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利用拉曼镊子、微分干涉对比显微镜和核酸染料荧光显微镜监测芽孢杆菌属单孢子的湿热失活动力学。

Monitoring the wet-heat inactivation dynamics of single spores of Bacillus species by using Raman tweezers, differential interference contrast microscopy, and nucleic acid dye fluorescence microscopy.

机构信息

Department of Physics, East Carolina University, Greenville, NC 27858-4353, USA.

出版信息

Appl Environ Microbiol. 2011 Jul;77(14):4754-69. doi: 10.1128/AEM.00194-11. Epub 2011 May 20.

DOI:10.1128/AEM.00194-11
PMID:21602365
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3147409/
Abstract

Dynamic processes during wet-heat treatment of individual spores of Bacillus cereus, Bacillus megaterium, and Bacillus subtilis at 80 to 90°C were investigated using dual-trap Raman spectroscopy, differential interference contrast (DIC) microscopy, and nucleic acid stain (SYTO 16) fluorescence microscopy. During spore wet-heat treatment, while the spores' 1:1 chelate of Ca(2+) with dipicolinic acid (CaDPA) was released rapidly at a highly variable time T(lag), the levels of spore nucleic acids remained nearly unchanged, and the T(lag) times for individual spores from the same preparation were increased somewhat as spore levels of CaDPA increased. The brightness of the spores' DIC image decreased by ~50% in parallel with CaDPA release, and there was no spore cortex hydrolysis observed. The lateral diameters of the spores' DIC image and SYTO 16 fluorescence image also decreased in parallel with CaDPA release. The SYTO 16 fluorescence intensity began to increase during wet-heat treatment at a time before T(lag) and reached maximum at a time slightly later than T(release). However, the fluorescence intensities of wet-heat-inactivated spores were ~15-fold lower than those of nutrient-germinated spores, and this low SYTO 16 fluorescence intensity may be due in part to the low permeability of the dormant spores' inner membranes to SYTO 16 and in part to nucleic acid denaturation during the wet-heat treatment.

摘要

采用双捕集拉曼光谱、微分干涉对比(DIC)显微镜和核酸染料(SYTO 16)荧光显微镜研究了 80-90°C 下单个蜡状芽孢杆菌、巨大芽孢杆菌和枯草芽孢杆菌孢子湿热处理过程中的动态变化。在孢子湿热处理过程中,当孢子中 1:1 的钙(Ca 2+ )与二吡啶羧酸(CaDPA)螯合物快速释放时,其孢子核酸水平几乎保持不变,且随着 CaDPA 含量的增加,同一批次中各孢子的 T lag 时间略有增加。DIC 图像中孢子的亮度随着 CaDPA 的释放而降低约 50%,且未观察到孢子皮层水解。DIC 图像和 SYTO 16 荧光图像的孢子横向直径也随着 CaDPA 的释放而平行减小。SYTO 16 荧光强度在 T lag 之前的某个时间点开始随着湿热处理而增加,并在稍晚于 T release 的时间点达到最大值。然而,湿热失活孢子的荧光强度比营养发芽孢子低约 15 倍,这种低 SYTO 16 荧光强度可能部分归因于休眠孢子内膜对 SYTO 16 的低渗透性,部分归因于湿热处理过程中核酸变性。

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