholin iodide (acetylcholinesterase substrate), or 0.4 mmol/L of butyrylcholin iodide (butyrylcholinesterase substrate), 1 ml of the buffer solution of 25 mmol/L of phosphate of pH 7.4, and water to make up to 4 ml (including the amount of the enzyme solution and the testing reagent added afterwards). After the solution was kept at 37° C. for 5 minutes, 0.1-0.2 ml of enzyme solution (red cell membrane or serum of rat) was added, or 0.1-0.3 ml of the testing reagent was added at the same time. The solution was kept at the same temperature for another 8 minutes. Then 1 ml of 3% of sodium lauryl sulphate was added to terminate the reaction. Finally 1 ml of 0.2% 5,5-dithio-2,2′-nitro-benzoic acid solution was added for developing. “721” spectrophotometer was used to determine the density of light at 440 nm. A solution without addition of the pharmaceutical to inhibit the enzyme activity was used as a control (100%). A diagram was plotted with the percentage of the remaining enzyme activity against gram molecule concentration of the pharmaceutical, so as to obtain the dose of the pharmaceutical at 50% of inhibition of the enzyme activity, i.e., IC

50

. The results of the test showed that all the derivatives exhibited inhibition effect on acetylcholinesterase; derivatives No. 1, No. 17, No. 18 and No. 19 exhibited remarkable inhibition effect on acetylcholinesterase; their effect was slightly weaker than that of huperzine A, but apparently stronger than that of physostigmine and galanthamine. They exhibited weaker inhibition effect on butyrylcholinesterase (pseudo enzyme) than huperzine A. Derivatives No. 1 and No. 17 exhibited greater selective inhibition effect on acetylcholinesterase than huperzine A (see Tables 1, 2 and 6). A study on kinetics of enzyme indicated that the combination of derivatives No. 17, No. 18 and No. 19 respectively with acetylcholinesterase was reversible.

The two memory model test, mouse passive escape operation (Platform jumping method) and 8-arm maze spatial distinction operation of rat, indicated that both derivatives No. 18 and No. 19 exhibited very strong effect, similar to that of the compound of formula (I), on improving memory (see Tables 3 and 4).

The critical toxicity test on mice indicated that LD50 of derivatives No. 18 and No. 19 were smaller than, only ⅓ of, that of the compound of formula (I) (see Table 5).

TABLE 1

In-vitro anticholinesterase effect of huperzine

A derivatives (determined by colorimetric method)

concentration for inhibition

of 50% of enzyme activity

(IC

50

μM)

acetylcholin-

butyrylcholin-

esterase

esterase

IC

50

ratio

Compound No.

(AChE)

(BuChE)

BuChE/AChE

1

0.348

380.19

1092.5

2

9.05

>346.7

3

3.63

>331.1

4

>12.88

58.9

5

>10.96

>275.4

6

>12.3

>309.1

17

0.172

199.5

1159.9

18

0.151

107.2

709.9

19

0.145

104.7

722.1

10

>15.85

109.6

11

>14.45

363

compound(I)

0.06309

63.09

1000

Physostigmine

0.251

1.259

5.02

galanthamine

1.995

12.59

6.3

AChE taken from rat's red cell membrane. BuChE taken from rat's serum.

TABLE 2

In-vitro anticholinesterase effect of huperzine

A derivatives

concentration for

inhibition of 50%

of enzyme activity

(IC

50

μM)

acetyl-

butyryl-

cholin-

cholin-

esterase

esterase

IC

50

ratio

Compound No.

MW

(AChE)

(BuChE)

BuChE/AChE

huperzine A

242

0.0977

100.0

1023.3

1

342

0.3475

380.2

1094.1

12

376

0.1259

251.2

1995.2

15

390

0.6310

502.0

795.6

17

428

0.1718

199.5

1161.2

18

376

0.1514

107.2

708.2

19

406

0.1445

104.7

724.6

20

346

0.1778

125.9

708.1

21

420

0.1413

158.5

1121.3

22

406

0.1259

125.9

1000.0

23

362

0.2512

199.5

794.2

24

362

0.1000

158.5

1585.0

25

378

0.1585

251.2

1584.9

27

356

0.1259

100.0

794.3

MW: molecular weight

AChE taken from homogenate of rat's cortex. BuChE taken from rat's serum.

TABLE 3

Improvement by huperzine A derivatives on the

condition of memory impairment caused by scopolamine in

passive escape operation

No.

delitescence of

dosage

of

get-down Δ

Group

(mg/kg ip + po)

mice

(sec ± SEM)

physiological saline +

−+−

20

71.9 ± 12.9

physiological saline

scopolamine +

2+ −

20

29.5 ± 2.7

physiological saline

scopolamine +

2 + 0.2

20

67.7 ± 11.7**

derivative No. 18

3 + 0.3

20

64.0 ± 9.8*

2 + 0.4

20

48.7 ± 6.9

physiological saline +

−+−

18

81.7 ± 19.0

physiological saline

scopolamine +

2+ −

23

32.8 ± 8.2

physiological saline

scopolamine +

2 + 0.1

11

48.9 ± 12.6

derivative No. 19

2 + 0.2

16

71.6 ± 14.5

2 + 0.3

21

99.8 ± 16.4**

2 + 0.4

18

92.2 ± 15.5*

Δ: Once trained, the mice were administered, and tested after 24 hours. comparison with the physiological saline group P < 0.01

