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Antimicrobial activity of açaí against Listeria innocua
Accepted Manuscript Antimicrobial activity of açaí against Listeria innocua Clara Miracle Belda-Galbis, Antonio Jiménez, María Consuelo Pina-Pérez, Antonio Martínez, Dolores Rodrigo PII:
S0956-7135(15)00033-X
DOI:
10.1016/j.foodcont.2015.01.018
Reference:
JFCO 4251
To appear in:
Food Control
Received Date: 18 September 2014 Revised Date:
19 December 2014
Accepted Date: 3 January 2015
Please cite this article as: Belda-Galbis C.M., Jiménez A., Pina-Pérez M.C., Martínez A. & Rodrigo D., Antimicrobial activity of açaí against Listeria innocua, Food Control (2015), doi: 10.1016/ j.foodcont.2015.01.018. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT Antimicrobial activity of açaí against Listeria innocua
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Clara Miracle Belda-Galbis, Antonio Jiménez, María Consuelo Pina-Pérez, Antonio Martínez,
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Dolores Rodrigo*
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Instituto de Agroquímica y Tecnología de Alimentos (IATA-CSIC), Carrer del Catedràtic
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Agustín Escardino Benlloch 7, 46980, Paterna, València, Spain.
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Corresponding author. Tel.: +34 963 900 022 (ext. 2218). Fax: +34 963 636 301. E-mail
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address: [email protected]
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ACCEPTED MANUSCRIPT Abstract
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A study was carried out to evaluate antimicrobial activity of açaí against Listeria innocua, as a
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non-pathogenic surrogate for Listeria monocytogenes, at different temperatures (37, 22, and 10
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°C), from a kinetic point of view. With this aim, first the Minimum Inhibitory Concentration
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(MIC) under optimal growth conditions was established (37 °C), and then the effect of 3 non-
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inhibitory doses (3, 5, and 7 g/L) at 37, 22, and 10 °C was evaluated on the basis of the kinetic
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parameters lag time (λ) and maximum specific growth rate (µ max). The Total Phenolic Content
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(TPC) of the samples tested as a function of açaí concentration was also determined. Results
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obtained showed that the MIC was 10 g/L, containing 2154.91 ± 126.10 mg of Gallic Acid
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Equivalents (GAE)/L. At non-inhibitory doses, regardless of temperature, the higher the açaí
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concentration, the higher the value of λ, and the effect of a variation in açaí concentration on λ
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was greater at high temperatures. Therefore, the addition of non-inhibitory doses of açaí could
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provide a means of controlling the growth of L. monocytogenes if a cold chain failure occurs, or
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if any other reason compromises the microbiological safety of minimally processed foods.
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Consequently, the present study is important both for the science community and for the food
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industry because it provides the first mathematical characterization of açaí antimicrobial activity
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and reveals its potential use to control the concentration and growth of pathogenic bacteria in
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foods free of non-synthetic additives.
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Keywords: Food preservatives; microbial safety; açaí; phenolic compounds; Listeria innocua;
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mathematical modelling
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Introduction
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Açaí palm (Euterpe oleracea Martius), also known as cabbage palm or palisade pine, is a
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monoecious plant native of tropical regions of northern South America, where açaí has been
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consumed since pre-Columbian times (Alonso 2012). From then until now, the distribution and
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sale of açaí and açaí-based products has increased in North America, Europe, China, and Japan,
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Brazil being the main producer of açaí pulp-based drinks (Alonso 2012). The increasing interest
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in this kind of product is partly due to studies which show that açaí consumption could have
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beneficial effects on consumer health (del Pozo-Insfran et al. 2006; Schauss et al. 2006;
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Mertens-Talcott et al. 2008; Sun et al. 2010; Horiguchi et al. 2011; Udani et al. 2011; de Moura
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et al. 2012; Feio et al. 2012; Bonomo et al. 2014).
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Nowadays, it is well known that açaí contains as much fiber as whole wheat flour or rice bran,
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and a fair amount of heart-healthy fatty acids (Sanabria and Sangronis 2007), in addition to
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flavonoids, lignans, and other polyphenols with an extremely high antioxidant potential.
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According to Schauss et al. (2006), the antioxidant capacity of freeze-dried açaí pulp (1027
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µmol of Trolox Equivalents (TE)/g) is higher than the antioxidant capacity of any other fruit or
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vegetable that has been analyzed, including blueberries (62.20 µmol of TE/g), strawberries
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(35.77 µmol of TE/g), and raspberries (49.25 µmol of TE/g) (Wu et al. 2004). For this reason,
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açaí is considered a “superfruit.”
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Although açaí health benefits and its nutritional composition have been studied in depth, its
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antimicrobial activity has not yet been exploited because, to date, the antimicrobial activity of
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açaí has scarcely been studied (Lian et al. 2012; Melhorança and Pereira 2012; Bonomo et al.
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2014). According to Lian et al. (2012), açaí antimicrobial activity depends on its phenolic
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content. Some exotic tropical fruit extracts have been reported to exert a wide spectrum of
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antimicrobial activity due to phenolic compounds with bacteriostatic and bactericidal properties
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(Kabuki et al. 2000; Esquenazi et al. 2002). These compounds are able to modify membrane
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permeability and to complex with macro- and micronutrients. Consequently, the affect the
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ACCEPTED MANUSCRIPT retention of macromolecules within the cell, the electron transport and the nutrient uptake
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(Cowan 1999; Daglia 2012).
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Until today no standardized methods for determining the antimicrobial activity of any
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compound or mix are described in the literature, but so far no standardized test has been
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developed to evaluate the antibacterial activity of possible preservatives against food-related
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microorganisms, although the need for such a test has been indicated (Burt 2004). Normally,
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researchers adapt experimental methods to provide a better representation of possible future
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applications of antimicrobials in their particular field. In this connection, a count of viable cells
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after incubation of a microorganism in the presence of a supposedly antimicrobial compound or
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mixture makes it possible to characterize the bacteriostatic or bactericidal effect of the
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compound or mixture, and also to quantify its effect in terms of kinetic parameters (maximum
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specific growth rate, µ max, and lag phase duration, λ) that define the behavior of the
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microorganism in the presence of the antimicrobial substance or mixture, and that also permit an
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exposure assessment in a risk assessment system.
