Performance and precision of double digestion RAD (ddRAD) genotyping in large multiplexed datasets of marine fish species

Maroso, Francesco; Hillen, Jasmien; Pardo, Belén G.; Gkagkavouzis, Konstantinos; Coscia, Ilaria; Hermida, Miguel; Franch, Rafaella; Hellemans, Bart; Houdt, J. K. J. Van; Simionati, Barbara; Taggart, John B.; Nielsen, Einar Eg; Maes, Grégory E.; Ciavaglia, Sherryn A.; Webster, Lucy M.I.; Volckaert, Filip; Martı́nez, Paulino; Bargelloni, Luca; Ogden, R. Todd

doi:10.1016/j.margen.2018.02.002

Cited by 26 publications

(38 citation statements)

References 35 publications

(5 reference statements)

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“…S8a-c). This is in line with the earlier observation that variance in read coverage between individuals and between loci in the same individual introduce biases (Maroso et al 2018). However, based on results from this study, larger sample sizes are likely also needed in search of reliable outliers between populations (Fig.…”

Section: Frankham 1996; Allendorf and Ryman 2014)supporting

confidence: 92%

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Genome wide analysis reveals genetic divergence between Goldsinny wrasse populations

Jansson¹,

Besnier²,

Malde³

et al. 2020

Preprint

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Background: Marine fish populations are often characterized by high levels of gene flow and correspondingly low genetic divergence. This presents a challenge to define management units. Goldsinny wrasse (Ctenolabrus rupestris) is a heavily exploited species due to its importance as a cleaner-fish in commercial salmonid aquaculture. However, at the present, the population genetic structure of this species is still largely unresolved. Here, full-genome sequencing was used to produce the first genomic reference for this species, to study population-genomic divergence among four geographically distinct populations, and, to identify informative SNP markers for future studies. Results: After construction of a de novo assembly, the genome was estimated to be highly polymorphic and of ~600Mbp in size. 33 235 SNPs were thereafter selected to assess genomic diversity and differentiation among four populations collected from Scandinavia, Scotland, and Spain. Global FST among these populations was 0.015–0.092. Approximately 4% of the investigated loci were identified as putative global outliers, and ~1% within Scandinavia. SNPs showing large divergence (FST>0.15) were picked as candidate diagnostic markers for population assignment. 173 of the most diagnostic SNPs between the two Scandinavian populations were validated by genotyping 47 individuals from each end of the species’ Scandinavian distribution range. 69 of these SNPs were significantly (p<0.05) differentiated (mean FST_173_loci=0.065, FST_69_loci=0.140). Using these validated SNPs, individuals were assigned with high probability (≥ 94%) to their populations of origin.Conclusions: Goldsinny wrasse displays a highly polymorphic genome, and substantial population genomic structure. Diversifying selection likely affects population structuring globally and within Scandinavia. The diagnostic loci identified now provide a promising and cost-efficient tool to investigate goldsinny wrasse populations further.

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Section: Frankham 1996; Allendorf and Ryman 2014)supporting

confidence: 92%

“…On the other hand, this in turn would have come on the expense of genomic coverage, and thus possibility to detect (any) adaptive outliers (Hoban et al 2016), and could also introduce other type of errors and biases (see e.g. Maroso et al 2018;Wright et al 2019;Graham et al 2020).…”

Section: Frankham 1996; Allendorf and Ryman 2014)mentioning

confidence: 99%

Genome wide analysis reveals genetic divergence between Goldsinny wrasse populations

Jansson¹,

Besnier²,

Malde³

et al. 2020

Preprint

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“…Both RAD and ddRAD-seq have been widely applied in aquaculture breeding and genetics studies (Robledo et al 2018). In particular, ddRAD-seq has been applied for genotyping large multiplexed datasets (e.g., Maroso et al 2018), construction of genetic linkage maps (e.g., Recknagel et al 2013;Oral et al 2017), analyzing life history traits (e.g., Pukk 2016), mapping sex determining loci (e.g., Palaiokostas et al 2015;Brown et al 2016), genomic predictions and genome-wide association studies (e.g., Barria et al 2018), assessing genetic diversity (e.g., Hosoya et al 2018;Tony et al 2015;Siccha-Ramirez et al 2018;Torati et al 2019), phylogeography (e.g., Stobie et al 2018, and species identification in tilapias (Syaifudin et al 2019).…”