**comparison with scopolamine group *P < 0.05, **P < 0.01

TABLE 4

Improvement by huperzine derivatives on the

condition of memory impairment caused by scopolamine in

spatial distinction operation

No. of mistakes in

operation before reaching

the standard Δ

X + SEM)

dosage

No.

refer-

(mg/kg

of

ence

working

Group

ip + po)

rats

memory

memory

physiological saline +

−+−

24

0.42 ± 0.1

0.08 ± 0.01

physiological saline

scopolamine +

0.2+ −

6

1.67 ± 0.21

0.33 ± 0.42

physiological saline

scopolamine +

0.2 ± 0.1

6

1.33 ± 0.21

1.33 ±

derivative No. 19

0.49**

0.2 ± 0.3

6

0.33 ±

0.17 ±

0.21**

0.17**

physiological saline +

−+−

24

0.33 ± 0.13

0.08 ± 0.006

physiological saline

scopolamine +

0.125+ −

6

2.0 ± 0.45

2.0 ± 0.52

physiological saline

scopolamine +

0.124 + 0.2

6

0.67 ±

0.33 ±

derivative No. 18

0.33**

0.13**

physiological saline +

−+−

14

0.21 ± 0.11

0.07 ± 0.07

physiological saline

scopolamine +

0.15+ −

7

2.14 ± 0.14

2.57 ± 0.29

physiological saline

scopolamine +

0.15 + 0.25

10

0.57 ±

0.86 ±

huperzine A

0.30**

0.14**

Δ: 8-arm maze test. After trained to reach the standard (no. of mistake less than one per day for three successive days), the rats were tested. The rat first entering the arm on which there is no food is taken as the reference emory mistake. The rat re-entering the arm on which there is food is taken as the working memory mistake, comparison with the physiological saline group P > 0.01

**comparison with scopolamine group P < 0.01

TABLE 5

Critical toxicity of huperzine A derivatives on

mice (Bliss method)

mg/kg p.o. (95% confidence limit)*

Compound

LD

50

LD

50

compound (I)

3.1(3.5-3.8)

4.6(4.2-5.1)

derivative No. 18

9.6(7.3-12.5)

14.4(12.9-16.4)

derivative No. 19

11.1(9.6-12.9)

14.1(15.5-20.5)

*10 mice per group, with equal no. of males and females.

Test of each pharmaceutical was carried out using 4-5 dosage group.

Mortality within 7 days was observed.

TABLE 6

In-vitro anticholinesterase effect of huperzine

A derivatives

inhibition activity

Compound

AChE

BuChE

No.

1(μM)

IC

50(M)

10(μM)

BuChE/AChE

(18)

90.2

8.4 × 10

−8

0

>500

(20)

83.7

9.4 × 10

−8

0

>500

(21)

84.9

1.0 × 10

7

0

>500

(22)

68.7

0

(23)

34.4

0

(15)

60.8

0

(24)

78.3

2.8 × 10

−7

0

>100

(25)

62.0

0

(27)

84.0

1.1 × 10

−7

3.3

>500

(26)

79.7

1.8 × 10

−7

1.1

>300

(16)

80.7

2.1 × 10

−7

1.8

>200

(14)

76.4

3.6 × 10

−7

2.5

>100

(44)

85.6

1.1 × 10

−7

1.8

>500

(45)

87.0

1.0 × 10

−7

1.8

>500

(46)

78.7

2.9 × 10

−7

1.2

>100

E-2020

86.2

6.6 × 10

−8

2.9

>500

huperzine A

88.3

1.2 × 10

−7

0

>500

The results of the above pharmacological study show that derivatives No. 17, No. 18 and No. 19 are highly effective selective inhibitors of acetylcholinesterase and have lower critical toxicity than compound (I). Hence, it can be deduced that they have prospect of clinical application and development for use in the treatment of relieving serious amyasthenia and of dysmnesia caused by failure in central cholinergic system.

EXAMPLE 1

Preparation of Derivative No. 2

Compound (I) (0.50 mmole) into 5 ml three-neck flask was weight out. 20 ml of anhydrous pyridine was added to dissolve compound (I). While cooling in ice-bath, phenyl acetyl chloride (0.55 mmole) was added dropwise. Then the whole mixture was stirred overnight at room temperature (25° C.). When thin-layer chromatography indicated substantial disappearance of the starting materials, the reaction was stopped. Pressure was reduced by means of water pump to vaporize pyridine. Separation was carried out using silica gel layer chromatography. Elution was carried out with dichloromethane:acetone:methanol=5:45:5 to produce the crude product, which was recrystallized using a mixed solvent of acetone and petroleum ether to produce the product with 75% yield.

UV λ

max

=229 nm (∈=17360); λ

max

=316 nm(∈=9320); [α]

D

25° C.

=29.43;

1

HNMR: [CDCl

3

]; 3H 6.31(1H,d,J=9.9 Hz); 4H 7.20 (1H,d,J=9.9 Hz); 10H 2.89(2H,m); 9H 3.52 (1H,m); 8H 5.38(1H,d,J=5.0 Hz); 14-H 1.62(3H,d,J=6.7 Hz); 13-H 5.08(1H,q,J=6.7 Hz); 6-H 2.15,2.45(2H,m); 12-H 1.50(3H,s); 2′,4′-H 7.36(2H,m); 3′,5′-H 7.29(2H,m); 6′-H 7.24(1H,m); 7′-H 3.59(s); MS(m/z) 360(M

+

) 345 269 252 227 224 210(100%) 91; mp: 171-173° C.; IR: υ

max

3280, 1660(s), 1620(s), 1550, 1450, 1350, 1300, 1175, 1130, 840, 620 cm

−1

The same process was used to prepare derivatives No. 3, No. 5, No. 6, No. 7, No. 8, No. 9, No. 10, No. 11, and No. 13.