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The main goal of this work was to assess the antimicrobial capability of açaí against Listeria
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innocua at different temperatures by means of mathematical modeling of microbial behavior in
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reference media, given that L. innocua is a non-pathogenic surrogate for Listeria
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monocytogenes (Char et al. 2010; Belda-Galbis et al. 2013; Jadhav et al. 2013; Belda-Galbis et
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al. 2014), a psychrotrophic facultative anaerobic pathogen, frequently found in minimally
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processed ready-to-eat foods, that is able to grow in very hostile environments (CCFH 2002;
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FSAI 2005), and that is able to form biofilms on all the materials commonly used in the industry
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(Møretrø and Langsrud 2004; Zhu et al. 2005).
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Material and methods 2.1.
Bacterial culture
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ACCEPTED MANUSCRIPT Vials containing around 9.51 × 109 (± 1.52 × 109) cfu/mL of L. innocua (CECT 910) were
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obtained from a lyophilized pure culture provided by the Spanish Type Culture Collection,
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using the method described by Saucedo-Reyes et al. (2009).
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The average cell concentration of the stock was determined by viable plate count from 4
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samples after incubation at 37 °C for 48 h. Aliquots of samples were serially diluted in 1 g/L of
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buffered peptone water (Scharlau Chemie, SA, Barcelona, Spain), and 100 µL of each dilution
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was spread on Tryptic Soy Agar (TSA; Scharlau Chemie, SA, Barcelona, Spain). 2.2.
Experimental procedure
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A commercial açaí berry extract (Nature’s Way® Products, Inc., Utah, USA) was selected. Its
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antimicrobial activity was assessed at different temperatures (37, 22, and 10 °C) by viable plate
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count. In brief, the bacteria were inoculated in Tryptic Soy Broth (TSB; Scharlau Chemie, SA,
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Barcelona, Spain) at a concentration of ca. 1 × 105 cfu/mL, in the absence and presence of açaí
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at different concentrations. Samples of the culture were taken every 60 min, up to stationary
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phase achievement, diluted in 1 g/L buffered peptone water, and plate counted in TSA after 48 h
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of incubation at 37 °C.
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As a first step, a range of concentrations [2–10 g/L] of açaí was tested at optimal L. innocua
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growth temperature (37 °C) (Rowan and Anderson 1998; FSAI 2005) to determine the
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Minimum Inhibitory Concentration (MIC) and the range of non-inhibitory doses that modify
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bacterial kinetic behavior at this temperature. As a second step, the effect of 3 non-inhibitory
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açaí concentrations (3, 5, and 7 g/L) was analyzed in depth at 37, 22, and 10 °C, following the
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method described previously.
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For all the experiments, 3 separate repetitions were performed for each of the conditions tested,
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with a minimum number of 4 replicates per repetition.
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2.3.
Total phenolic content determination
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according to the Folin–Ciocalteu colorimetric method (Singleton and Rossi 1965). Gallic acid
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calibration standards with concentrations of 0, 0.1, 0.2, 0.3, 0.4, 0.5, 0.6, 0.7, 0.8, and 1 g/L
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were prepared. Three mL of sodium carbonate solution (20 g/L) (Sigma-Aldrich® Co., LLC,
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Missouri, USA) and 100 µL of Folin-Ciocalteu reagent (1:1 (v/v)) (Sigma-Aldrich® Co., LLC,
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Missouri, USA) were added to an aliquot of 100 µL from each gallic acid standard or sample
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tube. The mixture was vortexed and allowed to stand at room temperature, in the dark, for 1 h.
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Absorbance was then measured at 750 nm, using a Lan Optics Model PG1800
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spectrophotometer (Labolan, Navarra, Spain). The results were expressed as mg of Gallic Acid
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Equivalents (GAE) per L. 2.4.
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Modeling of Listeria innocua growth in the presence of non-inhibitory doses of açaí
Growth curves obtained at non-inhibitory açaí concentrations (2, 3, 5, 7, and 8 g/L) were fitted
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to the modified Gompertz model (Gibson et al. 1988) (Eq. (1)), in accordance with previous
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studies by other authors (Koutsoumanis et al. 1998; Valbuena et al. 2008; Gupta et al. 2012;
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Pina-Pérez et al. 2013), modeling the antimicrobial activity of compounds derived from
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vegetable origins.
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logଵሺܰ௧ ሻ = ܣ+ × ܥeିୣ
(1)
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where Nt represents the number of microorganisms at time t (cfu/mL); A the lower asymptote
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value (log10 cfu/mL); C the difference between the curve asymptotes (log10 cfu/mL); B the
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relative growth rate when t = M ((log10 cfu/mL)/h); and M the elapsed time until the maximum
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growth rate is reached (h).
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Fits were performed by nonlinear regression, using the Marquardt algorithm to determine the
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value of the model parameters by minimizing the residual sum of squares (Zwietering et al.
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1990). A, B, C, and M were then used to calculate the lag phase duration (λ; h) and the
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maximum growth rate (µmax; (log10 cfu/mL)/h) reached by L. innocua in each of the scenarios
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studied (Eqs. (2) and (3)) (Gibson et al. 1988; McMeekin et al. 1993).
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ߣ = ܯ− ቀቁ +
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ߤ௫ =
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The goodness of the fits was evaluated by calculating the corrected determination coefficient
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(corrected R2) and the Mean Square Error (MSE) associated with each of them (Saucedo-Reyes
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et al. 2009). The data analysis was performed using Statgraphics® Centurion XV software
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(Statpoint Technologies, Inc., Virginia, USA).
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Results and discussion 3.1.
MIC determination at optimal growth temperature (37 °C)
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L. innocua was inoculated in TSB with different açaí concentrations (0, 2, 3, 5, 7, 8, and 10 g/L)
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to assess açaí MIC at optimum growth temperature (37 °C) (Rowan and Anderson 1998; FSAI
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2005). Figure 1 presents the growth and inactivation curves obtained. Furthermore, Table 1
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shows the N0, Nf, and λ values obtained as a function of açaí concentration. According to these
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results, the concentration of 10 g/L proved to be the MIC for L. innocua growth in TSB at 37
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°C, and it was a bactericidal concentration capable of achieving inactivation of nearly 3 log10
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cycles after 18 h of incubation, and non-detection of viables after 24 h of incubation. Based on
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this value and according to previous works, açaí seems less effective than other antimicrobial
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food additives such as carvacrol or citral. Under similar conditions, the MIC of those
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compounds for L. innocua and L. monocytogenes is lower (≤ 2,22 g/ L) (Kim et al. 1995;
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Veldhuizen et al. 2007; Gutiérrez et al. 2009; Belda-Galbis et al. 2013, 2014), as expected
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taking into account that both are highly pure compounds. Nevertheless, the use of açaí as an
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ACCEPTED MANUSCRIPT antimicrobial preservative could be more convenient considering consumer’s preference for
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high quality fresh (or fresh-like) foods, free from synthetic additives, where açaí could be added
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with no legal restrictions, not only as a preservative but also as a nutritional and functional
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ingredient.
