首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Colony formation by sublethally heat-injured Zygosaccharomyces rouxii as affected by solutes in the recovery medium and procedure for sterilizing medium.
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Colony formation by sublethally heat-injured Zygosaccharomyces rouxii as affected by solutes in the recovery medium and procedure for sterilizing medium.

机译:在恢复培养基中溶质的影响下肉豆蔻热损伤的合子酵母菌落形成菌落并进行灭菌步骤。

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摘要

Recovery and colony formation by healthy and sublethally heat-injured cells of Zygosaccharomyces rouxii as influenced by the procedure for sterilizing recovery media (YM agar [YMA], wort agar, cornmeal agar, and oatmeal agar) were investigated. Media were supplemented with various concentrations of glucose, sucrose, glycerol, or sorbitol and sterilized by autoclaving (110 degrees C, 15 min) and by repeated treatment with steam (100 degrees C). An increase in sensitivity was observed when heat-injured cells were plated on glucose-supplemented YMA at an aw of 0.880 compared with aws of 0.933 and 0.998. Colonies which developed from unheated and heated cells on YMA at aws of 0.998 and 0.933 generally exceeded 0.5 mm in diameter within 3.5 to 4 days of incubation at 25 degrees C, whereas colonies formed on YMA at an aw of 0.880 typically did not exceed 0.5 mm in diameter until after 5.5 to 6.5 days of incubation. The number of colonies exceeding 0.5 mm in diameter which were formed by heat-injured cells on YMA at an aw of 0.880 was 2 to 3 logs less than the total number of colonies detected, i.e., on YMA at an aw of 0.933 and using no limits of exclusion based on colony diameter. A substantial portion of cells which survived heat treatment were sublethally injured as evidenced by increased sensitivity to a suboptimum aw (0.880). In no instance was recovery of Z. rouxii significantly affected by medium sterilization procedure when glucose or sorbitol was used as the aw-suppressing solute.(ABSTRACT TRUNCATED AT 250 WORDS)
机译:研究了健康和致死性损伤的鲁氏酵母菌的恢复和集落形成,该过程受灭菌培养基(YM琼脂[YMA],麦芽汁琼脂,玉米面琼脂和燕麦片琼脂)灭菌程序的影响。向培养基中补充各种浓度的葡萄糖,蔗糖,甘油或山梨糖醇,并通过高压灭菌(110摄氏度,15分钟)和蒸汽重复处理(100摄氏度)进行灭菌。当将热损伤的细胞以0.880的aw接种到补充了葡萄糖的YMA上时,灵敏度从0.933和0.998的aw上提高了。在25℃孵育3.5至4天内,在0.998和0.933的aws下从YMA上未加热和加热的细胞形成的菌落直径通常超过0.5 mm,而在aw为0.880的aaw上在YMA上形成的菌落通常不超过0.5 mm直到培养5.5到6.5天后再进行培养。由热损伤细胞在aw为0.880时在YMA上形成的直径超过0.5毫米的菌落数比检测到的菌落总数少2至3个对数,即在aw为0.933且不使用a基于菌落直径的排斥极限。对亚最佳aw(0.880)的敏感性增加证明,大部分在热处理后存活的细胞都受到了致命的皮下损伤。当使用葡萄糖或山梨糖醇作为抑制aw的溶质时,中等灭菌程序绝不会对鲁氏沼虾的恢复产生显着影响(摘要截断为250个单词)

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