agents in the actual product. There

agents in the actual product. Therefore, the objectives of the pre- sentstudywere: (a)toevaluate theinvitroantimicrobialactivityof vanillin and geraniol against typical food pathogens; and (b) to apply the selected natural compounds in vivo in strawberry juice inoculated with E. coli O157:H7.
2. Material and methods
2.1. Determination of MIC in vitro of natural compounds
The minimum inhibitory concentration (MIC) is the minimum concentration that produces a 90% reduction in the growth of mi- crobialcolonies.Itisalsodefinedasthelowestconcentrationof the corresponding compound that is able to inhibit visible growth of the microorganism (Hammer, Carson, & Riley, 1996). MIC of the selected natural compounds was determined using the Broth Microdilution Method. Vanillin and geraniol antimicrobial activity was evaluated against two Gram positive bacteria: Listeria monocytogenes pro- vided by CERELA (Centro de Referencia de Lactobacilos, Tucuman, Argentina) and Staphylococcus aureus ATCC 25923; and two Gram negative bacteria: E. coli O157H:7 ATCC 43895 and Pseudomona aeruginosa ATCC 27853. The selected strains were maintained on tryptic soy broth (Britania, Argentina) at 4
C. Before used, they were cultured in Brain Heart Infusion (BHI) (Britania, Argentina) for 24 h at 37
C. Assays were performed by triplicate in sterile 96-well micro- plates using Muller Hilton broth (MH) (Britania, Argentina) with the addition of the selected natural compounds. Vanillin (Sigma Aldrich) was previously dissolved in dimethyl sulfoxide (DMSO) and was used in a concentration range from 0.2 to 4.0 mg/mL. On the other hand, geraniol (Sigma Aldrich) was previously dissolved in tween 80 (Cicarelli, Argentina), and was used in concentrations from 0.2 to 2.4 mL mL 1 Wells were filled with 200 mL of MH plus the corresponding natural compound and inoculated with each bacterial strain at a final bacterial density of 5.105 CFU mL1 (which was achieved by adding 5 mL in each well of a 107 CFU mL1 suspension of the in- dicator strain in MH). The microplates were incubated at 37
C for 24 h. Different controls were used in this study: awell filled with MH with no biopreservative and inoculated with each bacterial strain, inordertoassessthegrowthofthepathogens;andwells filledwith MH plus DMSO and MH plus tween 80, respectively, inoculated with each bacterial strain, in order to prove that neither of the solvents had antimicrobial effects by themselves.
2.2. Juice preparation
Strawberries(Fragaria x ananassa) weregrownandharvestedin
Sierra de los Padres, Mar del Plata, Argentine. The strawberries were destemmed and the juices were prepared with a commercial juice extractor. Once juices were inoculated and the treatments were applied, the strawberry juices were stored in sterile poly- propylene flasks at 5
C for 14 days to assess the evolution of E. coli O157:H7.
2.3. Inoculation with E. coli O157:H7
2.3.1. Culture maintenance and inoculum preparation E. coli O157:H7, ATCC 43895 was used. A stock culture was maintained in tryptic soy broth (Britania, Buenos Aires, Argentina) at 4
C. Before use, E. coli O157:H7 was cultured in brain heart infusion (BHI) broth (Britania) for 24 h at 37
C. A 0.1 mL aliquot of the culture was transferred to 9.9 mL of BHI broth at two consec- utive 24 h intervals followed by incubation at 37
C before each experiment. A bacterial suspension was prepared by adding 10 mL oftheE.colicultureto90mLofsterilepeptonatedwater(0.1%w/v).
2.3.2. Inoculation of the samples Samples were inoculated with E. coli O157:H7 before the application of the treatments, simulating an inadequate manipu- lationof thestrawberriesatpostharvest.Tocarrythisout,100 mLof the bacterial suspension previously prepared were added to 10 mL of fresh strawberry juice to reach a final pathogen concentration of ~5 log colony-forming units (CFU) mL1. Control samples were untreated strawberry juice inoculated with E. coli. After being treated, the strawberry juices were stored in refrigerated chambers at 5
C for 14 days.
2.4. Application of biopreservatives to inoculated strawberry juice
Once the MIC in vitro was determined, in order to evaluate the antimicrobial effects of vanillin and geraniol in vivo, the natural antimicrobial agents were applied directly to the strawberry juice attwodifferentconcentrationsforeachnaturalcompound:1and2 MIC (Van1MIC and Van2MIC for vanillin, and Ger1MIC and Ger2- MIC for geraniol, respectively). A juice with no treatment (untreated) was used as control sample.
2.5. Microbiological analysis
ViableE.colicountsweremonitoredasfollows:0.1mLaliquotof each sample were spread on the surface of eosin methylene blue (EMB)agarplatesandthecolonieswerecountedafterincubationat 37
C for 24e48 h. EMB is a selective medium that allows the characterization of typical E. coli colonies; those that were dark centered, flat and with a metallic sheen were taken into account. Randomly, selected E. coli colonies were confirmed using an E. coli chromogenic test kit (Chromobrit, Britania). All culture media used were purchased from Britania. Microbial counts were expressed as log CFU mL1.
2.6. Statistical analysis
A completely randomized design was used. Three independent runswereperformed.DataobtainedwasanalyzedusingRv.2.12.2. (R Development Core Team, 2011). Results reported in this article are mean values accompanied by their standard errors (Kuehl, 2001). Analysis of variance ANOVA was performed and TukeyeK- ramer comparison test was used to estimate significant differences between treatments (p < 0.05).
Fig. 1. Chemical structures of (a) vanillin and (b) geraniol.