- Email: [email protected]
Mutagenicity screening of popular thai spices
,q Chm. Toxic. Vol. 20. pp. 527 IO 530. 1982 Printed in Grcnf Britain. All rights rcscrved
Copyright
MUTAGENICITY
SCREENING
OF POPULAR
M. UNGSURUNGSIE* and 0. Department
of Microbiology, tPub/ic Health,
THAI
0278-69lS/82/050~27-04M3.~/0 0 1982 Pergamon Press Ltd
SPICES
.%WI-JJENKULt
Faculties oj *Pharmacy Mahidol University
und
and C. PAOVALO Department
Phwnaceutical Mahidol Unioersity. of
(Receioed
II
Chemistry, Faculty of Pharmacy, Bangkok 4, Thailand January
1982)
Abstract-Mutagenicity screeningwascarriedout on 31samples of popular Thai spices derived from 12 different families of plants, namely the Amaryllidaceae(2). Graminae(1). Labiatae(4). Lauraceae(1). Magnoliaceae(1).Myristicaceae(21,Myrtaceae(2).Piperaceae (3).Rutaceae(2),Solanaceae(2).Umbelliferae(2) and Zingiberaceae(9).Two variationsof the rapid streakmethodof ret-assayin Bacillus subtilis strains HI7 (ret+) and M45 (ret-) wereused.Only Ceylon cinnamon(the bark of Cinnamomum zeylanicum Neesof the family Lauraceae)showed mutagenicactivity. The crude form of this spice and its water-heatedand water-maceratedresiduesall producedthe ret effect,while water-heatedand watermaceratedfiltrates did not, evenin concentrationsequivalentto as muchas 50 mg solids/testdisc.
INTRODUCHON
Spices have been used for centuries to preserve foodsor to make them more appetizing by improving tasteand/or aroma. Many spices have also been used in both folk medicines and modern drug preparations, since they contain active medicinal ingredients (Cantoria, 1976; Morton, 1980; Swinyard & Harvey, 1975). Becauseof these widespread uses, the chemical constituents, the pharmacological actions and the antimicrobial activities of spices have been widely studied (Dasgupta & Datta, 1980; Isogai, Suzuki & Tamura, 1976;Monsereenusorn, 1980; Prasad & Joshi, 1949). However, little work has been carried out on the possible carcinogenic properties of spices and this may be useful since many are consumed in fairly large quantities over long periods of time. Mutagenicity is the capacity of a substance to induce changes in genes or chromosomes (Hollstein, McCann, Angelosante & Nichols, 1979) and many studies have revealed a close relationship between mutagenicity and carcinogenicity (Ames, Durston, Yamasaki & Lee, 1973; McCann, Choi, Yamasaki & Ames, 1975; Slater, Anderson & Rosenkranz, 1971). About SO-90%of the substancesrecognized as mutagenic also show carcinogenic action. Consequently, any spice showing a mutagenic effect may also have an associatedcarcinogenic capacity. In this investigation, 31 samples of popular Thai spiceswere screened for mutagenicity using the rapid stre’akmethod of the ret-assaysystem.
of the plants used are identified in Table 1. To reduce the residuesof any insecticides that might be present, the fresh spiceswere washed twice, drained and finally ground. The dried spices were powdered directly, except for turmeric which was purchased in the powdered form. Each ground spice was divided into three portions for treatment according to the following three protocols, which reflected some of the cooking procedures to which the spices are commonly subjected and which together could provide some information on the heat stability and water solubility of active constituents of the spices:
(1) One portion was not treated and was designated the ‘crude form’ of the spice. (2) The second portion was mixed with water (log spice in 50 ml, except turmeric for which lOOmi water was used) and the mixture was heated in a boiling water-bath for 1 hr, cooled to room temperature and filtered through gauze or cotton wool to yield the ‘water-heated residue’ and ‘water-heated filtrate’. The latter was divided into two parts, one part remaining untreated while the other was dried at 85”C, 0.5-l g of the residue being redissolved in 1 ml water. (3) The third portion was treated in the sameway as the second portion, except that the mixture was macerated for 5 days at room temperature instead of being boiled and the treated part of the ‘water-macerated filtrate’ separated from the ‘water-macerated residue’ was dried at 45°C rather than at 85°C. Bacteria. Bacillus subtilis strain H17 (ret+), possessEXPERIMENTAL ing regular DNA recombination repair properties, Test spices.Thirty-one samples of fresh and dried and strain M45 (ret-), a mutant with a much lower Thai spiceswere bought from local markets and herb DNA-repair efficiency, were used as test organisms. shops,respectively, in Bangkok. The spices and Parts These two strains were kindly provided by Dr T. F.C.T. 2u/s-c
527
M. UNGSURUNGSIE, 0. SUTHIENKULand C. PAOVALO
528
Table
I. Tested spices and their planr sources
Common name
Source
Family
Fresh spices
minimum Roxb. var.
