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Inulin increases Bifidobacterium animalis Bb-12 in vitro gastrointestinal resistance in margarine
Accepted Manuscript Inulin increases Bifidobacterium animalis Bb-12 in vitro gastrointestinal resistance in margarine Cínthia Hoch Batista de Souza, Luiz Antonio Gioielli, Susana Marta Isay Saad PII:
S0023-6438(17)30032-4
DOI:
10.1016/j.lwt.2017.01.032
Reference:
YFSTL 5984
To appear in:
LWT - Food Science and Technology
Received Date: 20 July 2016 Revised Date:
6 January 2017
Accepted Date: 12 January 2017
Please cite this article as: de Souza, C.H.B., Gioielli, L.A., Saad, S.M.I., Inulin increases Bifidobacterium animalis Bb-12 in vitro gastrointestinal resistance in margarine, LWT - Food Science and Technology (2017), doi: 10.1016/j.lwt.2017.01.032. 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.
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Inulin increases Bifidobacterium animalis Bb-12 in vitro gastrointestinal resistance in
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margarine
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6 Cínthia Hoch Batista de Souza a,1, Luiz Antonio Gioielli a, Susana Marta Isay Saad a,*
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a
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Universidade de São Paulo. Av. Prof. Lineu Prestes, 580, 05508-000 - São Paulo, SP, Brazil.
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Rua Marselha, 591, 86041-140 - Londrina, PR, Brazil.
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Departamento de Tecnologia Bioquímico-Farmacêutica, Faculdade de Ciências Farmacêuticas,
Present address: Mestrado em Ciência e Tecnologia de Leite e Derivados, Universidade Norte do Paraná.
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*
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Tel: +55-11-30912378; Fax: +55-11-38156386
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E-mail address: [email protected] (S.M.I. Saad)
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Corresponding author:
Shortened running title: In vitro GI resistance of Bifidobacterium Bb-12 in margarine.
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Abstract
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This study aimed to investigate the effect of inulin, whey protein concentrate (WPC), and/or
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caseinomacropeptide (CMP), in different proportions up to 3%, on the viability and resistance to simulated
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gastric and enteric conditions of Bifidobacterium animalis Bb-12 added in probiotic and synbiotic margarine,
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during 35 days of storage at 5°C. Supplementation was important, since the control margarine presented very
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low Bb-12 populations. Inulin at 3% resulted in higher Bb-12 counts (8 log cfu g-1). CMP contributed for
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higher Bb-12 counts, compared to WPC. Inulin increased Bb-12 in vitro survival significantly after 6h
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(P<0.05). In margarines with WPC at 3%, Bb-12 populations decreased drastically during the in vitro assays
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for all storage periods. For the other formulations, Bb-12 populations decreased 2 log cfu g-1 after 2h. Taken
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together, results on viability of B. animalis Bb-12 and on in vitro GI resistance of the strain incorporated in
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margarine produced with inulin were unique, but the addition of inulin was necessary.
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Keywords: Synbiotic; Probiotic; Prebiotic; Spread; Gastrointestinal resistance.
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1. Introduction
Probiotics are “live microorganisms that, when administered in adequate amounts, confer a health
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benefit on the host” (Hill, Guarner, Reid, Gibson, Merenstein, & Pot, 2014). One of the well-investigated
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probiotics is Bifidobacterium animalis subsp. lactis Bb-12, with demonstrated efficacy through clinical trials
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(Haschke et al., 1998). In order to exert their functional properties, probiotics need to be delivered to human
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intestine in an active and viable form (Vandenplas, Huys, & Daube, 2015). Therefore, it is important to
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develop probiotic food with suitable probiotic populations throughout shelf life and that are ingested as part
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of a normal diet for maintaining a regular probiotic intake. Nevertheless, ingested microorganisms are
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exposed to several stress factors that influence their viability through the human gastrointestinal tract (GIT).
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Among these factors, probiotics must tolerate the stomach acidic environment and also the reduced water activity and the presence of bile in the upper small intestine (Vandenplas, Huys, & Daube, 2015). Once probiotic bacteria must preserve viability and arrive at high populations in the colon after
surviving the food processing steps and the digestive process, a careful selection of the food matrix is an
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important factor that should be considered in developing a probiotic product. The food matrix is considered
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as one of the major factors in regulating colonization of microorganisms in the GIT. Food helps to buffer the
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bacteria through the stomach and may contain other functional ingredients that could interact with probiotics
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to alter their functionality. Fat content, concentration and type of proteins, sugars, and pH of foods are some
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factors that could affect probiotic growth and survival in food products (Ranadheera, Baines, & Adams,
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2010). These features might help probiotic survival during passage through the GIT, where survival is
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dependent on both the strain and the food matrix involved. Likewise, the supplementation of food with some
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ingredients like the prebiotic fibre inulin and milk proteins may stimulate probiotic bifidobacteria growth and
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also protect them during GIT passage (Janer, Peláez, & Requena, 2004; Kos, Šušković, Goreta, & Matošić,
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2000).
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Limitations of dairy products such as the presence of allergens and the requirement for cold storage
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facilities, as well as an increasing demand for new foods and tastes have initiated a trend in non-dairy
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probiotic product development (Martins, Ramos, Vanzela, Stringheta, Pinto, & Martins, 2013; Rößle, Auty,
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Brunton, Gormley, & Butler, 2010; Tripathi & Giri, 2014). Among these new food matrices, margarine has
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excellent perspectives as a matrix for probiotic incorporation. Margarine has several advantages over
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yoghurt-type products in terms of delivery of viable probiotics, including its higher pH. Moreover, desirable
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characteristics for probiotic foods as higher fat content and more solid consistency (Ong, Henriksson, &
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Shah, 2006) are observed in a margarine food matrix and may offer protection to probiotics through the GIT
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transit. Also, spreads, like margarine, are a particularly interesting vehicles for functional ingredients,
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because they are eaten daily. Therefore, the aim of this study was to investigate the effect of inulin, WPC,
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and/or CMP, in different proportions up to 3%, on the viability and resistance to simulated gastric and enteric
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conditions of a commercial probiotic strain of Bifidobacterium animalis Bb-12 added in probiotic and
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synbiotic margarine.
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2. Materials and methods
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2.1. Experimental design and margarine manufacture
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Seven pilot scale margarine-making trials, named as M1-M7, were produced according to Table 1,
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using a simplex-centroid design, changing the inulin, whey protein concentrate (WPC), and
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caseinomacropeptide (CMP) proportions in the margarines (three repetitions of each trial were produced on different days). For each formulation, 3 kg of margarine were obtained. Combinations of the ingredients inulin (Beneo ST-Gel, Orafti, Oreye, Belgium), whey protein concentrate (Lacprodan 80, Arla Foods Ingredients, Sønderhøj, Denmark), and caseinomacropeptide (Lacprodan CGMP 10, Arla Foods Ingredients)
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were used. A control trial, without supplementation with inulin, WPC and/or CMP (M8) was also prepared.
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All trials were produced using the freeze-dried probiotic culture of Bifidobacterium animalis subsp. lactis
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Bb-12 (Christian Hansen, Hørsholm, Denmark).
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Margarine production was carried out in five steps: 1) fat phase production, 2) water phase
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production, 3) emulsification, 4) crystallization process, and 5) packaging and storage. Different ingredients
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were employed for preparing the fat and water margarine phases (Table 2).
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The following commercial ingredients were employed for the preparation of the fat phase: palm oil
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(Agropalma, Tailândia, Brazil), canola oil (Liza, Mairinque, Brazil), emulsifiers monoacylglycerol (Myvatex
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Smooth 5Z10729 and Myverol 18-92K) and polyglycerol esters of ricinoleic acid (Admul Wol 1408K)
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(Kerry Bio-Science, Campinas, Brazil), colouring agent β-carotene (DSM, São Paulo, Brazil), butter flavour
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(Danisco, Cotia, Brazil), and vitamin A (Fortitech, Campinas, Brazil). For the water phase, the following
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ingredients were employed: water, NaCl (Cisne, Cabo Frio, Brazil), food-grade lactic acid 85% solution
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(Purac Sínteses, Rio de Janeiro, Brazil), skimmed powdered milk (Nestlé, Araçatuba, Brazil). Additionally,
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according to experimental design (Table 1), the following ingredients were also used in the water phase:
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inulin (Beneo ST-Gel), whey protein concentrate (Lacprodan 80), and caseinomacropeptide (Lacprodan
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CGMP 10). Water phase ingredients were manually mixed, after which the probiotic inoculum was added.
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The probiotic inoculum of Bb-12 was grown in 40 ml of reconstituted skimmed powdered milk for 2
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h at 37°C, prior to its addition to the water phase, in order to obtain Bb-12 populations of a minimum
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between 8 and 9 log cfu g-1 after margarine production (day 1). For the preparation of the fat phase, palm oil
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was heated at 45°C and manually mixed with the additional fat phase ingredients mentioned above. During the emulsification step (step 3), the water phase was gently added to the fat phase under
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agitation using a mixer (Stand Mixer 300, Brastemp, São Paulo, Brazil) until the emulsion formation took
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place. For the crystallization step (step 4), the emulsion obtained on step 3 was transferred to an associated
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equipment consisting of a 10 l jacketed emulsion tank, fitted with a refrigerated scraped-surface (Skymsen,
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Brusque, Brazil), similarly to that described by Goli, Sahri, and Keramat (2009). The emulsion (35°C) was
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submitted to a crystallization process until reaching the temperature of 17°C. Subsequently, the margarine
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was transferred to a manual dispenser (Delgo, Cotia, Brazil) and packaged in individual polypropylene plastic pots for food products (Tries Aditivos Plásticos, São Paulo, Brazil) in portions of 60 g of product. The margarines were then stored at 5±1°C for up to 35 days.
2.2. Determination of B. animalis Bb-12 viability during refrigerated storage
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Margarines from each batch were used for microbiological analysis. Counts of B. animalis Bb-12
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were monitored during margarine production (day 0), and after 1, 7, 14, 21, 28, and 35 days of refrigerated
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storage at 5±1°C, for all trials. For this purpose, 25 g portions of duplicate margarine samples were collected
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aseptically, blended in a Bag Mixer 400 (Interscience, St. Nom, France) with 225 ml of 0.1% peptone water
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preheated to 40°C, according to Charteris, Kelly, Morelli, and Collins (2002), during 3.5 min, to obtain a
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suitable dispersion, and submitted to serial dilutions with the same diluent.
