Microarray-based uncovering reference genes for quantitative real time PCR in grapevine under abiotic stress

Coito, João L.; Rocheta, Margarida; Carvalho, Luísa C.; Amâncio, Sara

doi:10.1186/1756-0500-5-220

Cited by 45 publications

(50 citation statements)

References 45 publications

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“…Therefore, to get an accurate expression profiling among multiple samples, more than one reference genes should be used (Brunner et al 2004;Coito et al 2012;Nicot et al 2005;Xu et al 2012;Zhong et al 2011).…”

Section: Discussionmentioning

confidence: 99%

Systematic selection and validation of appropriate reference genes for gene expression studies by quantitative real-time PCR in pear

et al. 2015

Acta Physiol Plant

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RT-qPCR is a widely used method in gene expression and transcriptome studies. Normalization based on reference genes is necessary to accurately analyze RTqPCR data. Thus, an accurate and systematic evaluation of these reference genes before experiments are conducted is necessary. In this study, 18 candidate reference genes were evaluated under various experimental conditions covering a range of tissue types and cultivars, NaCl, CaCl 2 and temperature treatments, hormones (6-BA, ABA and NAA) and a set of osmotic stress (mannitol and PEG6000) treatments. Gene expression across 48 pear samples was evaluated using geNorm, NormFinder and BestKeeper statistical algorithms. Actin2/7 (ACT2/7), ubiquitin extension protein (UBI) and Yellow-leaf-specific gene 8 (YLS8) exhibited the most stable expression across all the pear samples tested. While in the other experimental groups, different sets of samples had their own best reference genes. In addition, the gene expression of PbCBL7, a member of the calcineurin B-like protein, was measured across all the 48 samples using the best three reference genes, it displayed variation in gene expression across different tissues and cultivars, and exhibited diverse up-or down-regulated expression patterns under various treatments, which indicate that PbCBL7 may play a role in response to specific abiotic stress in pear. These results are valuable for future research on gene expression and abiotic stress tolerance in pear.

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Section: Discussionmentioning

confidence: 99%

Systematic selection and validation of appropriate reference genes for gene expression studies by quantitative real-time PCR in pear

et al. 2015

Acta Physiol Plant

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“…Transcripts coding sHSPs (obtained when using the GrapeGene 520510F array (Affymetrix) in plants subjected to 42 °C for 1 h), reference genes (Coito et al . ) and oxidative stress genes (Carvalho et al . ).…”

Section: Methodsmentioning

confidence: 99%

Heat stress in grapevine: the pros and cons of acclimation

Carvalho

Coito

Colaço

et al. 2014

Plant Cell & Environment

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Heat stress is a major limiting factor of grapevine production and quality. Acclimation and recovery are essential to ensure plant survival, and the recovery mechanisms can be independent of the heat response mechanisms. An experimental set up with and without acclimation to heat followed by recovery [stepwise acclimation and recovery (SAR) and stepwise recovery (SR), respectively] was applied to two grapevine varieties, Touriga Nacional (TN), and Trincadeira (TR), with different tolerance to abiotic stress. Major differences were found between leaves of SAR and SR, especially after recovery; in SAR, almost all parameters returned to basal levels while in SR they remained altered. Acclimation led to a swifter and short-term antioxidative response, affecting the plant to a lesser extent than SR. Significant differences were found among varieties: upon stress, TN significantly increased ascorbate and glutathione reduction levels, boosting the cell's redox-buffering capacity, while TR needed to synthesize both metabolites, its response being insufficient to keep the redox state at working levels. TR was affected by stress for a longer period and the up-regulation pattern of antioxidative stress genes was more obvious. In TN, heat shock proteins were significantly induced, but the canonical heat-stress gene signature was not evident probably because no shutdown of the housekeeping metabolism was needed.

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“…In recent years, real-time quantitative PCR (RTqPCR) has been becoming a mainstream technology for gene expression profile analysis due to the higher sensitivity and specificity (Coito et al 2012). Reliable gene expression assays based on RT-qPCR technology are dependent on multiple factors, such as RNA quality, amount of input RNA, the efficiency of RNA reverse transcription and so on (Udvardi et al 2008).…”

Section: Introductionmentioning

confidence: 99%

Reference gene selection in Artemisia annua L., a plant species producing anti-malarial artemisinin

Liu

Zhao

Wang

et al. 2014

Plant Cell Tiss Organ Cult

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The selection and validation of reference genes are essential for gene expression studies by real-time quantitative PCR. The genetic map of Artemisia annua L., a Chinese medicinal plant species producing anti-malarial artemisinin, has been reported. However, few reference genes of A. annua have been estimated for real-time quantitative PCR until now. In this study, ten putative housekeeping genes, including ACT, UBQ, TUB, 18S rRNA, EF1a, CYP, RPL13D, TUA, RPII and GAPDH, were chosen for identifying expression stability using geNorm and NormFinder software tools in 11 different sample pools, containing those from different plant organs and from plants treated with phytohormones and abiotic stresses. As

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Microarray-based uncovering reference genes for quantitative real time PCR in grapevine under abiotic stress

Cited by 45 publications

References 45 publications

Systematic selection and validation of appropriate reference genes for gene expression studies by quantitative real-time PCR in pear

Systematic selection and validation of appropriate reference genes for gene expression studies by quantitative real-time PCR in pear

Heat stress in grapevine: the pros and cons of acclimation

Reference gene selection in Artemisia annua L., a plant species producing anti-malarial artemisinin

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