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Taking into account the TPC of the samples tested, which ranged from 363.40 ± 20.07 to
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3221.25 ± 23.80 mg of GAE/L as a function of açaí concentration (Table 2), the TPC of the
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MIC obtained (10 g/L) was 2154.91 ± 126.10 mg of GAE/L. On the basis of this value, the MIC
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obtained is in the range defined by Wen et al. (2003) (1600−2600 mg/L) when they studied the
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antilisterial activity of phenolic acids, such as caffeic and ferulic acid, against various L.
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monocytogenes strains in TSB at 30 °C. In the literature there are studies that show that açaí
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contains not only flavonoids and lignans, but also vanillic acid, syringic acid, p-hydroxybenzoic
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acid, protocatechuic acid, gallic acid, ferulic acid, caffeic acid, chlorogenic acid, p-coumaric
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acid, and ellagic acid (del Pozo-Insfran et al. 2006; Pacheco-Palencia et al. 2008; Rojano et al.
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2011). They could all be responsible for the antimicrobial potential of the açaí extract studied.
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At non-inhibitory doses, L. innocua growth was dependent on açaí concentration. In general
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terms, the higher the açaí concentration, the higher the value of λ. This influence of the
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concentration on λ has also been observed by other researchers evaluating the antimicrobial
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potential of other vegetable products (Ferrer et al. 2009; Pina-Pérez et al. 2012).
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Açaí effect on Listeria innocua growth kinetics
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L. innocua growth curves were obtained at three different temperatures (37, 22, and 10 °C), in
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TSB supplemented with açaí at concentrations below the MIC (3, 5, and 7 g/L) (Figure 2). The
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growth curves obtained were fitted to the modified Gompertz equation with corrected R2 values
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ranging from 0.98 to 0.99 and MSE values ranging from 0.01 to 0.05. From the fits, the kinetic
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parameters λ and µ max were also calculated (Table 3).
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Regardless of the açaí concentration, L. innocua growth in TSB was dependent on incubation
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temperature. Decreasing the temperature in the range studied prolonged λ and reduced µ max. 8
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the effect of temperature on bacterial growth (Gospavic et al. 2008; Pina-Pérez et al. 2012).
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According to the results obtained (Table 3), reducing the temperature from 37 to 10 °C led to a
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10-fold increase in λ and a 6-fold decrease in µ max, in the absence of açaí.
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Regardless of temperature, addition of açaí to the culture broth at the concentrations studied (3,
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5, and 7 g/L) did not affect µ max (Table 3). However, it was observed that the higher the açaí
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concentration, the higher the value of λ. This means that under isothermal conditions the
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presence of açaí could prolong lag phase duration, whereas the maximum growth rate reached in
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log phase would remain unchanged. In particular, incubation in the presence of 7 g/L of açaí
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multiplied λ by 15, 7, and 4 at 37, 22, and 10 °C, respectively. This implies that if a cold chain
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failure occurs (temperatures between 10 and 22 °C) the use of 7 g/L of açaí would increase the
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time without growth up to a maximum of 31 (± 2.24) h.
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The relationship between the natural logarithm of λ (ln λ) and the concentration of açaí (g/L) as
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a function of temperature is presented in Figure 3. As can be seen in this figure, there is a linear
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relationship between the two variables, with r2 ≥ 0.95. The value of the slope of the curves
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obtained also demonstrates that the effect of varying the açaí concentration on the value of λ is
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greater at high temperatures; açaí proved to be more effective at 37 °C than at 22 and 10 °C.
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Perhaps temperature alters the antimicrobial potential of açaí, although it is also possible that L.
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innocua may be more sensitive to changes in concentration when it is incubated at optimum
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growth temperature. When bacteria grow at low temperatures, they alter the composition of
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their membranes to increase their cold tolerance; these changes might also increase their
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resistance to açaí, (i) because it has been shown that adaptation to a particular stress can
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generate resistance to other stresses (Wesche et al. 2009), and especially (ii) because
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polyphenols are antimicrobials that act on the membrane (Cowan 1999; Daglia 2012).
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Conclusion
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safety during shelf life. The use of preservatives with antimicrobial properties can avoid the
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proliferation of spoilage and/or pathogenic microorganisms after processing if a cold chain
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failure occurs, or if any other situation promotes or facilitates microbial growth during storage.
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In this context, the present study provides the first mathematical characterization and
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quantification of the effect of açaí concentration on survival and growth of L. innocua, as a non-
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pathogenic surrogate for L. monocytogenes, in the presence of various açaí concentrations [3–7
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g/L], at various temperatures [37–10 °C].
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The results obtained show that at 37 °C açaí can control or inhibit growth of L. innocua,
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depending on the concentration. In this case, 10 g/L was the MIC and was also a concentration
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capable of inactivating almost 3 log cycles after 18 h of incubation, and of producing non-
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detection of viables after 24 h of incubation in the presence of açaí. Moreover, at lower doses it
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was observed that açaí was capable of slowing bacterial growth and prolonging the latent phase
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to a maximum value of 31.01 (± 2.24) h in the presence of 7 g/L of açaí at 10 °C.
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Consequently, açaí could be included in the formulation of minimally processed foods, not only
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for its nutritional quality but also for its preservative potential, taking into account that it could
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be an effective additional control measure to ensure microbiological safety, even at slightly
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abusive refrigeration temperatures (10 °C).
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Acknowledgments
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Clara Miracle Belda-Galbis holds a JAE-Predoctoral fellowship granted by CSIC in 2010. This
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study was carried out with FEDER funds and with funds from the Interministerial Commission
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for Science and Innovation projects AGL2010-22206-C02-01 ALI and AGL2013-48993-C2-2-
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R.
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Alonso, J. R. (2012). El fruto de asaí (Euterpe oleracea) como antioxidante. Revista de
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Melhorança, A. L., & Pereira, M. R. R. (2012). Atividade antimicrobiana de óleos extraídos de
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açaí e de pupunha sobre o desenvolvimento de Pseudomonas aeruginosa e
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Staphylococcus aureus. Bioscience Journal, 28(4), 598-603.
