A note on sampling chironomids for RNA-based studies of natural populations that retains critical morphological vouchers

Krosch, Matt N.; Bryant, Litticia M.

doi:10.5324/cjcr.v0i28.1877

Cited by 3 publications

(2 citation statements)

References 22 publications

(18 reference statements)

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“…Cultures were kept in separate rooms for each species, and adult males and females were collected between 3 and 5 days after emergence, killed by freezing and transferred immediately to RNA later for transport to the Molecular Genetics Research Facility (MGRF), QUT, Brisbane, Australia. One individual of each sex per species was pooled in a single replicated RNA extraction, conducted using a modified Trizol/Trisure RNA isolation as described in Krosch and Bryant (). RNA quality and quantity were assessed on an Agilent 2100 Bioanalyser (Agilent Technologies, USA) and an RNA 6000 Nano kit for total RNA.…”

Section: Methodsmentioning

confidence: 99%

A transcriptome‐based analytical workflow for identifying loci for species diagnosis: a case study with Bactrocera fruit flies (Diptera: Tephritidae)

et al. 2017

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Development of novel molecular methods for accurate and economical identification of species has become critical both for pure biological research and for a wide range of applied areas. The most widely used current molecular diagnostic tool, the mitochondrial cytochrome c oxidase subunit 1 gene (COI), the so-called DNA barcode, has been highly criticised and is known to be ineffective at distinguishing species in many groups. Alternative markers are needed to circumvent these issues and provide diagnosticians with a greater range of tools for making accurate identifications. To address this, we describe here a novel analytical workflow for diagnostic marker development that utilises near-genomic-scale data to search for potential informative loci. The workflow takes advantage of orthologous gene databases, in combination with tests of phylogenetic resolution, and benchmarking of nucleotide variation against COI, to determine putative loci that might outperform COI. We use transcriptomes of 14 tephritid fruit flies and especially the taxonomically complex genus Bactrocera, as a case study. Of 1646 orthologues searched, our workflow retained a total of five loci following our conservative filtering strategy. One locus, POP4, had strong potential as a novel diagnostic marker for Bactrocera fruit flies. POP4 discriminates most species in the training set of taxa, but like COI fails to separate the sibling species Bactrocera tryoni and Bactrocera neohumeralis. Further validation of this potential new marker against a broader taxonomic sample is ongoing. We advocate that this simple and efficient workflow is, with minor modification, customisable for diagnostic development in almost any taxonomic group.

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Section: Methodsmentioning

confidence: 99%

A transcriptome‐based analytical workflow for identifying loci for species diagnosis: a case study with Bactrocera fruit flies (Diptera: Tephritidae)

et al. 2017

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“…Here, we utilise RNAseq data for C. draysoni obtained in a previous comparative transcriptomic study to explore patterns of differential expression within-species 40 (BioProject PRJNA350713, Transcriptome Shotgun Assembly Accession GFNI00000000, Short Read Archive Accessions in Table 1 ). Details of specimen collection, preservation, processing, RNA extraction, sequencing and read filtering are described in Krosch & Bryant (2015) 58 and Krosch (2017) 40 . Cleaned reads were assembled with Trinity Version 2014–04–13pl package 59 .…”

Section: Methodsmentioning

confidence: 99%

Differential gene expression of Australian Cricotopus draysoni (Diptera: Chironomidae) populations reveals seasonal association in detoxification gene regulation

Krosch

Bryant

Vink

2017

Sci Rep

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Understanding the molecular mechanisms of organismal response to human-derived ecosystem change is recognised as a critical tool in monitoring and managing impacts, especially in freshwater systems. Fundamental to this approach is to determine the genes involved in responding to ecosystem change and detect modifications to their expression and activity in natural populations. Potential targets for this approach include well-known detoxification genes that are upregulated in response to stress. Here, we tested whether expression of such genes varied in association with differences in ecosystem health and could be detected in the field. We sampled populations of the freshwater midge, Cricotopus draysoni, from two geographically proximate sites in southeast Queensland, Australia, which differed in their ecosystem health, at multiple time points. We assessed transcriptome-level differential gene expression and predicted greatest differential expression between sites, associated with organismal responses to local physico-chemical factors. In contrast, we observed a clear and dramatic difference in gene expression – including of known detoxification genes – between time points, specifically between periods at the start and end of the austral summer rainfall when in-stream water levels are most different. These data suggest that these waterways experience greatest pollution load when water levels are high following rainfall events.

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Comparative analysis of larval transcriptomes from co-occurring species of AustralianCricotopus(Diptera: Chironomidae)

Krosch

2016

Austral Entomology

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A note on sampling chironomids for RNA-based studies of natural populations that retains critical morphological vouchers

Cited by 3 publications

References 22 publications

A transcriptome‐based analytical workflow for identifying loci for species diagnosis: a case study with Bactrocera fruit flies (Diptera: Tephritidae)

A transcriptome‐based analytical workflow for identifying loci for species diagnosis: a case study with Bactrocera fruit flies (Diptera: Tephritidae)

Differential gene expression of Australian Cricotopus draysoni (Diptera: Chironomidae) populations reveals seasonal association in detoxification gene regulation

Comparative analysis of larval transcriptomes from co-occurring species of AustralianCricotopus(Diptera: Chironomidae)

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