1 Kumamoto Prefectural Fisheries Research Center, Ohyano, Amakusa, Kumamoto 869-3603; 2 Laboratory of Marine Resource Chemistry, Graduate School of Agriculture, Kyushu University, 6-10-1, Hakozaki, Fukuoka 812-8581; 3 The Chemo-Sero-Therapeutic Research Institute, Kikuchi Research Center, Kyokushi, Kikuchi, Kumamoto 869-1298, Japan
Received 2 January 2002; returned 4 July 2002; revised 10 August 2002; accepted 28 August 2002
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Abstract |
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Introduction |
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The present study was undertaken in order to examine the bactericidal effects of crude and purified phlorotannins from the brown alga E. kurome on pathogenic bacteria, primarily including food-borne pathogenic bacteria and MRSA. In addition, the effect of the administration of phlorotannins on male and female mice was investigated in order to confirm the safety of phlorotannins for mammals.
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Materials and methods |
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Bacillus cereus (two strains), MRSA (nine strains), S. aureus, Streptococcus pyogenes, Campylobacter fetus, Campylobacter jejuni (three strains), Escherichia coli (three strains), Salmonella enteritidis (nine strains), Salmonellae typhimurium (four strains) and Vibrio parahaemolyticus (two strains) were obtained from our collection or from clinical isolates held within The Chemo-Sero-Therapeutic Research Institute.
The reference strains used in tests were S. aureus Smith, S. aureus ATCC 25923 (MRSA), S. pyogenes ATCC 19615, B. cereus ATCC 19637, C. fetus CIP 53105, C. jejuni CIP 702, E. coli ATCC 25922, E. coli NIHJ JC-2, S. enteritidis S-48, S. enteritidis L-248, S. enteritidis L-540, S. typhimurium L-719, S. typhimurium L-767, S. typhimurium SIC-8401 and S. typhimurium ATCC 14028.
All the bacteria except for Campylobacter spp. were cultured aerobically without shaking in 10 mL of brain heart infusion (BHI) broth (Nissui, Tokyo, Japan) at 37°C for 18 h. NaCl (2.5%) was added to the medium used for V. parahaemolyticus. Campylobacter spp. were grown on fresh Skirrow agar plates (Merck, Tokyo, Japan) at 37°C for 48 h in a Campy Pouch (Becton Dickinson, San Jose, CA, USA).
Preparation of phlorotannins
The brown alga E. kurome Okamura was collected from an undersea forest of algae near Tsuji Island, Kumamoto, Japan, in May 2000 and washed with tap water to remove sediment and epiphytes, before being air-dried and pulverized. The algal powder (800 g, moisture 10%) was extracted with methanol (2400 mL) with shaking (90 rpm) at 5°C for 48 h. The extracts were concentrated in vacuo to a small volume before methanol (240 mL), chloroform (480 mL) and deionized water (180 mL) were added, and then the upper and lower layers were separated.13 The upper layer was extracted twice with ethylacetate (300 mL). The ethylacetate fraction was evaporated in vacuo. The extract is hereafter referred to as crude phlorotannins. The algal powder produced a yield of phlorotannins of
3%.
The crude phlorotannins were composed of phloroglucinol (2%) and its oligomers: eckol (trimer, 9%), phlorofucofuroeckol A (pentamer, 28%), dieckol (hexamer, 24%), 8,8'-bieckol (hexamer, 7%) and others (unidentified tetramer, etc., 30%). The components were identified by thin-layer chromatography (TLC)12 and determined quantitatively by high-performance liquid chromatography (Inertsil ODS column, 6 x 150 mm, GL Science, Tokyo, Japan). Elution was performed at a flow rate of 1.0 mL/min using a linear gradient of 30100% methanol with UV detection at 290 nm. These compounds were fractionated by silicic acid chromatography on a column (15 mm i.d. x 150 cm, Wakogel C-300HG; Wako Pure Chemical Industries, Osaka, Japan) with chloroform: methanol:water (80:20:2, v/v) as the eluent. Each 5 mL fraction was collected and evaporated in vacuo. Consecutive fractions that showed a single spot representing eckol, phlorofucofuroeckol A, dieckol or 8,8'-bieckol on TLC were pooled (>90% purity). Phloroglucinol (as dihydrate, >98% purity) was obtained from Wako Pure Chemical Industries. Terrestrial polyphenols, catechin (>90% purity) and EGCG (>95% purity) were obtained from Kurita Water Industries (Tokyo, Japan).
