Multiplicação e regeneração in vitro de marmeleiro
Autor(a) principal: | |
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Data de Publicação: | 2013 |
Tipo de documento: | Tese |
Idioma: | por |
Título da fonte: | Repositório Institucional da UFPel - Guaiaca |
Texto Completo: | http://repositorio.ufpel.edu.br/handle/ri/1993 |
Resumo: | Pear orchards with high density planting were possible due to the use of rootstock quince (Cydonia oblonga Mill.), thus obtaining small plants and rapid fruiting, and provide uniformity to these orchards. Techniques that may improve the ability to propagation this rootstock are of great interest. The aim of this study was to adjust protocols for in vitro multiplication and regeneration of quince cultivars MC and Adams. The results of this word are presented in chapter. Material used in the experiments was obtained from in vitro propagation in culture medium consisting of MS salts and vitamins supplemented with myo-inositol (100 mg L-1), 6 - benzylaminopurine (BA) (0.3 mg L-1), sucrose (30 g L-1) and agar (8 g L-1). Chapter 1 we used MS medium added agar (8 g L-1) on solidified medium and vermiculite (3 g flask-1) in the liquid medium and the flasks were sealed with aluminum foil, PVC film and polypropylene cap. In Chapter 2 how carbon source in culture medium was added sucrose, fructose or sorbitol at concentrations 0, 15, 30, 45 and 60 g L-1. For in vitro regeneration the Chapter 3 was divided in two experiments. In experiment 1 the culture medium consisted of salts and vitamins MS and SH supplemented with myoinositol (100 mg L-1), sucrose (30 g L-1), agar (8 g L-1), NAA (2 mM) and TDZ at concentrations 0, 1.5, 3, 4.5 and 6 μM. In experiment 2 the culture medium consisted of SH salts and vitamins supplemented with myo-inositol (100 mg L-1), sucrose (30 g L-1), agar (8 g L-1), TDZ (0 , 1.5, 3, 4.5 and 6 μM) combined with NAA or IBA at concentrations of 0, 1.0, 1.5 and 2 μM. All experiments were evaluated after 60 days. Considering the results presented in Chapter 1 is possible to conclude that the use of culture medium solidified with agar and the flasks sealed with aluminum foil or polypropylene cap favored the in vitro multiplication of quince 'MC' and 'Adams'. In the second chapter it was found that the sucrose concentration of 45 g L-1 to cultivar MC and 30 g L-1 to cultivar Adams are the best concentrations and carbon source for in vitro multiplication quince. In the Chapter 3 first verified in experiment 1 that the in vitro regeneration of adventitious shoots quince cultivars MC and Adams was favored by the use of SH culture medium and addition of 4.5 μM TDZ to cultivar MC and 6 μM TDZ for cultivar Adams. And in experiment 2 it was concluded that multiple shoots were formed from the combination of 4.5 μM TDZ and 2 μM NAA for cultivar MC and 6 μM TDZ and 2 μM NAA to cultivar Adams. |
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2014-08-20T13:59:05Z2013-04-292014-08-20T13:59:05Z2013-03-28RIBEIRO, Mirian de Farias. In vitro multiplication and regeneration of quince. 2013. 157 f. Tese (Doutorado em Biologia) - Universidade Federal de Pelotas, Pelotas, 2013.http://repositorio.ufpel.edu.br/handle/ri/1993Pear orchards with high density planting were possible due to the use of rootstock quince (Cydonia oblonga Mill.), thus obtaining small plants and rapid fruiting, and provide uniformity to these orchards. Techniques that may improve the ability to propagation this rootstock are of great interest. The aim of this study was to adjust protocols for in vitro multiplication and regeneration of quince cultivars MC and Adams. The results of this word are presented in chapter. Material used in the experiments was obtained from in vitro propagation in culture medium consisting of MS salts and vitamins supplemented with myo-inositol (100 mg L-1), 6 - benzylaminopurine (BA) (0.3 mg L-1), sucrose (30 g L-1) and agar (8 g L-1). Chapter 1 