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B. animalis Bb-12 was counted by pour-plating 1 ml of each dilution in DeMan-Rogosa-Sharpe agar
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(MRS agar, Oxoid, Basingstoke, UK) to which sodium propionate (0.3 g 100 ml-1) and lithium chloride (0.2
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g 100 ml-1) were added (Lithium Propionate MRS, LP-MRS). Plates were incubated during 3 days under
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anaerobic condition (Anaerobic System Anaerogen, Oxoid) at 37°C (Vinderola & Reinheimer, 2000). Counts
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of Bb-12 populations were carried out in quadruplicates.
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2.3. Survival of B. animalis Bb-12 under in vitro simulated gastrointestinal conditions
The in vitro evaluation of probiotic B. animalis Bb-12 survival in refrigerated margarines submitted
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to gastric and enteric simulated conditions was carried out according to the methods described by Buriti,
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Castro, and Saad (2010), with modifications, as described below. The in vitro assays were carried out after 7,
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14, 21, and 28 days of refrigerated storage, since some trials did not present sufficient counts for a probiotic
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food product on day 35 (end of storage period). In order to enumerate Bb-12 before and after the in vitro
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assays, samples were collected initially (time 0) and after 2h (first step – after the gastric phase), 4h (after the
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first enteric phase), and 6h after the beginning of the assay (after the second enteric phase).
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For the in vitro procedure, in each sample collection, 10 ml from each triplicate dilution of
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margarine in 0.5% NaCl solution (blended in a Bag Mixer 400) was transferred to 3 sterile flasks, totalizing 9
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flasks containing the samples, and the pH of flasks was adjusted to 1.6-2.0 with 0.2 ml of 1 N HCl. Pepsin
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(from porcine stomach mucosa, Sigma-Aldrich, St. Louis, USA) and lipase (Amano lipase from Penicillium
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camemberti, Aldrich Chemical Company Inc., Milwaukee, USA) solutions were added to samples to reach a
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concentration of 3 g l-1 and of 1.3 mg l-1, respectively. Flasks were incubated at 37°C, with agitation of
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approximately 150 r.p.m in a metabolic water bath (Dubnoff MA-095, Marconi, Piracicaba, Brazil), during
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2h (first step - gastric phase). In the next step (first enteric phase), the pH of samples was increased to 4.05.2, using an alkaline solution pH 12 (1N NaOH, PO4H2Na.2H2O and distilled water). Bile (bovine bile, Sigma-Aldrich) and pancreatin (from porcine pancreas, Sigma-Aldrich) were added to reach a concentration of 5 g l-1 and of 1.6 g l-1, respectively. Samples were incubated again at 37°C for 2h under agitation. In the
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last step, the pH was increased to 6.77-7.21, using the same alkaline solution. Bile and pancreatin
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concentrations were adjusted (7.95 g l-1 and 0.79 g l-1, respectively), and samples were incubated again at
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37°C for 2h under agitation (second enteric phase), achieving 6h of the in vitro assay.
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Enumeration of B. animalis Bb-12 was carried out as described above in aliquots collected from
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triplicate samples after 2h, 4h, and 6h (three different flasks of the same trial for each time) of the in vitro
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assays. All results were presented as log cfu g-1 of margarine.
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2.4. Statistical analysis Statistical analysis of results obtained was carried out using STATISTICA v.8.0 software (Statsoft,
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Tulsa, OK, USA). Analysis of variance (ANOVA) was used to determine significant differences (P<0.05)
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for every parameter analysed among different margarine trials and different days of storage of each
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margarine, using repeated measures. Differences between means were detected using post hoc Tukey test.
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Data were checked for the homogeneity of variances before ANOVA evaluation, using the Brown-Forsythe
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test. When homogeneity of variances was not verified, equivalent non-parametric tests were applied: Kruskal
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Wallis test followed by post hoc Mann Whitney U (different margarines in the same period of storage) or
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Friedman test followed by post hoc LSD rank (different storage period for a same margarine) (Bower,
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1998a,b).
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The experimental results obtained both for B. animalis Bb-12 viability in margarines and for the in
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vitro resistance tests after 21 days of refrigerated storage were applied to obtain the linear, quadratic, and
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special cubic regression models, as a function of the proportions of each ingredient (x1: inulin, x2: WPC, and
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x 3:
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(
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coefficients estimated by the least square method, and xi = dependent variables (x1: inulin, x2: WPC, and x3:
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CMP) with
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was evaluated by ANOVA and F test. Also, the lack of fit and adjusted coefficient of determination (R2) were
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in
margarine
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present
yˆ ( i ) = b1 x1 + b2 x 2 + b3 x 3 + b2 b3 x 2 x 3 ),
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formulations. where
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∑ i = 1 x =1, 1> x > 0 was used to describe data obtained. The quality of the models obtained i
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CMP)
determined and used to evaluate the model.
3. Results and Discussion 3.1. Probiotic viability during refrigerated storage of margarines
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Table 3 shows the viability of B. animalis Bb-12 added to margarines M1-M8 during the
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refrigerated storage at 5±1°C for up to 35 days. Brazilian present legislation states that the minimum viable
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quantity of probiotic culture should be between 8.00 and 9.00 log cfu per daily serving portion and 10 g is the
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portion recommended for margarine, butter, and spreads (Anvisa, 2003, 2008). Therefore, if a portion of
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around 10 g of margarine is consumed daily, each gram of the product would necessarily contain, at least,
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7.00 log cfu of probiotic bacteria.
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The addition of inulin, WPC, and CMP was necessary for the survival of Bb-12 in margarine, since
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M8 (control) presented mean counts of 5.12±0.10 and 3.10±0.15 log cfu g-1, respectively, after the 1st and the
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7th day of storage. After 7 days of storage, Bb-12 was not detected in M8. Except for M2, M3, and M7 after
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14, 35, and 28 days of storage, respectively, and M8, all other margarines presented populations of Bb-12
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above the minimum required for a probiotic food during the whole storage period.
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Among the different margarines studied, the formulation M1, containing higher amounts of inulin
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(3%), presented populations of Bb-12 above 8.00 log cfu g-1 throughout the whole storage period. On days 28
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and 35, populations in M1 were significantly higher (P<0.05). Margarines M3, M5, and M6 revealed
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populations of Bb-12 above 8.00 log cfu g-1 from day 0 up to day 21 of storage. After this period, significant
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reductions were observed (P<0.05). In the same way, M4 and M7 Bb-12 populations were above 8.00 log
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cfu g-1 until day 14. In contrast, M2 was not considered a probiotic margarine after 14 days of storage, since
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it presented Bb-12 populations below 7.00 log cfu g-1. Regarding the margarines supplemented with milk
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proteins (WPC and CMP), Bb-12 populations in M3 (3% of CMP) were significantly higher than in M2 (3%
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of WPC) (P<0.05). On day 35, they were as low as 4.64 log cfu g-1 (M2) and 6.87 log cfu g-1 (M3).
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The lipid food matrix is in fact a great technological challenge for probiotic incorporation, since the
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water-in-oil emulsion which makes up the margarine structure is a relatively inhospitable environment for
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their growth. The size of the water phase droplets, the absence of nutrients inside the droplets, the addition of
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some ingredients like salt, and the lack of ability of microorganisms to move between droplets also reduce
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the ability of margarine to support microbial growth (Charteris, Kelly, Morelli, & Collins, 2002). Preliminary
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tests carried out by our research group revealed that Lactobacillus acidophilus La-5 was not able to survive
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in margarine matrix (data not shown). Therefore, margarine features reinforce the importance of the aqueous
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phase supplementation in order to obtain suitable populations of a specific probiotic microorganism. The presence of ingredients that could be fermented by beneficial microorganisms added during margarine manufacture may ensure their growth and/or survival during shelf life. The results obtained for margarine M1 probably are related to the fact that B. animalis Bb-12 is able
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to metabolize prebiotic ingredients. The inulin employed in the presented study has a low polymerization
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degree (DP ~ 10) (Beneo®
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M1 containing 3% inulin presented lower pH values, varying from 4.89 (day 1) to 4.50 (day 35) when
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compared to M2 (5.42-5.10), M3 (5.28-5.12), and M6 (5.36-5.10). Inulin has a stimulant effect on the
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bifidobacteria growth, acting as a bifidogenic factor. Fermentation of inulin by bifidobacteria results in the
HP), therefore easily metabolized by Bifidobacterium spp. In fact, margarine
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production of organic acids (Bosscher, Loo, & Franck, 2006). These compounds, especially lactic acid, might
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also be formed in synbiotic food, and probably contributed for the decrease in margarine pH values.
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Some studies revealed Bifidobacterium animalis subsp. lactis populations of 107 cfu g-1 , when dairy
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foods were manufactured with inulin (Bruno, Lankaputhra, & Shah, 2002; Cardarelli, Buriti, Castro, & Saad,
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2008), whereas, in the present study, M1 presented even higher Bb-12 populations - of 108 cfu g-1. Several factors, including the presence of oxygen and acid, are responsible for the loss in viability of
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probiotic bacteria in foods (Tripathi & Giri, 2014). However, in margarine M1, the presence of 3% of inulin
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probably contributed for Bb-12 increased survival, particularly conferring protection against the presence of
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organic acids and salt. Regarding supplementation of margarine with WPC and/or CMP, probably CMP was
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more easily metabolized by Bb-12. Caseinomacropeptide (CMP) contains not only available nitrogen for
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bacterial growth but also amino-sugars, such as sialic acid and N-acetylgalactosamine, which could be
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fermented by bifidobacteria (Janer, Peláez, & Requena, 2004).
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A noticeable difference in the composition of WPC that may influence upon growth of probiotic
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microorganisms is the content of mainly β-lactoglobulin and α-lactoalbumin, which were selectively
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removed during the isolation of the CMP fraction (Martín-Diana, Fraga, & Fontecha, 2014). WPC also
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includes whey proteins with excessively high molecular weight to be rendered available for direct bacterial
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uptake, but could be enzymatically cleaved, leading to formation of bifidobacterial growth factors (Janer,
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Peláez, & Requena, 2004). In the present study, according to the manufacturer (Arla Foods Ingredients,
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Sønderhøj, Denmark), CMP added in margarines M3, M5, and M7 had higher glutamine, isoleucine, proline,
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serine, and threonine levels than those of WPC. The presence of these amino acids contributed for the high
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Bb-12 populations observed in M3 (above 8.00 log cfu g-1 up to the 21st day of storage). Probably, the
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probiotic culture here employed was not capable of using the proteins present in M2, since several
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bifidobacteria strains were reported as being only weakly proteolytic (Bergamini, Hynes, Palma, Sabbag, &
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Zalazar, 2009).