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Mertens-Talcott, S. U., Rios, J., Jilma-Stohlawetz, P., Pacheco-Palencia, L. A., Meibohm, B.,
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Talcott, S. T., et al. (2008). Pharmacokinetics of anthocyanins and antioxidant effects
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Møretrø, T., & Langsrud, S. (2004). Listeria monocytogenes: Biofilm formation and persistence in food-processing environments. Biofilms, 1(02), 107-121. Pacheco-Palencia, L. A., Mertens-Talcott, S., & Talcott, S. T. (2008). Chemical Composition,
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antioxidant properties, and thermal stability of a phytochemical enriched oil from açai
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Pina-Pérez, M. C., Martínez-López, A., & Rodrigo, D. (2012). Cinnamon antimicrobial effect
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against Salmonella Typhimurium cells treated by pulsed electric fields (PEF) in
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pasteurized skim milk beverage. Food Research International, 48(2), 777-783.
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Pina-Pérez, M. C., Rodrigo, D., & Martínez-López, A. (2013). Antimicrobial potential of
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flavoring ingredients against Bacillus cereus in a milk-based beverage. Foodborne
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Pathogens and Disease, 10(11), 969-976.
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Rojano, B. A., Zapata, I. C., Alzate, A. F., Mosquera, A. J., Cortés, F. B., & Gamboa, L. (2011).
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Polifenoles y actividad antioxidante del fruto liofilizado de palma naidi (açai
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colombiano) (Euterpe oleracea Mart.). Revista Facultad Nacional de Agronomía,
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64(2), 6213-6220.
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Rowan, N. J., & Anderson, J. G. (1998). Effects of above-optimum growth temperature and cell
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morphology on thermotolerance of Listeria monocytogenes cells suspended in bovine
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milk. Applied and Environmental Microbiology, 64(6), 2065-2071.
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Sanabria, N., & Sangronis, E. (2007). Caracterización del acai or manaca (Euterpe oleracea
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Mart.): Un fruto del Amazonas. Archivos Latinoamericanos de Nutricion, 57(1), 94-98.
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Saucedo-Reyes, D., Marco-Celdrán, A., Pina-Pérez, M. C., Rodrigo, D., & Martínez-López, A.
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(2009). Modeling survival of high hydrostatic pressure treated stationary- and
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exponential-phase Listeria innocua cells. Innovative Food Science & Emerging
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Technologies, 10(2), 135-141.
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Schauss, A. G., Wu, X., Prior, R. L., Ou, B., Huang, D., Owens, J., et al. (2006). Antioxidant
342
capacity and other bioactivities of the freeze-dried amazonian palm berry, Euterpe
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oleraceae Mart. (Acai). Journal of Agricultural and Food Chemistry, 54(22), 8604-
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8610. Singleton, V. L., & Rossi, J. A. (1965). Colorimetry of total phenolics with phosphomolybdic-
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phosphotungstic acid reagents. American Journal of Enology and Viticulture, 16(3),
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144-158.
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Sun, X., Seeberger, J., Alberico, T., Wang, C., Wheeler, C. T., Schauss, A. G., et al. (2010).
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Açai palm fruit (Euterpe oleracea Mart.) pulp improves survival of flies on a high fat
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diet. Experimental Gerontology, 45(3), 243-251.
Udani, J. K., Singh, B. B., Singh, V. J., & Barrett, M. L. (2011). Effects of açai (Euterpe
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oleracea Mart.) berry preparation on metabolic parameters in a healthy overweight
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population: A pilot study. Nutrition Journal, 10.
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Valbuena, E., Barreiro, J., Sánchez, E., Castro, G., Kutchinskaya, V., & Brinez, W. (2008).
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Growth prediction of Lactococcus lactis subsp. lactis in sterile skimed milk as a
356
function of temperature. Revista Científica, 18(6), 745-758.
Veldhuizen, E. J. A., Creutzberg, T. O., Burt, S. A., & Haagsman, H. P. (2007). Low
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temperature and binding to food components inhibit the antibacterial activity of
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carvacrol against Listeria monocytogenes in steak tartare. Journal of Food Protection,
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70(9), 2127-2132.
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Wen, A. M., Delaquis, P., Stanich, K., & Toivonen, P. (2003). Antilisterial activity of selected phenolic acids. Food Microbiology, 20(3), 305-311.
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Wesche, A. M., Gurtler, J. B., Marks, B. P., & Ryser, E. T. (2009). Stress, sublethal injury,
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resuscitation, and virulence of bacterial foodborne pathogens. Journal of Food
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Protection, 72(5), 1121-1138.
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Wu, X. L., Beecher, G. R., Holden, J. M., Haytowitz, D. B., Gebhardt, S. E., & Prior, R. L.
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(2004). Lipophilic and hydrophilic antioxidant capacities of common foods in the
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United States. Journal of Agricultural and Food Chemistry, 52(12), 4026-4037.
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Zhu, M., Du, M., Cordray, J., & Ahn, D. U. (2005). Control of Listeria monocytogenes
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contamination in ready-to-eat meat products. Comprehensive Reviews in Food Science
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and Food Safety, 4(2), 34-42.
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Zwietering, M. H., Jongenburger, I., Rombouts, F. M., & van't Riet, K. (1990). Modeling of the bacterial growth curve. Applied and Environmental Microbiology, 56(6), 1875-1881.
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Fig. 1. Listeria innocua growth and inactivation in the presence of açaí (g/L).
377
Fig. 2. Listeria innocua growth curves according to açaí concentration (g/L) at different
378
temperatures. The Gompertz model is presented fitting experimental data points.
379
Fig. 3. Relationship between the natural logarithm of lag time (ln λ) and the concentration of
380
açaí (g/L) at the temperatures studied.
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ACCEPTED MANUSCRIPT Table 1. Listeria innocua initial concentration (N0), final concentration (Nf) and lag phase
Açaí (g/L)
N0 (log10 cfu/mL)
Nf (log10 cfu/mL)
λ (h)
0
5.62 ± 0.06
9.38 ± 0.04a
00.83 ± 0.08
2
5.65 ± 0.05
9.13 ± 0.01
a
01.20 ± 0.04
2
5.64 ± 0.02
9.26 ± 0.11a
02.34 ± 0.24
5
5.57 ± 0.06
9.16 ± 0.04a
5.54 ± 0.01
9.22 ± 0.04
a a
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duration (λ), at 37 °C, as a function of açaí concentration.
