Towards Quantitative Microbiome Community Profiling Using Internal Standards

WOS:000459327600015 International audience An inherent issue in high-throughput rRNA gene tag sequencing microbiome surveys is that they provide compositional data in relative abundances. This often leads to spurious correlations, making the interpretation of relationships to biogeochemical rates ch...

Full description

Bibliographic Details
Published in:Applied and Environmental Microbiology
Main Authors: Lin, Yajuan, Gifford, Scott, Ducklow, Hugh, Schofield, Oscar, Cassar, Nicolas
Other Authors: Laboratoire des Sciences de l'Environnement Marin (LEMAR) (LEMAR), Institut de Recherche pour le Développement (IRD)-Institut Français de Recherche pour l'Exploitation de la Mer (IFREMER)-Université de Brest (UBO)-Institut Universitaire Européen de la Mer (IUEM), Institut de Recherche pour le Développement (IRD)-Institut national des sciences de l'Univers (INSU - CNRS)-Université de Brest (UBO)-Centre National de la Recherche Scientifique (CNRS)-Institut de Recherche pour le Développement (IRD)-Institut national des sciences de l'Univers (INSU - CNRS)-Université de Brest (UBO)-Centre National de la Recherche Scientifique (CNRS)-Centre National de la Recherche Scientifique (CNRS), Nicholas School of the Environment, Duke University Durham, University of North Carolina Chapel Hill (UNC), University of North Carolina System (UNC), Lamont-Doherty Earth Observatory (LDEO), Columbia University New York, School of Environmental and Biological Sciences New Brunswick, Rutgers, The State University of New Jersey New Brunswick (RU), Rutgers University System (Rutgers)-Rutgers University System (Rutgers), ANR-10-LABX-0019,LabexMER,LabexMER Marine Excellence Research: a changing ocean(2010)
Format: Article in Journal/Newspaper
Language:English
Published: HAL CCSD 2019
Subjects:
ACL
ocean
phytoplankton
variability
marine
quantification
bacteria
abundances
amplicon sequencing
community profiling
genome sequence
internal standard
marine microbiome
metagenomics
phaeocystis-antarctica
[SDE.BE]Environmental Sciences/Biodiversity and Ecology
Antarc*
Antarctica
Online Access:https://hal.science/hal-02871388
https://doi.org/10.1128/AEM.02634-18
Description
Summary:WOS:000459327600015 International audience An inherent issue in high-throughput rRNA gene tag sequencing microbiome surveys is that they provide compositional data in relative abundances. This often leads to spurious correlations, making the interpretation of relationships to biogeochemical rates challenging. To overcome this issue, we quantitatively estimated the abundance of microorganisms by spiking in known amounts of internal DNA standards. Using a 3-year sample set of diverse microbial communities from the Western Antarctica Peninsula, we demonstrated that the internal standard method yielded community profiles and taxon cooccurrence patterns substantially different from those derived using relative abundances. We found that the method provided results consistent with the traditional CHEMTAX analysis of pigments and total bacterial counts by flow cytometry. Using the internal standard method, we also showed that chloroplast 16S rRNA gene data in microbial surveys can be used to estimate abundances of certain eukaryotic phototrophs such as cryptophytes and diatoms. In Phaeocystis, scatter in the 16S/18S rRNA gene ratio may be explained by physiological adaptation to environmental conditions. We conclude that the internal standard method, when applied to rRNA gene microbial community profiling, is quantitative and that its application will substantially improve our understanding of microbial ecosystems. IMPORTANCE High-throughput-sequencing-based marine microbiome profiling is rapidly expanding and changing how we study the oceans. Although powerful, the technique is not fully quantitative; it provides taxon counts only in relative abundances. In order to address this issue, we present a method to quantitatively estimate microbial abundances per unit volume of seawater filtered by spiking known amounts of internal DNA standards into each sample. We validated this method by comparing the calculated abundances to other independent estimates, including chemical markers (pigments) and total bacterial cell ...

Similar Items