Bird pepper Cherry pepper
Fruit of Fruit ol
Galangal Garlic Ginger (old) (young) Hoary basil Holy-basil Kitchen mint Kra chai Leech lime Lemon grass Shallot Sweet basil Zedoary
longum Bail Rhizome of Alpinia galanga Swartz Bulb of Allium~satiu~m Linn. Rhizome of Zinaiber oficinale Roscoe Roscoe Rhizome of Ziniiber o&inale Leaf of Ocimum americana Linn. Leaf of Ocium sanctum Linn. Leaf of Mentha cordifolia Apir Ridl. Root of Gastrochilus-pandurkus Leaf of Citrus hysrrix DC Stem of Cymbopogon citratus Stapf. Bulb or Allium ascalonicum Linn. Leaf of Ocimum basilicurn Linn. Rhizome of Curcuma zedoaria Rose
Capsicum Capsicum
frutescens
Dried
Bay leaf Black pepper Caraway Ceylon cinnamon Chinese star anise Clove Coriander Dee plee Mace Nutmeg Phlai Phrik horn Siam cardamom Turmeric White pepper Wild ginger
Kada, National Japan.
Media and culture preparation. The composition of the liquid medium used for bacterial culture was log
beef extract (Difco Laboratories, Detroit, MI, USA), log polypeptone (Daiko Chemical Co., Osaka, Japan) and 5 g NaCl (Sigma Chemical Co., St. Louis, MO, USA) in 1 litre distilled water, pH 7. For solid medium, 15g bacto-agar (Difco Laboratories) was added and 10ml medium was dispensed into each lo-cm Petri dish. Culture preparations. B. subtilis strains H17 and M45 were separately cultivated in liquid medium at 37°C for 18 hr in a shaker incubator, and 50% (w/v) glycerol was then added to each culture (glycerol:culture = 1: 3). The cultures were then divided into small vials and kept in the freezer at -80°C. One vial was used for each experiment. Mutagenicity screening of spices. The rapid streak method of the ret-assay system described by Kada and his colleagues (Kada, Moriya & Shirasu, 1974; Kada, Tutikawa & Sadaie, 1972)was used with slight modification. Briefly, the frozen cultures of B. subtilis strains H17 and M45 were thawed at room temperature, each strain was streaked on the agar plate in a long line and spices were tested using IS-mm paper discs. These discs were wetted with 0.05ml water
Zingiberaceae Amaryllidaceae Zingiberaceae Zingiberaceae Labiatae Labiatae Labiatae Zingiberaceae Rutaceae Graminae Amaryllidaceae Labiatae Zingiberaceae
spices
Leaf of Pimenta racemoso Moiller Fruit of Piper nigrum Linn. Fruit ol Cuminum cyminum Linn. Bark of Cinnamomum zeylanicum Nees Fruit of Illicium serum Hook Flower of Eugenia caryophyllus Bullock et Harris Fruit of Coriandrum sativum Linn. Fruit ol’ Piper chaba Hunt Arillode of Myrisrica J-agans Linn. Seed of Myristica fiagans Linn. Rhizome of Zingiber cassumunar Roxb. Fruit of Zanthoxylum limonella Alston Fruit of Amomum kreruanh Pierre Rhizome of Curcuma longa Linn. Fruit of Piper nigrum Linn. Rhizome of Zingiber zerumbet Smith
