References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)

Detalhes bibliográficos
Autor(a) principal: Schimpl, Flávia Camila
Data de Publicação: 2015
Outros Autores: Domingues Júnior, Adilson Pereira, Gonçalves, José Francisco Carvalho de, Silva, José Ferreira da, Mazzafera, Paulo
Tipo de documento: Artigo
Idioma: eng
Título da fonte: Repositório Institucional do INPA
Texto Completo: https://repositorio.inpa.gov.br/handle/1/15305
Resumo: Gene expression has been extensively studied in plant science research, mainly for the assessment of plant stress responses. Real-time-quantitative polymerase chain reaction (RT-qPCR) is an important tool for obtaining this information because it is a quick and easy technique to acquire a large amount of molecular data for both model and non-model plants. For a successful RT-qPCR analysis, gene expression should be carefully normalised. Genes involved in essential biological processes that exhibit constitutive expression are commonly selected as internal standards to normalise RT-qPCR experiments. In this study, the transcription profiles of 13 candidate reference genes for RT-qPCR were evaluated in three guarana cultivars (BRS-Amazonas, BRS-Maués and BRS-Luzéia) using different tissues (vegetative and fruit) in varying developmental stages. Two different algorithms, NormFinder and GeNorm, were utilised to assess gene stability. In general, the two algorithms did not select the same pairs of genes for all analysed conditions. For the largest group (the fruits of all cultivars), NormFinder selected the pair EF1A/UBQ, whereas GeNorm chose ACT/GAPDH as the best normalising genes. Thus, we recommend the use of at least four reference genes for the normalisation of gene expression in guarana plant studies. © 2015, Botanical Society of Sao Paulo.
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spelling Schimpl, Flávia CamilaDomingues Júnior, Adilson PereiraGonçalves, José Francisco Carvalho deSilva, José Ferreira daMazzafera, Paulo2020-05-07T16:33:58Z2020-05-07T16:33:58Z2015https://repositorio.inpa.gov.br/handle/1/1530510.1007/s40415-015-0147-9Gene expression has been extensively studied in plant science research, mainly for the assessment of plant stress responses. Real-time-quantitative polymerase chain reaction (RT-qPCR) is an important tool for obtaining this information because it is a quick and easy technique to acquire a large amount of molecular data for both model and non-model plants. For a successful RT-qPCR analysis, gene expression should be carefully normalised. Genes involved in essential biological processes that exhibit constitutive expression are commonly selected as internal standards to normalise RT-qPCR experiments. In this study, the transcription profiles of 13 candidate reference genes for RT-qPCR were evaluated in three guarana cultivars (BRS-Amazonas, BRS-Maués and BRS-Luzéia) using different tissues (vegetative and fruit) in varying developmental stages. Two different algorithms, NormFinder and GeNorm, were utilised to assess gene stability. In general, the two algorithms did not select the same pairs of genes for all analysed conditions. For the largest group (the fruits of all cultivars), NormFinder selected the pair EF1A/UBQ, whereas GeNorm chose ACT/GAPDH as the best normalising genes. Thus, we recommend the use of at least four reference genes for the normalisation of gene expression in guarana plant studies. © 2015, Botanical Society of Sao Paulo.Volume 38, Número 2, Pags. 281-288Attribution-NonCommercial-NoDerivs 3.0 Brazilhttp://creativecommons.org/licenses/by-nc-nd/3.0/br/info:eu-repo/semantics/openAccessReferences genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)info:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/articleRevista Brasileira de Botanicaengreponame:Repositório Institucional do INPAinstname:Instituto Nacional de Pesquisas da Amazônia (INPA)instacron:INPAORIGINALartigo-inpa.pdfapplication/pdf583856https://repositorio.inpa.gov.br/bitstream/1/15305/1/artigo-inpa.pdf6deee2b051c0a77a2979f1c6a3f423f3MD51CC-LICENSElicense_rdfapplication/octet-stream914https://repositorio.inpa.gov.br/bitstream/1/15305/2/license_rdf4d2950bda3d176f570a9f8b328dfbbefMD521/153052020-07-14 11:07:54.594oai:repositorio:1/15305Repositório de PublicaçõesPUBhttps://repositorio.inpa.gov.br/oai/requestopendoar:2020-07-14T15:07:54Repositório Institucional do INPA - Instituto Nacional de Pesquisas da Amazônia (INPA)false
dc.title.en.fl_str_mv References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
title References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
spellingShingle References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
Schimpl, Flávia Camila
title_short References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
title_full References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
title_fullStr References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
title_full_unstemmed References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
title_sort References genes for qRT-PCR in guaraná (Paullina cupana var. sorbilis)
author Schimpl, Flávia Camila
author_facet Schimpl, Flávia Camila
Domingues Júnior, Adilson Pereira
Gonçalves, José Francisco Carvalho de
Silva, José Ferreira da
Mazzafera, Paulo
author_role author
author2 Domingues Júnior, Adilson Pereira
Gonçalves, José Francisco Carvalho de
Silva, José Ferreira da
Mazzafera, Paulo
author2_role author
author
author
author
dc.contributor.author.fl_str_mv Schimpl, Flávia Camila
Domingues Júnior, Adilson Pereira
Gonçalves, José Francisco Carvalho de
Silva, José Ferreira da
Mazzafera, Paulo
description Gene expression has been extensively studied in plant science research, mainly for the assessment of plant stress responses. Real-time-quantitative polymerase chain reaction (RT-qPCR) is an important tool for obtaining this information because it is a quick and easy technique to acquire a large amount of molecular data for both model and non-model plants. For a successful RT-qPCR analysis, gene expression should be carefully normalised. Genes involved in essential biological processes that exhibit constitutive expression are commonly selected as internal standards to normalise RT-qPCR experiments. In this study, the transcription profiles of 13 candidate reference genes for RT-qPCR were evaluated in three guarana cultivars (BRS-Amazonas, BRS-Maués and BRS-Luzéia) using different tissues (vegetative and fruit) in varying developmental stages. Two different algorithms, NormFinder and GeNorm, were utilised to assess gene stability. In general, the two algorithms did not select the same pairs of genes for all analysed conditions. For the largest group (the fruits of all cultivars), NormFinder selected the pair EF1A/UBQ, whereas GeNorm chose ACT/GAPDH as the best normalising genes. Thus, we recommend the use of at least four reference genes for the normalisation of gene expression in guarana plant studies. © 2015, Botanical Society of Sao Paulo.
publishDate 2015
dc.date.issued.fl_str_mv 2015
dc.date.accessioned.fl_str_mv 2020-05-07T16:33:58Z
dc.date.available.fl_str_mv 2020-05-07T16:33:58Z
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dc.identifier.doi.none.fl_str_mv 10.1007/s40415-015-0147-9
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identifier_str_mv 10.1007/s40415-015-0147-9
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dc.relation.ispartof.pt_BR.fl_str_mv Volume 38, Número 2, Pags. 281-288
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http://creativecommons.org/licenses/by-nc-nd/3.0/br/
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publisher.none.fl_str_mv Revista Brasileira de Botanica
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