Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros

Detalhes bibliográficos
Autor(a) principal: Machado, Caroline de Araújo
Data de Publicação: 2012
Tipo de documento: Dissertação
Idioma: por
Título da fonte: Repositório Institucional da UFS
Texto Completo: https://ri.ufs.br/handle/riufs/6595
Resumo: The conservation of the coconut palm has been investigated in recent years by research organizations, public and private. These studies have concentrated on obtaining conservation protocols in vitro using slow growth and cryopreservation. Storage as a means of maintaining the viability of pollen, it is important for the preservation of genetic variability, facilitates the exchange of germplasm and contributes greatly to the generation of variability obtained from artificial crosses increasing the efficiency of breeding programs. The objective of this work was to study the effect of mannitol and abscisic acid (ABA) on growth of seedlings of coconut dwarf accessions for conservation purposes, and in vivo studies of the viability and storage conditions of pollen grains. For the study of conservation by slow growth were used mature zygotic embryos of Gramame Red Dwarf (AVG) and Malayan Yellow Dwarf (AAM). The coconut embryos were inoculated in culture medium Y3 (Eeuwens, 1976) supplemented with 30 g L-1 sucrose, gelled with 0.7% agar in presence of 2.5 g L-1 of activated charcoal. Were tested the following concentrations of mannitol: 0; 0.1; 0.2, 0.3 and 0.4 M. In other experiment was tested the following ABA concentrations: 0, 10, 20, 30 and 40 mM. The 0.1 and 0.2 M mannitol reduced the plantlets length of AAM and AVG accessions, respectively at 180 and 270 days of cultivation. Concentrations above 20 μM ABA were viable to inhibit the plantlets growth to 180 and 270 days. The ABA concentrations tested not inhibit the access AVG growth. For the study of determining the culture medium in germination of pollen grains, it was evaluated four culture media: Brewbaker and Kwack (1983) modified by Sousa et al. (2010); Lora et al. (2006); Sousa et al. (1998) and Sousa et al. (1998) modified by the author, in different times: 0, 24, 48 and 72 hours. The Lora culture medium promoted the major in vitro germination of AVeJBr pollen grains. Pollen grains of AVeJBr access showed viability up to 72 hours (3 days). The condition of storage at -20°C and -80°C promotes more viable pollen germination of AVC access up to 60 days. The condition of storage at -196°C promotes greater availability of pollen germination by AVeJBr access up to 60 days.
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spelling Machado, Caroline de AraújoLédo, Ana da Silvahttp://lattes.cnpq.br/12273191060798822017-10-02T12:49:40Z2017-10-02T12:49:40Z2012-04-23https://ri.ufs.br/handle/riufs/6595The conservation of the coconut palm has been investigated in recent years by research organizations, public and private. These studies have concentrated on obtaining conservation protocols in vitro using slow growth and cryopreservation. Storage as a means of maintaining the viability of pollen, it is important for the preservation of genetic variability, facilitates the exchange of germplasm and contributes greatly to the generation of variability obtained from artificial crosses increasing the efficiency of breeding programs. The objective of this work was to study the effect of mannitol and abscisic acid (ABA) on growth of seedlings of coconut dwarf accessions for conservation purposes, and in vivo studies of the viability and storage conditions of pollen grains. For the study of conservation by slow growth were used mature zygotic embryos of Gramame Red Dwarf (AVG) and Malayan Yellow Dwarf (AAM). The coconut embryos were inoculated in culture medium Y3 (Eeuwens, 1976) supplemented with 30 g L-1 sucrose, gelled with 0.7% agar in presence of 2.5 g L-1 of activated charcoal. Were tested the following concentrations of mannitol: 0; 0.1; 0.2, 0.3 and 0.4 M. In other experiment was tested the following ABA concentrations: 0, 10, 20, 30 and 40 mM. The 0.1 and 0.2 M mannitol reduced the plantlets length of AAM and AVG accessions, respectively at 180 and 270 days of cultivation. Concentrations above 20 μM ABA were viable to inhibit the plantlets growth to 180 and 270 days. The ABA concentrations tested not inhibit the access AVG growth. For the study of determining the culture medium in germination of pollen grains, it was evaluated four culture media: Brewbaker and Kwack (1983) modified by Sousa et al. (2010); Lora et al. (2006); Sousa et al. (1998) and Sousa et al. (1998) modified by the author, in different times: 0, 24, 48 and 72 hours. The Lora culture medium promoted the major in