The present application is a U.S. National Phase Application of International Application No. PCT/IB2010/000139 (filed Jan. 8, 2010) which is hereby incorporated by reference in its entirety.
The present invention is in the field of the methods for selecting food grade bacteria with anti-oxidative properties.
All living subjects maintain a reducing environment within their cells. However, due to the aerobic metabolism by the mitochondria and other factors, reactive oxygen-derived species such as peroxides and free oxygen radicals are produced. The reducing environment is preserved by enzymes such as superoxide dismutase, catalase and glutathion peroxidase. If the normal redox state is disturbed, the reactive oxygen species may damage all components of the cell, including protein, lipids and especially DNA. This imbalance between the production of reactive oxygen species and the ability to detoxify the reactive intermediates or repair the damage caused by the reactive oxygen species is called oxidative stress. In humans, oxidative stress is an important factor in aging and degenerative diseases associated with aging such as cancer, arthritis, diabetes, artherosclerosis, Lou Gehrig's disease, Parkinson's disease, heart failure, Alzheimers's disease, and Huntington's disease. The free-radical theory of aging states that organisms age because cells accumulate damage caused by reactive oxygen species over time.
In order to prevent the adverse effects of oxidative stress, there is a need for screening of dietary components which have anti-oxidative properties. Especially food grade bacteria, particularly lactic acid bacteria, are suitable anti-oxidative dietary components, since their use advantageously results in a long term effect of anti-oxidant action, via colonization of the intestinal tract.
The U.S. Pat. No. 6,884,415 discloses an antioxidant food product produced by fermenting a food product containing Lactobacillus plantarum having a superoxide dismutase (SOD)-like activity and a catalase (CAT) activity, in the presence of a manganese-containing natural material. Nevertheless, it is known that food grade bacteria, including lactic acid bacteria, can have anti-oxidative properties not dependent on the catalase or SOD activity.
The International Application WO 03/002131 discloses a Lactobacillus fermentum strain as anti-oxidative probiotic. The anti-oxidative properties of this strain were characterized in vitro by enzymatic tests and by measuring the glutathion red/ox potential.
The International Application WO 00/20013 discloses a Lactobacillus or Propionibacterium strain giving rise to increased amounts of propionic acid in the gut of a mammal for the manufacture of a medicament for reducing oxidative stress factors such as IL-6, reactive oxygen species and adhesion molecules.
Caenorhabditis elegans (C. elegans) is a free-living, transparent worm (nematode), which lives in temperate soil environments. C. elegans feeds on bacteria, particularly Escherichia coli OP50 strain. It has since been used extensively as a model organism for a variety of reasons. Strains are cheap and easy to breed and can be frozen. When subsequently thawed, they remain viable, allowing long-term storage. They have a short and reproducible life span. C. elegans has the advantage of being a multicellular eukaryotic organism that is simple enough to be studied in great detail. This worm has close to 40% of human orthologous genes among the whole genome, which make it an organism relevant for the human situation.
Caenorhabditis elegans has been used as animal model system for assessing the oxidative damage and effects on aging (Larsen, 1993, PNAS 90:8905-8909). The study has been carried out with a mutant strain having hyper-resistance to oxidative stress compared to its parental strain.
Further, Ikeda et al. (2007, AEM 73:6404-6409) have studied the effect of lactic acid bacteria on life span and Salmonella resistance of C. elegans. The authors suggest that C. elegans can be an appropriate model for screening probiotic bacteria strains (exerting beneficial effects on human health when ingested in sufficient numbers) or dietetic antiaging substances. However, resistance against oxidative stress was not assessed in this study. It is also known that the increased life span for C. elegans is related to the insulin pathway and related to orthologous genes in humans involved in the insulin-like growth factor and diabetes (Glenn et al., 2004, J Gerontol A Biol Sci Med Sci. 59:1251-1260).
The inventors have found that the animal model system Caenorhabditis elegans is a suitable model for screening the ability of food grade bacteria to counteract the damaging effects of oxidative stress. The screening assay can be performed in liquid media in microtiter plates to which bacteria are added, as well as on agar plates with lawns of bacteria as feed.
In particular, the effect of these food grade bacteria on prevention of damage occurring by oxidative stress, particularly in the form of oxidative reactive species, can be tested using C. elegans. A suitable way to impose oxidative stress to C. elegans was found to be the addition of hydrogen peroxide. The screening method of the present invention is relatively simple, yet the results obtained are relevant for the human situation. Finally, the method advantageously allows to select for strains of food grade bacteria with an overall anti-oxidative stress effect, without being restricted to the selection for a specific mechanism involved in an anti-oxidative effect such as the presence of a particular enzyme (e.g., CAT, SOD) or the release of a particular factor, as it is the case in the prior art.