Institute of Genetics, Mishima,
Solanaceae Solanaceae
Myrtaceae Piperaceae Umbellirerae Lauraceae Magnoliaceae Myrtaceae Umbelliferae Piperaceae Myristicaceae Myristicaceae Zingiberaceae Rutaceae Zingiberaceae Zingiberaceae Piperaceae Zingiberaceae
before application of the sample. For testing of the crude samples and residues (water-heated and water-
macerated), the wetted disc was placed on the agar, with the margin of the paper touching the two streaked lines, and a 15-mm diameter and S-mm high metal ring was placed on top of the disc for easy loading with the spice powder or residue. After loading, the ring was removed. For the test filtrates (wattir-heated and water-macerated). a volume of O.OSmlwas pipetted/inoculated into the wetted disc before the disc was put on the agar. In this case the concentrated filtrate gave approximately 25-50 mg solids/disc. Mitomycin C (Kyowa Hokko Kogko Co. Ltd, Tokyo, Japan) at 0.05 pg/disc was used as the positive control, while water and cellulose (Sigmacell@Type 100; Sigma Chemical Co.) were used as negative controls: Two setsof plate tests were carried out and each set was duplicated. The first set was incubated at 37°C for 24 hr (the ‘standard streak method’). The second set was first put in the refrigerator (4°C) overnight and then incubated continuously at 37°C for 24 hr (the ‘cold method’). A result was interpreted as pOSitive for mutagenicity if the clear zone on the streaked line of strain M45 appeared 3 mm or more longer than that on the line of strain H17.
Mutagenicity Table
screening
2. Test samples showing antimicrobial activity* in the water-maceraced filtrates and residues, using
of Thai
spices
529
ret-assa)!of crude forms of Bacillussubtilis HI 7 (ret+) Lengths
spices and their and M45 (ret-)
Cold method
B. subrilis
Crude forms Galangal Garlic Shallot Zedoary Ceylon cinnamon Chinese star anise Clove Turmeric Wild ginger Water-heated residues Ceylon cinnamon Clove
B. subrilis
Hl7
M45
Difference
Ret effectt
5 41
5 42
0
-
I
-
0 6.5 0
2.5 I.5 I4 2
I 1.5 7.5 2
T -
5 0
5 0
0 0
-
4
6
2
17.5 7
23.5 6
I.5
6
HI 7
M45
Difference
Ret effectt
5.5 41 65 2.5 7 2
7 43 9 4 I4 2
I.5 2
-
2.5 1.5 7 0
I +
II
9
2 3
2 5
20 I2
+
-I
-2
29.5 I4
Water-heatedfiltrates Chinese star anise (50 mg solids/disc) Clove (50 mg solids/disc)
Water-macerated residues Garlic Ceylon
6.5
II
2
ginger
Water-macerated filtrates Garlic (50mg solids/disc) Clove
2 2
6 2
(50 mg solids/disc)
I -
-I
5 2
5 2
8
1
-
IO.5
4
+
IO II
II 25
0
-
23 I.5
23 3
I
-
I2 2
II
7
cinnamon
Clove Wild
I 3
I2
I
2
7 I
and
of clear zone (mm)
Standardstreakmethod
Spice
water-heated
-1
*The other samples tested (see Table 1) showed no antimicrobial activity cold method). tlndicating no mutagenic activity (-) and with mutagenic activity (+).
