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Pergamon Phytochemistry, Vol. 44, No. 1, pp. 79-81, 1997
Copyright © 1996 Elsevier Science Ltd
Printed in Great Britain. All rights reserved
PII: S0031-9422(96)00516-X 0031-9422/97 $17.00 + 0.00
BIOTRANSFORMATION OF (+)- AND (-)-CAMPHORQUINONES TO
CAMPHANEDIOLS BY GLOMERELLA CINGULATA
MITSUOM1YAZAWA,*MASAHIRONOBATA,MITSUROHYAKUMACHI~"and HIROMUKAMEOKA
Department of Applied Chemistry, Faculty of Science and Engineering, Kinki University, Kowakae, Higasioska-shi, Osaka
577, Japan; -~Laboratoryof Plant Disease, Faculty of Agriculture, Gifu University, l-l, Yanagido, Gifu, 501-11, Japan
(Receivedin revisedform 27 June 1996)
Key Word Index--Glomerella cingulata; fungus; biotransformation; (+)-camphorquinone; (-)-
camphorquinone; (+)-2-exo-3-exo-camphane-2,3-diol; (+)-2-endo-3-exo-camphane-2,3-diol; re-
duction; stereoselectivity; enantioselectivity.
Abstract--The reduction of (+)-camphorquinone by the plant pathogen Glomerella cingulata produced (+)-2-
exo-3-exo-2,3-diol with high stereoselectivity, whereas (-)-camphorquinone yielded (+)-2-endo-3-exo-2,3-diol
with high stereo- and enantioselectivity. Copyright © 1996 Elsvier Science Ltd
INTRODUCTION Camphorquinone (la and lb) disappeared after 9 hr, as
shown in a previous paper [1], and a-ketoalcohols were
In our previous paper, (+)- and (-)-camphorquinones
(la, lb) were shown to be readily reduced to keto produced in about 100% yield at 9 hr, and then
decreased from 12 hr to 10 days. Compounds la-5 and
alcohols by short time (24 hr) fermentation with various
lb-6 were obtained 10-20% yield at 10 days (Figs 1
fungi [1]. In particular, Glomerella cingulata gave high and 2).
yields of hydroxycamphors in a short time. However,
In order to isolate these metabolites, a large scale
further reduction to diols in the biotransformation of
incubation of la and lb with G. cingulata was carried
compounds la and lb have not been reported.
out. After the biotransformation, the metabolites were
This report deals with the biotransformation of la
extracted and purified as described in the Experimental.
and lb to camphanediols by G. cingulata.
The structures of these compounds were determined by
spectral methods. Metabolites la-5 and lb-6 were
identified as (+)-(1R, 2R, 3R)-3-exo-I,7,7-tri-
RESULTS AND DISCUSSION
methylbicyclo [2.2.1 ] heptane- 2,3- diol((+)- 2- exo- 3-
In time-course experiments, small amounts of either exo-camphane-2,3-diol, la-5) and (+) - (1S, 2R, 3R)-
(+)-camphorquinone (la) or (-)-camphorquinone (lb) 3-exo-hydroxy-l,7,7-trimethyl-bicyclo [2.2.1] heptane-
were incubated with G. cingulata for 10 days, respec- 2,3-diol ((+)-2-endo-3-exo-camphane-2,3-diol, lb-6)
tively (Figs 1 and 2). The hiotransformation of com- by comparison with literature data [2]. It was consid-
pounds la and lb proceeded readily to give the eredthat compound la was transformedto (+)-2-exo-
oe-ketoaicohols (+)-2R-exo-hydroxyepicamphor(la-1), 3-exo-2,3-diol (la-5), yield 10%) via ~-ketoalcohols
(-)-2S-endo-hydroxyepicamphor (la-2), (-)-3S-exo- (+)-2R-exo-hydroxyepicamphor (la-1) and/or (-)-3S-
hydroxycamphor (la-3) and (+)-3R-endo-hydroxy- exo-hydroxycamphor (la-3), and compound lb to (+)-
camphor (la-4) from la, and (-)-2S-exo-hydroxy- 2-endo-3-exo-2,3-diol (lb-6), yield 20%) via (+)-2R-
epicamphor (lb-1), (+)-2R-endo-hydroxyepicamphor endo-hydroxyepicamphor (lb-2) and/or (+)-3R-exo-
(lb-2), (+)-3R-exo-hydroxycamphor (lb-3) and (-)- hydroxyepicamphor (lb-3) (Scheme 1). These biocon-
3S-endo-hydroxycamphor (lb-4)from lb with reduc- version processes exhibited high regio- and stereo-
tion of the carbonyl group [1]. These compounds of selective reduction.