7
5.54 ± 0.01
9.24 ± 0.03
10
5.61 ± 0.06
2.78 ± 0.06b
12.35 ± 0.23 11.20 ± 0.17 11,20 -0,17
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Value obtained after 24 h of incubation; b Value obtained after 18 h of incubation
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05.35 ± 0.68
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2
363.40 ± 20.07
3
726.80 ± 63.20
5
1209.21 ± 101.30
7
1533.60 ± 120.30
8
1623.00 ± 136.32
10
2154.91 ± 126.10
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TPC (mg of GAEa/L)
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Gallic Acid Equivalents
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Açaí (g/L)
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Tabla 3. Lag time (λ) and maximum growth rate (µmax) reached by Listeria innocua according to incubation conditions. λ (h) 37 °C
22 °C
10 °C
0
00.82 ± 0.07
02.12 ± 0.59
08.12 ± 1.37
3
02.35 ± 0.22
06.01 ± 0.81
16.86 ± 3.34
5
05.35 ± 0.71
10.57 ± 0.21
30.38 ± 0.76
7
12.32 ± 0.26
13.99 ± 2.97
31.01 ± 2.24
37 °C
22 °C
10 °C
0.65 ± 0.03
0.30 ± 0.00
0.11 ± 0.01
0.51 ± 0.03
0.24 ± 0.03
0.18 ± 0.03
0.53 ± 0.03
0.25 ± 0.03
0.11 ± 0.03
0.47 ± 0.03
0.30 ± 0.03
0.14 ± 0.03
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(g/L)
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µ max ((log10 cfu/mL)/h)
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2
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2
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1 0 4
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12 t (h)
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0 3
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5
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log10 cfu/mL
9
7
6
37 °C
5 2
4
6
8
10
12 t (h)
14
16
log10 cfu/mL
9
8
7
5
22
2
4
6
8
10
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14 16 t (h)
0 3 5 7
22 °C 18
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22
24
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0
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5 7
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10 °C
5 0
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12
18
24
30
36 42 t (h)
48
54
60
66
72
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4
22 °C 10 °C
3
ln λ
2
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ln λ 37 = 2.18 × açaí + 2.13 (r2 = 0.95)
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ln λ 22 = 2.94 × açaí + 0.79 (r2 = 0.99) ln λ 10 = 4.06 × açaí − 0.30 (r2 = 0.98)
0
0.2
-1
0.4
0.8
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Açaí concentration (g/L)
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ACCEPTED MANUSCRIPT Highlights
►Açaí antimicrobial effect was mathematically assessed, from a kinetic point of view. ►The total phenolic content of samples tested was determined spectrophotometrically. ►Açaí was able to inhibit and slow bacterial growth, in a dose-dependent manner ► At non-
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minimally processed foods for its preservative potential.
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inhibitory doses, increasing açaí concentration increased lag time. ►Açaí could be added to
S0956-7135(15)00033-X
DOI:
10.1016/j.foodcont.2015.01.018
Reference:
JFCO 4251
To appear in:
Food Control
Received Date: 18 September 2014 Revised Date:
19 December 2014
Accepted Date: 3 January 2015
Please cite this article as: Belda-Galbis C.M., Jiménez A., Pina-Pérez M.C., Martínez A. & Rodrigo D., Antimicrobial activity of açaí against Listeria innocua, Food Control (2015), doi: 10.1016/ j.foodcont.2015.01.018. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT Antimicrobial activity of açaí against Listeria innocua
1 2 3
Clara Miracle Belda-Galbis, Antonio Jiménez, María Consuelo Pina-Pérez, Antonio Martínez,
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Dolores Rodrigo*
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Instituto de Agroquímica y Tecnología de Alimentos (IATA-CSIC), Carrer del Catedràtic
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Agustín Escardino Benlloch 7, 46980, Paterna, València, Spain.
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Corresponding author. Tel.: +34 963 900 022 (ext. 2218). Fax: +34 963 636 301. E-mail
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*
address: [email protected]
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ACCEPTED MANUSCRIPT Abstract
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A study was carried out to evaluate antimicrobial activity of açaí against Listeria innocua, as a
15
non-pathogenic surrogate for Listeria monocytogenes, at different temperatures (37, 22, and 10
16
°C), from a kinetic point of view. With this aim, first the Minimum Inhibitory Concentration
17
(MIC) under optimal growth conditions was established (37 °C), and then the effect of 3 non-
18
inhibitory doses (3, 5, and 7 g/L) at 37, 22, and 10 °C was evaluated on the basis of the kinetic
19
parameters lag time (λ) and maximum specific growth rate (µ max). The Total Phenolic Content
20
(TPC) of the samples tested as a function of açaí concentration was also determined. Results
21
obtained showed that the MIC was 10 g/L, containing 2154.91 ± 126.10 mg of Gallic Acid
22
Equivalents (GAE)/L. At non-inhibitory doses, regardless of temperature, the higher the açaí
23
concentration, the higher the value of λ, and the effect of a variation in açaí concentration on λ
24
was greater at high temperatures. Therefore, the addition of non-inhibitory doses of açaí could
25
provide a means of controlling the growth of L. monocytogenes if a cold chain failure occurs, or
26
if any other reason compromises the microbiological safety of minimally processed foods.
27
Consequently, the present study is important both for the science community and for the food
28
industry because it provides the first mathematical characterization of açaí antimicrobial activity
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and reveals its potential use to control the concentration and growth of pathogenic bacteria in
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foods free of non-synthetic additives.
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Keywords: Food preservatives; microbial safety; açaí; phenolic compounds; Listeria innocua;
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mathematical modelling
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Introduction
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Açaí palm (Euterpe oleracea Martius), also known as cabbage palm or palisade pine, is a
36
monoecious plant native of tropical regions of northern South America, where açaí has been
37
consumed since pre-Columbian times (Alonso 2012). From then until now, the distribution and
38
sale of açaí and açaí-based products has increased in North America, Europe, China, and Japan,
39
Brazil being the main producer of açaí pulp-based drinks (Alonso 2012). The increasing interest
40
in this kind of product is partly due to studies which show that açaí consumption could have
41
beneficial effects on consumer health (del Pozo-Insfran et al. 2006; Schauss et al. 2006;
42
Mertens-Talcott et al. 2008; Sun et al. 2010; Horiguchi et al. 2011; Udani et al. 2011; de Moura
43
et al. 2012; Feio et al. 2012; Bonomo et al. 2014).