we used MS medium added agar (8 g L-1) on solidified medium and vermiculite (3 g flask-1) in the liquid medium and the flasks were sealed with aluminum foil, PVC film and polypropylene cap. In Chapter 2 how carbon source in culture medium was added sucrose, fructose or sorbitol at concentrations 0, 15, 30, 45 and 60 g L-1. For in vitro regeneration the Chapter 3 was divided in two experiments. In experiment 1 the culture medium consisted of salts and vitamins MS and SH supplemented with myoinositol (100 mg L-1), sucrose (30 g L-1), agar (8 g L-1), NAA (2 mM) and TDZ at concentrations 0, 1.5, 3, 4.5 and 6 μM. In experiment 2 the culture medium consisted of SH salts and vitamins supplemented with myo-inositol (100 mg L-1), sucrose (30 g L-1), agar (8 g L-1), TDZ (0 , 1.5, 3, 4.5 and 6 μM) combined with NAA or IBA at concentrations of 0, 1.0, 1.5 and 2 μM. All experiments were evaluated after 60 days. Considering the results presented in Chapter 1 is possible to conclude that the use of culture medium solidified with agar and the flasks sealed with aluminum foil or polypropylene cap favored the in vitro multiplication of quince 'MC' and 'Adams'. In the second chapter it was found that the sucrose concentration of 45 g L-1 to cultivar MC and 30 g L-1 to cultivar Adams are the best concentrations and carbon source for in vitro multiplication quince. In the Chapter 3 first verified in experiment 1 that the in vitro regeneration of adventitious shoots quince cultivars MC and Adams was favored by the use of SH culture medium and addition of 4.5 μM TDZ to cultivar MC and 6 μM TDZ for cultivar Adams. And in experiment 2 it was concluded that multiple shoots were formed from the combination of 4.5 μM TDZ and 2 μM NAA for cultivar MC and 6 μM TDZ and 2 μM NAA to cultivar Adams.Pomares de pereira com plantio em alta densidade foram possíveis devido a utilização de portaenxerto de marmeleiro (Cydonia oblonga Mill.), obtendo-se assim plantas de pequeno porte e rápida frutificação, além de proporcionar uniformidade a esses pomares. Técnicas que venham melhorar a capacidade de propagação deste portaenxerto são de grande interesse. O objetivo desse trabalho foi ajustar protocolos de multiplicação e regeneração in vitro de marmeleiro cultivares MC e Adams. Os resultados do trabalho estão apresentados na forma de capítulos. O material vegetal utilizado nos experimentos foi obtido a partir da multiplicação in vitro em meio de cultura básico composto dos sais e vitaminas MS, suplementados com mio-inositol (100 mg L-1), 6- benzilaminopurina (BAP) (0,3 mg L-1), sacarose (30 g L- 1) e ágar (8 g L-1). No capítulo 1, utilizou-se meio básico acrescentado de ágar (8 g L- 1) no meio solidificado e vermiculita (3 g frasco-1) no meio líquido e os frascos foram vedados com papel alumínio, filme PVC e tampa de polipropileno. No capítulo 2, como fonte de carbono no meio de cultura foi utilizado sacarose, frutose ou sorbitol nas concentrações de 0, 15, 30, 45 e 60 g L-1. Para regeneração in vitro o capítulo 3 foi dividido em dois experimentos. No experimento 1 os meios de cultura constituíram-se dos sais e vitaminas MS e SH, suplementados com mio-inositol (100 mg L-1), sacarose (30 g L-1), ágar (8 g L-1), ANA (2 μM) e TDZ nas concentrações de 0, 1,5, 3, 4,5 e 6 μM. No experimento 2 o meio de cultura constituiu-se dos sais e vitaminas SH, suplementado com mio-inositol (100 mg L-1), sacarose (30 g L-1), ágar (8 g L-1), TDZ (0, 1,5, 3, 4,5 e 6 μM) combinado com ANA ou AIB nas concentrações de 0; 1,0; 1,5 e 2 μM. Todos os experimentos foram avaliados após 60 dias. Diante dos resultados apresentados no capítulo 1 é possível concluir que a utilização de meio de cultura solidificado com ágar e os frascos vedados com papel alumínio ou tampa de polipropileno favorecem a multiplicação in vitro de marmeleiro 'MC' e 'Adams'. No capítulo 2 constatou-se que a sacarose na concentração de 45 g L-1 para cultivar MC e 30 