Determination of bactericidal effects
The MBC of the phlorotannins, taken as the lowest concentration that could kill 99.9% of the initial inoculum within 24 h, was determined using a broth microdilution method. All tests were performed in sensitivity test broth (StB; Eiken Chemical, Tokyo, Japan) in 24-well microtitre plates. All cultured cells were suspended in StB to give a concentration of 104105 cfu/mL, and 1 mL of broth culture was pipetted into each well. The concentration of each inoculum was determined using viable counts on BHI agar (BHIA) plates for bacteria. Fresh Skirrow agar plates or 2.5% NaCl-added BHIA plates were used for Campylobacter or Vibrio spp., respectively. The isolated or crude phlorotannins and catechins were dissolved in 70% methanol, and 20 µL of the solution was added to each well, before being incubated with shaking (60 rpm) aerobically at 37°C for 24 h. To determine the MBCs, 20200 µL of culture was removed from each well at various time points and incubated in BHIA. After aerobic incubation at 37°C for 24 h, the colonies were enumerated. V. parahaemolyticus was tested in medium supplemented with 2.5% NaCl. Fresh Skirrow agar plates were used for Campylobacter spp. instead of BHIA, and these were incubated for 72 h. The microtitre and fresh agar plates seeded with Campylobacter spp. were incubated in a Campy Pouch. The methanol (final concentration, 1.4%) in the medium did not affect the growth of the strains during the experiments. The experiments were repeated two or three times.
Administration of crude phlorotannins to mice
Two hundred inbred 4-week-old ICR (Institute of Cancer Research) mice were obtained from Japan SLC (Shizuoka, Japan). After they had been acclimatized for 1 week, they were maintained throughout the study in a specific pathogen-free environment with a temperature of 24 ± 2°C, a humidity of 60 ± 15% and a 12 h lightdark cycle. The mice were housed in aluminum cages, each of which held 10 mice, and they were provided with the pellet diet CE-2 (CLEA Japan, Tokyo, Japan) ad libitum. In Experiment 1, crude phlorotannins were freely available. The mice were provided with the phlorotannins in solution (5000, 2500, 1250, 625 or 0 mg/L in tap water) ad libitum in 200 mL plastic water bottles. In Experiment 2, the crude phlorotannins were administered only once. After intragastric administration of 1 mL of the phlorotannin solution (5000, 2500, 1250, 625 or 0 mg/L in phosphate buffered saline), the mice were allowed free access to food and tap water. Each group comprised 10 male and 10 female mice. Body weights were recorded every 2 or 3 days: the initial weights of the male and female mice were 30.1 ± 1.6 and 25.8 ± 1.4 g (mean ± S.D.), respectively. The consumption of the phlorotannin solution was measured every day in Experiment 1. The experiments continued for 14 days. This study was approved by the Ethics Committee for Animal Experiments, the Chemo-Sero-Therapeutic Research Institute.
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Results |
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The crude phlorotannins showed bactericidal activity against all 35 strains tested: S. aureus (MRSA) (MBCs, 100200 mg/L), S. aureus (MBC, 100 mg/L), S. pyogenes (MBC, 400 mg/L), B. cereus (MBCs, 200400 mg/L), C. fetus (MBC, 50 mg/L), C. jejuni (MBC, 50 mg/L), E. coli (MBCs, 200400 mg/L), S. enteritidis (MBCs, 200800 mg/L), S. typhimurium (MBC, 200 mg/L) and V. parahaemolyticus (MBC, 200 mg/L). Overall, Campylobacter spp. were the most susceptible, followed by S. aureus. There was considerable variation in the MBCs among the different strains of S. enteritidis. Of all the bacteria tested, only two strains of Vibrio were killed within 2 h at twice the MBC. The other bacteria were largely unaffected by this concentration, even at 4 h (data not shown).