-
in either
variant
0 2
-
9.5 2
+ -
0 0
-
I
-
I4 0
+ -
I.5 -I
3
I
of the assay (standard
streak
or
the spice and also by the water-heated and watermacerated residues, but not by the water-heated and The results in Table 2 show that many of the tested water-macerated filtrates, showing the responsible spices showed antimicrobial activity against strains component(s) to be heat stable but not water soluble. H17 and M45. In the crude form, these spices were Organic-solvent fractions have not been prepared and galangal. garlic, shallot. zedoary, Ceylon cinnamon, it is not yet known whether the fractions showing a Chinese star anise, clove, turmeric and wild ginger. mutagenic action are also carcinogenic. Another Among these,garlic produced the longest clear zones aspectrequiring investigation is the possible influence for both strains, with lengths of about 40 mm by both of metabolic processeson the mutagenic activity of the standard streak and cold methods. When the spice constituents, and work is at present in progress spiceshad been heated with water, only the residues on the mutagenicity of various Ceylon cinnamon of Ceylon cinnamon and clove retained their antimic- extracts using the spore ret-assay in the presenceand robial activity, while the untreated water-heated fil- absenceof a hepatic metabolizing system. trates had no such effect. However, when these filtrateswere concentrated, Chinese star anise and clove Acknowledgements-We are indebted to Dr T. Kada, at 50 mg/disc produced some clear zones on the Department of Induced Mutation, National Institute of streak lines of HI7 and M45. The water-macerated Genetics, Mishima, Japan, for generous supplies of the test residuesof four samplesof spices,namely, garlic, Cey- organisms and we gratefully acknowledge the help of Dr T. lon cinnamon, clove and wild ginger, possessedanti- Flagel, Departmentof Microbiology, Faculty of Science. microbial activity, and again the corresponding fil- Mahidol University, in reviewingthis paper.The work described was supported by a grant from Mahidol Univertrates showed no activity until after their concen- sity. tration to 50 mg/disc, at which point both garlic and clove caused inhibition of both test strains. When the lengths of the clear zones for strains HI7 REFERENCES and M45 were compared, only Ceylon cinnamon had a ret effect, indicating the possession of mutagenic Ames, B. N., Durston, W. E., Yamasaki, E. & Lee, F. D. (1973). Carcinogensare mutagens:A simple test system activity. This effect was exhibited by the crude form of RESULTS
AND
DISCUSSION
M. UNGSURUNGSIE,0. SUTHIENKUL and C. PAOVALO
530
combining liver homogenates for activation and bacteria for detection. Proc. na&. Acad. Sci. U.S.A. 70, 2281. Cantoria. M. (1976).Aromatic and medicinal spices of the Philippines.’ Q. Ji Crude Drug Res. 14, 97. . Dasgupta, A. & Data, P. C. (1980). Medicinal spices of piper, pharmacognostic delimitation. Q. JI Crude Drug Res. 18, 17. Hollstein, M.. McCann. J., Angelosante, F. A. & Nichols, W. W. (1979):Short-term tests for carcinogens and mutagens. Mutation Res. 65, 133. Isogai, A., Suzuki, A. & Tamura, S. (1976). Structure of cinnzeylanin and cinnzeylanol, polyhydroxylated pentazeylanicum Nees. cyclic diterpenes from Cinnamomum Agric.
hiol. khem.
40, 2305.
Kada. T.. Moriva. M. & Shirasu. Y. (1974). Screening of pesticides for- DNA interactions by “ret-assay” and mutagenesis testing, and frameshift mutagens detected. Mutation
Res. 26. 243.
Kada. T., Tutikawa, K. & Sadaie, Y. (1972). In vitro and host mediated “ret-assay” procedures for screening chemical mutagens; and phloxine. a mutagenic red dye detected. Marorion Res. 16. 165.
McCann, J., Choi, E., Yamasaki. E. & Ames, B. N. (1975). Detection of carcinogens as mutagens in the Salmonella/ microsome test: assay of 300 chemicals. Proc. natn. Acad. Sci. U.S.A.
72. 5135.
Monsereenusorn, Y. (1980). Effect of Capsicum annum on blood glucose level. Q. J/ Crude Drug Res. 18, 1. Morton, J. F. (1980). Caribbean and Latin American folk medicine and its influence in the United States. Q. J/ Crude Drug Rex
18, 57.
Prasad, H. H. & Joshi. N. V. (1949).The preservative value of spices used in pickling raw fruit in India. Agric. J. India.
34, 402.
Slater. E. E.. Anderson, M. D. & Rosenkranz, H. S. (1971). Rapid detection of mutagens and carcinogens. Cancer Res. 31, 970.
Swinyard. E. A. & Harvey, S. C. (1975). Gastrointestinal drugs. In Remington’s Pharmaceurical Sciences. Edited by G. D. Chase, R. S. Deno, A. R. Gennaro, M. R. Gibson, S. C. Harvey, R. E. King, A. N. Martin, E. A. Swinyard, C. T. Van Meter & B. Willin. 15th Ed. p. 787. Mack Printing Co., Easton. PA.