vitro germination of AVeJBr pollen grains. Pollen grains of AVeJBr access showed viability up to 72 hours (3 days). The condition of storage at -20°C and -80°C promotes more viable pollen germination of AVC access up to 60 days. The condition of storage at -196°C promotes greater availability of pollen germination by AVeJBr access up to 60 days.A conservação do coqueiro tem sido alvo de estudos nos últimos anos por organizações de pesquisa pública e privada. Essas pesquisas têm se concentrado na obtenção de protocolos por crescimento lento ou criopreservação. O armazenamento, como meio de manutenção da viabilidade do pólen, é importante para a preservação da variabilidade genética, facilita o intercâmbio de germoplasma e contribui muito na geração de variabilidade obtida através de cruzamentos artificiais aumentando a eficiência dos programas de melhoramento genético. O objetivo do trabalho foi de estudar o efeito do manitol e do ácido abscísico (ABA) no crescimento de plântulas de acessos de coqueiro anão para fins de conservação, além de estudos da viabilidade in vivo e condições de armazenamento de grãos de pólen. Para o estudo de conservação por crescimento lento foram utilizados embriões zigóticos maduros de acessos de coqueiro anão vermelho de Gramame (AVG) e anão amarelo da Malásia (AAM) e para estudos da viabilidade in vivo e condições de armazenamento de grãos de pólen o acesso anão verde de Jiqui do Brasil (AVeJBr). Os embriões foram inoculados em meio de cultura Y3 com 30 g L-1 de sacarose, geleificado com 0,7% de ágar na presença de 2,5 g L-1 de carvão ativado. Foram testadas as seguintes concentrações de manitol: 0; 0,1; 0,2; 0,3 e 0,4 M. Em outro ensaio o ABA foi adicionado ao meio de cultura nas concentrações de 0; 10; 20; 30 e 40 μM. As concentrações de 0,1 e 0,2 M de manitol reduziram o comprimento da parte aérea para os acessos AAM e AVG, respectivamente aos 180 e 270 dias de cultivo. Concentrações acima de 20μM do ABA foram viáveis para inibir o crescimento de plântulas aos 180 e 270 dias. O acesso AVG não sofreu inibição do comprimento da parte aérea, quando concentrações de ABA foram adicionadas ao meio de cultura. Foram avaliados quatro meios de cultura para germinação in vitro do acesso AVeJBr: Brewbaker & Kwack (1983) modificado por Sousa et al. (2010); Lora et al. (2006); Sousa et al. (1998) e Sousa et al. (1998) modificado pelo autor, em diferentes tempos: 0, 24, 48 e 72 horas. O meio de cultura de Lora promoveu a maior germinação de grãos de pólen do acesso AVeJBr. Grãos de pólen de coqueiro AVeJBr apresentaram viabilidade média, sob temperatura ambiente, até 72 horas (3 dias). A condição de armazenamento a -20°C e -80°C promove maior viabilidade de grãos de pólen por germinação do acesso AVC até os 60 dias. A condição de armazenamento a -196°C promove maior viabilidade de grãos de pólen por germinação do acesso AVeJBr até os 60 dias.application/pdfporUniversidade Federal de SergipePós-Graduação em AgroecossistemasUFSBRCocos nucifera L.GermoplasmaGrãos de pólenArmazenamentoEmbriões zigóticosCocos nucifera L.GermplasmGrain pollenStorageZygotic embryosCNPQ::CIENCIAS AGRARIAS::AGRONOMIAEstratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros CosteirosConservation strategies for coconut dwarf accessions of Embrapa Coastal Tablelands BAGinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesisinfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UFSinstname:Universidade Federal de Sergipe (UFS)instacron:UFSORIGINALCAROLINE_ARAUJO_MACHADO.pdfapplication/pdf2623624https://ri.ufs.br/jspui/bitstream/riufs/6595/1/CAROLINE_ARAUJO_MACHADO.pdf4b01798737eac42a2e75534c0d7f1537MD51TEXTCAROLINE_ARAUJO_MACHADO.pdf.txtCAROLINE_ARAUJO_MACHADO.pdf.txtExtracted texttext/plain109829https://ri.ufs.br/jspui/bitstream/riufs/6595/2/CAROLINE_ARAUJO_MACHADO.pdf.txt6180b4a5972c4ffaf4d9347904befb46MD52THUMBNAILCAROLINE_ARAUJO_MACHADO.pdf.jpgCAROLINE_ARAUJO_MACHADO.pdf.jpgGenerated Thumbnailimage/jpeg1349https://ri.ufs.br/jspui/bitstream/riufs/6595/3/CAROLINE_ARAUJO_MACHADO.pdf.jpg561d6d4c1276e27dbcae998374de3867MD53riufs/65952017-11-24 20:58:53.554oai:ufs.br:riufs/6595Repositório InstitucionalPUBhttps://ri.ufs.br/oai/requestrepositorio@academico.ufs.bropendoar:2017-11-24T23:58:53Repositório Institucional da UFS - Universidade Federal de Sergipe (UFS)false
dc.title.por.fl_str_mv Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
dc.title.alternative.eng.fl_str_mv Conservation strategies for coconut dwarf accessions of Embrapa Coastal Tablelands BAG
title Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
spellingShingle Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
Machado, Caroline de Araújo
Cocos nucifera L.
