Commercial DNA extraction kits impact observed microbial community composition in permafrost samples

Vishnivetskaya, Tatiana A.; Layton, Alice C.; Lau, Maggie C. Y.; Chauhan, Archana; Cheng, Karen R.; Meyers, A. J.; Murphy, Jasity R.; Rogers, Alexandra; Saarunya, Geetha; Williams, Daniel E.; Pfiffner, Susan M.; Biggerstaff, John; Stackhouse, B. T.; Phelps, Tommy J.; Whyte, Lyle G.; Sayler, Gary S.; Onstott, Tullis C.

doi:10.1111/1574-6941.12219

Cited by 92 publications

(90 citation statements)

References 50 publications

(64 reference statements)

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“…The greater amount of DNA extracted by the Fast kit is consistent with much higher 16s rRNA gene copy numbers using this kit. Similar to our studyVishnivetskaya et al (2014) [38] extracted more DNA using the Fast kit than the MoBio kit from permafrost soils in the Arctic; although in their study both the Fast and MoBio kits extracted high quality DNA (see Table 1 of Vishnivetskaya et al (2014) for comparison of the kits) [38]. The DNA extracted by the MoBio kit in our study was of a higher quality than that extracted using the Fast kit.…”

Section: Effect Of Different Methods Of Soil Sampling and Dna Extractsupporting

confidence: 84%

Impact of Different Methods of Soil Sampling and DNA Extraction on the Identification of Soil Bacterial Abundance under Elevated CO2

Li¹,

Bowatte²,

Newton³

et al. 2017

OALib

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Elevated atmospheric CO 2 (eCO 2 ) is anticipated to have marked effects on soil microbial populations. While there is experimental evidence to support this view there are also studies where changes in microbial populations, such as the abundance of bacteria, are suggested but cannot be statistically established. We conducted this study to identify whether the sampling and sample treatment methods used could influence the results obtained using bacterial abundance as the variable of interest. We tested three different sampling methods and two different DNA extraction kits. The first because microbes are distributed heterogeneously in soil so the sampling procedure might be expected to influence the accuracy and precision of the population estimate and the second because the quantity and quality of DNA extracted influences the microbial analyses that can be performed and can introduce bias. Samples were taken from a long-running FACE experiment on grassland from under plants of Agrostis capillaris. We found that bacterial abundance was consistently lower under eCO 2 but we were only able to establish a statistical difference where a more intense sampling regime was used and bulking of the soil sample was avoided. A reduction in bacterial abundance is a consistent outcome in eCO 2 field experiments but the only other occasion where this reduction has been found to be significant was also where individual soil cores were analysed rather than the samples being bulked. We conclude that while there is extra work and cost attached to more detailed sampling this approach is highly desirable if we are to make robust conclusions about the impacts of eCO 2 on soil microbes.

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Section: Effect Of Different Methods Of Soil Sampling and Dna Extractsupporting

confidence: 84%

Impact of Different Methods of Soil Sampling and DNA Extraction on the Identification of Soil Bacterial Abundance under Elevated CO2

Li¹,

Bowatte²,

Newton³

et al. 2017

OALib

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“…Even if an equimolar mix of samples was used for sequencing, significantly different numbers of reads were obtained depending on the primer set used (see Table S4), as previously noted in other projects (A. Dheilly, Biogenouest Platform, Rennes, France, personal communication). This variability may reflect differences in the sample titration in the equimolar mix (16) or may have been due to the fusion primer set used. Indeed, association of primers with tag sequences and pyrosequencing adaptors may reduce the hybridization efficiency on DNA capture beads, which is required for emulsion PCR and sequencing, and/or may be a disadvantage in amplification.…”

Section: Discussionmentioning

confidence: 99%

“…While molecular analyses provide a less biased picture of environmental microbial communities than culturebased methods, each step of the analysis needs to be taken into account. Indeed, the DNA extraction method, PCR amplification, or data analysis can all lead to distortions of the compositions of analyzed samples (10)(11)(12)(13)(14)(15)(16)(17)(18).…”

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confidence: 99%

Influence of DNA Extraction Method, 16S rRNA Targeted Hypervariable Regions, and Sample Origin on Microbial Diversity Detected by 454 Pyrosequencing in Marine Chemosynthetic Ecosystems