Copyright
MUTAGENICITY
SCREENING
OF POPULAR
M. UNGSURUNGSIE* and 0. Department
of Microbiology, tPub/ic Health,
THAI
0278-69lS/82/050~27-04M3.~/0 0 1982 Pergamon Press Ltd
SPICES
.%WI-JJENKULt
Faculties oj *Pharmacy Mahidol University
und
and C. PAOVALO Department
Phwnaceutical Mahidol Unioersity. of
(Receioed
II
Chemistry, Faculty of Pharmacy, Bangkok 4, Thailand January
1982)
Abstract-Mutagenicity screeningwascarriedout on 31samples of popular Thai spices derived from 12 different families of plants, namely the Amaryllidaceae(2). Graminae(1). Labiatae(4). Lauraceae(1). Magnoliaceae(1).Myristicaceae(21,Myrtaceae(2).Piperaceae (3).Rutaceae(2),Solanaceae(2).Umbelliferae(2) and Zingiberaceae(9).Two variationsof the rapid streakmethodof ret-assayin Bacillus subtilis strains HI7 (ret+) and M45 (ret-) wereused.Only Ceylon cinnamon(the bark of Cinnamomum zeylanicum Neesof the family Lauraceae)showed mutagenicactivity. The crude form of this spice and its water-heatedand water-maceratedresiduesall producedthe ret effect,while water-heatedand watermaceratedfiltrates did not, evenin concentrationsequivalentto as muchas 50 mg solids/testdisc.
INTRODUCHON
Spices have been used for centuries to preserve foodsor to make them more appetizing by improving tasteand/or aroma. Many spices have also been used in both folk medicines and modern drug preparations, since they contain active medicinal ingredients (Cantoria, 1976; Morton, 1980; Swinyard & Harvey, 1975). Becauseof these widespread uses, the chemical constituents, the pharmacological actions and the antimicrobial activities of spices have been widely studied (Dasgupta & Datta, 1980; Isogai, Suzuki & Tamura, 1976;Monsereenusorn, 1980; Prasad & Joshi, 1949). However, little work has been carried out on the possible carcinogenic properties of spices and this may be useful since many are consumed in fairly large quantities over long periods of time. Mutagenicity is the capacity of a substance to induce changes in genes or chromosomes (Hollstein, McCann, Angelosante & Nichols, 1979) and many studies have revealed a close relationship between mutagenicity and carcinogenicity (Ames, Durston, Yamasaki & Lee, 1973; McCann, Choi, Yamasaki & Ames, 1975; Slater, Anderson & Rosenkranz, 1971). About SO-90%of the substancesrecognized as mutagenic also show carcinogenic action. Consequently, any spice showing a mutagenic effect may also have an associatedcarcinogenic capacity. In this investigation, 31 samples of popular Thai spiceswere screened for mutagenicity using the rapid stre’akmethod of the ret-assaysystem.
of the plants used are identified in Table 1. To reduce the residuesof any insecticides that might be present, the fresh spiceswere washed twice, drained and finally ground. The dried spices were powdered directly, except for turmeric which was purchased in the powdered form. Each ground spice was divided into three portions for treatment according to the following three protocols, which reflected some of the cooking procedures to which the spices are commonly subjected and which together could provide some information on the heat stability and water solubility of active constituents of the spices:
(1) One portion was not treated and was designated the ‘crude form’ of the spice. (2) The second portion was mixed with water (log spice in 50 ml, except turmeric for which lOOmi water was used) and the mixture was heated in a boiling water-bath for 1 hr, cooled to room temperature and filtered through gauze or cotton wool to yield the ‘water-heated residue’ and ‘water-heated filtrate’. The latter was divided into two parts, one part remaining untreated while the other was dried at 85”C, 0.5-l g of the residue being redissolved in 1 ml water. (3) The third portion was treated in the sameway as the second portion, except that the mixture was macerated for 5 days at room temperature instead of being boiled and the treated part of the ‘water-macerated filtrate’ separated from the ‘water-macerated residue’ was dried at 45°C rather than at 85°C. Bacteria. Bacillus subtilis strain H17 (ret+), possessEXPERIMENTAL ing regular DNA recombination repair properties, Test spices.Thirty-one samples of fresh and dried and strain M45 (ret-), a mutant with a much lower Thai spiceswere bought from local markets and herb DNA-repair efficiency, were used as test organisms. shops,respectively, in Bangkok. The spices and Parts These two strains were kindly provided by Dr T. F.C.T. 2u/s-c
527
M. UNGSURUNGSIE, 0. SUTHIENKULand C. PAOVALO
528
Table
I. Tested spices and their planr sources
Common name
Source
Family
Fresh spices
minimum Roxb. var.
