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The determination of viable counts in probiotic cultures microencapsulated by spray-coating

机译:喷雾包衣微囊化益生菌培养物中活菌计数的测定

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An assessment of various methods to determine viable counts (CFU) in freeze-dried and dried micro-encapsulated (ME) probiotic cultures was carried out. Microencapsulation was done by spray-coating of dried Lactobacillus rhamnosus R0011 or Bifidobacterium longum ATCC 15708 cultures with fat Rehydra-tion of the ME powders was incomplete when they were added to water and gently agitated. As a result analytical methods based on vortexing of rehydrated ME cultures and which did not incorporate a high-shear homogenization (HSH) step underestimated the viable counts. The CFU of ME cultures were identical when methods using either blender or generator probes high-shear homogenization (HSH) were carried out. Furthermore HSH reduced the variability of the CFU results of both free-cell and ME cultures by a factor of three. The addition of an emulsifier (Tween 80) in the rehydrating medium to dissolve fat did not improve CFU counts when generator probes were used for HSH. The presence of fat in the ME product, or when added to the rehydration medium, improved CFU counts of B. longum but not of L. rhamnosus.
机译:对确定冻干和干燥的微囊化(ME)益生菌培养物中活菌计数(CFU)的各种方法进行了评估。通过将鼠李糖乳杆菌R0011或长双歧杆菌ATCC 15708培养物用脂肪喷雾包衣来完成微囊化。将ME粉末加到水中并轻轻搅动后,其水合不完全。结果,基于再水化的ME培养物涡旋的分析方法没有包括高剪切均质化(HSH)步骤,因此低估了可行的计数。当使用混合器或发生器探针进行高剪切均质化(HSH)的方法时,ME培养物的CFU相同。此外,HSH将游离细胞和ME培养物CFU结果的变异性降低了三倍。当将生成器探针用于HSH时,在补液介质中添加乳化剂(吐温80)以溶解脂肪不会提高CFU计数。 ME产品中存在脂肪,或者添加到补液介质中,可以提高长双歧杆菌的CFU计数,但不能提高鼠李糖乳杆菌的CFU计数。

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