EXAMPLE 2

Preparation of Derivative No. 4

Compound (I) (0.5 mmole) into 50 ml three-neck flask was weight out. 20 ml of anhydrous pyricline to dissolve compound (I) was added. While cooling in ice-bath, DBU (0.6 mmole) was first added, and then 0.55 mmole of hydrochloric acid pyridine-2-formyl chloride was added. The whole mixture was placed overnight at room temperature. When thin-layer chromatography determination indicated substantial completion of the reaction, pressure was reduced by means of water pump to vaporize pyridine. Separation was carried out using silica gel layer chromatography. Elutioni was carried out with dichloromethane:acetone:methanol=50:45:5 to produce the crude product, which was recrystallized using a mixed solvent of acetone and petroleum ether to produce the product with 74% yield.

UV λ

max

=226 nm (∈=1.35×10

4

); λ

max

=264 nm (∈=5.4·10

3

); λ

max

=315 nm (∈=5730); [α]

D

=77.85°;

1

HNMR: [CDCl

3

]; 3-H 6.36(1H,J=9.2 Hz); 4-H 7.44(1H,J=9.2 Hz); 10-H 3.05(2H,m); 9-H 3.74(1H,m); 8-H 5.42(1H,d,J=4.7 Hz); 14-H 1.65(3H,d,J=6.6 Hz); 13-H 5.35(1H,q=6.6 Hz); 6-H 2.42(2H,s); 12-H 1.55(3H,s); 2′-H 8.58(1H,m); 4′-H 7.85(1H,m); 5′-H 7.48(1H,m); 6′-H′ 8.15(1H,m); MS(m/z) 347(M

+

), 241(100%) 169, 149, 106, 95, 79, 71, 55; mp: 170-171° C.; IR: u

max

3450, 2900, 1660(s), 1615(s), 1530(s), 1460, 1300, 1180, 1140, 1000, 830, 750 cm

−1

The same process was used to prepare derivatives No. 12 and No. 14.

EXAMPLE 3

Preparation of Derivative No. 19

Compound (I) (0.5 mmole) was weight out into 50 ml three-neck flask. Anhydrous ethanol and 4,6-dimethoxy-2-hydroxy benzaldehyde (0.51 mmole) were added. The mixture was heated slightly under reflux. Through a water segregator part of the ethanol was vaporized continuously. The solvent in the reaction was constantly replenished. The reaction was carried out for several hours and the reaction state was constantly determined by means of thin-layer chromatography. When the reaction was completed, the pressure was reduced to remove the ethanol to produce a solid crude product, which was recrystallized using a mixed solvent of acetone and petroleum ether to produce the product with 92% yield.

The same process was used to prepare derivatives No. 17, 18, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29, 30, 31, 32, 33, 34, 35, 36, 37, 38, 39, 40, 41, 42, and 43.

Derivative No. 19

m.p. 207-210° C.; MS: m/z 406(M

+

); 391(M

+

-CH

3

), 351(M

+

-C

4

H

7

);

1

H NMR (CDCl

3

); 1-H 13.12(1H,br,s); 3-H 6.41(1H,d,J=9.1 Hz); 4-H 7.25(1H,d,J=9.1 Hz); 6-H 2.85 (2H,s); 8-H 3.45(1H,d,J=4.7 Hz); 9-H 3.61(1H,m); 10-H 2.85(2H,m); 12-H

3

1.60(3H,s); 13-H 5.22(1H,q,J=7.7 Hz); 14-H

3

1.25(3H,d,J=7.7 Hz); 2′-OH 14.58(1H,br,s); 3′-H 5.57 (1H,s); 4′-OCH

3

3.79(3H,s); 5′-H 5.85(1H,s); 6′-OCH

3

3.70 (3H,s); 7′-H 8.15(1H,s); IR: υ

max

3480(m), 2960(s), 2930(s), 2870(s), 1670(s), 1620(s), 1540(s), 1450(s), 1330 (s), 1300 (s), 1218(sh), 1186(m), 1155(s), 1110(s), 1080(m), 1050(m), 1000(m), 930(m), 840(s), 730(m), 670(m), 610(m), 520(s) cm

−1

.