44
Nowadays, it is well known that açaí contains as much fiber as whole wheat flour or rice bran,
45
and a fair amount of heart-healthy fatty acids (Sanabria and Sangronis 2007), in addition to
46
flavonoids, lignans, and other polyphenols with an extremely high antioxidant potential.
47
According to Schauss et al. (2006), the antioxidant capacity of freeze-dried açaí pulp (1027
48
µmol of Trolox Equivalents (TE)/g) is higher than the antioxidant capacity of any other fruit or
49
vegetable that has been analyzed, including blueberries (62.20 µmol of TE/g), strawberries
50
(35.77 µmol of TE/g), and raspberries (49.25 µmol of TE/g) (Wu et al. 2004). For this reason,
51
açaí is considered a “superfruit.”
52
Although açaí health benefits and its nutritional composition have been studied in depth, its
53
antimicrobial activity has not yet been exploited because, to date, the antimicrobial activity of
54
açaí has scarcely been studied (Lian et al. 2012; Melhorança and Pereira 2012; Bonomo et al.
55
2014). According to Lian et al. (2012), açaí antimicrobial activity depends on its phenolic
56
content. Some exotic tropical fruit extracts have been reported to exert a wide spectrum of
57
antimicrobial activity due to phenolic compounds with bacteriostatic and bactericidal properties
58
(Kabuki et al. 2000; Esquenazi et al. 2002). These compounds are able to modify membrane
59
permeability and to complex with macro- and micronutrients. Consequently, the affect the
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ACCEPTED MANUSCRIPT retention of macromolecules within the cell, the electron transport and the nutrient uptake
61
(Cowan 1999; Daglia 2012).
62
Until today no standardized methods for determining the antimicrobial activity of any
63
compound or mix are described in the literature, but so far no standardized test has been
64
developed to evaluate the antibacterial activity of possible preservatives against food-related
65
microorganisms, although the need for such a test has been indicated (Burt 2004). Normally,
66
researchers adapt experimental methods to provide a better representation of possible future
67
applications of antimicrobials in their particular field. In this connection, a count of viable cells
68
after incubation of a microorganism in the presence of a supposedly antimicrobial compound or
69
mixture makes it possible to characterize the bacteriostatic or bactericidal effect of the
70
compound or mixture, and also to quantify its effect in terms of kinetic parameters (maximum
71
specific growth rate, µ max, and lag phase duration, λ) that define the behavior of the
72
microorganism in the presence of the antimicrobial substance or mixture, and that also permit an
73
exposure assessment in a risk assessment system.
74
The main goal of this work was to assess the antimicrobial capability of açaí against Listeria
75
innocua at different temperatures by means of mathematical modeling of microbial behavior in
76
reference media, given that L. innocua is a non-pathogenic surrogate for Listeria
77
monocytogenes (Char et al. 2010; Belda-Galbis et al. 2013; Jadhav et al. 2013; Belda-Galbis et
78
al. 2014), a psychrotrophic facultative anaerobic pathogen, frequently found in minimally
79
processed ready-to-eat foods, that is able to grow in very hostile environments (CCFH 2002;
80
FSAI 2005), and that is able to form biofilms on all the materials commonly used in the industry
81
(Møretrø and Langsrud 2004; Zhu et al. 2005).
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2.
Material and methods 2.1.
Bacterial culture
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86
obtained from a lyophilized pure culture provided by the Spanish Type Culture Collection,
87
using the method described by Saucedo-Reyes et al. (2009).
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The average cell concentration of the stock was determined by viable plate count from 4
89
samples after incubation at 37 °C for 48 h. Aliquots of samples were serially diluted in 1 g/L of
90
buffered peptone water (Scharlau Chemie, SA, Barcelona, Spain), and 100 µL of each dilution
91
was spread on Tryptic Soy Agar (TSA; Scharlau Chemie, SA, Barcelona, Spain). 2.2.
Experimental procedure
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A commercial açaí berry extract (Nature’s Way® Products, Inc., Utah, USA) was selected. Its
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antimicrobial activity was assessed at different temperatures (37, 22, and 10 °C) by viable plate
95
count. In brief, the bacteria were inoculated in Tryptic Soy Broth (TSB; Scharlau Chemie, SA,
96
Barcelona, Spain) at a concentration of ca. 1 × 105 cfu/mL, in the absence and presence of açaí
97
at different concentrations. Samples of the culture were taken every 60 min, up to stationary
98
phase achievement, diluted in 1 g/L buffered peptone water, and plate counted in TSA after 48 h
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of incubation at 37 °C.
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As a first step, a range of concentrations [2–10 g/L] of açaí was tested at optimal L. innocua
101
growth temperature (37 °C) (Rowan and Anderson 1998; FSAI 2005) to determine the
102
Minimum Inhibitory Concentration (MIC) and the range of non-inhibitory doses that modify
103
bacterial kinetic behavior at this temperature. As a second step, the effect of 3 non-inhibitory
104
açaí concentrations (3, 5, and 7 g/L) was analyzed in depth at 37, 22, and 10 °C, following the
105
method described previously.
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For all the experiments, 3 separate repetitions were performed for each of the conditions tested,
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with a minimum number of 4 replicates per repetition.
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2.3.
Total phenolic content determination
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according to the Folin–Ciocalteu colorimetric method (Singleton and Rossi 1965). Gallic acid
111
calibration standards with concentrations of 0, 0.1, 0.2, 0.3, 0.4, 0.5, 0.6, 0.7, 0.8, and 1 g/L
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were prepared. Three mL of sodium carbonate solution (20 g/L) (Sigma-Aldrich® Co., LLC,
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Missouri, USA) and 100 µL of Folin-Ciocalteu reagent (1:1 (v/v)) (Sigma-Aldrich® Co., LLC,
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Missouri, USA) were added to an aliquot of 100 µL from each gallic acid standard or sample
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tube. The mixture was vortexed and allowed to stand at room temperature, in the dark, for 1 h.
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Absorbance was then measured at 750 nm, using a Lan Optics Model PG1800
117
spectrophotometer (Labolan, Navarra, Spain). The results were expressed as mg of Gallic Acid
118
Equivalents (GAE) per L. 2.4.
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Modeling of Listeria innocua growth in the presence of non-inhibitory doses of açaí
Growth curves obtained at non-inhibitory açaí concentrations (2, 3, 5, 7, and 8 g/L) were fitted
121
to the modified Gompertz model (Gibson et al. 1988) (Eq. (1)), in accordance with previous
122
studies by other authors (Koutsoumanis et al. 1998; Valbuena et al. 2008; Gupta et al. 2012;
123
Pina-Pérez et al. 2013), modeling the antimicrobial activity of compounds derived from
124
vegetable origins.