Only a few studies were reported on probiotic lipid-based emulsions. Charteris, Kelly, Morelli, and
Collins (2002) studied a table biospread containing Lactobacillus casei and Bifidobacterium infantis and reported populations of 4.5×108 cfu ml-1 (L. casei) and 1.0×106 cfu ml-1 (B. infantis), when different
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ingredients like L-cysteine and sodium alginate were added to the water phase. Similarly, Dommels,
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Kemperman, Zebregs, Draaisma, and Jol (2009) evaluated the viability of Lactobacillus reuteri DSM 17938
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and Lactobacillus rhamnosus GG added to a low fat spread with 28% of lipids. Populations of, respectively,
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2.85×108 and of 1.65×109 cfu g-1 were observed after 6 weeks of refrigerated storage.
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Considering the results obtained for probiotic viability in margarine formulations on day 21 (all
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margarines presented suitable Bb-12 populations, homogeneity of variances, and significant differences
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between formulations), a quadratic model was generated for this variable response, in order to verify the
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influence of inulin, WPC, and CMP on Bb-12 viability. The quadratic model and its coefficients and quality
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analysis are presented in Table 4. The model obtained was statistically significant (P < 0.01) and able to
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explain 86% of results (variation). Also, lack of fit was not statistically significant (P=0.065). The model
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obtained revealed that B. animalis Bb-12 viability on day 21 was dependent on the individual presence inulin,
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WPC, and CMP. The simultaneous supplementation with WPC and CMP was also important. The contour
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plot generated from the quadratic model for viability revealed that inulin was more important than WPC and
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CMP to maintain Bb-12 viability in margarine (Fig. 1). Higher populations of Bb-12 were observed with
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inulin concentrations between 3% and 0.75% (1.00 and 0.25 in the diagram). The same behaviour was
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observed with CMP between 2.25 and 3%.
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3.2. Probiotic survival in margarines under in vitro simulated human gastrointestinal conditions The survival of B. animalis Bb-12 in margarines M1-M7 submitted to simulated in vitro human
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gastrointestinal conditions after 7, 14, 21, and 28 days of storage at 5±1°C is presented in Fig. 2. The control
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trial (M8) was not submitted to in vitro evaluation, since Bb-12 populations observed after 7 days of storage
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were below 6.00 log cfu g-1).
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During the whole in vitro assays - simulated gastric (2 h) and enteric (4 h and 6 h) conditions,
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considering the storage period evaluated (28 days), reductions in Bb-12 populations varied from 0.95 - 2.98
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log cfu g-1; 1.0 - 3.26 log cfu g-1, and 0.71 - 3.47 log cfu g-1 after 2, 4, and 6h, respectively, for most of the
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margarines. M2 presented higher reductions, varying from 4.3 to 5.5 log cfu g-1 during the same period of the
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in vitro assays.
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Significant decreases in Bb-12 populations were observed after 2 h of the in vitro assays for all
margarines tested during storage for up to 28 days (P<0.05). On day 7, after 2h of in vitro assays, M2 presented a 5.00 log cfu g-1 decrease (P<0.05). In contrast, others margarines presented a reduction of 2.00 log cfu g-1 after the gastric phase. M1, M3, and M7 presented the lowest reductions, probably due to the
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presence of inulin and CMP. At the end of the in vitro assays (6h) significant reductions in Bb-12
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populations were observed only for M5 after 7 days, M3 after 21 days, and M4 and M6 after 28 days. M1
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and M6 on day 7, M1, M2 and M7 on day 14, M2 on day 21, and M5 on day 28 presented significant
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increase in probiotic populations (P<0.05). Probably these results reflect a recovery of Bb-12 when it was
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submitted to enteric phase 1 and 2 (pH 5 and 7, respectively). The hydrochloric acid present in the gastric
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phase resulted in an injury of Bb-12 cells, and their recovery through the microbiological analysis was
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difficult. After 7 days, all margarines studied, except M5, presented an increase or maintenance in the Bb-12
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populations until the end of the in vitro assays (6h). From day 7 to 14, a decrease in probiotic populations
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was observed during the whole in vitro assay, but with counts always above 6.00 log cfu g-1, except for M2
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(1.20 cfu g-1 and of 1.98 log cfu g-1 after 2 and 6 hours).
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After 21 days of storage, most margarines presented probiotic populations below 6.00 log cfu g-1,
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varying from 1.14 (M2) to 5.85 log cfu g-1 (M7) after 6h of the in vitro assay. M1 and M2 differed
285
significantly from the other formulations (P<0.05), since populations of, respectively, 7.15 cfu g-1 and 1.14
286
cfu g-1 were observed after 6h of the in vitro assays. At 28 days of storage, after 6h of in vitro assays, Bb-12
287
populations in M3 were significantly higher than in M4 (P<0.05). In margarine supplemented with inulin +
288
WPC (M4), a significantly increase in Bb-12 populations was observed between 4 and 6h of the in vitro
289
assay on day 7 (P<0.05).
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During the whole in vitro assays period, margarines supplemented with inulin presented lower
291
reductions in Bb-12 populations when compared to initial counts. As mentioned earlier, inulin protected
292
probiotic microorganism during the in vitro assays, since when mixed with water inulin forms a particle gel
293
network. This gel probably avoided the action of HCl and enzymes over Bb-12 during the in vitro assays.
294
Inulin assured probiotic viability in suitable concentrations for margarines M4, M5, M7, and especially for
295
M1 during storage. On day 28, by the end of in vitro assays (6h), inulin assured populations of 6.32 log cfu g-
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1
in M1.
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High reductions in probiotic viability after simulated gastric phase are expected results, since to
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reach the intestine, strains must first pass through the stomach, which provides a powerful barrier against the
299
entrance in the gut (Morelli, 2007). Similarly to what was observed in the present study, Hansen, Allan-
300
Wojtas, Jin, and Paulson (2002) reported a 1.3 log cfu g-1 decrease in B. animalis Bb-12 populations after
302 303 304
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exposure to pH 2.0 during 2 hours. Charteris, Kelly, Morelli, and Collins (1998) reported that milk proteins protected probiotic
Lactobacillus casei and Bifidobacterium lactis during simulated gastric transit. This was not observed here when whey protein concentrate was employed, since margarines supplemented with WPC solely did not
305
present suitable Bb-12 populations after 2, 4, and 6h of the in vitro assays during all the sampling periods.
306
Probiotic counts in M2 during shelf life were the lowest (P<0.05) (Table 4). This fact contributed towards
307
the unsatisfactory results observed after the in vitro assays of margarine M2. Different results were reported
308
by Kos, Šušković, Goreta, & Matošić (2000), regarding the addition of WPC. The authors observed that
309
WPC was an important protector for Lactobacillus acidophilus M92 exposed to simulated gastric and small
10
310
intestinal juices, whereas, in the present study, the addition of WPC did not protect Bb-12 and M2 presented
311
a progressive decrease in Bb-12 populations during the in vitro assays along storage. After 28 days, Bb-12
312
counts observed in all sampling periods of the in vitro assay of M2 were below the detection limits of the
313
method (<1.14 log cfu g-1).
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Guo, Wang, Yan, Chen, Liu, and Zhang (2009) observed that the incubation of B. animalis Bb-12 in
315
simulated gastric juice containing pepsin at pH 2.5 resulted in significant decreases in its survival rate. In the
316
present study, reductions observed in probiotic populations were lower, due to the presence of the food
317
matrix and its constituents, mainly its fat content, a factor that could affect probiotic growth and survival in
318
food during the digestive process (Ranadheera, Baines, & Adams, 2010).
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As observed in the present study, Buriti, Castro, and Saad (2010) reported that the supplementation of
320
synbiotic guava musses with inulin and WPC simultaneously did not influence L. acidophilus La-5
321
protection positively during in vitro resistance assays. However, in refrigerated synbiotic guava musses the
322
authors observed counts below 2.00 log cfu g-1 when products supplement with different percentages of
323
inulin (1.33%, 2% or 4%) where submitted to in vitro resistance assays after 28 days. Similarly, Bedani,
324
Rossi, and Saad (2013) observed that inulin did not protect La-5 in fermented soy product during in vitro
325
resistance assays, whereas B. animalis Bb-12 presented mean populations above 7.00 log cfu g-1 up to the
326
end of in vitro assays.
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The presence of inulin was important to protect Bb-12, since margarine with 3% of inulin (M1)
328
presented Bb-12 populations of 6.32 log cfu g-1 after 6h of in vitro assays. The survival rate of Bb-12 in M1
329
after in vitro assays was 91.33% and 78.51% after 7 and 28 days of storage, respectively. Similar results
330
regarding protection given by the prebiotic ingredient inulin, when combined with fructooligosacharide, to
331
Bb-12 during GI in vitro assays were reported by Padilha, Villarreal-Morales, Vieira, Costa, and Saad (2016)
332
in petit-suisse cheese. The authors observed mean Bb-12 survival rates of 79% in the synbiotic cheese,
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whereas this rate was reduced to 60% in the probiotic product. In order to verify the influence of inulin, WPC, and CMP on Bb-12 resistance, results obtained after
6h of the in vitro assays on day 21 were used, since the parameters mentioned previously regarding Bb-12 viability were observed. A quadratic model was generated for this variable response and it was statistically
337
significant (P < 0.01) and able to explain 98% of results (variation). Also, lack of fit was not statistically
338
significant (P=0.665). The model and its coefficients and quality analysis are presented in Table 5. The
339
contour plot generated from the quadratic model obtained for Bb-12 survival during in vitro assays is
340
presented in Fig. 3.
11
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The quadratic model obtained revealed that probiotic Bb-12 survival was dependent on isolated
342
ingredients and some ingredients interactions. The higher viability of Bb-12 (>7.00 log cfu g-1) after the in
343
vitro tests was observed when inulin was added in concentrations varying between 3 and 2.25%. Similarly, a
344
satisfactory result was observed when margarine was supplemented with CMP, since concentrations between
345
3 and 2.25% resulted in Bb-12 populations between 5.25 and 6.25 log cfu g-1 after the entire in vitro assay
346
(6h). In contrast, WPC in the same concentrations resulted in Bb-12 populations below 4.25 log cfu g-1 after
347
6h of the in vitro assay.
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The conditions found in human gastrointestinal tract are hostile for probiotic microorganisms.
349
Nevertheless, the food matrix protects the cells, and avoids high reductions in probiotic populations (El-
350
Shafei, Tawfik, Dabiza, Sharaf, & Effat, 2010). Therefore, the food matrix and its composition are very
351
important for protecting probiotic strains. The fat content, the pH and the solid matrix, may protect probiotic
352
bacteria more efficiently than a fluid environment during storage of the food product and its transit through
353
the human gastrointestinal tract (Ranadheera, Baines, & Adams, 2010). In the present study, the solid matrix
354
and the fat present in margarine assured the survival of the probiotic strain Bb-12 during the in vitro
355
resistance assays. However, it is important to emphasize that high counts during the shelf life of a specific
356
product are necessary to obtain appropriate populations of probiotic viable cells by the end of the digestive
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process.