Derivative No. 20

1

H NMR (CDCl

3

): 1-H 12.72(1H,br,s); 3-H 6.34(1H,d, J=9.4 Hz); 4-H 7.11(1H,d,J=9.4 Hz); 6

a

-H 2.79(1H,d,J=16.0 Hz); 6

b

-H 2.75(1H,d,J=16.0 Hz); 8-H 5.41(1H,d,J=5.0 Hz); 9-H 3.63(1H,m); 10

a

-H 2.95(1H,dd,J=16.6, 4.9 Hz); 10

b

-H 2.27(1H,d,J=16.6 Hz); 12-H 1.57(3H,s); 13-H 5.07(1H,q,J=6.8 Hz); 14-H 1.55(3H,d,J=6.8 Hz); 2′-OH 13.77(1H,br,s); 3′-H 6.94(1H,d,J=8.4 Hz); 4′-H 7.30(1H,t with small splitts, J=8.4 Hz); 5′-H 6.85(1H,t with small splitts, J=7.4 Hz); 6′-H 7.22(1H,dd,J=7.4, 1.6 Hz); 7′-H 8.31(1H,s); MS: 346(M

+

), 331, 317, 303, 291, 253, 239, 226, 210, 197, 184, 167, 128, 121, 97. IR: υ

max

3420, 2900, 1660, 1620, 1580, 1560, 1500, 1460, 1420, 1380, 1350, 1280, 1205, 1150, 1120, 1080, 1010, 970, 910, 840, 790, 755(s), 650, 630, 610, 520 cm

−1

Derivative No. 21;

1

H NMR (CDCl

3

); 1-H 12.87(1H,br,s); 3-H 6.32(1H,d, J=9.4 Hz); 4-H 7.07(1H,d,J=9.4 Hz); 6

a

-H 2.79(1H,d,J=16.0 Hz); 6

b

-H 2.75(1H,d,J=16.0 Hz); 8-H 5.43(1H,d,J=5.0 Hz); 9-H 3.63(1H,m); 10

a

-H 2.97(1H,dd,J=16.0, 4.0 Hz); 10

b

-H 2.18(1H,d,J=16.0 Hz); 12-H 1.58(3H,s); 13-H 5.14(1H,q,J=6.8 Hz); 14-H 1.57(3H,d,J=6.8 Hz); 2′,6′-2H 7.04(2H,s); 7′-H 8.25(1H,s); 3′,5′-2(OCH

3

) 3.87(6H,s); 4′-OCH

3

3.84 (3H,s); MS: 420(M

+

), 405(M

+

-CH

3

), 391, 365, 351, 313, 284, 239, 226, 210, 196, 181, 140, 124. IR: υ

max

2940, 1660(s), 1590, 1560, 1500, 1565, 1420, 1370, 1330, 1300, 1230, 1190, 1130(s), 1005, 960, 930, 840, 770, 735, 725, 660, 605, 540, 530 cm

−1

.

Derivative No. 22

1

H NMR(CDCl

3

): 1-H 13.03(1H,br,s); 3-H 6.34(1H,d,J=9.4 Hz); 4-H 7.14(1H,d,J=9.4 Hz); 6-H

2

2.73(2H,s); 8-H 5.39(1H,d,J=4.7 Hz); 9-H 3.61(1H,m); 10

a

-H 2.94(1H,dd, J=16.8, 4.9 Hz); 10

b

-H 2.27(1H,d,J=16.8 Hz); 12-H 1.55 (3H,s); 13-H 5.09(1H,q,J=6.8 Hz); 14-H 1.54(3H,d,J=6.8 Hz); 2′-OH 14.39(1H,br.s); 3′-OCH

3

3.87(3H,s); 4′-OCH

3

3.85(3H,s); 5′-H 6.43(1H,d,J=8.7 Hz); 6′-H 6.91(1H,d,J=8.7 Hz); 7′-H 8.14(1H,s); MS: 406(M

+

), 391(M

+

-CH

3

), 373, 351, 239, 226, 197, 182, 167, 139, 101; IR: υ

max

3450-3350 (br), 2940(m), 1660(s), 1620(s), 1555, 1510, 1455, 1415, 1290, 1270(s), 1210, 1110(s), 1060, 970, 930, 835, 785, 695, 675, 640, 625 cm

−1

.

Derivative No. 23

1

H NMR(d

6

-DMSO): 1-H 11.48(1H,br,s); 3-H 6.13(1H, d,J=9.4 Hz); 4-H 7.07(1H,d,J=9.4 Hz); 6

a

-H 2.68(1H,d,J=16.7 Hz); 6

b

-H 2.59(1H,d,J=16.7 Hz); 8-H 5.48(1H,d,J=4.7 Hz); 9-H 3.65(1H,m); 10

a

-H 2.77(1H,dd,J=16.3, 4.0 Hz); 10

b

-H 2.28(1H,d,J=16.3 Hz); 12-H 1.59(3H,s); 13-H 5.05 (1H,q,J=6.8 Hz); 14-H 1.60(3H,d,J=6.8 Hz); 2′-OH 14.40 (1H,br,s); 3′-H 6.18(1H,s); 4′-OH 10.09(1H,br,s); 5′-H 6.30 (1H,d, with small splitts, J=8.4 Hz); 6′-H 7.31(1H,d,J=8.4 Hz); 7′-H 8.47(1H,s); MS: 362(M

+

), 347, 319, 307, 242, 226, 210, 197, 167, 137. IR: υ

max

3500-2800(br), 1665(s), 1625(s), 1605(s), 1550, 1540, 1450, 1345, 1300, 1230, 1180, 1120, 1080, 975 cm

−1

.