absolute configuration la-1-4 and lb-1-4 were de- In the case of biotransformation of racemic camphor-
scribed in a previous paper [1]. It was confirmed that quinones by G. cingulata for 10 days, optically active
the ot-keto-alcohols were further transformed by G. camphanediol (lb-6 yield 10%, optical purity 99.9%)
cingulata to give la-5 and lb-6 over the ten-day period was isolated from the extract. This revealed that the
of the experiment. Two secondary metabolites (la-5 reduction of racemic camphorquinones by G. cingulata
and lb-6) were detected by TLC and GC analysis, proceeded with high stereo-and enantioselectivity. The
yield of compound la-5 was very poor (about 5%,
optical purity 99.9%). Thus, the racemic camphor-
*Author to whom correspondence should be addressed, quinones (la, lb) were reduced by G. cingulata to
79
80 M. M]YAZAWA et al.
I00
80-
0
0 1 2 3 4 S 6 7 8 9 10
Time (day)
Fig. I. Time course of the biotransformationof (+)-camphorquinone (la) by Glomerella cingulata,lq, la; A, ketoalcohols
(la-l-4); ©, 2-exo-3-exo-camphane-2, 3-diol(la-5).
100-
==
4o
0 1 2 3 4 S 6 7 8 9 10
Time (day)
Fig. 2. Time course of the biolransformationof (-)-camphurquinone (Ib) by Glomerella cingulata.B, lb; A, l<etoalcohols
(lb-1-4); O, 2 endo-3-exo-camphane-2,3,-diol(lb-6).
8 9
OGcingulata: "1- OH 4" "1" "l"
5 "~0 "
H OH H
la la-1 la-2 111-3 1t1=4 (+)-(1s, 2R,3S)
la-5
H HO H
I b I b'l I b-2 I b'3 I b-4 (+)-(1R,2R,3R)
lb-6
Scheme 1. Reduction of (+)-(la) and (-)-camphorquinone (lb) to ketoalcohols (la-l-4, lb-l-4) and diols (la-5, lb-6) by
Glomerella cingulata.
Biotransformation of camphorquinonesby Glomerellacingulata 81
yield 2,3-diol with high-stereo- and enantioselectivity, lected, saturated with NaC1, and extracted with EtOAc.
respectively. The mycelia were also collected and extracted with
In 1971, Robertson et al. [3] reported the reduction EtOAc. The EtOAc extracts were combined and the
of camphorquinone in rabbits. This reduction provided solvent removed under red. pres. The extract was
2-endo-3-endo-camphanediol and 2-endo-3-exo- chromatographed on silica gel using n-hexane-EtOAc
camohanediol. However, there have been no detailed and the substrate and metabolites isolated. In the case
reports of the stereoselectivity. To our knowledge, this of compound la: la-l-4: 161mg; la-5:82 mg. In the
is the first report of the reduction of compound la to case of lb: lb-l-4:188 mg lb-6: 40mg).
