Exploring the lag phase and growth initiation of a yeast culture by means of an individual-based model

Gisbert, Marta Ginovart; Prats, Clara; Portell, Xavier; Silbert, M.

doi:10.1016/j.fm.2010.05.004

Cited by 27 publications

(30 citation statements)

References 36 publications

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“…It is known that temperature is one of the most critical factors influencing the industrial fermentation, including specific growth rate and biomass yield. [17,18] Figure 1(B) shows that the maximal yeast count (1.01£10 9 CFU/g) was obtained at 30 C. After that, with increasing the temperature, the yeast count decreased rapidly. Thus, 30 C was defined as the optimal temperature.…”

Section: Single-factor Experimentsmentioning

confidence: 93%

Optimization ofSaccharomyces boulardiiproduction in solid-state fermentation with response surface methodology

Qin

Zhan³

et al. 2015

Biotechnology & Biotechnological Equipment

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Saccharomyces boulardii preparations are promising probiotics and clinical agents for animals and humans. This work focused on optimizing the nutritional conditions for the production of S. boulardii in solid-state fermentation by using classical and statistical methods. In single-factor experiments, the S. boulardii production was significantly increased by the addition of glucoamylase and the optimal carbon and nitrogen sources were found to be soluble starch and NH 4 Cl, respectively. The effects of the glucoamylase, soluble starch and NH 4 Cl on S. boulardii production were evaluated by a three-level three-factor BoxÀBehnken design and response surface methodology (RSM). The maximal yeast count (4.50 £10 9 CFU/g) was obtained under the optimized conditions (198 U/g glucoamylase, 2.37% soluble starch and 0.9% NH 4 Cl), which was in a good agreement with the predicted value of the model. This study has provided useful information on how to improve the accumulation of yeast cells by RSM.

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Section: Single-factor Experimentsmentioning

confidence: 93%

Optimization ofSaccharomyces boulardiiproduction in solid-state fermentation with response surface methodology

Qin

Zhan³

et al. 2015

Biotechnology & Biotechnological Equipment

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“…For this study, we used INDISIM-YEAST as the individual-based simulator, which is based on the generic simulator INDISIM [9,[11][12][13][14]. Although the reader can refer to some previously published papers for a description of different parts of INDISIM-YEAST [11,12], a formal and brief description of this simulation model is presented below in order to make this study more self-contained and autonomous.…”

Section: Methodsmentioning

confidence: 99%

“…This is a proof of the ability of INDISIM-YEAST to distinguish differences in the evolution of a population that emerges from small inocula with different age structures. In fact, it is particularly useful in the study of small inocula during the initial steps of growth because of the large influence of the discrete and asymmetrical nature of yeast cellular division [13]. It is here that this model has an edge over top-down continuous models, which are useful when the initial population contains a large number of cells and the interest is the inspection of average behaviours exhibited by those cells.…”

Section: Initial Growth Of the Yeast Populationmentioning

confidence: 99%

“…INDISIM-YEAST constitutes the adaptation of INDISIM to the study of the specific characteristics of the yeast cell cycle, and is designed to deal with yeast populations growing in liquid media [11,12]. Recently, this simulator was used to study the influence of cell ageing and inoculum size on the lag phase and first division time of a yeast culture [13]. The aim of this contribution is to explore, by means of the simulator INDISIM-YEAST, the effects of inoculum size and cell genealogical age on the dynamics of yeast fermentation, focussing on: (1) the first stages of yeast population growth, (2) the mean biomass evolution of the population, (3) the rate of glucose uptake and ethanol production, and (4) the biomass and genealogical age distributions, in order to be able to integrate these results and to advance understanding of the composition of yeast populations and their temporal evolution in beer fermentations.…”

Section: Introductionmentioning

confidence: 99%

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Analysis of the effect of inoculum characteristics on the first stages of a growing yeast population in beer fermentations by means of an individual-based model

