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Assessing and Maximizing Cultivated Diversity with Plate-Wash PCR and High Throughput Sequencing

View ORCID ProfileEmily N. Junkins, View ORCID ProfileBradley S. Stevenson
doi: https://doi.org/10.1101/2020.11.19.390864
Emily N. Junkins
aDepartment of Microbiology and Plant Biology, University of Oklahoma, Norman, OK, USA
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Bradley S. Stevenson
aDepartment of Microbiology and Plant Biology, University of Oklahoma, Norman, OK, USA
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  • For correspondence: bradley.stevenson@ou.edu
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Abstract

Molecular techniques continue to reveal a growing disparity between the immense diversity of microbial life and the small proportion that is in pure culture. The disparity, originally dubbed “the great plate count anomaly” by Staley and Konopka, has become even more vexing given our increased understanding of the importance of microbiomes to a host and the role of microorganisms in the vital biogeochemical functions of our biosphere. Searching for novel antimicrobial drug targets often focuses on screening a broad diversity of microorganisms. If diverse microorganisms are to be screened, they need to be cultivated. Recent innovative research has used molecular techniques to assess the efficacy of cultivation efforts, providing invaluable feedback to cultivation strategies for isolating targeted and/or novel microorganisms. Here, we aimed to determine the efficiency of cultivating representative microorganisms from a non-human, mammalian microbiome, identify those microorganisms, and determine the bioactivity of isolates. Molecular methods indicated that around 57% of the ASVs detected in the original inoculum were cultivated in our experiments, but nearly 53% of the total ASVs that were present in our cultivation experiments were not detected in the original inoculum. In light of our controls, our data suggests that when molecular tools were used to characterize our cultivation efforts, they provided a more complete, albeit more complex, understanding of which organisms were present compared to what was eventually cultivated. Lastly, about 3% of the isolates collected from our cultivation experiments showed inhibitory bioactivity against a multidrug-resistant pathogen panel, further highlighting the importance of informing and directing future cultivation efforts with molecular tools.

Importance Cultivation is the definitive tool to understand a microorganism’s physiology, metabolism, and ecological role(s). Despite continuous efforts to hone this skill, researchers are still observing yet-to-be cultivated organisms through high-throughput sequencing studies. Here, we use the very same tool that highlights biodiversity to assess cultivation efficiency. When applied to drug discovery, where screening a vast number of isolates for bioactive metabolites is common, cultivating redundant organisms is a hindrance. However, we observed that cultivating in combination with molecular tools can expand the observed diversity of an environment and its community, potentially increasing the number of microorganisms to be screened for natural products.

Competing Interest Statement

The authors have declared no competing interest.

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The copyright holder for this preprint is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. All rights reserved. No reuse allowed without permission.
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Posted November 24, 2020.
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Assessing and Maximizing Cultivated Diversity with Plate-Wash PCR and High Throughput Sequencing
Emily N. Junkins, Bradley S. Stevenson
bioRxiv 2020.11.19.390864; doi: https://doi.org/10.1101/2020.11.19.390864
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Assessing and Maximizing Cultivated Diversity with Plate-Wash PCR and High Throughput Sequencing
Emily N. Junkins, Bradley S. Stevenson
bioRxiv 2020.11.19.390864; doi: https://doi.org/10.1101/2020.11.19.390864

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