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logଵሺܰ௧ ሻ = ܣ+ × ܥeିୣ
(1)
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షಳ×ሺషಾሻ
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where Nt represents the number of microorganisms at time t (cfu/mL); A the lower asymptote
128
value (log10 cfu/mL); C the difference between the curve asymptotes (log10 cfu/mL); B the
129
relative growth rate when t = M ((log10 cfu/mL)/h); and M the elapsed time until the maximum
130
growth rate is reached (h).
131
Fits were performed by nonlinear regression, using the Marquardt algorithm to determine the
132
value of the model parameters by minimizing the residual sum of squares (Zwietering et al.
133
1990). A, B, C, and M were then used to calculate the lag phase duration (λ; h) and the
6
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maximum growth rate (µmax; (log10 cfu/mL)/h) reached by L. innocua in each of the scenarios
135
studied (Eqs. (2) and (3)) (Gibson et al. 1988; McMeekin et al. 1993).
136
ߣ = ܯ− ቀቁ +
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ߤ௫ =
ଵ
୪୭భబ ேబ ି ఓೌೣ
(2)
× ୣ
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(3)
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The goodness of the fits was evaluated by calculating the corrected determination coefficient
140
(corrected R2) and the Mean Square Error (MSE) associated with each of them (Saucedo-Reyes
141
et al. 2009). The data analysis was performed using Statgraphics® Centurion XV software
142
(Statpoint Technologies, Inc., Virginia, USA).
143
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3.
Results and discussion 3.1.
MIC determination at optimal growth temperature (37 °C)
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L. innocua was inoculated in TSB with different açaí concentrations (0, 2, 3, 5, 7, 8, and 10 g/L)
147
to assess açaí MIC at optimum growth temperature (37 °C) (Rowan and Anderson 1998; FSAI
148
2005). Figure 1 presents the growth and inactivation curves obtained. Furthermore, Table 1
149
shows the N0, Nf, and λ values obtained as a function of açaí concentration. According to these
150
results, the concentration of 10 g/L proved to be the MIC for L. innocua growth in TSB at 37
151
°C, and it was a bactericidal concentration capable of achieving inactivation of nearly 3 log10
152
cycles after 18 h of incubation, and non-detection of viables after 24 h of incubation. Based on
153
this value and according to previous works, açaí seems less effective than other antimicrobial
154
food additives such as carvacrol or citral. Under similar conditions, the MIC of those
155
compounds for L. innocua and L. monocytogenes is lower (≤ 2,22 g/ L) (Kim et al. 1995;
156
Veldhuizen et al. 2007; Gutiérrez et al. 2009; Belda-Galbis et al. 2013, 2014), as expected
157
taking into account that both are highly pure compounds. Nevertheless, the use of açaí as an
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high quality fresh (or fresh-like) foods, free from synthetic additives, where açaí could be added
160
with no legal restrictions, not only as a preservative but also as a nutritional and functional
161
ingredient.
162
Taking into account the TPC of the samples tested, which ranged from 363.40 ± 20.07 to
163
3221.25 ± 23.80 mg of GAE/L as a function of açaí concentration (Table 2), the TPC of the
164
MIC obtained (10 g/L) was 2154.91 ± 126.10 mg of GAE/L. On the basis of this value, the MIC
165
obtained is in the range defined by Wen et al. (2003) (1600−2600 mg/L) when they studied the
166
antilisterial activity of phenolic acids, such as caffeic and ferulic acid, against various L.
167
monocytogenes strains in TSB at 30 °C. In the literature there are studies that show that açaí
168
contains not only flavonoids and lignans, but also vanillic acid, syringic acid, p-hydroxybenzoic
169
acid, protocatechuic acid, gallic acid, ferulic acid, caffeic acid, chlorogenic acid, p-coumaric
170
acid, and ellagic acid (del Pozo-Insfran et al. 2006; Pacheco-Palencia et al. 2008; Rojano et al.
171
2011). They could all be responsible for the antimicrobial potential of the açaí extract studied.
172
At non-inhibitory doses, L. innocua growth was dependent on açaí concentration. In general
173
terms, the higher the açaí concentration, the higher the value of λ. This influence of the
174
concentration on λ has also been observed by other researchers evaluating the antimicrobial
175
potential of other vegetable products (Ferrer et al. 2009; Pina-Pérez et al. 2012).
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Açaí effect on Listeria innocua growth kinetics
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L. innocua growth curves were obtained at three different temperatures (37, 22, and 10 °C), in
178
TSB supplemented with açaí at concentrations below the MIC (3, 5, and 7 g/L) (Figure 2). The
179
growth curves obtained were fitted to the modified Gompertz equation with corrected R2 values
180
ranging from 0.98 to 0.99 and MSE values ranging from 0.01 to 0.05. From the fits, the kinetic
181
parameters λ and µ max were also calculated (Table 3).
182
Regardless of the açaí concentration, L. innocua growth in TSB was dependent on incubation
183
temperature. Decreasing the temperature in the range studied prolonged λ and reduced µ max. 8
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the effect of temperature on bacterial growth (Gospavic et al. 2008; Pina-Pérez et al. 2012).
186
According to the results obtained (Table 3), reducing the temperature from 37 to 10 °C led to a
187
10-fold increase in λ and a 6-fold decrease in µ max, in the absence of açaí.
188
Regardless of temperature, addition of açaí to the culture broth at the concentrations studied (3,
189
5, and 7 g/L) did not affect µ max (Table 3). However, it was observed that the higher the açaí
190
concentration, the higher the value of λ. This means that under isothermal conditions the
191
presence of açaí could prolong lag phase duration, whereas the maximum growth rate reached in
192
log phase would remain unchanged. In particular, incubation in the presence of 7 g/L of açaí
193
multiplied λ by 15, 7, and 4 at 37, 22, and 10 °C, respectively. This implies that if a cold chain
194
failure occurs (temperatures between 10 and 22 °C) the use of 7 g/L of açaí would increase the
195
time without growth up to a maximum of 31 (± 2.24) h.
196
The relationship between the natural logarithm of λ (ln λ) and the concentration of açaí (g/L) as
197
a function of temperature is presented in Figure 3. As can be seen in this figure, there is a linear
198
relationship between the two variables, with r2 ≥ 0.95. The value of the slope of the curves
199
obtained also demonstrates that the effect of varying the açaí concentration on the value of λ is
200
greater at high temperatures; açaí proved to be more effective at 37 °C than at 22 and 10 °C.