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4. Conclusion
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The results obtained showed that the production of probiotic margarine with suitable populations of
362
B. animalis Bb-12, and without hydrogenation process, with palm and canola oil, is possible. The
363
supplementation of the water phase was very important, since the control margarine (without the addition of
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inulin, WPC, and/or CMP) presented very low and insufficient Bb-12 populations. The presence of inulin, especially in the proportion of 3% resulted in significant higher Bb-12 populations (P<0.05) and assured Bb12 resistance through the in vitro assays. Populations observed for margarines (except M2) by the end of in vitro assays (after 6h) revealed that recovery of Bb-12 viable cells in satisfactory populations was possible,
368
even after the digestive process. As far as we know, taken together, results on viability of B. animalis Bb-12
369
and on in vitro GI resistance of the strain incorporated in margarine produced with inulin were unique, when
370
compared to other probiotic products described in the scientific literature. Therefore, functional margarine
371
supplemented with a probiotic strain like B. animalis Bb-12 ought to be produced commercially, though the
372
addition of inulin is necessary to lead to promising probiotic potential.
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375 The authors would like to thank Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
377
(Projects 07/59260-0 and 06/54843-5), and Conselho Nacional de Desenvolvimento Científico e Tecnológico
378
(CNPq) for financial support and fellowships. The authors would also like to thank Agropalma, Kerry Bio-
379
Science, DSM, Danisco, Fortitech, Purac Sínteses, Orafti, and Arla Foods, for providing part of the material
380
resources employed in this study. The authors gratefully acknowledge Regina Célia Cabral Estrotra for her
381
technical assistance.
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Table 1
2
Simplex-centroid experimental design employed in the present study. Quantities of each ingredient (%) CMP3 (x3)
0 3.0 0 1.5 0 1.5 1.0 -
0 0 3.0 0 1.5 1.5 1.0 -
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WPC2 (x2)
2
Whey protein concentrate (Arla Foods Ingredients, Sønderhøj, Denmark; 82% protein).
3
Caseinomacropeptide (Arla Foods Ingredients, 85% protein).
4
M8: control trial.
– = without inulin, WPC and/or CMP addition.
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8
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3 4 5 6 7
Proportion of ingredients in the mixture Inulin1 (x1) (x1, x2, x3) M1 (1, 0, 0) 3.0 M2 (0, 1, 0) 0 M3 (0, 0, 1) 0 M4 (½, ½, 0) 1.5 M5 (½, 0, ½) 1.5 M6 (0, ½, ½) 0 (⅓, ⅓, ⅓) 1.0 M7 M84 (0, 0, 0) 1 Inulin (Orafti, 92% inulin + 8% fructose, glucose, and sucrose).
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Margarine Trials
1
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Table 2
10
Ingredients used for the production of the margarine trials studied, according to the experimental design
11
described in Table 1. Margarine formulations Ingredients (%)
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60.000 3.400 0.001 0.050 0.880 3.000
Control trial.
**
33.999 0.760 0.010 0.400 0.500
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30.999 0.760 0.010 0.400 0.500
60.000 3.400 0.001 0.050 0.880 -
60% of palm oil (Agropalma, Tailândia, Brazil) + 40% of canola oil (Liza, Mairinque, Brazil).
***
Margarines M1 - M7 were supplemented with a mixture containing inulin, WPC, and/or CMP, according to
Table 1. 1
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– = without supplementation with inulin, WPC, and/or CMP. : (Cisne, Cabo Frio, Brazil); 2: (food-grade lactic acid 85% solution, Purac Sínteses, Rio de Janeiro, Brazil); 3:
(Nestlé, Araçatuba, Brazil); 4: (Christian Hansen, Hørsholm, Denmark);
5
(Kerry Bio-Science, Campinas,
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Brazil); 6: (β-carotene, DSM, São Paulo, Brazil); 7: (Danisco, Cotia, Brazil), 8: (Fortitech, Campinas, Brazil).
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*
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Water phase Water Salt1 Lactic acid2 Skimmed powdered milk3 Probiotic culture4 Fat phase Fat** Emulsifiers5 Colouring agent6 Butter flavour7 Vitamin A8 Mixture***
12 13 14 15 16 17 18 19
M8*
M1-M7
2
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Table 3
22
Populations (mean values1 ± standard deviation) of B. animalis Bb-12 (log cfu g-1) in margarines M1-M8 after 0, 1, 7, 14, 21, 28, and 35 days of storage
23
at 5±1°C. Margarines M2
M3
M4
M5
M6
M7
03
8.39±0.33BCab
8.24±0.14Ca
8.71±0.10Aa
8.49±0.11Ba
8.77±0.10Aa
8.42±0.14Ba
8.14±0.12Ca
1
8.77±0.24Aa
7.82±0.19Bb
8.60±0.16Aa
8.43±0.05Aa
8.42±0.09Aab
8.63±0.22Aa
8.44±0.14Aa
5.12±0.10Cb
7
8.19±0.23Bb
7.55±0.17Cb
8.36±0.15ABab
8.18±0.07Bb
8.55±0.18Aa
8.26±0.13ABb
8.29±0.12Ba
3.10±0.15Dc
14
8.54±0.01Aa
6.74±0.17Cc
8.19±0.08ABb
8.03±0.06Bb
8.16±0.10ABbc
8.27±0.13ABb
8.40±0.16Aa
-
21
8.23±0.20Aab
6.54±0.14Dc
8.07±0.21ABbc
7.62±0.08Cc
8.10±0.04ABc
8.03±0.15ABc
7.81±0.29BCb
-
28
8.05±0.04Ab
5.40±0.16Dd
7.64±0.03Bc
7.56±0.15Bcd
7.52±0.09Bd
7.62±0.12Bd
6.81±0.01Cc
-
35
8.01±0.22Ab
4.64±0.26De
6.87±0.52Bd
7.32±0.04Bd
7.29±0.23Bd
7.27±0.09Be
6.26±0.16Cd
-
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See Table 1 for description of trials M1-M8. n=6.
2
Control trial.
3
Day 0: counts observed in the same day of margarine production.
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A,B,C,D
8.52±0.07Ba
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(Days)
24 25 26 27 28 29 30
M82
M1
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Storage
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21
: For each day of storage, different capital letters in a row denote significant differences (P<0.05) between different trials.
a,b,c,d,e
: For each trial, different lowercase superscripts in a column denote significant differences (P<0.05) between different days of storage.
– = not detected.
31
3
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Table 4
33
Coefficients (b1, b2, b3) with their respective standard deviations, P values (model and lack of fit), and adjusted
34
R2 of the quadratic model obtained for B. animalis Bb-12 viability in margarines at 21 days of storage at 5±1°C.
35
Coefficients Inulin (b1) WPC (b2) CMP (b3) Inulin + WPC (b12) Inulin + CMP (b13) WPC + CMP (b23) P value P lack of fit Adjusted R2 n.s: non-significant.
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Values 8.26 (0.08) 6.61 (0.09) 8.03 (0.09) n.s n.s 2.72 (0.34) <0.01 0.065230 0.86
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Table 5
40
Coefficients (b1, b2, b3) with their respective standard deviations, P values (model and lack of fit), and adjusted
41
R2 of the quadratic model obtained for B. animalis Bb-12 survival during in vitro tests at 21 days of storage at
42
5±1°C. Values 7.14 (0.12) 1.14 (0.07) 5.48 (0.08) 6.16 (0.48) -3.31 (0.39) 8.28 (0.34) <0.01 0.665 0.98
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Coefficients Inulin (b1) WPC (b2) CMP (b3) Inulin + WPC (b12) Inulin + CMP (b13) WPC + CMP (b23) P value P lack of fit Adjusted R2
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Figure caption
Figure 1. Contour plot showing the effect of inulin, whey protein concentrate (WPC), and
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caseinomacropeptide (CMP) on B. animalis Bb-12 viability (log cfu g-1) at 21 days of refrigerated storage.
Figure 2. Survival of B. animalis Bb-12 (log cfu g-1) in margarines M1-M7 submitted to in
at 5±1°C (a, b, c, and d, respectively) before ( )], and enteric [4h (
) and 6h (
) and during exposition to simulated gastric
)] conditions. A,B,C,D,E: different superscript capital
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[2h (
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vitro simulated gastrointestinal conditions after 7, 14, 21, and 28 days of refrigerated storage
letters denote significant differences between margarines for the same sampling period of the in vitro assay.
a,b,c
: different lowercase superscript letters denote significant differences
between the sampling periods of the in vitro assays for the same margarine. See Table 1 for
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description of margarines M1-M7.
Figure 3. Contour plot showing the effect of inulin, WPC, and CMP on B. animalis Bb-12
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resistance (log cfu g-1) during in vitro assays at 21 days of refrigerated storage.
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B. animalis Bb-12 (log cfu g-1)
10
Ba
8
Aa
ABa
Ab Ab Ac
Bb
Bb BCb
6 4
ABa
Ba
Ca
Ba ABb Bb Ab
Ab ABb
BCb Cb c Cc
Bb Bb Cc
Cc
M4
M5
M6
Db Db Db
2 0 M1
M2
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ACCEPTED MANUSCRIPT Original manuscript “Margarine produced with inulin increases Bifidobacterium animalis Bb-12 gastrointestinal survival in vitro”, authors Cínthia Hoch Batista de Souza, Luiz Antonio Gioielli, and Susana Marta Isay Saad.
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Research Highlights
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Submission – LWT - Food Science and Technology
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Margarine with inulin, whey protein concentrate, and/or caseinomacropeptide at 3% was studied.
Viability and GI in vitro resistance of Bifidobacterium Bb-12 was evaluated Inulin improved Bb-12 survival in probiotic margarine during storage. Margarine with inulin improved Bb-12 resistance to in vitro GI assays.
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Inulin in the proportion of 3% resulted in significant higher Bb-12 survival.
S0023-6438(17)30032-4
DOI:
10.1016/j.lwt.2017.01.032
Reference:
YFSTL 5984
To appear in:
LWT - Food Science and Technology
Received Date: 20 July 2016 Revised Date:
6 January 2017
Accepted Date: 12 January 2017
Please cite this article as: de Souza, C.H.B., Gioielli, L.A., Saad, S.M.I., Inulin increases Bifidobacterium animalis Bb-12 in vitro gastrointestinal resistance in margarine, LWT - Food Science and Technology (2017), doi: 10.1016/j.lwt.2017.01.032. 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.