Gisbert

Prats

Portell

et al. 2010

J Ind Microbiol Biotechnol

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The yeast Saccharomyces cerevisiae has a limited replicative lifespan. The cell mass at division is partitioned unequally between a larger, old parent cell and a smaller, new daughter cell. Industrial beer fermentations maintain and reuse yeast. At the end of fermentation a portion of the yeast is 'cropped' from the vessel for 'serial repitching'. Harvesting yeast may select a population with an imbalance of young and aged individuals, but the output of any bioprocess is dependent on the physiology of each single cell in the population. Unlike continuous models, individual-based modelling is an approach that considers each microbe as an individual, a unique and discrete entity, with characteristics that change throughout its life. The aim of this contribution is to explore, by means of individual-based simulations, the effects of inoculum size and cell genealogical age on the dynamics of virtual yeast fermentation, focussing on: (1) the first stages of population growth, (2) the mean biomass evolution of the population, (3) the rate of glucose uptake and ethanol production, and (4) the biomass and genealogical age distributions. The ultimate goal is to integrate these results in order to make progress in the understanding of the composition of yeast populations and their temporal evolution in beer fermentations. Simulation results show that there is a clear influence of these initial features of the inocula on the subsequent growth dynamics. By contrasting both the individual and global properties of yeast cells and populations, we gain insight into the interrelation between these two types of data, which helps us to deal with the macroscopic behaviour observed in experimental research.

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“…Furthermore, the exhaustion of utilisable carbon dioxide (Sezonov, Joseleau-Petit, & D'Ari, 2007) in the fermentation pots (18 mL in 50 mL), where cells are increasing in number, may also explain entry into the stationary phase of growth, although L. plantarum strains isolated from fermented maize porridges have been found to withstand low pH (2.5) (Kalui, Mathara, Kutima, Kiiyukia, & Wongo, 2009). The absence of lag time could be influenced by several factors such as the inoculum quantity, the environmental conditions of the original and the new growth medium, the growth stage of the microorganisms during the time of inoculation (Ginovart, Prats, Portell, & Silbert, 2011;Swinnen, Bernaerts, Dens, Geeraerd, & Van Impe, 2004) and probably the investigation period. The L. plantarum strains and the yeasts were suspended in PBS at an active growth stage and inoculated into the maize slurry environment that had enough nutrients to support their growth.…”

Section: Microbial Growthmentioning

confidence: 99%

Fermentation and antimicrobial characteristics of Lactobacillus plantarum and Candida tropicalis from Nigerian fermented maize (akamu)

2014

IJFS

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This study investigated the ability of Lactobacillus plantarum strains (NGL5 and NGL7) and Candida tropicalis (NGY1) previously identified from akamu-a Nigerian fermented maize food with probiotic L. plantarum LpTx and Saccharomyces boulardii SB20 to ferment ground maize slurries based on pH, acidity, microbial biomass, levels of sugars and organic acids, and their antimicrobial activity against Salmonella enterica serovar Enteritidis NCTC 5188, Escherichia coli NCTC 11560, Bacillus cereus NCIMB 11925, Staphylococcus aureus NCTC 3750 and Listeria monocytogenes NCTC 7973 using an agar spot assay. L. plantarum strains either as single or mixed starter cultures with the yeasts had growth rates ≥0.15 h −1 , with pH significantly (p≤0.05) decreased to ≤3.93 after 12 h and then to ≤3.52 after 72 h and lactic acid >84 mmol L −1 . The yeasts had growth rates ≥0.18 h −1 but pH was ≥4.57 with lactic acid levels ≤20.23 mmol L −1 after 72 h in the single culture fermentation. There was no inhibition in modified MRS agar: 0.2% glucose and 0.2% glucose without Tween 80. Inhibition halos in MRS agar varied from 10.6 to 23.9 mm. S. bourladii was more inhibitory towards L. monocytogenes (8.6 mm) and B. cereus (5.4 mm ) than was C. tropicalis (1.1 and 3.3 mm for L. monocytogenes NCTC 7973 and B. cereus NCIMB 11925 respectively) (0.9 mm) in malt extract agar. This study showed that C. tropicalis was less inhibitory to the pathogens while antimicrobial activities of the L. plantarum strains were mainly due to acidity and the L. plantarum strains either as single or mixed cultures with the yeasts demonstrated strong fermentation ability, with significant decrease in pH which is vital in the choice of starter for product safety.

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Exploring the lag phase and growth initiation of a yeast culture by means of an individual-based model

Cited by 27 publications

References 36 publications

Optimization ofSaccharomyces boulardiiproduction in solid-state fermentation with response surface methodology

Optimization ofSaccharomyces boulardiiproduction in solid-state fermentation with response surface methodology

Analysis of the effect of inoculum characteristics on the first stages of a growing yeast population in beer fermentations by means of an individual-based model

Fermentation and antimicrobial characteristics of Lactobacillus plantarum and Candida tropicalis from Nigerian fermented maize (akamu)

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