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通过流式细胞术定量土壤细菌丰度的方法优化。

Optimization of a Method To Quantify Soil Bacterial Abundance by Flow Cytometry.

机构信息

Department of Ecology and Evolutionary Biology, University of California, Irvine, Irvine, California, USA.

Center for Environmental Biology, University of California, Irvine, Irvine, California, USA.

出版信息

mSphere. 2019 Oct 9;4(5):e00435-19. doi: 10.1128/mSphere.00435-19.

Abstract

Bacterial abundance is a fundamental metric for understanding the population dynamics of soil bacteria and their role in biogeochemical cycles. Despite its importance, methodological constraints hamper our ability to assess bacterial abundance in terrestrial environments. Here, we aimed to optimize the use of flow cytometry (FCM) to assay bacterial abundances in soil while providing a rigorous quantification of its limitations. Soil samples were spiked with to evaluate the levels of recovery efficiency among three extraction approaches. The optimized method added a surfactant (a tetrasodium pyrophosphate [TSP] buffer) to 0.1 g of soil, applied an intermediate degree of agitation through shaking, and used a Nycodenz density gradient to separate the cells from background debris. This procedure resulted in a high (average, 89%) level of cell recovery. Recovery efficiencies did not differ significantly among sites across an elevation gradient but were positively correlated with percent carbon in the soil samples. Estimated abundances were also highly repeatable between technical replicates. The method was applied to samples from two field studies and, in both cases, was sensitive enough to detect treatment and site differences in bacterial abundances. We conclude that FCM offers a fast and sensitive method to assay soil bacterial abundance from relatively small amounts of soil. Further work is needed to assay differential biases of the method across a wider range of soil types. The ability to quantify bacterial abundance is important for understanding the contributions of microbial communities in soils, but such assays remain difficult and time-consuming. Flow cytometry offers a fast and direct way to count bacterial cells, but several concerns remain in applying the technique to soils. This study aimed to improve the efficiency of the method for soil while quantifying its limitations. We demonstrated that an optimized procedure was sensitive enough to capture differences in bacterial abundances among treatments and ecosystems in two field studies.

摘要

细菌丰度是理解土壤细菌种群动态及其在生物地球化学循环中作用的基本指标。尽管它很重要,但方法上的限制阻碍了我们评估陆地环境中细菌丰度的能力。在这里,我们旨在优化使用流式细胞术(FCM)来测定土壤中的细菌丰度,同时对其局限性进行严格的量化。通过向土壤中添加[细菌丰度标准物质]来评估三种提取方法的回收率水平。优化的方法是在 0.1 克土壤中添加一种表面活性剂(四磷酸钠[TSP]缓冲液),通过振荡施加中等程度的搅拌,并使用 Nycodenz 密度梯度将细胞与背景碎片分离。该程序导致细胞回收率高(平均 89%)。回收率效率在不同海拔梯度的站点之间没有显著差异,但与土壤样品中的碳百分比呈正相关。在技术重复之间,估计的丰度也具有高度的可重复性。该方法应用于两项野外研究的样本中,在这两种情况下,该方法都足够灵敏,可以检测到细菌丰度的处理和地点差异。我们得出结论,FCM 提供了一种快速灵敏的方法,可以从小量土壤中测定土壤细菌丰度。需要进一步的工作来检测该方法在更广泛的土壤类型中的差异偏倚。定量细菌丰度对于理解微生物群落在土壤中的贡献很重要,但此类测定仍然困难且耗时。流式细胞术提供了一种快速直接的方法来计数细菌细胞,但在将该技术应用于土壤时仍然存在一些问题。本研究旨在提高该方法在土壤中的效率,同时量化其局限性。我们证明,一种优化的程序足够灵敏,可以捕捉到两个野外研究中处理和生态系统之间细菌丰度的差异。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/79cf/6796974/be54e5c918b9/mSphere.00435-19-f0001.jpg

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