dc.contributor.author |
Florez Liz |
en |
dc.contributor.author |
Scheper Reiny |
en |
dc.contributor.author |
Fisher Brent |
en |
dc.contributor.author |
Sutherland Paul |
en |
dc.contributor.author |
Templeton Matthew |
en |
dc.contributor.author |
Bowen Joanna |
en |
dc.date.accessioned |
2020-10-12T00:45:07Z |
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dc.date.available |
2020-10-12T00:45:07Z |
|
dc.date.issued |
2020-8-12 |
en |
dc.identifier.citation |
12 Aug 2020. BioRxiv. 37 pages |
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dc.identifier.uri |
http://hdl.handle.net/2292/53217 |
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dc.description.abstract |
Abstract European canker, caused by the necrotrophic fungal phytopathogen Neonectria ditissima , is one of the most damaging apple diseases worldwide. An understanding of the molecular basis of N. ditissima virulence is currently lacking. Identification of genes with an up-regulation of expression during infection, which are therefore probably involved in virulence, is a first step towards this understanding. Real-time quantitative reverse transcription PCR (qRT-PCR) can be used to identify these candidate virulence genes, but relies on the use of reference genes for relative gene expression data normalisation. However, no report that addresses selecting appropriate fungal reference genes for use in the N. ditissima -apple pathosystem has been published to date. In this study, eight N. ditissima genes were selected as candidate qRT-PCR reference genes for gene expression analysis. A subset of the primers (six) designed to amplify regions from these genes were specific for N. ditissima , failing to amplify PCR products with template from other fungal pathogens present in the apple orchard. The efficiency of amplification of these six primer sets was satisfactory, ranging from 81.8 to 107.53%. Analysis of expression stability when a highly pathogenic N. ditissima isolate was cultured under 10 regimes, using the statistical algorithms geNorm, NormFinder and BestKeeper, indicated that actin and myo-inositol-1-phosphate synthase ( mips ), or their combination, could be utilised as the most suitable reference genes for normalisation of N. ditissima gene expression. As a test case, these reference genes were used to study expression of three candidate virulence genes during a time course of infection. All three, which shared traits with fungal effector genes, had up-regulated expression in planta compared to in vitro with expression peaking between five and six weeks post inoculation (wpi). Thus, these three genes may well be involved in N. ditissima pathogenicity and are priority candidates for further functional characterization. |
en |
dc.rights |
Items in ResearchSpace are protected by copyright, with all rights reserved, unless otherwise indicated. Previously published items are made available in accordance with the copyright policy of the publisher. |
en |
dc.rights.uri |
https://researchspace.auckland.ac.nz/docs/uoa-docs/rights.htm |
en |
dc.rights.uri |
https://creativecommons.org/licenses/by/4.0/ |
|
dc.title |
Reference genes for gene expression analysis in the fungal pathogen Neonectria ditissima and their use demonstrating expression up-regulation of candidate virulence genes |
en |
dc.type |
Journal Article |
en |
dc.identifier.doi |
10.1101/2020.08.12.247601 |
en |
dc.date.updated |
2020-09-29T02:55:12Z |
en |
dc.rights.holder |
Copyright: The authors |
en |
pubs.publication-status |
Published |
en |
dc.rights.accessrights |
http://purl.org/eprint/accessRights/OpenAccess |
en |
pubs.subtype |
Preprint |
en |
pubs.elements-id |
812752 |
en |