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Inulin increases Bifidobacterium animalis Bb-12 in vitro gastrointestinal resistance in
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margarine
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6 Cínthia Hoch Batista de Souza a,1, Luiz Antonio Gioielli a, Susana Marta Isay Saad a,*
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a
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Universidade de São Paulo. Av. Prof. Lineu Prestes, 580, 05508-000 - São Paulo, SP, Brazil.
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Rua Marselha, 591, 86041-140 - Londrina, PR, Brazil.
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Departamento de Tecnologia Bioquímico-Farmacêutica, Faculdade de Ciências Farmacêuticas,
Present address: Mestrado em Ciência e Tecnologia de Leite e Derivados, Universidade Norte do Paraná.
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*
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Tel: +55-11-30912378; Fax: +55-11-38156386
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E-mail address: [email protected] (S.M.I. Saad)
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Corresponding author:
Shortened running title: In vitro GI resistance of Bifidobacterium Bb-12 in margarine.
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Abstract
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This study aimed to investigate the effect of inulin, whey protein concentrate (WPC), and/or
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caseinomacropeptide (CMP), in different proportions up to 3%, on the viability and resistance to simulated
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gastric and enteric conditions of Bifidobacterium animalis Bb-12 added in probiotic and synbiotic margarine,
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during 35 days of storage at 5°C. Supplementation was important, since the control margarine presented very
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low Bb-12 populations. Inulin at 3% resulted in higher Bb-12 counts (8 log cfu g-1). CMP contributed for
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higher Bb-12 counts, compared to WPC. Inulin increased Bb-12 in vitro survival significantly after 6h
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(P<0.05). In margarines with WPC at 3%, Bb-12 populations decreased drastically during the in vitro assays
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for all storage periods. For the other formulations, Bb-12 populations decreased 2 log cfu g-1 after 2h. Taken
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together, results on viability of B. animalis Bb-12 and on in vitro GI resistance of the strain incorporated in
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margarine produced with inulin were unique, but the addition of inulin was necessary.
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Keywords: Synbiotic; Probiotic; Prebiotic; Spread; Gastrointestinal resistance.
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1. Introduction
Probiotics are “live microorganisms that, when administered in adequate amounts, confer a health
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benefit on the host” (Hill, Guarner, Reid, Gibson, Merenstein, & Pot, 2014). One of the well-investigated
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probiotics is Bifidobacterium animalis subsp. lactis Bb-12, with demonstrated efficacy through clinical trials
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(Haschke et al., 1998). In order to exert their functional properties, probiotics need to be delivered to human
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intestine in an active and viable form (Vandenplas, Huys, & Daube, 2015). Therefore, it is important to
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develop probiotic food with suitable probiotic populations throughout shelf life and that are ingested as part
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of a normal diet for maintaining a regular probiotic intake. Nevertheless, ingested microorganisms are
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exposed to several stress factors that influence their viability through the human gastrointestinal tract (GIT).
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Among these factors, probiotics must tolerate the stomach acidic environment and also the reduced water activity and the presence of bile in the upper small intestine (Vandenplas, Huys, & Daube, 2015). Once probiotic bacteria must preserve viability and arrive at high populations in the colon after
surviving the food processing steps and the digestive process, a careful selection of the food matrix is an
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important factor that should be considered in developing a probiotic product. The food matrix is considered
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as one of the major factors in regulating colonization of microorganisms in the GIT. Food helps to buffer the
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bacteria through the stomach and may contain other functional ingredients that could interact with probiotics
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to alter their functionality. Fat content, concentration and type of proteins, sugars, and pH of foods are some
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factors that could affect probiotic growth and survival in food products (Ranadheera, Baines, & Adams,
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2010). These features might help probiotic survival during passage through the GIT, where survival is
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dependent on both the strain and the food matrix involved. Likewise, the supplementation of food with some
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ingredients like the prebiotic fibre inulin and milk proteins may stimulate probiotic bifidobacteria growth and
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also protect them during GIT passage (Janer, Peláez, & Requena, 2004; Kos, Šušković, Goreta, & Matošić,
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2000).
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Limitations of dairy products such as the presence of allergens and the requirement for cold storage
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facilities, as well as an increasing demand for new foods and tastes have initiated a trend in non-dairy
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probiotic product development (Martins, Ramos, Vanzela, Stringheta, Pinto, & Martins, 2013; Rößle, Auty,
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Brunton, Gormley, & Butler, 2010; Tripathi & Giri, 2014). Among these new food matrices, margarine has
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excellent perspectives as a matrix for probiotic incorporation. Margarine has several advantages over
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yoghurt-type products in terms of delivery of viable probiotics, including its higher pH. Moreover, desirable
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characteristics for probiotic foods as higher fat content and more solid consistency (Ong, Henriksson, &
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Shah, 2006) are observed in a margarine food matrix and may offer protection to probiotics through the GIT
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transit. Also, spreads, like margarine, are a particularly interesting vehicles for functional ingredients,
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because they are eaten daily. Therefore, the aim of this study was to investigate the effect of inulin, WPC,
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and/or CMP, in different proportions up to 3%, on the viability and resistance to simulated gastric and enteric
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conditions of a commercial probiotic strain of Bifidobacterium animalis Bb-12 added in probiotic and
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synbiotic margarine.
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2. Materials and methods
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2.1. Experimental design and margarine manufacture
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Seven pilot scale margarine-making trials, named as M1-M7, were produced according to Table 1,
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using a simplex-centroid design, changing the inulin, whey protein concentrate (WPC), and
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caseinomacropeptide (CMP) proportions in the margarines (three repetitions of each trial were produced on different days). For each formulation, 3 kg of margarine were obtained. Combinations of the ingredients inulin (Beneo ST-Gel, Orafti, Oreye, Belgium), whey protein concentrate (Lacprodan 80, Arla Foods Ingredients, Sønderhøj, Denmark), and caseinomacropeptide (Lacprodan CGMP 10, Arla Foods Ingredients)
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were used. A control trial, without supplementation with inulin, WPC and/or CMP (M8) was also prepared.
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All trials were produced using the freeze-dried probiotic culture of Bifidobacterium animalis subsp. lactis
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Bb-12 (Christian Hansen, Hørsholm, Denmark).
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Margarine production was carried out in five steps: 1) fat phase production, 2) water phase
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production, 3) emulsification, 4) crystallization process, and 5) packaging and storage. Different ingredients
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were employed for preparing the fat and water margarine phases (Table 2).
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The following commercial ingredients were employed for the preparation of the fat phase: palm oil
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(Agropalma, Tailândia, Brazil), canola oil (Liza, Mairinque, Brazil), emulsifiers monoacylglycerol (Myvatex
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Smooth 5Z10729 and Myverol 18-92K) and polyglycerol esters of ricinoleic acid (Admul Wol 1408K)
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(Kerry Bio-Science, Campinas, Brazil), colouring agent β-carotene (DSM, São Paulo, Brazil), butter flavour
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(Danisco, Cotia, Brazil), and vitamin A (Fortitech, Campinas, Brazil). For the water phase, the following
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ingredients were employed: water, NaCl (Cisne, Cabo Frio, Brazil), food-grade lactic acid 85% solution
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(Purac Sínteses, Rio de Janeiro, Brazil), skimmed powdered milk (Nestlé, Araçatuba, Brazil). Additionally,
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according to experimental design (Table 1), the following ingredients were also used in the water phase:
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inulin (Beneo ST-Gel), whey protein concentrate (Lacprodan 80), and caseinomacropeptide (Lacprodan
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CGMP 10). Water phase ingredients were manually mixed, after which the probiotic inoculum was added.
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The probiotic inoculum of Bb-12 was grown in 40 ml of reconstituted skimmed powdered milk for 2
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h at 37°C, prior to its addition to the water phase, in order to obtain Bb-12 populations of a minimum
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between 8 and 9 log cfu g-1 after margarine production (day 1). For the preparation of the fat phase, palm oil
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was heated at 45°C and manually mixed with the additional fat phase ingredients mentioned above. During the emulsification step (step 3), the water phase was gently added to the fat phase under
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agitation using a mixer (Stand Mixer 300, Brastemp, São Paulo, Brazil) until the emulsion formation took
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place. For the crystallization step (step 4), the emulsion obtained on step 3 was transferred to an associated
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equipment consisting of a 10 l jacketed emulsion tank, fitted with a refrigerated scraped-surface (Skymsen,
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Brusque, Brazil), similarly to that described by Goli, Sahri, and Keramat (2009). The emulsion (35°C) was
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submitted to a crystallization process until reaching the temperature of 17°C. Subsequently, the margarine
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was transferred to a manual dispenser (Delgo, Cotia, Brazil) and packaged in individual polypropylene plastic pots for food products (Tries Aditivos Plásticos, São Paulo, Brazil) in portions of 60 g of product. The margarines were then stored at 5±1°C for up to 35 days.
2.2. Determination of B. animalis Bb-12 viability during refrigerated storage
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Margarines from each batch were used for microbiological analysis. Counts of B. animalis Bb-12
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were monitored during margarine production (day 0), and after 1, 7, 14, 21, 28, and 35 days of refrigerated
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storage at 5±1°C, for all trials. For this purpose, 25 g portions of duplicate margarine samples were collected
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aseptically, blended in a Bag Mixer 400 (Interscience, St. Nom, France) with 225 ml of 0.1% peptone water
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preheated to 40°C, according to Charteris, Kelly, Morelli, and Collins (2002), during 3.5 min, to obtain a
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suitable dispersion, and submitted to serial dilutions with the same diluent.
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B. animalis Bb-12 was counted by pour-plating 1 ml of each dilution in DeMan-Rogosa-Sharpe agar
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(MRS agar, Oxoid, Basingstoke, UK) to which sodium propionate (0.3 g 100 ml-1) and lithium chloride (0.2
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g 100 ml-1) were added (Lithium Propionate MRS, LP-MRS). Plates were incubated during 3 days under
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anaerobic condition (Anaerobic System Anaerogen, Oxoid) at 37°C (Vinderola & Reinheimer, 2000). Counts
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of Bb-12 populations were carried out in quadruplicates.
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2.3. Survival of B. animalis Bb-12 under in vitro simulated gastrointestinal conditions
The in vitro evaluation of probiotic B. animalis Bb-12 survival in refrigerated margarines submitted
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to gastric and enteric simulated conditions was carried out according to the methods described by Buriti,
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Castro, and Saad (2010), with modifications, as described below. The in vitro assays were carried out after 7,
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14, 21, and 28 days of refrigerated storage, since some trials did not present sufficient counts for a probiotic
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food product on day 35 (end of storage period). In order to enumerate Bb-12 before and after the in vitro
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assays, samples were collected initially (time 0) and after 2h (first step – after the gastric phase), 4h (after the
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first enteric phase), and 6h after the beginning of the assay (after the second enteric phase).