Section: Introductionmentioning

confidence: 99%

Characterizing the genetic structure of introduced Nile tilapia (Oreochromis niloticus) strains in Tanzania using double digest RAD sequencing

et al. 2019

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Tilapia hatcheries in Tanzania rely heavily on importing germplasm. Nevertheless, the genetic structure of the imported stocks is poorly understood. In the current study, the level of genetic diversity and differentiation of eight populations of Nile tilapia (Oreochromis niloticus) strains imported in Tanzania was investigated. Four of the studied strains originated from Thailand, three from Uganda, and one from the Netherlands. Double-digest restriction site-associated DNA sequencing (ddRAD-seq) was applied to identify and genotype single nucleotide polymorphisms (SNPs). In total, 2214 SNPs passed all the quality control steps and were utilized for downstream analysis. Mean heterozygosity estimates were higher for the Thailand strains (Ho, 0.23) compared with the strains from Uganda (Ho, 0.12). Low genetic distance was observed amongst populations from the same geographic origin (Fst, 0.01-0.04). However, genetic distance between populations from different geographic origins was substantial (Fst, 0.24-0.44). Bayesian model-based clustering (STRUCTURE) and discriminant analysis of principal components (DAPC) grouped the studied animals into three distinct clusters. A cross-validation approach (where 25% of animals from each population were considered of unknown origin) was conducted in order to test the efficiency of the SNP dataset for identifying the population of origin. The cross-validation procedure was repeated 10 times resulting in approximately 97% of the tested animals being allocated to the correct geographic population of origin. The breeding history and hatchery practices used to manage these stocks prior and after import appear to be the main factors for the genetic diversity observed in this study. Our study will help inform hatchery stock management and future breeding program designs in Tanzania.

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“…We assessed three main measures as proxies for evaluating ddRAD sequencing success: number of polymorphic loci, sequencing read depth, and levels of missing loci between treatments within a species. While number of loci is often utilized as a standard measurement of sequencing success (Graham et al, ), depth of coverage (number of sequence reads for a given locus) is also an important metric of sequence quality, as higher depth allows for greater detection of sequencing errors, heterozygous loci, and differences between individuals and populations (Maroso et al, ; Sims, Sudbery, Ilott, Heger, & Ponting, ). Quantifying the amount of missing data is also an important aspect of assessing RAD success, as there is a finite number of sequencing reads spread across multiple individuals during sequencing, and the assembly of genomes, either de novo or mapped to a reference, depends on sequence similarity (low levels of missing data) between specimens (Catchen, Amores, & Hohenlohe, ).…”

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Utilizing field collected insects for next generation sequencing: Effects of sampling, storage, and DNA extraction methods

Ballare

Pope

Castilla

et al. 2019

Ecology and Evolution

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DNA sequencing technologies continue to advance the biological sciences, expanding opportunities for genomic studies of non‐model organisms for basic and applied questions. Despite these opportunities, many next generation sequencing protocols have been developed assuming a substantial quantity of high molecular weight DNA (>100 ng), which can be difficult to obtain for many study systems. In particular, the ability to sequence field‐collected specimens that exhibit varying levels of DNA degradation remains largely unexplored. In this study we investigate the influence of five traditional insect capture and curation methods on Double‐Digest Restriction Enzyme Associated DNA (ddRAD) sequencing success for three wild bee species. We sequenced a total of 105 specimens (between 7–13 specimens per species and treatment). We additionally investigated how different DNA quality metrics (including pre‐sequence concentration and contamination) predicted downstream sequencing success, and also compared two DNA extraction methods. We report successful library preparation for all specimens, with all treatments and extraction methods producing enough highly reliable loci for population genetic analyses. Although results varied between species, we found that specimens collected by net sampling directly into 100% EtOH, or by passive trapping followed by 100% EtOH storage before pinning tended to produce higher quality ddRAD assemblies, likely as a result of rapid specimen desiccation. Surprisingly, we found that specimens preserved in propylene glycol during field sampling exhibited lower‐quality assemblies. We provide recommendations for each treatment, extraction method, and DNA quality assessment, and further encourage researchers to consider utilizing a wider variety of specimens for genomic analyses.

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Performance and precision of double digestion RAD (ddRAD) genotyping in large multiplexed datasets of marine fish species

Cited by 26 publications

References 35 publications

Genome wide analysis reveals genetic divergence between Goldsinny wrasse populations

Genome wide analysis reveals genetic divergence between Goldsinny wrasse populations

Characterizing the genetic structure of introduced Nile tilapia (Oreochromis niloticus) strains in Tanzania using double digest RAD sequencing

Utilizing field collected insects for next generation sequencing: Effects of sampling, storage, and DNA extraction methods

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