Bactericidal activity of purified phlorotannins
The MBCs of five purified phlorotannins (phloroglucinol, eckol, phlorofucofuroeckol A, dieckol and 8,8'-bieckol), catechin and EGCG against six reference strains and the clinical isolate of V. parahaemolyticus were determined (Table 1). For all the polyphenols, the MBCs were lowest for C. jejuni among the bacteria tested. The lowest MBCs against C. jejuni and the other bacteria were 0.03 and 0.13 0.54 µmol/mL of both dieckol and 8,8'-bieckol; 0.08 and 0.331.08 µmol/mL of both eckol and phlorofucofuroeckol A; and 0.03 and 0.441.75 µmol/mL for EGCG, respectively. On the whole, the bactericidal effects of eckol, phlorofucofuroeckol A, dieckol and 8,8'-bieckol were more pronounced than those of the catechins, although EGCG had a similar MBC to both dieckol and 8,8'-bieckol against C. jejuni.
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In Experiment 1, the maximum daily intake of phlorotannins was 1500 mg/kg of initial body weight in males and 1286 mg/kg in females. In Experiment 2, the maximum dose of phlorotannins was 168.2 mg/kg in males and 193.7 mg/kg in females. Survival in all groups at the end of 14 days was 100% (Table 2). Moreover, no harmful effects were observed even with the largest administration of crude phlorotannins, and the rate of weight gain in all groups was no less than that of the controls. No signs or symptoms of disorder were observed in any of the groups, in either experiment.
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Discussion |
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Several studies have found that catechins exhibit stronger antibacterial effects on Gram-positive bacteria than on Gram-negative bacteria.14,15 However, in the present study, we could not find any remarkable difference in susceptibility to phlorotannins between Gram-positive and Gram-negative bacteria. For example, Campylobacter spp., which are Gram-negative, were the most susceptible among the bacteria tested. Moreover, the species specificity of the bactericidal effect of the phlorotannins may be smaller than that of EGCG (Table 1). However, since the sample size (the number and kinds of strains) was small, further experiments may be necessary to confirm these tendencies. Moreover, tests to determine whether or not mutants resistant to the phlorotannins can be generated need to be performed in the future.
Interestingly, the phlorotannins killed V. parahaemolyticus within 0.52 h when administered at twice the MBC (Figure 1). The reason for this is unclear; however, a similar effect of phlorotannins was found against other Vibrio spp., Vibrio vulnificus, Vibrio colerae and Vibrio anguillarum (data not shown).
In this paper, the MBCs of polyphenols are expressed as µmol/mL to allow a comparison of activities per molecule (Table 1). The bactericidal effects of phlorotannins tend to increase with polymerization of phloroglucinol. This tendency is different from the case of tea catechins, whose effects are augmented with the addition of the gallate group.
Schulz et al.16 suggested that the antimicrobial activity of polyphenols may result from their interaction with bacterial enzymes and proteins. Ikigai et al.14 reported that catechins damage bacterial cell membranes. Furthermore, strong interactions between algal phlorotannins and proteins have been reported by Stern et al.17 Although the mode of activity of phlorotannins is still obscure, the interactions of phlorotannins with bacterial proteins may play an important role in the bactericidal action of phlorotannins.
E. kurome as well as Eisenia bicyclis is used as a food product in some areas of Japan. Accordingly, it is of interest to note that no harmful effects were observed on oral administration of a large quantity of phlorotannins in mice, corresponding to a human dose of 90.0 g/60 kg per day in males and 64.3 g/50 kg per day in females, or a single dose of 10.1 g/60 kg in males and 9.7 g/50 kg in females.
The results obtained in the present study suggest that phlorotannins have pronounced bactericidal activity against pathogenic bacteria. Therefore, phlorotannins as well as E. kurome and E. bicyclis may be useful as a food product or as a drug with antibacterial activity.
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Acknowledgements |
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Footnotes |
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References |
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