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For the in vitro procedure, in each sample collection, 10 ml from each triplicate dilution of
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margarine in 0.5% NaCl solution (blended in a Bag Mixer 400) was transferred to 3 sterile flasks, totalizing 9
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flasks containing the samples, and the pH of flasks was adjusted to 1.6-2.0 with 0.2 ml of 1 N HCl. Pepsin
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(from porcine stomach mucosa, Sigma-Aldrich, St. Louis, USA) and lipase (Amano lipase from Penicillium
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camemberti, Aldrich Chemical Company Inc., Milwaukee, USA) solutions were added to samples to reach a
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concentration of 3 g l-1 and of 1.3 mg l-1, respectively. Flasks were incubated at 37°C, with agitation of
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approximately 150 r.p.m in a metabolic water bath (Dubnoff MA-095, Marconi, Piracicaba, Brazil), during
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2h (first step - gastric phase). In the next step (first enteric phase), the pH of samples was increased to 4.05.2, using an alkaline solution pH 12 (1N NaOH, PO4H2Na.2H2O and distilled water). Bile (bovine bile, Sigma-Aldrich) and pancreatin (from porcine pancreas, Sigma-Aldrich) were added to reach a concentration of 5 g l-1 and of 1.6 g l-1, respectively. Samples were incubated again at 37°C for 2h under agitation. In the
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last step, the pH was increased to 6.77-7.21, using the same alkaline solution. Bile and pancreatin
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concentrations were adjusted (7.95 g l-1 and 0.79 g l-1, respectively), and samples were incubated again at
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37°C for 2h under agitation (second enteric phase), achieving 6h of the in vitro assay.
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Enumeration of B. animalis Bb-12 was carried out as described above in aliquots collected from
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triplicate samples after 2h, 4h, and 6h (three different flasks of the same trial for each time) of the in vitro
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assays. All results were presented as log cfu g-1 of margarine.
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2.4. Statistical analysis Statistical analysis of results obtained was carried out using STATISTICA v.8.0 software (Statsoft,
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Tulsa, OK, USA). Analysis of variance (ANOVA) was used to determine significant differences (P<0.05)
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for every parameter analysed among different margarine trials and different days of storage of each
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margarine, using repeated measures. Differences between means were detected using post hoc Tukey test.
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Data were checked for the homogeneity of variances before ANOVA evaluation, using the Brown-Forsythe
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test. When homogeneity of variances was not verified, equivalent non-parametric tests were applied: Kruskal
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Wallis test followed by post hoc Mann Whitney U (different margarines in the same period of storage) or
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Friedman test followed by post hoc LSD rank (different storage period for a same margarine) (Bower,
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1998a,b).
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The experimental results obtained both for B. animalis Bb-12 viability in margarines and for the in
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vitro resistance tests after 21 days of refrigerated storage were applied to obtain the linear, quadratic, and
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special cubic regression models, as a function of the proportions of each ingredient (x1: inulin, x2: WPC, and
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x 3:
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(
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coefficients estimated by the least square method, and xi = dependent variables (x1: inulin, x2: WPC, and x3:
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CMP) with
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was evaluated by ANOVA and F test. Also, the lack of fit and adjusted coefficient of determination (R2) were
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in
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yˆ ( i ) = b1 x1 + b2 x 2 + b3 x 3 + b2 b3 x 2 x 3 ),
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CMP)
determined and used to evaluate the model.
3. Results and Discussion 3.1. Probiotic viability during refrigerated storage of margarines
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Table 3 shows the viability of B. animalis Bb-12 added to margarines M1-M8 during the
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refrigerated storage at 5±1°C for up to 35 days. Brazilian present legislation states that the minimum viable
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quantity of probiotic culture should be between 8.00 and 9.00 log cfu per daily serving portion and 10 g is the
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portion recommended for margarine, butter, and spreads (Anvisa, 2003, 2008). Therefore, if a portion of
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around 10 g of margarine is consumed daily, each gram of the product would necessarily contain, at least,
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7.00 log cfu of probiotic bacteria.
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The addition of inulin, WPC, and CMP was necessary for the survival of Bb-12 in margarine, since
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M8 (control) presented mean counts of 5.12±0.10 and 3.10±0.15 log cfu g-1, respectively, after the 1st and the
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7th day of storage. After 7 days of storage, Bb-12 was not detected in M8. Except for M2, M3, and M7 after
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14, 35, and 28 days of storage, respectively, and M8, all other margarines presented populations of Bb-12
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above the minimum required for a probiotic food during the whole storage period.
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Among the different margarines studied, the formulation M1, containing higher amounts of inulin
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(3%), presented populations of Bb-12 above 8.00 log cfu g-1 throughout the whole storage period. On days 28
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and 35, populations in M1 were significantly higher (P<0.05). Margarines M3, M5, and M6 revealed
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populations of Bb-12 above 8.00 log cfu g-1 from day 0 up to day 21 of storage. After this period, significant
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reductions were observed (P<0.05). In the same way, M4 and M7 Bb-12 populations were above 8.00 log
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cfu g-1 until day 14. In contrast, M2 was not considered a probiotic margarine after 14 days of storage, since
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it presented Bb-12 populations below 7.00 log cfu g-1. Regarding the margarines supplemented with milk
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proteins (WPC and CMP), Bb-12 populations in M3 (3% of CMP) were significantly higher than in M2 (3%
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of WPC) (P<0.05). On day 35, they were as low as 4.64 log cfu g-1 (M2) and 6.87 log cfu g-1 (M3).
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The lipid food matrix is in fact a great technological challenge for probiotic incorporation, since the
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water-in-oil emulsion which makes up the margarine structure is a relatively inhospitable environment for
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their growth. The size of the water phase droplets, the absence of nutrients inside the droplets, the addition of
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some ingredients like salt, and the lack of ability of microorganisms to move between droplets also reduce
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the ability of margarine to support microbial growth (Charteris, Kelly, Morelli, & Collins, 2002). Preliminary
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tests carried out by our research group revealed that Lactobacillus acidophilus La-5 was not able to survive
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in margarine matrix (data not shown). Therefore, margarine features reinforce the importance of the aqueous
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phase supplementation in order to obtain suitable populations of a specific probiotic microorganism. The presence of ingredients that could be fermented by beneficial microorganisms added during margarine manufacture may ensure their growth and/or survival during shelf life. The results obtained for margarine M1 probably are related to the fact that B. animalis Bb-12 is able
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to metabolize prebiotic ingredients. The inulin employed in the presented study has a low polymerization
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degree (DP ~ 10) (Beneo®
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M1 containing 3% inulin presented lower pH values, varying from 4.89 (day 1) to 4.50 (day 35) when
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compared to M2 (5.42-5.10), M3 (5.28-5.12), and M6 (5.36-5.10). Inulin has a stimulant effect on the
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bifidobacteria growth, acting as a bifidogenic factor. Fermentation of inulin by bifidobacteria results in the
HP), therefore easily metabolized by Bifidobacterium spp. In fact, margarine
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production of organic acids (Bosscher, Loo, & Franck, 2006). These compounds, especially lactic acid, might
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also be formed in synbiotic food, and probably contributed for the decrease in margarine pH values.
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Some studies revealed Bifidobacterium animalis subsp. lactis populations of 107 cfu g-1 , when dairy
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foods were manufactured with inulin (Bruno, Lankaputhra, & Shah, 2002; Cardarelli, Buriti, Castro, & Saad,
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2008), whereas, in the present study, M1 presented even higher Bb-12 populations - of 108 cfu g-1. Several factors, including the presence of oxygen and acid, are responsible for the loss in viability of
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probiotic bacteria in foods (Tripathi & Giri, 2014). However, in margarine M1, the presence of 3% of inulin
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probably contributed for Bb-12 increased survival, particularly conferring protection against the presence of
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organic acids and salt. Regarding supplementation of margarine with WPC and/or CMP, probably CMP was
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more easily metabolized by Bb-12. Caseinomacropeptide (CMP) contains not only available nitrogen for
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bacterial growth but also amino-sugars, such as sialic acid and N-acetylgalactosamine, which could be
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fermented by bifidobacteria (Janer, Peláez, & Requena, 2004).
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A noticeable difference in the composition of WPC that may influence upon growth of probiotic
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microorganisms is the content of mainly β-lactoglobulin and α-lactoalbumin, which were selectively
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removed during the isolation of the CMP fraction (Martín-Diana, Fraga, & Fontecha, 2014). WPC also
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includes whey proteins with excessively high molecular weight to be rendered available for direct bacterial
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uptake, but could be enzymatically cleaved, leading to formation of bifidobacterial growth factors (Janer,
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Peláez, & Requena, 2004). In the present study, according to the manufacturer (Arla Foods Ingredients,
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Sønderhøj, Denmark), CMP added in margarines M3, M5, and M7 had higher glutamine, isoleucine, proline,
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serine, and threonine levels than those of WPC. The presence of these amino acids contributed for the high
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Bb-12 populations observed in M3 (above 8.00 log cfu g-1 up to the 21st day of storage). Probably, the
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probiotic culture here employed was not capable of using the proteins present in M2, since several
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bifidobacteria strains were reported as being only weakly proteolytic (Bergamini, Hynes, Palma, Sabbag, &
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Zalazar, 2009).
Only a few studies were reported on probiotic lipid-based emulsions. Charteris, Kelly, Morelli, and
Collins (2002) studied a table biospread containing Lactobacillus casei and Bifidobacterium infantis and reported populations of 4.5×108 cfu ml-1 (L. casei) and 1.0×106 cfu ml-1 (B. infantis), when different
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ingredients like L-cysteine and sodium alginate were added to the water phase. Similarly, Dommels,
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Kemperman, Zebregs, Draaisma, and Jol (2009) evaluated the viability of Lactobacillus reuteri DSM 17938
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and Lactobacillus rhamnosus GG added to a low fat spread with 28% of lipids. Populations of, respectively,
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2.85×108 and of 1.65×109 cfu g-1 were observed after 6 weeks of refrigerated storage.