Germoplasma
Grãos de pólen
Armazenamento
Embriões zigóticos
Cocos nucifera L.
Germplasm
Grain pollen
Storage
Zygotic embryos
CNPQ::CIENCIAS AGRARIAS::AGRONOMIA
title_short Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
title_full Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
title_fullStr Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
title_full_unstemmed Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
title_sort Estratégias para conservação de acessos de coqueiro anão do BAG da Embrapa Tabuleiros Costeiros
author Machado, Caroline de Araújo
author_facet Machado, Caroline de Araújo
author_role author
dc.contributor.author.fl_str_mv Machado, Caroline de Araújo
dc.contributor.advisor1.fl_str_mv Lédo, Ana da Silva
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/1227319106079882
contributor_str_mv Lédo, Ana da Silva
dc.subject.por.fl_str_mv Cocos nucifera L.
Germoplasma
Grãos de pólen
Armazenamento
Embriões zigóticos
topic Cocos nucifera L.
Germoplasma
Grãos de pólen
Armazenamento
Embriões zigóticos
Cocos nucifera L.
Germplasm
Grain pollen
Storage
Zygotic embryos
CNPQ::CIENCIAS AGRARIAS::AGRONOMIA
dc.subject.eng.fl_str_mv Cocos nucifera L.
Germplasm
Grain pollen
Storage
Zygotic embryos
dc.subject.cnpq.fl_str_mv CNPQ::CIENCIAS AGRARIAS::AGRONOMIA
description The conservation of the coconut palm has been investigated in recent years by research organizations, public and private. These studies have concentrated on obtaining conservation protocols in vitro using slow growth and cryopreservation. Storage as a means of maintaining the viability of pollen, it is important for the preservation of genetic variability, facilitates the exchange of germplasm and contributes greatly to the generation of variability obtained from artificial crosses increasing the efficiency of breeding programs. The objective of this work was to study the effect of mannitol and abscisic acid (ABA) on growth of seedlings of coconut dwarf accessions for conservation purposes, and in vivo studies of the viability and storage conditions of pollen grains. For the study of conservation by slow growth were used mature zygotic embryos of Gramame Red Dwarf (AVG) and Malayan Yellow Dwarf (AAM). The coconut embryos were inoculated in culture medium Y3 (Eeuwens, 1976) supplemented with 30 g L-1 sucrose, gelled with 0.7% agar in presence of 2.5 g L-1 of activated charcoal. Were tested the following concentrations of mannitol: 0; 0.1; 0.2, 0.3 and 0.4 M. In other experiment was tested the following ABA concentrations: 0, 10, 20, 30 and 40 mM. The 0.1 and 0.2 M mannitol reduced the plantlets length of AAM and AVG accessions, respectively at 180 and 270 days of cultivation. Concentrations above 20 μM ABA were viable to inhibit the plantlets growth to 180 and 270 days. The ABA concentrations tested not inhibit the access AVG growth. For the study of determining the culture medium in germination of pollen grains, it was evaluated four culture media: Brewbaker and Kwack (1983) modified by Sousa et al. (2010); Lora et al. (2006); Sousa et al. (1998) and Sousa et al. (1998) modified by the author, in different times: 0, 24, 48 and 72 hours. The Lora culture medium promoted the major in vitro germination of AVeJBr pollen grains. Pollen grains of AVeJBr access showed viability up to 72 hours (3 days). The condition of storage at -20°C and -80°C promotes more viable pollen germination of AVC access up to 60 days. The condition of storage at -196°C promotes greater availability of pollen germination by AVeJBr access up to 60 days.
publishDate 2012
dc.date.issued.fl_str_mv 2012-04-23
dc.date.accessioned.fl_str_mv 2017-10-02T12:49:40Z
dc.date.available.fl_str_mv 2017-10-02T12:49:40Z
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dc.publisher.country.fl_str_mv BR
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