Bird pepper Cherry pepper
Fruit of Fruit ol
Galangal Garlic Ginger (old) (young) Hoary basil Holy-basil Kitchen mint Kra chai Leech lime Lemon grass Shallot Sweet basil Zedoary
longum Bail Rhizome of Alpinia galanga Swartz Bulb of Allium~satiu~m Linn. Rhizome of Zinaiber oficinale Roscoe Roscoe Rhizome of Ziniiber o&inale Leaf of Ocimum americana Linn. Leaf of Ocium sanctum Linn. Leaf of Mentha cordifolia Apir Ridl. Root of Gastrochilus-pandurkus Leaf of Citrus hysrrix DC Stem of Cymbopogon citratus Stapf. Bulb or Allium ascalonicum Linn. Leaf of Ocimum basilicurn Linn. Rhizome of Curcuma zedoaria Rose
Capsicum Capsicum
frutescens
Dried
Bay leaf Black pepper Caraway Ceylon cinnamon Chinese star anise Clove Coriander Dee plee Mace Nutmeg Phlai Phrik horn Siam cardamom Turmeric White pepper Wild ginger
Kada, National Japan.
Media and culture preparation. The composition of the liquid medium used for bacterial culture was log
beef extract (Difco Laboratories, Detroit, MI, USA), log polypeptone (Daiko Chemical Co., Osaka, Japan) and 5 g NaCl (Sigma Chemical Co., St. Louis, MO, USA) in 1 litre distilled water, pH 7. For solid medium, 15g bacto-agar (Difco Laboratories) was added and 10ml medium was dispensed into each lo-cm Petri dish. Culture preparations. B. subtilis strains H17 and M45 were separately cultivated in liquid medium at 37°C for 18 hr in a shaker incubator, and 50% (w/v) glycerol was then added to each culture (glycerol:culture = 1: 3). The cultures were then divided into small vials and kept in the freezer at -80°C. One vial was used for each experiment. Mutagenicity screening of spices. The rapid streak method of the ret-assay system described by Kada and his colleagues (Kada, Moriya & Shirasu, 1974; Kada, Tutikawa & Sadaie, 1972)was used with slight modification. Briefly, the frozen cultures of B. subtilis strains H17 and M45 were thawed at room temperature, each strain was streaked on the agar plate in a long line and spices were tested using IS-mm paper discs. These discs were wetted with 0.05ml water
Zingiberaceae Amaryllidaceae Zingiberaceae Zingiberaceae Labiatae Labiatae Labiatae Zingiberaceae Rutaceae Graminae Amaryllidaceae Labiatae Zingiberaceae
spices
Leaf of Pimenta racemoso Moiller Fruit of Piper nigrum Linn. Fruit ol Cuminum cyminum Linn. Bark of Cinnamomum zeylanicum Nees Fruit of Illicium serum Hook Flower of Eugenia caryophyllus Bullock et Harris Fruit of Coriandrum sativum Linn. Fruit ol’ Piper chaba Hunt Arillode of Myrisrica J-agans Linn. Seed of Myristica fiagans Linn. Rhizome of Zingiber cassumunar Roxb. Fruit of Zanthoxylum limonella Alston Fruit of Amomum kreruanh Pierre Rhizome of Curcuma longa Linn. Fruit of Piper nigrum Linn. Rhizome of Zingiber zerumbet Smith
