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定量稳定同位素探测中的测量误差与分辨率:对实验设计的影响

Measurement Error and Resolution in Quantitative Stable Isotope Probing: Implications for Experimental Design.

作者信息

Sieradzki Ella T, Koch Benjamin J, Greenlon Alex, Sachdeva Rohan, Malmstrom Rex R, Mau Rebecca L, Blazewicz Steven J, Firestone Mary K, Hofmockel Kirsten S, Schwartz Egbert, Hungate Bruce A, Pett-Ridge Jennifer

机构信息

University of California Berkeley, Environmental Science and Policy Management, Berkeley, California, USA.

Center for Ecosystem Science and Society, Northern Arizona University, Flagstaff, Arizona, USA.

出版信息

mSystems. 2020 Jul 21;5(4):e00151-20. doi: 10.1128/mSystems.00151-20.

Abstract

Quantitative stable isotope probing (qSIP) estimates isotope tracer incorporation into DNA of individual microbes and can link microbial biodiversity and biogeochemistry in complex communities. As with any quantitative estimation technique, qSIP involves measurement error, and a fuller understanding of error, precision, and statistical power benefits qSIP experimental design and data interpretation. We used several qSIP data sets-from soil and seawater microbiomes-to evaluate how variance in isotope incorporation estimates depends on organism abundance and resolution of the density fractionation scheme. We assessed statistical power for replicated qSIP studies, plus sensitivity and specificity for unreplicated designs. As a taxon's abundance increases, the variance of its weighted mean density declines. Nine fractions appear to be a reasonable trade-off between cost and precision for most qSIP applications. Increasing the number of density fractions beyond that reduces variance, although the magnitude of this benefit declines with additional fractions. Our analysis suggests that, if a taxon has an isotope enrichment of 10 atom% excess, there is a 60% chance that this will be detected as significantly different from zero (with alpha 0.1). With five replicates, isotope enrichment of 5 atom% could be detected with power (0.6) and alpha (0.1). Finally, we illustrate the importance of internal standards, which can help to calibrate per sample conversions of %GC to mean weighted density. These results should benefit researchers designing future SIP experiments and provide a useful reference for metagenomic SIP applications where both financial and computational limitations constrain experimental scope. One of the biggest challenges in microbial ecology is correlating the identity of microorganisms with the roles they fulfill in natural environmental systems. Studies of microbes in pure culture reveal much about their genomic content and potential functions but may not reflect an organism's activity within its natural community. Culture-independent studies supply a community-wide view of composition and function in the context of community interactions but often fail to link the two. Quantitative stable isotope probing (qSIP) is a method that can link the identity and functional activity of specific microbes within a naturally occurring community. Here, we explore how the resolution of density gradient fractionation affects the error and precision of qSIP results, how they may be improved via additional experimental replication, and discuss cost-benefit balanced scenarios for SIP experimental design.

摘要

定量稳定同位素探测(qSIP)可估算同位素示踪剂掺入单个微生物DNA的情况,并能将复杂群落中的微生物多样性与生物地球化学联系起来。与任何定量估算技术一样,qSIP存在测量误差,更全面地了解误差、精度和统计功效有助于qSIP实验设计和数据解释。我们使用了几个qSIP数据集——来自土壤和海水微生物群落——来评估同位素掺入估算中的方差如何取决于生物体丰度和密度分级方案的分辨率。我们评估了重复qSIP研究的统计功效,以及非重复设计的敏感性和特异性。随着一个分类单元丰度的增加,其加权平均密度的方差会下降。对于大多数qSIP应用而言,九个级分似乎是成本与精度之间的合理权衡。增加密度级分的数量会降低方差,不过这种益处的幅度会随着额外级分的增加而减小。我们的分析表明,如果一个分类单元的同位素富集度超过10原子%,那么有60%的可能性会检测到其与零有显著差异(α = 0.1)。进行五次重复时,5原子%的同位素富集度能够以功效(0.6)和α(0.1)被检测到。最后,我们说明了内标的重要性,它有助于校准每个样品中%GC到平均加权密度的转换。这些结果应会使设计未来SIP实验的研究人员受益,并为宏基因组SIP应用提供有用的参考,在这些应用中,财务和计算方面的限制会制约实验范围。微生物生态学中最大的挑战之一是将微生物的身份与其在自然环境系统中所发挥的作用联系起来。对纯培养微生物的研究揭示了很多关于它们的基因组内容和潜在功能,但可能无法反映生物体在其天然群落中的活性。非培养研究提供了群落相互作用背景下群落组成和功能的全局视图,但往往无法将两者联系起来。定量稳定同位素探测(qSIP)是一种能够将自然群落中特定微生物的身份与功能活性联系起来的方法。在这里,我们探讨密度梯度分级的分辨率如何影响qSIP结果的误差和精度,如何通过额外的实验重复来改进这些结果,并讨论SIP实验设计中成本效益平衡的方案。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/88ca/7566279/a0fe1dd9707c/mSystems.00151-20-f0001.jpg

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