Screening Method using Caenorhabditis elegans
In one embodiment the present invention relates to a method for selecting food grade bacteria with anti-oxidative properties comprising:
a. a step of synchronizing the growth of Caenorhabditis elegans (C. elegans) worms;
b. a step of feeding said C. elegans worms on the food grade bacteria to be tested;
c. a step of incubating the C. elegans worms in the presence of oxidative stress;
d. a step of determining the viability of said C. elegans worms which were incubated in the presence of oxidative stress; and
e. a step of selecting the food grade bacteria which provide the highest survival of said C. elegans in the presence of oxidative stress.
In another embodiment the present invention relates to the use of Caenorhabditis elegans in a method for selecting food grade bacteria with anti-oxidant properties.
The growth of C. elegans is synchronized because the method according to the present invention is advantageously carried out on worms being in the same growth state. Methods to grow and synchronize C. elegans worms are known in the art (In: W. B. Wood (ed) “The nematode Caenorhabditis elegans”. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., pp 587-606; Chen et al., 2008, J. Cell Commun. Signal. 2:81-92). A suitable way to achieve synchronized growth is to harvest eggs from gravid adults and start with hatching the eggs. A suitable way to hatch the eggs is incubating them overnight in M9 medium (10% vol MRS (De Man, Rogosa and Sharpe medium), fluorodexouridine 100 μg/ml) plus 5 μg/ml cholesterol. Subsequently the L1-stage worms can be isolated and grown as known in the art (In: W. B. Wood (ed) “The nematode Caenorhabditis elegans”; above cited). Preferably the worms are grown in the wells of a microtiter plate. Preferably the worms are grown without agitation during three days at 25° C. and at 80-85% relative humidity.
In a preferred embodiment of the method of the present invention, C. elegans mutant strain BA17 fem-1(hc17) (Nelson et al., 1978, Dev. Biol. 66:386-409) is used. This strain has advantageously inhibited fertility at 25° C., thereby making it easier to control its growth and reproduction.
In a preferred embodiment of step b. of the method of the present invention, Escherichia coli (E. coli), preferably E. coli OP50 (which is a normal food source for C. elegans) is used as a control feed.
Instead of control feed the worms can be grown in the presence of the food grade bacteria to be tested.
Preferably at least 50 worms are present per condition tested (presence or absence of oxidative stress), in order to find relevant differences between the different conditions.
When the worms have reached adult stage, preferably after 3 days culture, they can be incubated in the presence of oxidative stress. A suitable way to apply oxidative stress is by addition of hydrogen peroxide, preferably, at a concentration comprised between 1 mM to 20 mM final concentration, more preferably between 2 mM to 10 mM, even more preferably between 2 mM and 5 mM H2O2. 5 mM hydrogen peroxide is an optimal concentration. Preferably, as a control no H2O2 is added.
In a preferred embodiment of step c. of the method of the present invention, C. elegans are incubated in the presence of oxidative stress for 5 minutes to 48 h, more preferably 1 h to 10 h. 5 h is a suitable time for this incubation step.
One way of performing the incubation step in the presence of oxidative stress is in liquid media, for example in the wells of microtiter plates. This method has as advantage that many conditions can be tested simultaneously. Alternatively, the method can be performed on a solid medium, for example agar plates. This method is more laborious and time consuming that the microtiter assay but has as advantage that direct effects of the food grade bacteria on the oxidative stress conferring agent such as hydrogen peroxide, can be excluded.
In an embodiment of step c. of the method of the present invention, C. elegans worms can also be incubated in the absence of oxidative stress as a control. In a preferred embodiment of step d. of the method of the present invention, assessment of anti-oxidant resistance is read out as viability. This can be performed by microscopy. The worms are considered to be dead if they are paralyzed and no motion is observed.
In an embodiment of step d. of the method of the present invention, when there are C. elegans worms which are incubated in the absence of oxidative stress as a control at step c., then the viability of said C. elegans worms which are incubated in the presence of oxidative stress, is compared to the viability of said C. elegans worms which are incubated in the absence of oxidative stress.
The final step e. of the method of the present invention can be made by selecting the food grade bacteria which confer a high survival rate to the C. elegans worms in the presence of oxidative stress.
In a preferred embodiment of said step e., the survival of C. elegans in the absence of oxidative stress is assessed concomitantly and set to 100%.