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Perhaps temperature alters the antimicrobial potential of açaí, although it is also possible that L.
202
innocua may be more sensitive to changes in concentration when it is incubated at optimum
203
growth temperature. When bacteria grow at low temperatures, they alter the composition of
204
their membranes to increase their cold tolerance; these changes might also increase their
205
resistance to açaí, (i) because it has been shown that adaptation to a particular stress can
206
generate resistance to other stresses (Wesche et al. 2009), and especially (ii) because
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polyphenols are antimicrobials that act on the membrane (Cowan 1999; Daglia 2012).
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4.
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Conclusion
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safety during shelf life. The use of preservatives with antimicrobial properties can avoid the
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proliferation of spoilage and/or pathogenic microorganisms after processing if a cold chain
212
failure occurs, or if any other situation promotes or facilitates microbial growth during storage.
213
In this context, the present study provides the first mathematical characterization and
214
quantification of the effect of açaí concentration on survival and growth of L. innocua, as a non-
215
pathogenic surrogate for L. monocytogenes, in the presence of various açaí concentrations [3–7
216
g/L], at various temperatures [37–10 °C].
217
The results obtained show that at 37 °C açaí can control or inhibit growth of L. innocua,
218
depending on the concentration. In this case, 10 g/L was the MIC and was also a concentration
219
capable of inactivating almost 3 log cycles after 18 h of incubation, and of producing non-
220
detection of viables after 24 h of incubation in the presence of açaí. Moreover, at lower doses it
221
was observed that açaí was capable of slowing bacterial growth and prolonging the latent phase
222
to a maximum value of 31.01 (± 2.24) h in the presence of 7 g/L of açaí at 10 °C.
223
Consequently, açaí could be included in the formulation of minimally processed foods, not only
224
for its nutritional quality but also for its preservative potential, taking into account that it could
225
be an effective additional control measure to ensure microbiological safety, even at slightly
226
abusive refrigeration temperatures (10 °C).
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5.
Acknowledgments
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Clara Miracle Belda-Galbis holds a JAE-Predoctoral fellowship granted by CSIC in 2010. This
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study was carried out with FEDER funds and with funds from the Interministerial Commission
231
for Science and Innovation projects AGL2010-22206-C02-01 ALI and AGL2013-48993-C2-2-
232
R.
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6.
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Alonso, J. R. (2012). El fruto de asaí (Euterpe oleracea) como antioxidante. Revista de
236
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376
Fig. 1. Listeria innocua growth and inactivation in the presence of açaí (g/L).
377
Fig. 2. Listeria innocua growth curves according to açaí concentration (g/L) at different
378
temperatures. The Gompertz model is presented fitting experimental data points.
379
Fig. 3. Relationship between the natural logarithm of lag time (ln λ) and the concentration of
380
açaí (g/L) at the temperatures studied.
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Açaí (g/L)
N0 (log10 cfu/mL)
Nf (log10 cfu/mL)
λ (h)
0
5.62 ± 0.06
9.38 ± 0.04a
00.83 ± 0.08
2
5.65 ± 0.05
9.13 ± 0.01
a
01.20 ± 0.04
2
5.64 ± 0.02
9.26 ± 0.11a
02.34 ± 0.24
5
5.57 ± 0.06
9.16 ± 0.04a
5.54 ± 0.01
9.22 ± 0.04
a a
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duration (λ), at 37 °C, as a function of açaí concentration.
7
5.54 ± 0.01
9.24 ± 0.03
10
5.61 ± 0.06
2.78 ± 0.06b
12.35 ± 0.23 11.20 ± 0.17 11,20 -0,17
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Value obtained after 24 h of incubation; b Value obtained after 18 h of incubation
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05.35 ± 0.68
ACCEPTED MANUSCRIPT Table 2. Total phenolic content (TPC) of the different açaí concentration samples tested in the study.
2
363.40 ± 20.07
3
726.80 ± 63.20
5
1209.21 ± 101.30
7
1533.60 ± 120.30
8
1623.00 ± 136.32
10
2154.91 ± 126.10
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TPC (mg of GAEa/L)
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Gallic Acid Equivalents
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Açaí (g/L)
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Tabla 3. Lag time (λ) and maximum growth rate (µmax) reached by Listeria innocua according to incubation conditions. λ (h) 37 °C
22 °C
10 °C
0
00.82 ± 0.07
02.12 ± 0.59
08.12 ± 1.37
3
02.35 ± 0.22
06.01 ± 0.81
16.86 ± 3.34
5
05.35 ± 0.71
10.57 ± 0.21
30.38 ± 0.76
7
12.32 ± 0.26
13.99 ± 2.97
31.01 ± 2.24
37 °C
22 °C
10 °C
0.65 ± 0.03
0.30 ± 0.00
0.11 ± 0.01
0.51 ± 0.03
0.24 ± 0.03
0.18 ± 0.03
0.53 ± 0.03
0.25 ± 0.03
0.11 ± 0.03
0.47 ± 0.03
0.30 ± 0.03
0.14 ± 0.03
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µ max ((log10 cfu/mL)/h)
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0
6
2
5
3
4
5
3
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8
8
2
10
1 0 4
8
12 t (h)
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ACCEPTED MANUSCRIPT 10
8
0 3
7
5
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log10 cfu/mL
9
7
6
37 °C
5 2
4
6
8
10
12 t (h)
14
16
log10 cfu/mL
9
8
7
5
22
2
4
6
8
10
12
14 16 t (h)
0 3 5 7
22 °C 18
20
22
24
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5 7
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10 °C
5 0
6
12
18
24
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36 42 t (h)
48
54
60
66
72
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4
22 °C 10 °C
3
ln λ
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ln λ 37 = 2.18 × açaí + 2.13 (r2 = 0.95)
1
ln λ 22 = 2.94 × açaí + 0.79 (r2 = 0.99) ln λ 10 = 4.06 × açaí − 0.30 (r2 = 0.98)
0
0.2
-1
0.4
0.8
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ACCEPTED MANUSCRIPT Highlights
►Açaí antimicrobial effect was mathematically assessed, from a kinetic point of view. ►The total phenolic content of samples tested was determined spectrophotometrically. ►Açaí was able to inhibit and slow bacterial growth, in a dose-dependent manner ► At non-
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minimally processed foods for its preservative potential.
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inhibitory doses, increasing açaí concentration increased lag time. ►Açaí could be added to