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Comparison of New and Traditional Culture-Dependent Media for Enumerating Foodborne Yeasts and Molds

机译:比较新的和传统的依赖文化的媒介来计数食源性酵母菌和霉菌

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摘要

Fifty-six foods and food ingredients were analyzed for populations of naturally occurring yeasts and molds using Petrifilm rapid yeast and mold (RYM) count plates, Petrifilm yeast and mold (YM) count plates, dichloran rose bengal chloramphenicol (DRBC) agar plates, acidified potato dextrose agar (APDA) plates, and dichloran 18% glycerol (DG18) agar plates. Colonies were counted after incubating plates for 48, 72, and 120 h at 25℃. Of 56 foods in which either yeasts or molds were detected on at least one medium incubated for 120 h, neither yeasts nor molds were detected in 55.4, 73.2, 21.4, 19.6, and 71.4% of foods plated on the five respective media and incubated for 48 h; 10.7, 14.3, 3.6, 1.8, and 19.6% of foods were negative after 72 h, and 3.6, 1.8,0,0, and 0% of foods were negative after 120 h. Considering all enumeration media, correlation coefficients were 0.03 to 0.97 at 48 h of incubation; these values increased to 0.75 to 0.99 at 120 h. Coefficients of variation for total yeasts and molds were as high as 30.0, 30.8, and 27.2% at 48, 72, and 120 h, respectively. The general order of performance was DRBC = APDA > RYM Petrifilm > YM Petrifilm > DG18 when plates were incubated for 48 h, DRBC > APDA > RYM Petrifilm > YM Petrifilm > DG18 when plates were incubated for 72 h, and DRBC > APDA > RYM Petrifilm = YM Petrifilm > DG18 when plates were incubated for 120 h. Differences in performance among media are attributed to the diversity of yeasts and molds likely to be present in test foods and differences in nutrient, pH, and water activity requirements for resuscitation of stressed cells and colony development.
机译:使用Petrifilm快速酵母和霉菌(RYM)计数板,Petrifilm酵母和霉菌(YM)计数板,二氯甲烷玫瑰孟加拉氯霉素(DRBC)琼脂板(酸化)对56种食品和食品成分进行了自然酵母和霉菌种群分析马铃薯右旋糖琼脂(APDA)平板和二氯氯丹18%甘油(DG18)琼脂平板。在25℃孵育平板48、72和120小时后,对菌落计数。在至少一种培养120小时的培养基中检测到酵母或霉菌的56种食物中,分别在5种,53.2%,73.2%,21.4%,19.6%和71.4%的食物中分别检测到酵母和霉菌,并分别孵育了5种。 48小时; 72小时后,分别有10.7、14.3、3.6、1.8和19.6%的食物为阴性,而120小时后为3.6、1.8、0、0和0%的食物为阴性。考虑所有计数介质,孵育48小时的相关系数为0.03至0.97;这些值在120 h时增加到0.75至0.99。在48、72和120 h时,总酵母和霉菌的变异系数分别高达30.0%,30.8和27.2%。一般性能顺序为:DRBC = APDA> RYM Petrifilm> YM Petrifilm> DG18平板孵育48小时,DRBC> APDA> RYM Petrifilm> YM Petrifilm> DG18平板孵育72 h,DRBC> APDA> RYM培养板孵育120小时后,Petrifilm = YM Petrifilm> DG18。培养基之间性能的差异归因于受试食品中可能存在的酵母和霉菌的多样性,以及用于应激细胞复苏和菌落发育的营养,pH和水分活度要求的差异。

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  • 来源
    《Journal of food protection》 |2016年第1期|95-111|共17页
  • 作者单位

    Center for Food Safety and Department of Food Science and Technology, University of Georgia, 1109 Experiment Street, Griffin, Georgia 30223-1797, USA;

    Center for Food Safety and Department of Food Science and Technology, University of Georgia, 1109 Experiment Street, Griffin, Georgia 30223-1797, USA;

  • 收录信息 美国《科学引文索引》(SCI);美国《化学文摘》(CA);
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

  • 入库时间 2022-08-17 23:24:43

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