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Comparison of methods for detection and enumeration of airborne microorganisms collected by liquid impingement.

机译:比较液体撞击收集的空气传播微生物的检测和计数方法。

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摘要

Bacterial agents and cell components can be spread as bioaerosols, producing infections and asthmatic problems. This study compares four methods for the detection and enumeration of aerosolized bacteria collected in an AGI-30 impinger. Changes in the total and viable concentrations of Pseudomonas fluorescens in the collection fluid with respect to time of impingement were determined. Two direct microscopic methods (acridine orange and BacLight) and aerodynamic aerosol-size spectrometry (Aerosizer) were employed to measure the total bacterial cell concentrations in the impinger collection fluid and the air, respectively. These data were compared with plate counts on selective (MacConkey agar) and nonselective (Trypticase soy agar) media, and the percentages of culturable cells in the collection fluid and the bacterial injury response to the impingement process were determined'. The bacterial collection rate was found to be relatively unchanged during 60 min of impingement. The aerosol measurements indicated an increased amount of cell fragments upstream of the impinger due to continuous bacterial nebulization. Some of the bacterial clusters, present in the air upstream of the impinger, deagglomerated during impingement, thus increasing the total bacterial count by both direct microscopic methods. The BacLight staining technique was also used to determine the changes in viable bacterial concentration during the impingement process. The percentage of viable bacteria, determined as a ratio of BacLight live to total counts was only 20% after 60 min of sampling. High counts on Trypticase soy agar indicated that most of the injured cells could recover. On the other hand, the counts from the MacConkey agar were very low, indicating that most of the cells were structurally damaged in the impinger. The comparison of data on the percentage of injured bacteria obtained by the traditional plate count with the data on percentage of nonviable bacteria obtained by the BacLight method showed good agreement.
机译:细菌剂和细胞成分可作为生物气溶胶传播,产生感染和哮喘病。这项研究比较了四种检测和枚举AGI-30冲击器中雾化细菌的方法。确定了收集液中荧光假单胞菌总浓度和可行浓度随撞击时间的变化。两种直接的显微镜方法(ac啶橙和BacLight)和空气动力学气溶胶尺寸光谱法(Aerosizer)被用来分别测量撞击收集器液体和空气中细菌细胞的总浓度。将这些数据与选择性培养基(MacConkey琼脂)和非选择性培养基(胰蛋白酶大豆琼脂)上的平板计数进行比较,确定收集液中可培养细胞的百分比以及细菌对撞击过程的伤害反应。发现在撞击60分钟期间细菌收集率相对不变。气雾剂测量表明由于连续细菌雾化,冲击器上游的细胞碎片数量增加。撞击器上游空气中存在的某些细菌簇在撞击过程中会解聚,从而通过两种直接显微镜方法都增加了细菌总数。 BacLight染色技术还用于确定撞击过程中活菌浓度的变化。采样60分钟后,以BacLight活菌占总数的比例确定的活菌百分比仅为20%。胰蛋白酶大豆琼脂的高计数表明大多数受损细胞可以恢复。另一方面,MacConkey琼脂的计数非常低,表明大多数细胞在撞击器中受到结构性破坏。通过传统平板计数获得的受伤细菌百分比数据与通过BacLight方法获得的非活细菌百分比数据的比较显示出很好的一致性。

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