Derivative No. 24

1

H-NMR(CDCl

3

): 1-H 13.09(1H,br,s); 3-H 6.37(1H,d,J=9.4 Hz); 4-H 7.15(1H,d,J=9.4 Hz); 6-H

2

2.76(2H,s); 8-H 5.42(1H,d,J=5.0 Hz); 9-H 3.60(1H,m); 10

a

-H 2.96(1H,dd, J=16.5, 4.9 Hz); 10

b

-H 2.32(1H,d,J=16.5 Hz); 12-H 1.56 (3H,s); 13-H 5.11(1H,q,J=6.8 Hz); 14-H 1.58(3H,d,J=6.8 Hz); 2′-OH 13.09(1H,br,s); 3′-OH 9.83(1H,br,s); 4′-H 6.68 (1H,dd,J=8.1, 1.5 Hz); 5′-H 6.57(1H,t,J=7.8 Hz); 6′-H 6.91 (1H,dd,J=7.6, 1.5 Hz); 7′-H 8.08(1H,s); MS: 362(M

+

), 347 (M

+

-CH

3

), 307, 253, 239, 226 197, 167, 149, 138, 137, 109, 92, 81. IR: υ

max

3500-2800(br), 1660(s), 1625(s), 1545, 1460, 1370, 1275, 1240, 1120, 1080, 1060, 1020, 835, 775, 740(s), 640, 630, 525 cm

−1

.

Derivative No. 26

1

HNMR(CDCl

3

): 1-H 13.10(1H,br,s); 3-H 6.33(1H,d J=9.4 Hz); 4-H 7.12(1H,d,J=9.4 Hz); 6-H

2

2.75(2H,s); 8-H 5.41(1H,d,J=4.8 Hz); 9-H 3.62(1H,m); 10

a

-H 2.95(1H,dd, J=16.5, 4.9 Hz); 10

b

-H 2.27(1H,d,J=16.5 Hz); 12-H

3

1.57 (3H,s); 13-H 5.08(1H,q,J=6.8 Hz); 14-H 1.54(3H,d,J=6.8 Hz); 2′-OH 14.36(1H,br,s); 3′-OCH

3

3.86(3H,s); 4′-H 6.83 (1H,dd,J=7.9, 1.5 Hz); 5′-H 6.76 (1H,t,J=7.9 Hz); 6′-H 6.89(1H,dd,J=7.9, 1.5 Hz); 7′-H 8.27(1H,s); MS: 376(M

+

), 361, 346, 331, 306, 270, 253, 239, 226, 210, 197, 167, 152, 109, 106, 82. IR: υ

max

3450-3360, 2940-2980, 1660(s), 1620(s), 1555, 1465(s), 1255(s), 1190, 1170, 1115, 1085, 970, 930, 840, 780, 740, 680, 640, 630, 520 cm

−1

.

Derivative No. 27

1

HNMR(CDCl

3

): 1-H 12.80(1H,br,s); 3-H 6.34(1H,d,J=9.4 Hz); 4-H 7.07(1H,d,J=9.4 Hz); 6-H

2

2.72(2H,s); 8-H 5.40(1H,d,J=5.0 Hz); 9-H 3.61(1H,m); 10

a

-H 2.94(1H,dd, J=16.2, 3.6 Hz); 10

b

-H 2.17(1H,d,J=16.2 Hz); 12-H 1.56 (3H,s); 13-H 5.08(1H,q,J=6.8 Hz); 14-H 1.57(3H,d,J=6.8 Hz); 2′,6′-2H 7.45(2H,dd,J=6.8, 1.4 Hz); 3′,5′,8′-3H 7.30 (3H,m); 4′-H 7.06(1H,m); 7′-H 6.99 (1H,d,J=15.9 Hz); 9′-H 8.06(1H,d,J=8.1 Hz); MS: 356(M

+

), 341(M

+

-CH

3

), 327, 301, 265, 237, 226, 210, 197, 167, 131, 115, 91, 77. IR: υ

max

3600-3400(br), 2950-2850(br), 1660(s), 1632, 1620, 1550, 1465, 1445, 1300(m), 1175, 1115, 975, 825, 750(s), 690(s), 630, 620, 520 cm

−1

.

Derivative No. 28

1

HNMR(CDCl

3

): 1-H 12.76(1H,br,s); 3-H 6.38(1H,d,J=9.3 Hz); 4-H 7.12(1H,d,J=9.3 Hz); 6

a

-H 2.81(1H,d,J=16.0 Hz); 6

b

-H 2.78(1H,d,J=16.0 Hz); 8-H 5.46(1H,br,s); 9-H 3.67(1H,m); 10

a

-H 3.00(1H,dd,J=16.4, 4.5 Hz); 10

b

-H 2.31 (1H,d,J=16.4 Hz); 12-H 1.62(3H,s); 13-H 5.07(1H,q,J=6.6 Hz); 14-H 1.60(3H,d,J=6.6 Hz); 2′-OH 13.76(1H,br,s); 3′-H 6.94(1H,d,J=8.7 Hz); 4′-H 7.29(1H,dd,J=8.7, 2.3 Hz); 5′,6′,7′,8′-4H 7.25(4H,m); 11′-H 8.30(1H,s); MS(m/z): 396(M

+

, 3%), 381(M

+

-CH

3,1

), 226(2), 172(4), 144(2), 127(1), 115 (5), 85(13), 71(22), 57(100). IR(KBr): 3408, 1660, 1626, 1479, 1280 cm

−1

.