(+)-2-exo-3-exo-camphane-2, 3-diol (la-5) with (+)-2-Exo-3-exo-camphane-2,3-diol (la-5). Mp
microorganisms. In this work, it is clear that the 256.5_258.50; [a]~o + 17.4° (EtOH; c = 6.0); El-MS
reduction of camphorquinones to diols via a-ketoal- m/z: 170 [M] ÷ (CloH~802); IR ~'maxcm-l: 3641(OH);
cohols occurs with higher stereo- and enantioselectivity 1H NMR (270.05 MHz, CDCI3, TMS as int. standard):
than the reduction to a-ketoalcohols, t50.94 (3H, s, H-10) 0.80 (3H, s, H-9), 1.11(3H, s,
H-8), 0.80 (1H, m, H-6-endo, 1.40 (1H, m, H-6-exo),
0.85 (1H, m, H-5-endo), 1.60 (1H, m, H-5-exo), 1.70
EXPERIMENTAL (1H, d, J = 4.7 Hz, H-4) 3.84 (1H, d, J = 7.0 Hz, H-3),
General. (+)- and (-)-camphorquinones were pur- 3.51 (1H, d, J = 7.0 Hz, H-2); ~3C NMR (67.80 MHz,
chased from Kanto Chemical Co., Inc. 1H and ~3C CDC13:8 79.9 (d, C-2), 76.2 (d, C-3), 51.5 (d, C-4),
NMR: 270.05 and 67.80 MHz, respectively, GC-MS: 48.8 (s, C-7), 46.43 (s, C-l), 33.1 (t, C-6), 24.1 (t, C-5),
20 eV (ion voltage) and 250° (ion source) using OV-1 21.8 (q, C-9), 21.0 (q, C-8), 11.1 (q, C-10).
(0.25 mm × 30 m) capillary column GC; column temp. (+)-2-Endo-3-exo-camphane-2,3-diol (lb-6). Mp
4° min1 from 140 to 240°, injection temp. 240°. TLC: 254.0-256.0°; [a]~° + 15.0° (EtOH; c = 1.5); El-MS
silica gel 60 F254 pre-coated (layer thickness 0.25 nun, re~z:170 [M] ÷ (CIoH1802); IR l'm,x cm-l: 3628 (OH);
Merck) with n-hexane-EtOAc (1 : 1). CC: silica gel IH NMR (270.05 MHz, CDCI3, TMS as int. standard):
with n-hexane-EtOAc gradient). ~ 0.88(3H, s, H-10), 1.07 (3H, s, H-9), 0.85 (3H, s,
Microorganisms and culture condition. Glomerella H-8), 1.72 (1H, m, H-6-endo), 1.19 (1H, m, H-6-exo),
cingulata was purchased from Gifu University. The 1.17 (1H, m, H-5-endo), 1.72 (1H, m, H-5-exo), 1.66
fungus was maintained on nutrient agar slants at 10° (1H, m, J=4.7 Hz, H-4), 3.54 (1H, d, J=2.5 Hz,
and was used to inoculate autoclaved culture medium H-3), 3.96 (1H, d, J = 2.5 Hz, H-2), 13C NMR (67.80
(g 1-1); sucrose 15, glucose 15, polypeptone 5, KC1 0.5 MHz, CDCI3): t5 86.1 (d, C-2), 84.6 (d, C-3), 52.5 (d,
MgSO4.7H20 0.5, K2HPO4 1, FeSO4"7H20 0.01. C-4), 50.3 (s, C-7), 47.2 (s, C-I), 25.4 (t, C-6), 25.1 (t,
Cultivation of G. cingulata. The spores were shaken C-5), 21.0 (q, C-8), 19.3 (q, C-9), 12.9 (q, C-10).
with culture medium at 27° for 72 hr in an incubator.
Mycelia were then transferred to the culture medium
, REFERENCES
(150 ml in a 300 ml Erlenmeyer flask) and stirred for
72 hr at 27°. After the growth of the fungus; the 1. Miyazawa, M., Nobata, M., Hyakumachi, M. and
substrates (la and lb) were added directly to each Kameoka, H. (1995)Phytochemistry 39 (3), 569.
medium (400 mg per 200 ml) and the incubation 2. Partanen, T., Malkonen, P. J. and Vainiotalo, P.
continued under the same conditions for 10 days. (1990) J. Chem. Soc., Perkin. Trans. II, 777.
