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向超临界二氧化碳中添加乙醇可增强 Bacillus cereus 生物膜中细菌孢子的失活动能。

Addition of ethanol to supercritical carbon dioxide enhances the inactivation of bacterial spores in the biofilm of Bacillus cereus.

机构信息

Department of Biotechnology, Korea University Graduate School, Seoul 136-713, Republic of Korea.

出版信息

Int J Food Microbiol. 2013 Sep 2;166(2):207-12. doi: 10.1016/j.ijfoodmicro.2013.07.015. Epub 2013 Jul 21.

Abstract

Supercritical carbon dioxide (SC-CO2) was used to inactivate Bacillus cereus spores inside biofilms, which were grown on stainless steel. SC-CO2 treatment was tested using various conditions, such as pressure treatment (10-30 MPa), temperature (35-60°C), and time (10-120 min). B. cereus vegetative cells in the biofilm were completely inactivated by treatment with SC-CO2 at 10 MPa and at 35°C for 5 min. However, SC-CO2 alone did not inactivate spores in biofilm even after the treatment time was extended to 120 min. When ethanol was used as a cosolvent with SC-CO2 in the SC-CO2 treatment using only 2-10 ml of ethanol in 100ml of SC-CO2 vessel for 60-90 min of treatment time at 10 MPa and 60°C, B. cereus spores in the biofilm were found to be completely inactivated in the colony-forming test. We also assessed the viability of SC-CO2-treated bacterial spores and vegetative cells in the biofilm by staining with SYTO 9 and propidium iodide. The membrane integrity of the vegetative cells was completely lost, while the integrity of the membrane was still maintained in most spores. However, when SC-CO2 along with ethanol was used, both vegetative cells and spores lost their membrane integrity, indicating that the use of ethanol as a cosolvent with SC-CO2 is efficient in inactivating the bacterial spores in the biofilm.

摘要

超临界二氧化碳(SC-CO2)被用于灭活不锈钢上生物膜内的蜡状芽孢杆菌孢子。使用不同的条件测试了 SC-CO2 处理,例如压力处理(10-30 MPa)、温度(35-60°C)和时间(10-120 min)。在 10 MPa 和 35°C 下用 SC-CO2 处理 5 min,可完全杀死生物膜中的蜡状芽孢杆菌营养细胞。然而,即使处理时间延长至 120 min,单独的 SC-CO2 也不能杀死生物膜中的孢子。当乙醇作为 SC-CO2 的共溶剂,在 10 MPa 和 60°C 下用 100ml 的 SC-CO2 容器中仅用 2-10ml 的乙醇处理 60-90 min 时,生物膜中的蜡状芽孢杆菌孢子在集落形成试验中被完全杀死。我们还通过用 SYTO 9 和碘化丙啶染色评估了 SC-CO2 处理后的生物膜中细菌孢子和营养细胞的活力。营养细胞的膜完整性完全丧失,而大多数孢子的膜完整性仍得以维持。然而,当使用 SC-CO2 与乙醇时,营养细胞和孢子都失去了膜完整性,表明将乙醇用作 SC-CO2 的共溶剂可有效地灭活生物膜中的细菌孢子。

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