Browsing by Author "Poddar, Devastotra"
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- ItemStability of the probiotic Lactobacillus paracasei CRL 431 under different environmental conditions : a thesis presented in partial fulfilment of the requirements for the degree of Doctor of Philosophy in Food Technology at Massey University, Manawatu, New Zealand(Massey University, 2015) Poddar, DevastotraProbiotics are live microorganisms which provide health benefits to the host upon consumption. There is a wealth of information available on the health benefits associated with the consumption of probiotics. However, currently probiotic microorganisms are delivered mainly through refrigerated, short shelf-life products. When incorporated into ambient shelf-life products, the products generally fail to meet the regulatory criteria, which require probiotic bacteria to be viable in high numbers at the end of shelf-life. Storage temperature, oxygen and residual moisture content often result in loss of viability of probiotics during storage and distribution. A preliminary study was carried out to explore the effects of matrix composition (fat, protein and carbohydrate) on the probiotic bacterial (Lactobacillus paracasei CRL 431) viability, during fluidized bed drying and subsequent storage. The finding suggests that whole milk powder provided a superior protection to bacteria during fluidized bed drying and subsequent storage, compared to skim milk powder or milk protein isolate. Moreover, water activity of the powders during storage played a key role in determining the probiotic viability. The effects of drying techniques, moisture content and water activity on the storage stability of L. paracasei in a whole milk matrix were studied. Whole milk powder-bacteria mixtures were dried using spray drying, freeze drying or fluidized bed drying and stored at 25 ÂșC under controlled water activity ( 0.11 aw, 0.33 aw and 0.52 aw) for 105 days. At 0.11 aw, cell viability loss was minimal, while at 0.52 aw viability was lost in all powders within 22 days. At the intermediate 0.33 aw, there were marked differences among stored powders. Further, various analytical techniques (X-ray diffraction, FT-IR, Raman, NMR spectroscopy) were used to explore why and how structural differences in the matrix-bacteria mixtures, produced using different drying technologies, under different water activity storage conditions, influence bacterial viability. The results suggest that fluidized bed drying provided a better protection to the bacteria during storage, which was attributed to unique powder structure that reduced the absorption of water. The lower absorption of water resulted in the maintenance of a more rigid structure, which limited molecular mobility. Lactobacillus sp. is known to accumulate large amounts of inorganic manganese which apparently provides defense against oxidative damage by scavenging free radicals. The ability of L. paracasei to maintain viability during long term ambient storage may be enhanced by the ability of microorganism to accumulate manganese, which may act as free radical scavenger. To investigate this hypothesis, X-ray fluorescent microscopy (XFM) was employed to determine the changes in the elemental composition of L. paracasei during growth in MRS medium with or without manganese as a function of physiological growth state (early log vs. stationary phase). The results revealed that lower level of manganese accumulation occurred during the early log phase of bacterial growth compared with the stationary phase cells. The lower level of manganese accumulation was found to be related to the loss in bacterial viability during storage. Manganese has been known to possess pro- and anti-oxidant properties, and understanding of the changes in the manganese oxidation state was considered to provide some further insights into the bacterial death mechanisms. In view of the relatively high concentration of manganese in lactobacilli, it was of interest to better understand the oxidation state, coordination number and ligands of the manganese in the bacteria. It was possible to characterize the changes of manganese within bacteria using XANES. The results confirmed that manganese present within L. paracasei is in Mn(II) oxidation state and no changes in the manganese ligands could be observed during storage. In summary, the thesis provides a mechanistic insight into the ways to improve the stability of probiotics for application into ambient long shelf-life products. Future studies on tracking the genetic and proteomic aspects of the bacteria during storage might be useful for further understanding and process optimization.