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Considering the results obtained for probiotic viability in margarine formulations on day 21 (all
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margarines presented suitable Bb-12 populations, homogeneity of variances, and significant differences
248
between formulations), a quadratic model was generated for this variable response, in order to verify the
249
influence of inulin, WPC, and CMP on Bb-12 viability. The quadratic model and its coefficients and quality
250
analysis are presented in Table 4. The model obtained was statistically significant (P < 0.01) and able to
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explain 86% of results (variation). Also, lack of fit was not statistically significant (P=0.065). The model
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obtained revealed that B. animalis Bb-12 viability on day 21 was dependent on the individual presence inulin,
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WPC, and CMP. The simultaneous supplementation with WPC and CMP was also important. The contour
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plot generated from the quadratic model for viability revealed that inulin was more important than WPC and
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CMP to maintain Bb-12 viability in margarine (Fig. 1). Higher populations of Bb-12 were observed with
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inulin concentrations between 3% and 0.75% (1.00 and 0.25 in the diagram). The same behaviour was
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observed with CMP between 2.25 and 3%.
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3.2. Probiotic survival in margarines under in vitro simulated human gastrointestinal conditions The survival of B. animalis Bb-12 in margarines M1-M7 submitted to simulated in vitro human
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gastrointestinal conditions after 7, 14, 21, and 28 days of storage at 5±1°C is presented in Fig. 2. The control
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trial (M8) was not submitted to in vitro evaluation, since Bb-12 populations observed after 7 days of storage
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were below 6.00 log cfu g-1).
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During the whole in vitro assays - simulated gastric (2 h) and enteric (4 h and 6 h) conditions,
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considering the storage period evaluated (28 days), reductions in Bb-12 populations varied from 0.95 - 2.98
266
log cfu g-1; 1.0 - 3.26 log cfu g-1, and 0.71 - 3.47 log cfu g-1 after 2, 4, and 6h, respectively, for most of the
267
margarines. M2 presented higher reductions, varying from 4.3 to 5.5 log cfu g-1 during the same period of the
268
in vitro assays.
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Significant decreases in Bb-12 populations were observed after 2 h of the in vitro assays for all
margarines tested during storage for up to 28 days (P<0.05). On day 7, after 2h of in vitro assays, M2 presented a 5.00 log cfu g-1 decrease (P<0.05). In contrast, others margarines presented a reduction of 2.00 log cfu g-1 after the gastric phase. M1, M3, and M7 presented the lowest reductions, probably due to the
273
presence of inulin and CMP. At the end of the in vitro assays (6h) significant reductions in Bb-12
274
populations were observed only for M5 after 7 days, M3 after 21 days, and M4 and M6 after 28 days. M1
275
and M6 on day 7, M1, M2 and M7 on day 14, M2 on day 21, and M5 on day 28 presented significant
276
increase in probiotic populations (P<0.05). Probably these results reflect a recovery of Bb-12 when it was
277
submitted to enteric phase 1 and 2 (pH 5 and 7, respectively). The hydrochloric acid present in the gastric
9
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phase resulted in an injury of Bb-12 cells, and their recovery through the microbiological analysis was
279
difficult. After 7 days, all margarines studied, except M5, presented an increase or maintenance in the Bb-12
280
populations until the end of the in vitro assays (6h). From day 7 to 14, a decrease in probiotic populations
281
was observed during the whole in vitro assay, but with counts always above 6.00 log cfu g-1, except for M2
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(1.20 cfu g-1 and of 1.98 log cfu g-1 after 2 and 6 hours).
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After 21 days of storage, most margarines presented probiotic populations below 6.00 log cfu g-1,
284
varying from 1.14 (M2) to 5.85 log cfu g-1 (M7) after 6h of the in vitro assay. M1 and M2 differed
285
significantly from the other formulations (P<0.05), since populations of, respectively, 7.15 cfu g-1 and 1.14
286
cfu g-1 were observed after 6h of the in vitro assays. At 28 days of storage, after 6h of in vitro assays, Bb-12
287
populations in M3 were significantly higher than in M4 (P<0.05). In margarine supplemented with inulin +
288
WPC (M4), a significantly increase in Bb-12 populations was observed between 4 and 6h of the in vitro
289
assay on day 7 (P<0.05).
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During the whole in vitro assays period, margarines supplemented with inulin presented lower
291
reductions in Bb-12 populations when compared to initial counts. As mentioned earlier, inulin protected
292
probiotic microorganism during the in vitro assays, since when mixed with water inulin forms a particle gel
293
network. This gel probably avoided the action of HCl and enzymes over Bb-12 during the in vitro assays.
294
Inulin assured probiotic viability in suitable concentrations for margarines M4, M5, M7, and especially for
295
M1 during storage. On day 28, by the end of in vitro assays (6h), inulin assured populations of 6.32 log cfu g-
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1
in M1.
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High reductions in probiotic viability after simulated gastric phase are expected results, since to
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reach the intestine, strains must first pass through the stomach, which provides a powerful barrier against the
299
entrance in the gut (Morelli, 2007). Similarly to what was observed in the present study, Hansen, Allan-
300
Wojtas, Jin, and Paulson (2002) reported a 1.3 log cfu g-1 decrease in B. animalis Bb-12 populations after
302 303 304
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exposure to pH 2.0 during 2 hours. Charteris, Kelly, Morelli, and Collins (1998) reported that milk proteins protected probiotic
Lactobacillus casei and Bifidobacterium lactis during simulated gastric transit. This was not observed here when whey protein concentrate was employed, since margarines supplemented with WPC solely did not
305
present suitable Bb-12 populations after 2, 4, and 6h of the in vitro assays during all the sampling periods.
306
Probiotic counts in M2 during shelf life were the lowest (P<0.05) (Table 4). This fact contributed towards
307
the unsatisfactory results observed after the in vitro assays of margarine M2. Different results were reported
308
by Kos, Šušković, Goreta, & Matošić (2000), regarding the addition of WPC. The authors observed that
309
WPC was an important protector for Lactobacillus acidophilus M92 exposed to simulated gastric and small
10
310
intestinal juices, whereas, in the present study, the addition of WPC did not protect Bb-12 and M2 presented
311
a progressive decrease in Bb-12 populations during the in vitro assays along storage. After 28 days, Bb-12
312
counts observed in all sampling periods of the in vitro assay of M2 were below the detection limits of the
313
method (<1.14 log cfu g-1).
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Guo, Wang, Yan, Chen, Liu, and Zhang (2009) observed that the incubation of B. animalis Bb-12 in
315
simulated gastric juice containing pepsin at pH 2.5 resulted in significant decreases in its survival rate. In the
316
present study, reductions observed in probiotic populations were lower, due to the presence of the food
317
matrix and its constituents, mainly its fat content, a factor that could affect probiotic growth and survival in
318
food during the digestive process (Ranadheera, Baines, & Adams, 2010).
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As observed in the present study, Buriti, Castro, and Saad (2010) reported that the supplementation of
320
synbiotic guava musses with inulin and WPC simultaneously did not influence L. acidophilus La-5
321
protection positively during in vitro resistance assays. However, in refrigerated synbiotic guava musses the
322
authors observed counts below 2.00 log cfu g-1 when products supplement with different percentages of
323
inulin (1.33%, 2% or 4%) where submitted to in vitro resistance assays after 28 days. Similarly, Bedani,
324
Rossi, and Saad (2013) observed that inulin did not protect La-5 in fermented soy product during in vitro
325
resistance assays, whereas B. animalis Bb-12 presented mean populations above 7.00 log cfu g-1 up to the
326
end of in vitro assays.
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The presence of inulin was important to protect Bb-12, since margarine with 3% of inulin (M1)
328
presented Bb-12 populations of 6.32 log cfu g-1 after 6h of in vitro assays. The survival rate of Bb-12 in M1
329
after in vitro assays was 91.33% and 78.51% after 7 and 28 days of storage, respectively. Similar results
330
regarding protection given by the prebiotic ingredient inulin, when combined with fructooligosacharide, to
331
Bb-12 during GI in vitro assays were reported by Padilha, Villarreal-Morales, Vieira, Costa, and Saad (2016)
332
in petit-suisse cheese. The authors observed mean Bb-12 survival rates of 79% in the synbiotic cheese,
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whereas this rate was reduced to 60% in the probiotic product. In order to verify the influence of inulin, WPC, and CMP on Bb-12 resistance, results obtained after
6h of the in vitro assays on day 21 were used, since the parameters mentioned previously regarding Bb-12 viability were observed. A quadratic model was generated for this variable response and it was statistically
337
significant (P < 0.01) and able to explain 98% of results (variation). Also, lack of fit was not statistically
338
significant (P=0.665). The model and its coefficients and quality analysis are presented in Table 5. The
339
contour plot generated from the quadratic model obtained for Bb-12 survival during in vitro assays is
340
presented in Fig. 3.
11
341
The quadratic model obtained revealed that probiotic Bb-12 survival was dependent on isolated
342
ingredients and some ingredients interactions. The higher viability of Bb-12 (>7.00 log cfu g-1) after the in
343
vitro tests was observed when inulin was added in concentrations varying between 3 and 2.25%. Similarly, a
344
satisfactory result was observed when margarine was supplemented with CMP, since concentrations between
345
3 and 2.25% resulted in Bb-12 populations between 5.25 and 6.25 log cfu g-1 after the entire in vitro assay
346
(6h). In contrast, WPC in the same concentrations resulted in Bb-12 populations below 4.25 log cfu g-1 after
347
6h of the in vitro assay.
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The conditions found in human gastrointestinal tract are hostile for probiotic microorganisms.
349
Nevertheless, the food matrix protects the cells, and avoids high reductions in probiotic populations (El-
350
Shafei, Tawfik, Dabiza, Sharaf, & Effat, 2010). Therefore, the food matrix and its composition are very
351
important for protecting probiotic strains. The fat content, the pH and the solid matrix, may protect probiotic
352
bacteria more efficiently than a fluid environment during storage of the food product and its transit through
353
the human gastrointestinal tract (Ranadheera, Baines, & Adams, 2010). In the present study, the solid matrix
354
and the fat present in margarine assured the survival of the probiotic strain Bb-12 during the in vitro
355
resistance assays. However, it is important to emphasize that high counts during the shelf life of a specific
356
product are necessary to obtain appropriate populations of probiotic viable cells by the end of the digestive
357
process.
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4. Conclusion
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The results obtained showed that the production of probiotic margarine with suitable populations of
362
B. animalis Bb-12, and without hydrogenation process, with palm and canola oil, is possible. The
363
supplementation of the water phase was very important, since the control margarine (without the addition of
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inulin, WPC, and/or CMP) presented very low and insufficient Bb-12 populations. The presence of inulin, especially in the proportion of 3% resulted in significant higher Bb-12 populations (P<0.05) and assured Bb12 resistance through the in vitro assays. Populations observed for margarines (except M2) by the end of in vitro assays (after 6h) revealed that recovery of Bb-12 viable cells in satisfactory populations was possible,
368
even after the digestive process. As far as we know, taken together, results on viability of B. animalis Bb-12
369
and on in vitro GI resistance of the strain incorporated in margarine produced with inulin were unique, when
370
compared to other probiotic products described in the scientific literature. Therefore, functional margarine
371
supplemented with a probiotic strain like B. animalis Bb-12 ought to be produced commercially, though the
372
addition of inulin is necessary to lead to promising probiotic potential.