g L-1 para cultivar Adams são as melhores concentrações e fonte de carbono para multiplicação in vitro dos portaenxertos de marmeleiro testados. No capítulo 3, primeiro verificou-se no experimento 1 que a regeneração in vitro de brotos adventícios de marmeleiro das cultivares MC e Adams foi favorecida pelo uso do meio de cultura SH e pela adição de 4,5 μM de TDZ para cultivar MC e 6 μM de TDZ para a cultivar Adams. No experimento 2 concluiu-se que houve maior taxa de regeneração a partir da combinação de 4,5 μM de TDZ e 2 μM de ANA para cultivar MC e 6 μM de TDZ e 2 μM de ANA para cultivar Adams.application/pdfporUniversidade Federal de PelotasPrograma de Pós-Graduação em Fisiologia VegetalUFPelBRBiologiaCydonia oblongaMicroambienteReguladores de crescimentoOrganogêneseCydonia oblongaMicroenvironmentGrowth regulatorsOrganogenesisCNPQ::CIENCIAS BIOLOGICAS::BOTANICA::FISIOLOGIA VEGETALMultiplicação e regeneração in vitro de marmeleiroIn vitro multiplication and regeneration of quinceinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/doctoralThesishttp://lattes.cnpq.br/5928016514739758http://lattes.cnpq.br/9373170196787637Bianchi, Valmor JoãoRibeiro, Mirian de Fariasinfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UFPel - Guaiacainstname:Universidade Federal de Pelotas (UFPEL)instacron:UFPELORIGINALtese_mirian_de_farias_ribeiro.pdfapplication/pdf2449435http://guaiaca.ufpel.edu.br/xmlui/bitstream/123456789/1993/1/tese_mirian_de_farias_ribeiro.pdf6695d40137c267cf6058be71ba7803e7MD51open accessTEXTtese_mirian_de_farias_ribeiro.pdf.txttese_mirian_de_farias_ribeiro.pdf.txtExtracted Texttext/plain121894http://guaiaca.ufpel.edu.br/xmlui/bitstream/123456789/1993/2/tese_mirian_de_farias_ribeiro.pdf.txte704b1e4a16b88590d61b9c644a6758fMD52open accessTHUMBNAILtese_mirian_de_farias_ribeiro.pdf.jpgtese_mirian_de_farias_ribeiro.pdf.jpgGenerated Thumbnailimage/jpeg1277http://guaiaca.ufpel.edu.br/xmlui/bitstream/123456789/1993/3/tese_mirian_de_farias_ribeiro.pdf.jpgedcca32aaae1fb910f426d14951f8ef6MD53open access123456789/19932019-08-19 12:02:49.643open accessoai:guaiaca.ufpel.edu.br:123456789/1993Repositório InstitucionalPUBhttp://repositorio.ufpel.edu.br/oai/requestrippel@ufpel.edu.br || repositorio@ufpel.edu.br || aline.batista@ufpel.edu.bropendoar:2019-08-19T15:02:49Repositório Institucional da UFPel - Guaiaca - Universidade Federal de Pelotas (UFPEL)false |
dc.title.por.fl_str_mv |
Multiplicação e regeneração in vitro de marmeleiro |
dc.title.alternative.eng.fl_str_mv |
In vitro multiplication and regeneration of quince |
title |
Multiplicação e regeneração in vitro de marmeleiro |
spellingShingle |
Multiplicação e regeneração in vitro de marmeleiro Ribeiro, Mirian de Farias Cydonia oblonga Microambiente Reguladores de crescimento Organogênese Cydonia oblonga Microenvironment Growth regulators Organogenesis CNPQ::CIENCIAS BIOLOGICAS::BOTANICA::FISIOLOGIA VEGETAL |
title_short |
Multiplicação e regeneração in vitro de marmeleiro |
title_full |
Multiplicação e regeneração in vitro de marmeleiro |
title_fullStr |
Multiplicação e regeneração in vitro de marmeleiro |
title_full_unstemmed |
Multiplicação e regeneração in vitro de marmeleiro |
title_sort |
Multiplicação e regeneração in vitro de marmeleiro |
author |
Ribeiro, Mirian de Farias |
author_facet |
Ribeiro, Mirian de Farias |
author_role |
author |
dc.contributor.authorLattes.por.fl_str_mv |
http://lattes.cnpq.br/5928016514739758 |
dc.contributor.advisorLattes.por.fl_str_mv |
http://lattes.cnpq.br/9373170196787637 |
dc.contributor.advisor1.fl_str_mv |
Bianchi, Valmor João |
dc.contributor.author.fl_str_mv |
Ribeiro, Mirian de Farias |
contributor_str_mv |
Bianchi, Valmor João |
dc.subject.por.fl_str_mv |
Cydonia oblonga Microambiente Reguladores de crescimento Organogênese |
topic |
Cydonia oblonga Microambiente Reguladores de crescimento Organogênese Cydonia oblonga Microenvironment Growth regulators Organogenesis CNPQ::CIENCIAS BIOLOGICAS::BOTANICA::FISIOLOGIA VEGETAL |
