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Impact of different water activities (aw) adjusted by solutes on high pressure high temperature inactivation of Bacillus amyloliquefaciens spores

机译:溶质调节的不同水分活度(aw)对解淀粉芽孢杆菌孢子的高压高温失活的影响

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摘要

Much research has been conducted to comprehend the mechanisms of high pressure (HP) inactivation of spores in aqueous systems but for food model systems these information are scarce. In these systems spores can interact with ingredients which then could possibly lead to retarded or reduced inactivation, which can cause a problem for the sterilization process. The protective mechanism of a reduced aw-value is still unclear. HP processing might prove valuable to overcome protective effects of solutes and achieve shorter process times for sterilization under HP. To gain insight into the underlying mechanisms five aw-values (0.9, 0.92, 0.94, 0.96, 1) were adjusted with two different solutes (NaCl, sucrose). Solutions were inoculated with spores of Bacillus amyloliquefaciens and treated at 105, 110, and 115°C at 600 MPa. Further a thermal inactivation was conducted at the same temperatures for a comparison with the HP data. Afterward, the influence of HP high temperature treatment on the inactivation, the dipicolinic acid (DPA)-release and membrane constitution was assessed by plate count, HPLC and flow cytometry (FCM). The results show that during HP treatments sucrose and salt both have a protective effect, in which the influence of sucrose on the retarded inactivation is higher. The threshold water activities (aw), which is 0.94, here salt and sucrose have a significant influence on the inactivation. The comparison of thermal (105–115°C) and HP and high temperature (600 MPa, 105–115°C) treated samples showed that the time needed to achieve a 4–5 log10 inactivation is reduced from 45 (aw = 1) to 75 (aw = 0.9) min at 105°C to 3 (aw = 1) to 15 (aw = 0.9) minutes at 600 MPa and 105°C. The release of DPA is the rate limiting step of the inactivation and therefore monitoring the release is of great interest. The DPA-release is slowed down in high concentrated solutions (e.g., sucrose, salt) in comparison to aw 1. Since there is a difference in the way the solutes protect the spore it could be seen as an inner spore membrane effect. Maybe as shown for vegetative microorganism the solutes can interact with membranes, e.g., the inner spore membrane. Flow cytometry (FCM) measurement data show a similar trend.
机译:已经进行了许多研究来理解含水系统中孢子的高压(HP)灭活机理,但是对于食品模型系统而言,这些信息很少。在这些系统中,孢子会与成分发生相互作用,从而可能导致灭活的延迟或减少,从而给灭菌过程带来麻烦。降低aw值的保护机制仍不清楚。 HP处理可能被证明对克服溶质的保护作用和缩短HP处理时间是很有价值的。为了深入了解潜在的机理,用两种不同的溶质(NaCl,蔗糖)调节了五个aw值(0.9、0.92、0.94、0.96、1)。用解淀粉芽孢杆菌的孢子接种溶液,并在105、110和115℃下在600MPa下处理。进一步在相同温度下进行热灭活以与HP数据进行比较。然后,通过平板计数,HPLC和流式细胞术(FCM)评估了HP高温处理对失活,二吡啶甲酸(DPA)释放和膜组成的影响。结果表明,在高压处理过程中,蔗糖和盐都具有保护作用,其中蔗糖对延迟失活的影响更高。水分活度阈值(aw)为0.94,此处的盐和蔗糖对失活有重要影响。热(105–115°C)和高压与高温(600 MPa,105–115°C)处理的样品的比较显示,实现4–5 log10灭活所需的时间从45(aw = 1)减少了在105°C下至75(aw = 0.9)分钟;在600 MPa和105°C下为3(aw = 1)至15(aw = 0.9)分钟。 DPA的释放是失活的速率限制步骤,因此监控释放非常重要。与aw 1相比,在高浓度溶液(例如蔗糖,盐)中,DPA的释放速度减慢。由于溶质保护孢子的方式有所不同,因此可以将其视为内部孢子膜效应。如对于营养微生物所示,溶质可以与膜例如内孢子膜相互作用。流式细胞仪(FCM)的测量数据显示了类似的趋势。

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