Institute of Genetics, Mishima,
Solanaceae Solanaceae
Myrtaceae Piperaceae Umbellirerae Lauraceae Magnoliaceae Myrtaceae Umbelliferae Piperaceae Myristicaceae Myristicaceae Zingiberaceae Rutaceae Zingiberaceae Zingiberaceae Piperaceae Zingiberaceae
before application of the sample. For testing of the crude samples and residues (water-heated and water-
macerated), the wetted disc was placed on the agar, with the margin of the paper touching the two streaked lines, and a 15-mm diameter and S-mm high metal ring was placed on top of the disc for easy loading with the spice powder or residue. After loading, the ring was removed. For the test filtrates (wattir-heated and water-macerated). a volume of O.OSmlwas pipetted/inoculated into the wetted disc before the disc was put on the agar. In this case the concentrated filtrate gave approximately 25-50 mg solids/disc. Mitomycin C (Kyowa Hokko Kogko Co. Ltd, Tokyo, Japan) at 0.05 pg/disc was used as the positive control, while water and cellulose (Sigmacell@Type 100; Sigma Chemical Co.) were used as negative controls: Two setsof plate tests were carried out and each set was duplicated. The first set was incubated at 37°C for 24 hr (the ‘standard streak method’). The second set was first put in the refrigerator (4°C) overnight and then incubated continuously at 37°C for 24 hr (the ‘cold method’). A result was interpreted as pOSitive for mutagenicity if the clear zone on the streaked line of strain M45 appeared 3 mm or more longer than that on the line of strain H17.
Mutagenicity Table
screening
2. Test samples showing antimicrobial activity* in the water-maceraced filtrates and residues, using
of Thai
spices
529
ret-assa)!of crude forms of Bacillussubtilis HI 7 (ret+) Lengths
spices and their and M45 (ret-)
Cold method
B. subrilis
Crude forms Galangal Garlic Shallot Zedoary Ceylon cinnamon Chinese star anise Clove Turmeric Wild ginger Water-heated residues Ceylon cinnamon Clove
B. subrilis
Hl7
M45
Difference
Ret effectt
5 41
5 42
0
-
I
-
0 6.5 0
2.5 I.5 I4 2
I 1.5 7.5 2
T -
5 0
5 0
0 0
-
4
6
2
17.5 7
23.5 6
I.5
6
HI 7
M45
Difference
Ret effectt
5.5 41 65 2.5 7 2
7 43 9 4 I4 2
I.5 2
-
2.5 1.5 7 0
I +
II
9
2 3
2 5
20 I2
+
-I
-2
29.5 I4
Water-heatedfiltrates Chinese star anise (50 mg solids/disc) Clove (50 mg solids/disc)
Water-macerated residues Garlic Ceylon
6.5
II
2
ginger
Water-macerated filtrates Garlic (50mg solids/disc) Clove
2 2
6 2
(50 mg solids/disc)
I -
-I
5 2
5 2
8
1
-
IO.5
4
+
IO II
II 25
0
-
23 I.5
23 3
I
-
I2 2
II
7
cinnamon
Clove Wild
I 3
I2
I
2
7 I
and
of clear zone (mm)
Standardstreakmethod
Spice
water-heated
-1
*The other samples tested (see Table 1) showed no antimicrobial activity cold method). tlndicating no mutagenic activity (-) and with mutagenic activity (+).