Purification of the metabolic products. At the end of 3. Robertson, J. S. and Solomon, E. (1971) Biochem. J.
the incubation period, the culture medium was col- 121, 503.

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  • 1. Pergamon Phytochemistry, Vol. 44, No. 1, pp. 79-81, 1997 Copyright © 1996 Elsevier Science Ltd Printed in Great Britain. All rights reserved PII: S0031-9422(96)00516-X 0031-9422/97 $17.00 + 0.00 BIOTRANSFORMATION OF (+)- AND (-)-CAMPHORQUINONES TO CAMPHANEDIOLS BY GLOMERELLA CINGULATA MITSUOM1YAZAWA,*MASAHIRONOBATA,MITSUROHYAKUMACHI~"and HIROMUKAMEOKA Department of Applied Chemistry, Faculty of Science and Engineering, Kinki University, Kowakae, Higasioska-shi, Osaka 577, Japan; -~Laboratoryof Plant Disease, Faculty of Agriculture, Gifu University, l-l, Yanagido, Gifu, 501-11, Japan (Receivedin revisedform 27 June 1996) Key Word Index--Glomerella cingulata; fungus; biotransformation; (+)-camphorquinone; (-)- camphorquinone; (+)-2-exo-3-exo-camphane-2,3-diol; (+)-2-endo-3-exo-camphane-2,3-diol; re- duction; stereoselectivity; enantioselectivity. Abstract--The reduction of (+)-camphorquinone by the plant pathogen Glomerella cingulata produced (+)-2- exo-3-exo-2,3-diol with high stereoselectivity, whereas (-)-camphorquinone yielded (+)-2-endo-3-exo-2,3-diol with high stereo- and enantioselectivity. Copyright © 1996 Elsvier Science Ltd INTRODUCTION Camphorquinone (la and lb) disappeared after 9 hr, as shown in a previous paper [1], and a-ketoalcohols were In our previous paper, (+)- and (-)-camphorquinones (la, lb) were shown to be readily reduced to keto produced in about 100% yield at 9 hr, and then decreased from 12 hr to 10 days. Compounds la-5 and alcohols by short time (24 hr) fermentation with various lb-6 were obtained 10-20% yield at 10 days (Figs 1 fungi [1]. In particular, Glomerella cingulata gave high and 2). yields of hydroxycamphors in a short time. However, In order to isolate these metabolites, a large scale further reduction to diols in the biotransformation of incubation of la and lb with G. cingulata was carried compounds la and lb have not been reported. out. After the biotransformation, the metabolites were This report deals with the biotransformation of la extracted and purified as described in the Experimental. and lb to camphanediols by G. cingulata. The structures of these compounds were determined by spectral methods. Metabolites la-5 and lb-6 were identified as (+)-(1R, 2R, 3R)-3-exo-I,7,7-tri- RESULTS AND DISCUSSION methylbicyclo [2.2.1 ] heptane- 2,3- diol((+)- 2- exo- 3- In time-course experiments, small amounts of either exo-camphane-2,3-diol, la-5) and (+) - (1S, 2R, 3R)- (+)-camphorquinone (la) or (-)-camphorquinone (lb) 3-exo-hydroxy-l,7,7-trimethyl-bicyclo [2.2.1] heptane- were incubated with G. cingulata for 10 days, respec- 2,3-diol ((+)-2-endo-3-exo-camphane-2,3-diol, lb-6) tively (Figs 1 and 2). The hiotransformation of com- by comparison with literature data [2]. It was consid- pounds la and lb proceeded readily to give the eredthat compound la was transformedto (+)-2-exo- oe-ketoaicohols (+)-2R-exo-hydroxyepicamphor(la-1), 3-exo-2,3-diol (la-5), yield 10%) via ~-ketoalcohols (-)-2S-endo-hydroxyepicamphor (la-2), (-)-3S-exo- (+)-2R-exo-hydroxyepicamphor (la-1) and/or (-)-3S- hydroxycamphor (la-3) and (+)-3R-endo-hydroxy- exo-hydroxycamphor (la-3), and compound lb to (+)- camphor (la-4) from la, and (-)-2S-exo-hydroxy- 2-endo-3-exo-2,3-diol (lb-6), yield 20%) via (+)-2R- epicamphor (lb-1), (+)-2R-endo-hydroxyepicamphor endo-hydroxyepicamphor (lb-2) and/or (+)-3R-exo- (lb-2), (+)-3R-exo-hydroxycamphor (lb-3) and (-)- hydroxyepicamphor (lb-3) (Scheme 1). These biocon- 3S-endo-hydroxycamphor (lb-4)from lb with reduc- version processes exhibited high regio- and stereo- tion of the carbonyl group [1]. These compounds of selective reduction. absolute configuration la-1-4 and lb-1-4 were de- In the case of biotransformation of racemic camphor- scribed in a previous paper [1]. It was confirmed that quinones by G. cingulata for 10 days, optically active the ot-keto-alcohols were further transformed by G. camphanediol (lb-6 yield 10%, optical purity 99.9%) cingulata to give la-5 and lb-6 over the ten-day period was isolated from the extract. This revealed that the of the experiment. Two secondary metabolites (la-5 reduction of racemic camphorquinones by G. cingulata and lb-6) were detected by TLC and GC analysis, proceeded with high stereo-and enantioselectivity. The yield of compound la-5 was very poor (about 5%, optical purity 99.9%). Thus, the racemic camphor- *Author to whom correspondence should be addressed, quinones (la, lb) were reduced by G. cingulata to 79
  • 2. 80 M. M]YAZAWA et al. I00 80- 0 0 1 2 3 4 S 6 7 8 9 10 Time (day) Fig. I. Time course of the biotransformationof (+)-camphorquinone (la) by Glomerella cingulata,lq, la; A, ketoalcohols (la-l-4); ©, 2-exo-3-exo-camphane-2, 3-diol(la-5). 100- == 4o 0 1 2 3 4 S 6 7 8 9 10 Time (day) Fig. 2. Time course of the biolransformationof (-)-camphurquinone (Ib) by Glomerella cingulata.B, lb; A, l<etoalcohols (lb-1-4); O, 2 endo-3-exo-camphane-2,3,-diol(lb-6). 8 9 OGcingulata: "1- OH 4" "1" "l" 5 "~0 " H OH H la la-1 la-2 111-3 1t1=4 (+)-(1s, 2R,3S) la-5 H HO H I b I b'l I b-2 I b'3 I b-4 (+)-(1R,2R,3R) lb-6 Scheme 1. Reduction of (+)-(la) and (-)-camphorquinone (lb) to ketoalcohols (la-l-4, lb-l-4) and diols (la-5, lb-6) by Glomerella cingulata.
  • 3. Biotransformation of camphorquinonesby Glomerellacingulata 81 yield 2,3-diol with high-stereo- and enantioselectivity, lected, saturated with NaC1, and extracted with EtOAc. respectively. The mycelia were also collected and extracted with In 1971, Robertson et al. [3] reported the reduction EtOAc. The EtOAc extracts were combined and the of camphorquinone in rabbits. This reduction provided solvent removed under red. pres. The extract was 2-endo-3-endo-camphanediol and 2-endo-3-exo- chromatographed on silica gel using n-hexane-EtOAc camohanediol. However, there have been no detailed and the substrate and metabolites isolated. In the case reports of the stereoselectivity. To our knowledge, this of compound la: la-l-4: 161mg; la-5:82 mg. In the is the