In another embodiment of said step e., the effect of the food grade bacteria on the survival (or viability) of the C. elegans worms is compared with the effect of the control feed, such as E. coli.
Food Grade Bacteria
Food grade bacteria according to the present invention relate to bacteria selected from the group consisting of bifidobacterium, lactobacillus, lactococcus, streptococcus, pediococcus, leuconostoc, oenococcus, enterococcus, aerococcus, carnobacterium, weisella, propionibacterium, bacillus, sporolactobacillus, corynebacterium and brevibacterium.
Preferably, the food grade bacteria are lactic acid bacteria (LAB). Lactic acid bacteria according to the present invention relate to bacteria selected from the group consisting of bifidobacterium, lactobacillus, lactococcus, streptococcus, pediococcus, leuconostoc, oenococcus, enterococcus, aerococcus, carnobacterium, and weisella. More preferably the food grade bacteria are selected from the group consisting of lactobacillus, streptococcus, lactococcus and bifidobacterium.
The food grade strains tested can be grown as known in the art. By way of example, strains belonging to Bifidobacterium, Lactobacillus and Streptococcus genera are grown in MRS with cysteine, MRS and Elliker media, respectively.
In a preferred embodiment of the method of the present invention, for the microtiter plate assay, the food grade bacteria tested are viable.
In another preferred embodiment of the method of the present invention, the food grade bacteria are precultured and harvested in the logaritmic phase growth.
In another preferred embodiment of the method of the present invention, the cultures of the different food grade bacteria are added to the C. elegans comprising liquid growth medium at a final concentration of 1×105 cells/ml to 1×108 cells/ml, more preferable of 1×106 cells/ml to 1×107 cells/ml. 4×107 cfu/ml is a preferred concentration for an assay in liquid media. Alternatively, when C. elegans is tested on agar plates, the food grade bacteria to be tested can be present in the form of colonies or lawns on the agar plates.
In another preferred embodiment of the method of the present invention, the food grade bacteria are added to the C. elegans growth medium in the presence of an antibiotic which inhibits the further growth of the food grade bacteria. Further, an antibiotic has to be present to prevent further growth of the bacteria during the assay. Preferably, the worms are grown and incubated in the presence of an antibiotic, more preferably kanamycin, even more preferably kanamycin in a concentration of 10 to 100 μg/ml. Advantageously, kanamycin also inhibits the growth of the control feed E. coli. Other suitable antibiotics to inhibit some strains of lactobacilli are vancomycin, neomycine and erythromycin.
Application
The method of the present invention is preferably used to select strains of food grade bacteria which protect against oxidative stress and/or to prevent the damage imposed by oxidative stress. These food grade bacteria can subsequently be used in the manufacture of pharmaceutical compositions, nutritional supplements, and/or food compositions products.
Such compositions are suitable for humans suffering from oxidative stress. Especially the elderly are an appropriate target group, since the aged gut and the immunosenescence is prone to less effective resistance to the oxidative stress and production of ROS.
100 food grade strains belonging to Bifidobacterium, Lactobacillus and Streptococcus genera were tested for their anti-oxidative properties. These genera were grown in MRS with cysteine, MRS and Elliker media respectively. As the bioassay of the in vivo antioxidant activity was carried out with samples of living cells of different lactic acid bacteria, cells were recovered in the logaritmic phase growth. After the analysis of the growth curves, the optimal time for cell recovery was after 15 h of incubation at DO600=1, 1.5 and 1.7 for Streptococcus, Lactobacillus and Bifidobacterium respectively. The cultures of the different lactic acid bacteria obtained as described above were added to the mixture at a final concentration of 4×106 cells/ml.
Subsequently, the sensibility of the 100 bacterial strains to kanamycin, an antibiotic used to avoid Escherichia coli growth, was analyzed. This antibiotic has to be present to prevent further growth of the bacteria during the assay. A concentration of 30 μg/ml kanamycin was found to be sufficient to inhibit E. coli OP50; 20% of the bacterial strains belonging to the genera Bifidobacterium and Lactobacillus were not inhibited by this antibiotic. However, since the bifidobacteria were not able to proliferate under the aerobic conditions, the presence of an antibiotic is not essential. Other suitable antibiotics to inhibit some strains of lactobacilli were vancomycin (250 μg/ml), neomycine (10-35 μg/ml), and erythromycine (1-100 μg/ml).