-
in either
variant
0 2
-
9.5 2
+ -
0 0
-
I
-
I4 0
+ -
I.5 -I
3
I
of the assay (standard
streak
or
the spice and also by the water-heated and watermacerated residues, but not by the water-heated and The results in Table 2 show that many of the tested water-macerated filtrates, showing the responsible spices showed antimicrobial activity against strains component(s) to be heat stable but not water soluble. H17 and M45. In the crude form, these spices were Organic-solvent fractions have not been prepared and galangal. garlic, shallot. zedoary, Ceylon cinnamon, it is not yet known whether the fractions showing a Chinese star anise, clove, turmeric and wild ginger. mutagenic action are also carcinogenic. Another Among these,garlic produced the longest clear zones aspectrequiring investigation is the possible influence for both strains, with lengths of about 40 mm by both of metabolic processeson the mutagenic activity of the standard streak and cold methods. When the spice constituents, and work is at present in progress spiceshad been heated with water, only the residues on the mutagenicity of various Ceylon cinnamon of Ceylon cinnamon and clove retained their antimic- extracts using the spore ret-assay in the presenceand robial activity, while the untreated water-heated fil- absenceof a hepatic metabolizing system. trates had no such effect. However, when these filtrateswere concentrated, Chinese star anise and clove Acknowledgements-We are indebted to Dr T. Kada, at 50 mg/disc produced some clear zones on the Department of Induced Mutation, National Institute of streak lines of HI7 and M45. The water-macerated Genetics, Mishima, Japan, for generous supplies of the test residuesof four samplesof spices,namely, garlic, Cey- organisms and we gratefully acknowledge the help of Dr T. lon cinnamon, clove and wild ginger, possessedanti- Flagel, Departmentof Microbiology, Faculty of Science. microbial activity, and again the corresponding fil- Mahidol University, in reviewingthis paper.The work described was supported by a grant from Mahidol Univertrates showed no activity until after their concen- sity. tration to 50 mg/disc, at which point both garlic and clove caused inhibition of both test strains. When the lengths of the clear zones for strains HI7 REFERENCES and M45 were compared, only Ceylon cinnamon had a ret effect, indicating the possession of mutagenic Ames, B. N., Durston, W. E., Yamasaki, E. & Lee, F. D. (1973). Carcinogensare mutagens:A simple test system activity. This effect was exhibited by the crude form of RESULTS
AND
DISCUSSION
M. UNGSURUNGSIE,0. SUTHIENKUL and C. PAOVALO
530
combining liver homogenates for activation and bacteria for detection. Proc. na&. Acad. Sci. U.S.A. 70, 2281. Cantoria. M. (1976).Aromatic and medicinal spices of the Philippines.’ Q. Ji Crude Drug Res. 14, 97. . Dasgupta, A. & Data, P. C. (1980). Medicinal spices of piper, pharmacognostic delimitation. Q. JI Crude Drug Res. 18, 17. Hollstein, M.. McCann. J., Angelosante, F. A. & Nichols, W. W. (1979):Short-term tests for carcinogens and mutagens. Mutation Res. 65, 133. Isogai, A., Suzuki, A. & Tamura, S. (1976). Structure of cinnzeylanin and cinnzeylanol, polyhydroxylated pentazeylanicum Nees. cyclic diterpenes from Cinnamomum Agric.
hiol. khem.
40, 2305.
Kada. T.. Moriva. M. & Shirasu. Y. (1974). Screening of pesticides for- DNA interactions by “ret-assay” and mutagenesis testing, and frameshift mutagens detected. Mutation
Res. 26. 243.
Kada. T., Tutikawa, K. & Sadaie, Y. (1972). In vitro and host mediated “ret-assay” procedures for screening chemical mutagens; and phloxine. a mutagenic red dye detected. Marorion Res. 16. 165.
McCann, J., Choi, E., Yamasaki. E. & Ames, B. N. (1975). Detection of carcinogens as mutagens in the Salmonella/ microsome test: assay of 300 chemicals. Proc. natn. Acad. Sci. U.S.A.
72. 5135.
Monsereenusorn, Y. (1980). Effect of Capsicum annum on blood glucose level. Q. J/ Crude Drug Res. 18, 1. Morton, J. F. (1980). Caribbean and Latin American folk medicine and its influence in the United States. Q. J/ Crude Drug Rex
18, 57.
Prasad, H. H. & Joshi. N. V. (1949).The preservative value of spices used in pickling raw fruit in India. Agric. J. India.
34, 402.
Slater. E. E.. Anderson, M. D. & Rosenkranz, H. S. (1971). Rapid detection of mutagens and carcinogens. Cancer Res. 31, 970.
Swinyard. E. A. & Harvey, S. C. (1975). Gastrointestinal drugs. In Remington’s Pharmaceurical Sciences. Edited by G. D. Chase, R. S. Deno, A. R. Gennaro, M. R. Gibson, S. C. Harvey, R. E. King, A. N. Martin, E. A. Swinyard, C. T. Van Meter & B. Willin. 15th Ed. p. 787. Mack Printing Co., Easton. PA.