Derivative No. 30

1

HNMR(CDCl

3

): 1-H 10.92(1H,br,s); 3-H 6.42(1H,d,J=9.3 Hz); 4-H 7.15(1H,d,J=9.3 Hz); 6

a

-H 2.82(1H,d,J=17.2 Hz); 6

b

-H 2.76(1H,d,J=17.2 Hz); 8-H 5.47(1H,br,s); 9-H 3.69(1H,m); 10

a

-H 2.99(1H,dd,J=16.0, 3.7 Hz); 10

b

-H 2.30 (1H,d,J=16.0 Hz); 12-H 1.63(3H,s); 13-H 5.07(1H,q,J=6.8 Hz); 14-H 1.61(3H,d,J=6.8 Hz); 3′-H 6.89(1H,d,J=6.8 Hz); 4′,6′-2H 7.42(2H,m); 7′-H 8.30(1H,s); MS(m/z): 426(M

+

+2,43%), 424(M

+

, 43), 411[(M

+

+2)-CH

3

,42], 409(M

+

-CH

3

, 45), 369(11), 289(5), 253(18), 239(33), 226(100), 210(54), 197(47), 167(31), 128(31), 115(46), 91(32), 77(59), 57(81). IR(KBr): 3400, 1660, 1630, 1475, 1280, 823 cm

−1

.

Derivative No. 32

1

HNMR(CDCl

3

): 1-H 12.70(1H,br,s); 3-H 6.39(1H,d,J=9.4 Hz); 4-H 7.11(1H,d,J=9.4 Hz); 6

a

-H 2.81(1H,d,J=16.2 Hz); 6

b

-H 2.77(1H,d,J=16.2 Hz); 8-H 5.45(1H,br,s); 9-H 3.67(1H,m); 10

a

-H 2.99(1H,dd,J=16.7, 4.9 Hz); 10

b

-H 2.31 (1H,d,J=16.7 Hz); 12-H 1.62(3H,s); 13-H 5.06(1H,q,J=6.8 Hz); 14-H 1.60(3H,d,J=6.8 Hz); 2′-OH 13.80(1H,br,s); 3′-H 6.89(1H,d,J=8.7 Hz); 4′-H 7.42(1H,dd,J=8.7, 2.4 Hz); 6′-H 7.39(1H,d,J=2.4 Hz); 7′-H 8.29(1H,s); MS(m/z): 392(M

+

+1,11%), 391(M

+

,45), 376(M

+

-CH

3

,60), 242(18), 226(53), 101(28), 83(53), 59(100). IR(KBr): 3419, 1660, 1616, 1549, 1336, 833 cm

−1

.

Derivative No. 33

1

HNMR(CDCl

3

): 1-H 12.40(1H,br,s); 3-H 6.42(1H,d,J=9.5 Hz); 4-H 7.15(1H,d,J=9.5 Hz); 6

a

-H 2.84(1H,d,J=16.3 Hz); 6

b

-H 2.77(1H,d,J=16.3 Hz); 8-H 5.47(1H,br,s); 9-H 3.70(1H,m); 10

a

-H 3.00(1H,dd,J=16.0, 4.9 Hz); 10

b

-H 2.39 (1H,d,J=16.0 Hz); 12-H 1.58(3H,s); 13-H 5.12(1H,q,J=6.8 Hz); 14-H 1.63(3H,d,J=6.8 Hz); 2′-OH 15.59(1H,br,s); 4′-H 8.16(1H,d,J=7.8 Hz); 5′-H 6.77(1H,t,J=7.8 Hz); 6′-H 7.46 (1H,d,J=7.8 Hz); 7′-H 8.24(1H,s); MS(m/z): 391(M

+

,66%), 376(M

+

-CH

3

,41), 356(45), 328(18), 288(14), 239(15), 226 (100), 210(25), 197(22), 83(61). IR(KBr): 3431, 1662, 1633, 1529, 1352, 1242, 754 cm

−1

.

Derivative No. 34

1

HNMR(CDCl

3

): 1-H 12.87(1H,br,s); 3-H 6.38(1H,d,J=9.6 Hz); 4-H 7.13(1H,d,J=9.6 Hz); 6-H

2

2.78(2H,s); 8-H 5.46(1H,br,s); 9-H 3.67(1H,m); 10

a

-H 3.00(1H,dd,J=16.5, 4.9 Hz); 10

b

-H 2.32(1H,d,J=16.5 Hz); 12-H 1.62(3H,s); 13-H 5.09(1H,q,J=6.7 Hz); 14-H 1.59(3H,d,J=6.7 Hz); 2′-OH 14.42(1H,br,s); 3′-OCH

3

3.90(3H,s); 4′,6′-2H 6.86 (2H,m); 7′-H 8.22(1H,s); MS(m/z): 412(M

+

+2,0.3%), 410 (M

+

,1.2), 395(M

+

-CH

3

,0.5), 239(1.4), 216(2), 83(100). IR(KBr): 3421, 2933, 1660, 1618, 1471, 1253, 839 cm

−1

.

Derivative No. 35

1

HNMR(CDCl

3

): 1-H 12.80(1H,br,s); 3-H 6.38(1H,d,J=9.3 Hz); 4-H 7.13(1H,d,J=9.3 Hz); 6-H

2

2.78(2H,s); 8-H 5.46(1H,br,s); 9-H 3.67(1H,m); 10

a

-H 3.00(1H,dd,J=16.7, 5.1 Hz); 10

b

-H 2.32(1H,d,J=16.7 Hz); 12-H 1.62(3H,s); 13-H 5.08(1H,q,J=6.8 Hz); 14-H 1.59(3H,d,J=6.8 Hz); 2′-OH 14.45(1H,br,s); 3′-OCH

3

3.89(3H,s); 4′,6′-2H 7.00 (2H,m); 7′-H 8.21(1H,s); MS(m/z): 456(M

+

2,79), 454(M

+

, 7a), 441[(M

+

+2)-CH

3

, 40], 439(M

+

-CH

3

,42), 401(7), 399 (8), 285(14), 239(24), 226(100), 210(33), 197(37), 83(84). IR(KBr): 3431, 1660, 1624, 1471, 1252 cm

−1

.