Experiments have been carried out with the C. elegans mutant strain BA17 fem-1(hc17) which has an inhibited fertility at 25° C. BA17 worms were synchronized by isolating eggs from gravid adults at 20° C., hatching the eggs overnight in M9 medium (10 vol % MRS, fluorodexouridine 110 μg/ml) plus 5 μg/ml cholesterol and isolating L1-stage worms in the wells of a microtiter plate. The worms were grown without agitation during 3 days at 25° C. and 80-85% relative humidity. These larvae were transferred to a plate comprising M9 medium plus cholesterol and incubated for 3 days at 25° C. 80-85% humidity while undergoing control or experimental feeding. At least 50 worm were present per well.
After 3 days, when the worms had reached adult stage, oxidative stress was applied by addition of hydrogen peroxide H2O2 (2 mM, 3 mM and 5 mM) or without H2O2 (no stress control). Two controls have been used during this experiment: wells with Escherichia coli instead of a lactic acid bacterium as the control of bacterial feeding and wells with E. coli and 2 mM, 3 mM or 5 mM H2O2 as the control for oxidative stress. H2O2 at a concentration of 5 mM was found to be optimal. Anti-oxidant resistance was read out as viability, assessed after 5 h by microsopy. Worms were incubated in these conditions during 5 hours. To score for antioxidant capacity the worms were consider to be dead (stressed) if they were paralyzed.
In the absence of oxidative stress during the incubation time with E. coli the viability varied between 100 to about 90%. In an initial test the lactic acid bacteria had similar or better survival rates, which is indicative for a similar or improved longevity. Results for an effect of some selected strains are shown in Table 1 below.
E. coli OP50
The effect of 99 strains of lactic acid bacteria on survival of C. elegans under oxidative stress was tested with 2, 3 and 5 mM H2O2. It was found that 5 mM H2O2 was the best concentration to test for oxidative stress. In the presence of 5 mM H2O2, the viability of the worms in the presence of E. coli OP50 was about 93% compared to the absence of oxidative stress. This is indicative for a 93% protection against oxidative stress for E. coli OP50.
Table 2 below shows the effect of selected lactic acid bacteria on the level protection against oxidative stress, compared to the protective effect exerted by the control E. coli OP50 strain set at 100%.
E. coli OP50
Lactobacilli
Bifidobacteria
Streptococci
It appears from the Table 2 above that, surprisingly, Bifidobacterium strains did not confer resistance to oxidative stress, while they confer a prolonged life span of C. elegans when cultured under anaerobic conditions (Ikeda et al., 2007; cited above). Further, surprisingly, only very few strains of Streptococcus and Lactobacillus were able to confer resistance to oxidative stress at a level higher than that of the control strain. The strains improving viability in the absence of oxidative stress were not necessarily the strains also giving the best protection against oxidative stress. This indicates that the improved effect of lactic acid bacteria on viability is not only caused by an effect on oxidative stress and that only very few, specifically selected strains of Streptococcus and Lactobacillus, have the ability to reduce anti-oxidative stress, compared to the control E. coli OP50.
Wild type C. elegans N2 were grown on nematode growth medium (NG) agar plates for 5 days (to synchronize the worms) with lawns of E. coli OP50 or with lawns of selected strains of lactic acid bacteria from Example 1 conferring a protection against oxidative stress, and incubated with 3 mM H2O2 for 5 h. The viability of the worms was assessed just before and after the 5 h incubation and the percentage of survival under oxidative stress was determined by determining the percentage of worms that died during the incubation time. The results are shown in Table 3.
In the assay with agar plates (instead of wells) specific strains of lactic acid bacteria were shown to exert a protective effect against oxidative stress, but not all strains tested in Example 1 turned out to be effective against oxidative stress. Of the 99 strains 3 lactobacillus strains, 10C, 11D and 3E were effective against oxidative stress.
Of the Streptococcus strains tested (S2B, S1E and S1D) none were able to protect against oxidative stress at a level above E. coli OP50 in the agar plate assay.
It appears from the foregoing that the agar plate method turns out to be more selective than the microtiter plate assay. Since the agar plate assay is more laborious and time consuming than the microtiter plate assay, the agar plate assay can be suitably used when only few food grade strains are tested.
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/IB2010/000139 | 1/8/2010 | WO | 00 | 11/30/2012 |
Publishing Document | Publishing Date | Country | Kind |
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WO2011/083353 | 7/14/2011 | WO | A |
Number | Name | Date | Kind |
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20030190312 | Kenyon et al. | Oct 2003 | A1 |
20080229436 | Reis et al. | Sep 2008 | A1 |
Number | Date | Country |
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03002131 | Jan 2003 | WO |
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20130078187 A1 | Mar 2013 | US |