12
373 374
ACCEPTED MANUSCRIPT Acknowledgments
375 The authors would like to thank Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
377
(Projects 07/59260-0 and 06/54843-5), and Conselho Nacional de Desenvolvimento Científico e Tecnológico
378
(CNPq) for financial support and fellowships. The authors would also like to thank Agropalma, Kerry Bio-
379
Science, DSM, Danisco, Fortitech, Purac Sínteses, Orafti, and Arla Foods, for providing part of the material
380
resources employed in this study. The authors gratefully acknowledge Regina Célia Cabral Estrotra for her
381
technical assistance.
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Table 1
2
Simplex-centroid experimental design employed in the present study. Quantities of each ingredient (%) CMP3 (x3)
0 3.0 0 1.5 0 1.5 1.0 -
0 0 3.0 0 1.5 1.5 1.0 -
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WPC2 (x2)
2
Whey protein concentrate (Arla Foods Ingredients, Sønderhøj, Denmark; 82% protein).
3
Caseinomacropeptide (Arla Foods Ingredients, 85% protein).
4
M8: control trial.
– = without inulin, WPC and/or CMP addition.
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8
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3 4 5 6 7
Proportion of ingredients in the mixture Inulin1 (x1) (x1, x2, x3) M1 (1, 0, 0) 3.0 M2 (0, 1, 0) 0 M3 (0, 0, 1) 0 M4 (½, ½, 0) 1.5 M5 (½, 0, ½) 1.5 M6 (0, ½, ½) 0 (⅓, ⅓, ⅓) 1.0 M7 M84 (0, 0, 0) 1 Inulin (Orafti, 92% inulin + 8% fructose, glucose, and sucrose).
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1
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Table 2
10
Ingredients used for the production of the margarine trials studied, according to the experimental design
11
described in Table 1. Margarine formulations Ingredients (%)
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60.000 3.400 0.001 0.050 0.880 3.000
Control trial.
**
33.999 0.760 0.010 0.400 0.500
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30.999 0.760 0.010 0.400 0.500
60.000 3.400 0.001 0.050 0.880 -
60% of palm oil (Agropalma, Tailândia, Brazil) + 40% of canola oil (Liza, Mairinque, Brazil).
***
Margarines M1 - M7 were supplemented with a mixture containing inulin, WPC, and/or CMP, according to
Table 1. 1
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– = without supplementation with inulin, WPC, and/or CMP. : (Cisne, Cabo Frio, Brazil); 2: (food-grade lactic acid 85% solution, Purac Sínteses, Rio de Janeiro, Brazil); 3:
(Nestlé, Araçatuba, Brazil); 4: (Christian Hansen, Hørsholm, Denmark);
5
(Kerry Bio-Science, Campinas,
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Brazil); 6: (β-carotene, DSM, São Paulo, Brazil); 7: (Danisco, Cotia, Brazil), 8: (Fortitech, Campinas, Brazil).
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*
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Water phase Water Salt1 Lactic acid2 Skimmed powdered milk3 Probiotic culture4 Fat phase Fat** Emulsifiers5 Colouring agent6 Butter flavour7 Vitamin A8 Mixture***
12 13 14 15 16 17 18 19
M8*
M1-M7
2
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Table 3
22
Populations (mean values1 ± standard deviation) of B. animalis Bb-12 (log cfu g-1) in margarines M1-M8 after 0, 1, 7, 14, 21, 28, and 35 days of storage
23
at 5±1°C. Margarines M2
M3
M4
M5
M6
M7
03
8.39±0.33BCab
8.24±0.14Ca
8.71±0.10Aa
8.49±0.11Ba
8.77±0.10Aa
8.42±0.14Ba
8.14±0.12Ca
1
8.77±0.24Aa
7.82±0.19Bb
8.60±0.16Aa
8.43±0.05Aa
8.42±0.09Aab
8.63±0.22Aa
8.44±0.14Aa
5.12±0.10Cb
7
8.19±0.23Bb
7.55±0.17Cb
8.36±0.15ABab
8.18±0.07Bb
8.55±0.18Aa
8.26±0.13ABb
8.29±0.12Ba
3.10±0.15Dc
14
8.54±0.01Aa
6.74±0.17Cc
8.19±0.08ABb
8.03±0.06Bb
8.16±0.10ABbc
8.27±0.13ABb
8.40±0.16Aa
-
21
8.23±0.20Aab
6.54±0.14Dc
8.07±0.21ABbc
7.62±0.08Cc
8.10±0.04ABc
8.03±0.15ABc
7.81±0.29BCb
-
28
8.05±0.04Ab
5.40±0.16Dd
7.64±0.03Bc
7.56±0.15Bcd
7.52±0.09Bd
7.62±0.12Bd
6.81±0.01Cc
-
35
8.01±0.22Ab
4.64±0.26De
6.87±0.52Bd
7.32±0.04Bd
7.29±0.23Bd
7.27±0.09Be
6.26±0.16Cd
-
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See Table 1 for description of trials M1-M8. n=6.
2
Control trial.
3
Day 0: counts observed in the same day of margarine production.
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A,B,C,D
8.52±0.07Ba
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(Days)
24 25 26 27 28 29 30
M82
M1
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Storage
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21
: For each day of storage, different capital letters in a row denote significant differences (P<0.05) between different trials.
a,b,c,d,e
: For each trial, different lowercase superscripts in a column denote significant differences (P<0.05) between different days of storage.
– = not detected.
31
3
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Table 4
33
Coefficients (b1, b2, b3) with their respective standard deviations, P values (model and lack of fit), and adjusted
34
R2 of the quadratic model obtained for B. animalis Bb-12 viability in margarines at 21 days of storage at 5±1°C.
35
Coefficients Inulin (b1) WPC (b2) CMP (b3) Inulin + WPC (b12) Inulin + CMP (b13) WPC + CMP (b23) P value P lack of fit Adjusted R2 n.s: non-significant.
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Values 8.26 (0.08) 6.61 (0.09) 8.03 (0.09) n.s n.s 2.72 (0.34) <0.01 0.065230 0.86
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4
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Table 5
40
Coefficients (b1, b2, b3) with their respective standard deviations, P values (model and lack of fit), and adjusted
41
R2 of the quadratic model obtained for B. animalis Bb-12 survival during in vitro tests at 21 days of storage at
42
5±1°C. Values 7.14 (0.12) 1.14 (0.07) 5.48 (0.08) 6.16 (0.48) -3.31 (0.39) 8.28 (0.34) <0.01 0.665 0.98
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Coefficients Inulin (b1) WPC (b2) CMP (b3) Inulin + WPC (b12) Inulin + CMP (b13) WPC + CMP (b23) P value P lack of fit Adjusted R2
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Figure caption
Figure 1. Contour plot showing the effect of inulin, whey protein concentrate (WPC), and
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caseinomacropeptide (CMP) on B. animalis Bb-12 viability (log cfu g-1) at 21 days of refrigerated storage.
Figure 2. Survival of B. animalis Bb-12 (log cfu g-1) in margarines M1-M7 submitted to in
at 5±1°C (a, b, c, and d, respectively) before ( )], and enteric [4h (
) and 6h (
) and during exposition to simulated gastric
)] conditions. A,B,C,D,E: different superscript capital
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[2h (
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vitro simulated gastrointestinal conditions after 7, 14, 21, and 28 days of refrigerated storage
letters denote significant differences between margarines for the same sampling period of the in vitro assay.
a,b,c
: different lowercase superscript letters denote significant differences
between the sampling periods of the in vitro assays for the same margarine. See Table 1 for
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description of margarines M1-M7.
Figure 3. Contour plot showing the effect of inulin, WPC, and CMP on B. animalis Bb-12
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resistance (log cfu g-1) during in vitro assays at 21 days of refrigerated storage.
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Figure 1
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B. animalis Bb-12 (log cfu g-1)
10
Ba
8
Aa
ABa
Ab Ab Ac
Bb
Bb BCb
6 4
ABa
Ba
Ca
Ba ABb Bb Ab
Ab ABb
BCb Cb c Cc
Bb Bb Cc
Cc
M4
M5
M6
Db Db Db
2 0 M1
M2
M3
M7
Aa
8
Ac
Ab
Ab
ABa Ab
Bb
Ab ABbCb
Db
Ab Bb Db
Cb Eb Bc
2 0 M1
M2
M3
M4
Ab Bb Db
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6 4
Aa
ABa
ABa
Ba
Ca
M5
M6
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B. animalis Bb-12 (log cfu g-1)
10
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Margarines
(a)
ABbc Bb Ac
M7
Margarines
10
Aa
8
ABa
Ab Ab Ab
4
M2
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(c)
Bb Cc Bb
Ba
Cc Cb Bbc
Bb Bb
M6
M7
Bb
M3
M4
M5
Margarines
10 8
Aa
Ba
Ba Bb
Da
6
Cb
Ba
Ba
Ab Ab Bb
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B. animalis Bb-12 (log cfu g-1)
BCb BCb Bb
Dc Db Cb
2 M1
Figure 2
ABa
ABa
Ca
Bb Bc CBc
6
0
(d)
Da
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B. animalis Bb-12 (log cfu g-1)
(b)
Bb Bb
Cc
Dc
Bc
Bc
Ca
Ab
Bb Cb
BCb Bb
Dc Ec
4 2 0
M1
M2
M3
M4
Margarines
M5
M6
M7
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Figure 3
ACCEPTED MANUSCRIPT Original manuscript “Margarine produced with inulin increases Bifidobacterium animalis Bb-12 gastrointestinal survival in vitro”, authors Cínthia Hoch Batista de Souza, Luiz Antonio Gioielli, and Susana Marta Isay Saad.
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Research Highlights
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Submission – LWT - Food Science and Technology
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Margarine with inulin, whey protein concentrate, and/or caseinomacropeptide at 3% was studied.
Viability and GI in vitro resistance of Bifidobacterium Bb-12 was evaluated Inulin improved Bb-12 survival in probiotic margarine during storage. Margarine with inulin improved Bb-12 resistance to in vitro GI assays.
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Inulin in the proportion of 3% resulted in significant higher Bb-12 survival.