EXAMPLE 4

Preparation of Derivative No. 15

Compound (I) (0.5 mmole) was weight out into 50 μl three-neck flask. 20 ml of anhydrous pyridine was added to dissolve compound (I). While cooling in ice-bath, o-phthalic acid anhydride was added. The mixture was stirred overnight at room temperature. When thin-layer chromatography determination indicated substantial completion of the reaction, the pressure was reduced by means of water pump to vaporize pyridine. Separation was carried out using silica gel layer chromatography. The development agent dichloromethane:methanol=3:1 was used to produce the crude product, which was recrystallized using propanol to produce white powders of derivative No. 15 with 78% yield.

The same process was used to prepare derivatives No. 1 to No. 16.

1

H NMR(d

6

-DMSO): 3-H 6.09(1H,d,J=9.4 Hz); 6-H

2

2.51(2H,s); 8-H 5.44(1H,d,J=4.8 Hz); 9-H 3.56(1H,m); 10

a

-H 2.66(1H,dd,J=16.8, 4.6 Hz); 10

b

-H 2.09(1H,d,J=16.8 Hz); 12-H

3

1.51(3H,s); 13-H 5.60(1H,q,J=6.8 Hz); 14-H

3

1.62(3H,d,J=6.8 Hz); 3′,4′,5′ and 4-H 7.51(4H,m); 6′-H 7.73(1H,d,J=7.5 Hz); N-H(amide) 7.90(1H,br,s); COO-H 8.46(1H,br,s); IR: υ

max

3650-2400, 1710, 1655, 1605, 1546, 1450, 1300 cm

−1

MS m/z: 372(M

+

), 357, 343, 329, 242, 227, 187, 147, 104(100).

EXAMPLE 5

Preparation of Derivative No. 44

Under argon gas stream 150 mg (0.620 mmole) of huperzine A and 200 mg of 4A molecular sieve were suspended in 4 ml of benzene. 76 μl (0.86 mmol) of pyridine-3-acetaldehyde and 20 mg of p-toluene sulphonic acid monohydrate were added. After reflux for three hours, the mixture was allowed to cool, and then neutralized with triethyl amine. The reaction solution was filtered with celite. After concentration, the residue was refined through silica gel column chromatography (methanol:dichloromethane=1:20) to produce derivative No. 44, a colorless solid (183 mg, 89% yield).

The same process was used to prepare derivatives No. 45 and No. 46, with 84% and 82% yield respectively.

Derivative No. 44

NMR(CDCL

3

) 1.64(3H,d,J=7.0 Hz), 1.65(3H,s); 2.25 (1H,d,J=16.0 Hz), 2.82(1H,d,J=17.0 Hz); 2.86(1H,d,J=16.0 Hz), 3.07(1H,dd,J=5.0,17.0 Hz) 8.65-3.75(1H,m); 5.14(1H, q,J=7.0 Hz), 5.50(1H,d,J=5.0 Hz); 6.34(1H,d,J=8.5 Hz), 7.09(1H,d,J=9.5 Hz); 7.40(1H,dd,J=5.0,8.0 Hz), 8.28(1H,dt, J=2.0,8.0 Hz), 8.47(1H,s); 8.70-8.72(1H,m), 8.94-8.96(1H, m), MS: 331(M

+

), 316(base), 226; HRMS calculated value: molecular formula C

22

H

21

N

2

O(M

+

): 331.16846; experimental value: 331.16888

Derivative No. 45

NMR(CDCL

3

) 1.64(3H,d,J=7.0 Hz), 1.65(3H,s); 2.25 (1H,d,J=16.0 Hz), 2.82(1H,d,J=16.5 Hz); 2.86(1H,d,J=16.0 Hz), 3.07(1H,dd,J=5.0,16.5 Hz),3.61-3.70(1H,m); 5.10(1H, q,J=7.0 Hz), 5.50(1H,d,J=4.0 Hz); 6.39(1H,d,J=9.5 Hz), 7.05(1H,d,J=9.5 Hz); 7.11-7.73(2H,m), 8.41(1H,s), 8.73-8.79(2H,m), MS: 331(M

+

), 316(base), 226; HRMS calculated value: molecular formula C

22

H

21

N

3

O(M

+

): 331.16846; experimental value: 331.18836

Derivative No. 46

NMR(CDCL

3

) 1.64(3H,d,J=6.5 Hz), 1.65(3H,s); 2.24 (1H,d,J=16.0 Hz), 2.82(1H,d,J=16.5 Hz); 2.85(1H,d,J=16.0 Hz), 3.07(1H,dd,J=5.0,16.5 Hz),3.67-3.70(1H,m); 3.96(6H, s), 5.22(1H,q,J=6.5 Hz), 5.30(1H,s); 5.47-5.49(1H,m), 6.39 (1H,d,J=9.5 Hz), 7.12(1H,s), 7.15(1H,d,J=9.5 Hz), 8.29(1H, s); MS: 406(M

