synDNA-a Synthetic DNA Spike-in Method for Absolute Quantification of Shotgun Metagenomic Sequencing

Livia S Zaramela; Megan Tjuanta; Oriane Moyne; Maxwell Neal; Karsten Zengler

doi:10.1128/msystems.00447-22

synDNA-a Synthetic DNA Spike-in Method for Absolute Quantification of Shotgun Metagenomic Sequencing

mSystems. 2022 Dec 20;7(6):e0044722. doi: 10.1128/msystems.00447-22. Epub 2022 Nov 1.

Authors

Livia S Zaramela¹, Megan Tjuanta¹, Oriane Moyne¹, Maxwell Neal², Karsten Zengler^{1

3

2}

Affiliations

¹ Department of Pediatrics, University of California, San Diegogrid.266100.3, La Jolla, California, USA.
² Department of Bioengineering, University of California, San Diegogrid.266100.3, La Jolla, California, USA.
³ Center for Microbiome Innovation, University of California, San Diegogrid.266100.3, La Jolla, California, USA.

Abstract

Microbiome studies have the common goal of determining which microbial taxa are present, respond to specific conditions, or promote phenotypic changes in the host. Most of these studies rely on relative abundance measurements to drive conclusions. Inherent limitations of relative values are the inability to determine whether an individual taxon is more or less abundant and the magnitude of this change between the two samples. These limitations can be overcome by using absolute abundance quantifications, which can allow for a more complete understanding of community dynamics by measuring variations in total microbial loads. Obtaining absolute abundance measurements is still technically challenging. Here, we developed synthetic DNA (synDNA) spike-ins that enable precise and cost-effective absolute quantification of microbiome data by adding defined amounts of synDNAs to the samples. We designed 10 synDNAs with the following features: 2,000-bp length, variable GC content (26, 36, 46, 56, or 66% GC), and negligible identity to sequences found in the NCBI database. Dilution pools were generated by mixing the 10 synDNAs at different concentrations. Shotgun metagenomic sequencing showed that the pools of synDNAs with different percentages of GC efficiently reproduced the serial dilution, showing high correlation (r = 0.96; R² ≥ 0.94) and significance (P < 0.01). Furthermore, we demonstrated that the synDNAs can be used as DNA spike-ins to generate linear models and predict with high accuracy the absolute number of bacterial cells in complex microbial communities. IMPORTANCE The synDNAs designed in this study enable accurate and reproducible measurements of absolute amount and fold changes of bacterial species in complex microbial communities. The method proposed here is versatile and promising as it can be applied to bacterial communities or genomic features like genes and operons, in addition to being easily adaptable by other research groups at a low cost. We also made the synDNAs' sequences and the plasmids available to encourage future application of the proposed method in the study of microbial communities.

Keywords: absolute abundance; metagenomics; microbial communities.

Publication types

Research Support, U.S. Gov't, Non-P.H.S.
Research Support, Non-U.S. Gov't

MeSH terms

Bacteria / genetics
DNA
Metagenome* / genetics
Microbiota* / genetics
Plasmids

Substances

DNA