first report of the reduction of compound la to case of lb: lb-l-4:188 mg lb-6: 40mg). (+)-2-exo-3-exo-camphane-2, 3-diol (la-5) with (+)-2-Exo-3-exo-camphane-2,3-diol (la-5). Mp microorganisms. In this work, it is clear that the 256.5_258.50; [a]~o + 17.4° (EtOH; c = 6.0); El-MS reduction of camphorquinones to diols via a-ketoal- m/z: 170 [M] ÷ (CloH~802); IR ~'maxcm-l: 3641(OH); cohols occurs with higher stereo- and enantioselectivity 1H NMR (270.05 MHz, CDCI3, TMS as int. standard): than the reduction to a-ketoalcohols, t50.94 (3H, s, H-10) 0.80 (3H, s, H-9), 1.11(3H, s, H-8), 0.80 (1H, m, H-6-endo, 1.40 (1H, m, H-6-exo), 0.85 (1H, m, H-5-endo), 1.60 (1H, m, H-5-exo), 1.70 EXPERIMENTAL (1H, d, J = 4.7 Hz, H-4) 3.84 (1H, d, J = 7.0 Hz, H-3), General. (+)- and (-)-camphorquinones were pur- 3.51 (1H, d, J = 7.0 Hz, H-2); ~3C NMR (67.80 MHz, chased from Kanto Chemical Co., Inc. 1H and ~3C CDC13:8 79.9 (d, C-2), 76.2 (d, C-3), 51.5 (d, C-4), NMR: 270.05 and 67.80 MHz, respectively, GC-MS: 48.8 (s, C-7), 46.43 (s, C-l), 33.1 (t, C-6), 24.1 (t, C-5), 20 eV (ion voltage) and 250° (ion source) using OV-1 21.8 (q, C-9), 21.0 (q, C-8), 11.1 (q, C-10). (0.25 mm × 30 m) capillary column GC; column temp. (+)-2-Endo-3-exo-camphane-2,3-diol (lb-6). Mp 4° min1 from 140 to 240°, injection temp. 240°. TLC: 254.0-256.0°; [a]~° + 15.0° (EtOH; c = 1.5); El-MS silica gel 60 F254 pre-coated (layer thickness 0.25 nun, re~z:170 [M] ÷ (CIoH1802); IR l'm,x cm-l: 3628 (OH); Merck) with n-hexane-EtOAc (1 : 1). CC: silica gel IH NMR (270.05 MHz, CDCI3, TMS as int. standard): with n-hexane-EtOAc gradient). ~ 0.88(3H, s, H-10), 1.07 (3H, s, H-9), 0.85 (3H, s, Microorganisms and culture condition. Glomerella H-8), 1.72 (1H, m, H-6-endo), 1.19 (1H, m, H-6-exo), cingulata was purchased from Gifu University. The 1.17 (1H, m, H-5-endo), 1.72 (1H, m, H-5-exo), 1.66 fungus was maintained on nutrient agar slants at 10° (1H, m, J=4.7 Hz, H-4), 3.54 (1H, d, J=2.5 Hz, and was used to inoculate autoclaved culture medium H-3), 3.96 (1H, d, J = 2.5 Hz, H-2), 13C NMR (67.80 (g 1-1); sucrose 15, glucose 15, polypeptone 5, KC1 0.5 MHz, CDCI3): t5 86.1 (d, C-2), 84.6 (d, C-3), 52.5 (d, MgSO4.7H20 0.5, K2HPO4 1, FeSO4"7H20 0.01. C-4), 50.3 (s, C-7), 47.2 (s, C-I), 25.4 (t, C-6), 25.1 (t, Cultivation of G. cingulata. The spores were shaken C-5), 21.0 (q, C-8), 19.3 (q, C-9), 12.9 (q, C-10). with culture medium at 27° for 72 hr in an incubator. Mycelia were then transferred to the culture medium , REFERENCES (150 ml in a 300 ml Erlenmeyer flask) and stirred for 72 hr at 27°. After the growth of the fungus; the 1. Miyazawa, M., Nobata, M., Hyakumachi, M. and substrates (la and lb) were added directly to each Kameoka, H. (1995)Phytochemistry 39 (3), 569. medium (400 mg per 200 ml) and the incubation 2. Partanen, T., Malkonen, P. J. and Vainiotalo, P. continued under the same conditions for 10 days. (1990) J. Chem. Soc., Perkin. Trans. II, 777. Purification of the metabolic products. At the end of 3. Robertson, J. S. and Solomon, E. (1971) Biochem. J. the incubation period, the culture medium was col- 121, 503.