dc.subject.eng.fl_str_mv |
Cydonia oblonga Microenvironment Growth regulators Organogenesis |
dc.subject.cnpq.fl_str_mv |
CNPQ::CIENCIAS BIOLOGICAS::BOTANICA::FISIOLOGIA VEGETAL |
description |
Pear orchards with high density planting were possible due to the use of rootstock quince (Cydonia oblonga Mill.), thus obtaining small plants and rapid fruiting, and provide uniformity to these orchards. Techniques that may improve the ability to propagation this rootstock are of great interest. The aim of this study was to adjust protocols for in vitro multiplication and regeneration of quince cultivars MC and Adams. The results of this word are presented in chapter. Material used in the experiments was obtained from in vitro propagation in culture medium consisting of MS salts and vitamins supplemented with myo-inositol (100 mg L-1), 6 - benzylaminopurine (BA) (0.3 mg L-1), sucrose (30 g L-1) and agar (8 g L-1). Chapter 1 we used MS medium added agar (8 g L-1) on solidified medium and vermiculite (3 g flask-1) in the liquid medium and the flasks were sealed with aluminum foil, PVC film and polypropylene cap. In Chapter 2 how carbon source in culture medium was added sucrose, fructose or sorbitol at concentrations 0, 15, 30, 45 and 60 g L-1. For in vitro regeneration the Chapter 3 was divided in two experiments. In experiment 1 the culture medium consisted of salts and vitamins MS and SH supplemented with myoinositol (100 mg L-1), sucrose (30 g L-1), agar (8 g L-1), NAA (2 mM) and TDZ at concentrations 0, 1.5, 3, 4.5 and 6 μM. In experiment 2 the culture medium consisted of SH salts and vitamins supplemented with myo-inositol (100 mg L-1), sucrose (30 g L-1), agar (8 g L-1), TDZ (0 , 1.5, 3, 4.5 and 6 μM) combined with NAA or IBA at concentrations of 0, 1.0, 1.5 and 2 μM. All experiments were evaluated after 60 days. Considering the results presented in Chapter 1 is possible to conclude that the use of culture medium solidified with agar and the flasks sealed with aluminum foil or polypropylene cap favored the in vitro multiplication of quince 'MC' and 'Adams'. In the second chapter it was found that the sucrose concentration of 45 g L-1 to cultivar MC and 30 g L-1 to cultivar Adams are the best concentrations and carbon source for in vitro multiplication quince. In the Chapter 3 first verified in experiment 1 that the in vitro regeneration of adventitious shoots quince cultivars MC and Adams was favored by the use of SH culture medium and addition of 4.5 μM TDZ to cultivar MC and 6 μM TDZ for cultivar Adams. And in experiment 2 it was concluded that multiple shoots were formed from the combination of 4.5 μM TDZ and 2 μM NAA for cultivar MC and 6 μM TDZ and 2 μM NAA to cultivar Adams. |
publishDate |
2013 |
dc.date.available.fl_str_mv |
2013-04-29 2014-08-20T13:59:05Z |
dc.date.issued.fl_str_mv |
2013-03-28 |
dc.date.accessioned.fl_str_mv |
2014-08-20T13:59:05Z |
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info:eu-repo/semantics/publishedVersion |
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info:eu-repo/semantics/doctoralThesis |
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doctoralThesis |
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publishedVersion |
dc.identifier.citation.fl_str_mv |
RIBEIRO, Mirian de Farias. In vitro multiplication and regeneration of quince. 2013. 157 f. Tese (Doutorado em Biologia) - Universidade Federal de Pelotas, Pelotas, 2013. |
dc.identifier.uri.fl_str_mv |
http://repositorio.ufpel.edu.br/handle/ri/1993 |
identifier_str_mv |
RIBEIRO, Mirian de Farias. In vitro multiplication and regeneration of quince. 2013. 157 f. Tese (Doutorado em Biologia) - Universidade Federal de Pelotas, Pelotas, 2013. |
url |
http://repositorio.ufpel.edu.br/handle/ri/1993 |
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UFPel |
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