−

,base), 391, 228, 167 HRMS calculated value: molecular formula C

24

H

26

N

2

O

4

(M

+

): 406.18926; experimental value: 406.18949

Claims

1. A huperzine A compound having tile following structural formula wherein Y and —R″ together form═CH, R is X is hydrogen, C1-C5 lower alkyloxy, nitro, halogen, hydroxymethyl, hydroxy, amino substituted by two C1-C5 lower alkyls or —CH═CH—G group, is phenyl or furanyl and R′ is hydrogen.
2. A method of treating myastheniaamyasthenia by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 110to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
3. A method of treating dysmnesia, caused by a failure in central cholinergic system by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 110to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
4. A method of inhibiting cholinesterase comprising administering a huperzine A compound according to claim 110in an amount effective to inhibit cholinesterase to a patient in need of such treatment.
5. A method of inhibiting cholinesterase according to claim 4, wherein said cholinesterase is an acetylcholinesterase.
6. A method of inhibiting cholinesterase according to claim 4, wherein the cholinesterase is butyrylcholinesterase.
7. A method of improving memory impairment comprising administering a huperzine A compound according to claim 110in an amount effective to improve mnemory imnpairmientmemory impairment to a patient in need of such treatment.
8. A compound according to claim 110, wherein R″ and Y are ═CH, prepared by a process of condensing huperzine A and the corresponding substituted aldehyde in an anhydrous solvent.
9. A method of inhibiting cholinesterase according to claim 4, wherein said huperzine A compound exhibits weaker inhibition effect on butyrylcholinesterase than huperzine A.
10. A huperzine A compound of the formula wherein Y and —R″ together form a ═CH group; R is wherein X is selected from the group consisting of hydrogen, C1-C5 lower alkoxy, nitro, halogen, hydroxymethyl, hydroxy, amino substituted by two C1-C5 lower alkyls and —CH═CH—G, wherein G is phenyl or furanyl; and R′ is hydrogen.
11. A huperzine A compound of the formula wherein Y and —R″ together form ═CH; R is selected from the group consisting of: and R′ is hydrogen.
12. A huperzine A compound of the formula wherein Y and —R″ together form ═CH; and R is
13. A huperzine A compound of the formula wherein Y and —R″ together form ═CH; and R is wherein each X is independently selected from the group consisting of hydrogen, methoxy, nitro, halogen, hydroxymethyl, and hydroxy; and R′ is H.
14. A method of treating amyasthenia by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 11 to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
15. A method of treating amyasthenia by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 12 to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
16. A method of treating amyasthenia by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 13 to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
17. A method of treating dysmnesia caused by a failure in central cholinergic system by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 11 to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
18. A method of treatment dysmnesia caused by a failure in central cholinergic system by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 12 to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
19. A method of treating dysmnesia caused by a failure in central cholinergic system by inhibiting cholinesterase comprising administering a huperzine A compound according to claim 13 to a patient in need of such treatment in an amount effective to inhibit cholinesterase.
20. A method of inhibiting cholinesterase comprising administering a huperzine A compound according to claim 11 in an amount effective to inhibit colinesterase to a patient in need of such treatment.
21. A method of inhibiting cholinesterase comprising administering a huperzine A compound according to claim 12 in an amount effective to inhibit colinesterase to a patient in need of such treatment.
22. A method of inhibiting cholinesterase comprising administering a huperzine A compound according to claim 13 in an amount effective to inhibit colinesterase to a patient in need of such treatment.
23. A method of improving memory impairment comprising administering a huperzine A compound according to claim 11 in an amount effective to improve memory impairment to a patient in need of such treatment.
24. A method of improving memory impairment comprising administering a huperzine A compound according to claim 12 in an amount effective to improve memory impairment to a patient in need of such treatment.
25. A method of improving memory impairment comprising administering a huperzine A compound according to claim 13 in an amount effective to improve memory impairment to a patient in need of such treatment.

Priority Claims (1)

Number	Date	Country	Kind
94114057	Dec 1994	CN

PCT Information

Filing Document	Filing Date	Country	Kind
PCT/CN95/00100		WO	00

Publishing Document	Publishing Date	Country	Kind
WO96/20176	7/4/1996	WO	A

US Referenced Citations (5)

Number	Name	Date	Kind
4929731	Kozikowski et al.	May 1990	A
4968672	Jacobson et al.	Nov 1990	A
5104880	Kozikowski	Apr 1992	A
5177082	Yu et al.	Jan 1993	A
5684018	Alexander	Nov 1997	A

Non-Patent Literature Citations (5)

Entry
Liu et al., Can. J. Chem, 64(4):837-839 (1986).
Qian et al., Tetrahedron Lett., 30(16):2089-90 (1989).
Tang et al., Acta Pharmacologica Sinica, 15(2):107-110 (1994) (Abstract Only).
Kozikowski et al., “Synthesis of Huperzine A and its Analogues and their Anticholinesterase Activity”, J. Org. Chem., 56:4636-4645 (1991).
Xiong et al., Acta Pharmacologica Sinica, 16(1):21-25 (1995).

Divisions (1)

	Number	Date	Country
Parent	08/860524	Jun 1997	US
Child	09/799127		US

Reissues (1)

	Number	Date	Country
Parent	08/860524	Jun 1997	US
Child	09/799127		US

Huperzine A derivatives, their preparation and their use

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Abstract