Cruaud

Vigneron

Lucchetti-Miganeh

et al. 2014

Appl Environ Microbiol

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dNext-generation sequencing (NGS) opens up exciting possibilities for improving our knowledge of environmental microbial diversity, allowing rapid and cost-effective identification of both cultivated and uncultivated microorganisms. However, library preparation, sequencing, and analysis of the results can provide inaccurate representations of the studied community compositions. Therefore, all these steps need to be taken into account carefully. Here we evaluated the effects of DNA extraction methods, targeted 16S rRNA hypervariable regions, and sample origins on the diverse microbes detected by 454 pyrosequencing in marine cold seep and hydrothermal vent sediments. To assign the reads with enough taxonomic precision, we built a database with about 2,500 sequences from Archaea and Bacteria from deep-sea marine sediments, affiliated according to reference publications in the field. Thanks to statistical and diversity analyses as well as inference of operational taxonomic unit (OTU) networks, we show that (i) while DNA extraction methods do not seem to affect the results for some samples, they can lead to dramatic changes for others; and (ii) the choice of amplification and sequencing primers also considerably affects the microbial community detected in the samples. Thereby, very different proportions of pyrosequencing reads were obtained for some microbial lineages, such as the archaeal ANME-1, ANME-2c, and MBG-D and deltaproteobacterial subgroups. This work clearly indicates that the results from sequencing-based analyses, such as pyrosequencing, should be interpreted very carefully. Therefore, the combination of NGS with complementary approaches, such as fluorescence in situ hybridization (FISH)/catalyzed reporter deposition (CARD)-FISH or quantitative PCR (Q-PCR), would be desirable to gain a more comprehensive picture of environmental microbial communities.

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“…Enumeration of the bacterial abundance in these permafrost samples by fluorescence in situ hybridization yielded 9.7 × 10 8 cells g À1 [Vishnivetskaya et al, 2014]. The assumed growth yield represents a maximum increase of at most 1 to 4% of the observed population since much of the anabolic activity during the initial thaw probably goes to cellular repair [Price and Sowers, 2004].…”

mentioning

confidence: 92%

Effects of simulated spring thaw of permafrost from mineral cryosol on CO₂ emissions and atmospheric CH₄ uptake

et al. 2015

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Previous studies investigating organic-rich tundra have reported that increasing biodegradation of Arctic tundra soil organic carbon (SOC) under warming climate regimes will cause increasing CO 2 and CH 4 emissions. Organic-poor, mineral cryosols, which comprise 87% of Arctic tundra, are not as well characterized. This study examined biogeochemical processes of 1 m long intact mineral cryosol cores (1-6% SOC) collected in the Canadian high Arctic. Vertical profiles of gaseous and aqueous chemistry and microbial composition were related to surface CO 2 and CH 4 fluxes during a simulated spring/summer thaw under light versus dark and in situ versus water saturated treatments. CO 2 fluxes attained 0.8 ± 0.4 mmol CO 2 m À2 h À1 for in situ treatments, of which 85 ± 11% was produced by aerobic SOC oxidation, consistent with field observations and metagenomic analyses indicating aerobic heterotrophs were the dominant phylotypes. The Q 10 values of CO 2 emissions ranged from 2 to 4 over the course of thawing. CH 4 degassing occurred during initial thaw; however, all cores were CH 4 sinks at atmospheric concentration CH 4 . Atmospheric CH 4 uptake rates ranged from À126 ± 77 to À207 ± 7 nmol CH 4 m À2 h À1 with CH 4 consumed between 0 and 35 cm depth.Metagenomic and gas chemistry analyses revealed that high-affinity Type II methanotrophic sequence abundance and activity were highest between 0 and 35 cm depth. Microbial sulfate reduction dominated the anaerobic processes, outcompeting methanogenesis for H 2 and acetate. Fluxes, microbial community composition, and biogeochemical rates indicate that mineral cryosols of Axel Heiberg Island act as net CO 2 sources and atmospheric CH 4 sinks during summertime thaw under both in situ and water saturated states.

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Commercial DNA extraction kits impact observed microbial community composition in permafrost samples

Cited by 92 publications

References 50 publications

Impact of Different Methods of Soil Sampling and DNA Extraction on the Identification of Soil Bacterial Abundance under Elevated CO2

Impact of Different Methods of Soil Sampling and DNA Extraction on the Identification of Soil Bacterial Abundance under Elevated CO2

Influence of DNA Extraction Method, 16S rRNA Targeted Hypervariable Regions, and Sample Origin on Microbial Diversity Detected by 454 Pyrosequencing in Marine Chemosynthetic Ecosystems

Effects of simulated spring thaw of permafrost from mineral cryosol on CO₂ emissions and atmospheric CH₄ uptake

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Commercial DNA extraction kits impact observed microbial community composition in permafrost samples

Cited by 92 publications

References 50 publications

Impact of Different Methods of Soil Sampling and DNA Extraction on the Identification of Soil Bacterial Abundance under Elevated CO2

Impact of Different Methods of Soil Sampling and DNA Extraction on the Identification of Soil Bacterial Abundance under Elevated CO2

Influence of DNA Extraction Method, 16S rRNA Targeted Hypervariable Regions, and Sample Origin on Microbial Diversity Detected by 454 Pyrosequencing in Marine Chemosynthetic Ecosystems

Effects of simulated spring thaw of permafrost from mineral cryosol on CO2 emissions and atmospheric CH4 uptake

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Effects of simulated spring thaw of permafrost from mineral cryosol on CO₂ emissions and atmospheric CH₄ uptake