GC bias affects genomic and metagenomic reconstructions, underrepresenting GC-poor organisms

Browne, Patrick; Nielsen, Tue Kjærgaard; Kot, Witold; Aggerholm, Anni; Gilbert, M. Thomas P.; Puetz, Lara; Rasmussen, Morten; Zervas, Athanasios; Hansen, Lars Hestbjerg

doi:10.1093/gigascience/giaa008

Cited by 119 publications

(106 citation statements)

References 37 publications

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“…Specifically, the abundance of each species differs among the methods. In addition to the presence of unculturable bacteria in the sequencing data, these differences could result from several biases in DNA extraction, PCR efficiency, primer selection, GC content, and data analyses, all of which have been investigated among various sequencing platforms [ 36 , 45 , 46 , 47 , 48 ]. In addition, the impact of bioinformatic methods used to achieve final results is well characterized.…”

Section: Resultsmentioning

confidence: 99%

Real-Time Culture-Independent Microbial Profiling Onboard the International Space Station Using Nanopore Sequencing

Stahl-Rommel

Nguyen

Arnold

et al. 2021

Genes

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For the past two decades, microbial monitoring of the International Space Station (ISS) has relied on culture-dependent methods that require return to Earth for analysis. This has a number of limitations, with the most significant being bias towards the detection of culturable organisms and the inherent delay between sample collection and ground-based analysis. In recent years, portable and easy-to-use molecular-based tools, such as Oxford Nanopore Technologies’ MinION™ sequencer and miniPCR bio’s miniPCR™ thermal cycler, have been validated onboard the ISS. Here, we report on the development, validation, and implementation of a swab-to-sequencer method that provides a culture-independent solution to real-time microbial profiling onboard the ISS. Method development focused on analysis of swabs collected in a low-biomass environment with limited facility resources and stringent controls on allowed processes and reagents. ISS-optimized procedures included enzymatic DNA extraction from a swab tip, bead-based purifications, altered buffers, and the use of miniPCR and the MinION. Validation was conducted through extensive ground-based assessments comparing current standard culture-dependent and newly developed culture-independent methods. Similar microbial distributions were observed between the two methods; however, as expected, the culture-independent data revealed microbial profiles with greater diversity. Protocol optimization and verification was established during NASA Extreme Environment Mission Operations (NEEMO) analog missions 21 and 22, respectively. Unique microbial profiles obtained from analog testing validated the swab-to-sequencer method in an extreme environment. Finally, four independent swab-to-sequencer experiments were conducted onboard the ISS by two crewmembers. Microorganisms identified from ISS swabs were consistent with historical culture-based data, and primarily consisted of commonly observed human-associated microbes. This simplified method has been streamlined for high ease-of-use for a non-trained crew to complete in an extreme environment, thereby enabling environmental and human health diagnostics in real-time as future missions take us beyond low-Earth orbit.

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Section: Resultsmentioning

confidence: 99%

Real-Time Culture-Independent Microbial Profiling Onboard the International Space Station Using Nanopore Sequencing

Stahl-Rommel

Nguyen

Arnold

et al. 2021

Genes

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“…The species of the samples is indicated. Tyler et al, 2016;Grützke et al, 2019;Sato et al, 2019;Uelze et al, 2019;Browne et al, 2020) (also compare Supplementary File S7). This is a concern since a high number of contigs in a genome assembly may cause a fragmentation of genes at the contig borders, thereby affecting gene annotation and multilocus sequence typing.…”

Section: Discussionmentioning

confidence: 99%

“…Nevertheless, we found that all assemblies were overall very similar, with respect to assembly length, N50, GC and the number of CDSs, with a few notable exceptions. In particular, assemblies constructed from short read data of laboratories LC06 and LC08 (both using a MiSeq Illumina instrument) had much lower N50 values and a greater number of contigs, probably due to their use of the Nextera XT DNA Library Preparation Kit, which was shown to have a strong GC bias ( Lan et al, 2015 ; Tyler et al, 2016 ; Grützke et al, 2019 ; Sato et al, 2019 ; Uelze et al, 2019 ; Browne et al, 2020 ) (also compare Supplementary File S7 ). This is a concern since a high number of contigs in a genome assembly may cause a fragmentation of genes at the contig borders, thereby affecting gene annotation and multilocus sequence typing.…”

Section: Discussionmentioning

confidence: 99%

German-Wide Interlaboratory Study Compares Consistency, Accuracy and Reproducibility of Whole-Genome Short Read Sequencing

et al. 2020

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“…As mentioned earlier, these observations could be interesting in terms of bone degradation, however, while amplicon metabarcoding has its clear advantages being both cost effective, fast and used in a variety of studies making the genetic databases available more exhaustive, the approach still has its disadvantages [ 32 ]. With the advancement of full shotgun metagenomic sequencing techniques, the sequence bias experienced with amplicon sequencing and issues of underrepresentation of uncultivable microorganisms in the databases, and therefore difficulties in characterisation, is reduced [ 70 ], although shotgun sequencing has recently been found to underrepresent low or high GC phyla with up to two logs [ 71 ]. A natural next step with this study would be to look into the functions of the different bacterial strains and examine how the bacterial communities are associated with bone tunneling using a shotgun metagenomics approach.…”

Section: Discussionmentioning

confidence: 99%

Bone biodeterioration—The effect of marine and terrestrial depositional environments on early diagenesis and bone bacterial community

et al. 2020

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Bacteria play an important role in the degradation of bone material. However, much remains to be learnt about the structure of their communities in degrading bone, and how the depositional environment influences their diversity throughout the exposure period. We genetically profiled the bacterial community in an experimental series of pig bone fragments (femur and humeri) deposited at different well-defined environments in Denmark. The bacterial community in the bone fragments and surrounding depositional environment were studied over one year, and correlated with the bioerosion damage patterns observed microscopically in the bones. We observed that the bacterial communities within the bones were heavily influenced by the local microbial community, and that the general bone microbial diversity increases with time after exposure. We found the presence of several known collagenase producing bacterial groups, and also observed increases in the relative abundance of several of these in bones with tunneling. We anticipate that future analyses using shotgun metagenomics on this and similar datasets will be able to provide insights into mechanisms of microbiome driven bone degradation.

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GC bias affects genomic and metagenomic reconstructions, underrepresenting GC-poor organisms

Cited by 119 publications

References 37 publications

Real-Time Culture-Independent Microbial Profiling Onboard the International Space Station Using Nanopore Sequencing

Real-Time Culture-Independent Microbial Profiling Onboard the International Space Station Using Nanopore Sequencing

German-Wide Interlaboratory Study Compares Consistency, Accuracy and Reproducibility of Whole-Genome Short Read Sequencing

Bone biodeterioration—The effect of marine and terrestrial depositional environments on early diagenesis and bone bacterial community

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