Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)

Detalhes bibliográficos
Autor(a) principal: Santos, Suzivany Almeida dos
Data de Publicação: 2017
Tipo de documento: Dissertação
Idioma: por
Título da fonte: Biblioteca Digital de Teses e Dissertações da UEFS
Texto Completo: http://tede2.uefs.br:8080/handle/tede/710
Resumo: The genus Hyptis is composed of about 400 species distributed throughout several countries, the majority being in a native and non-domesticated state. The genus has great importance for the pharmaceutical industry because of the high diversity found in its species. It has excellent pharmacological potential and is of great economic interest. Biological properties like it’s antimicrobial, anti - inflammatory, anesthetic, and insecticidal potential have already been demonstrated. However, in addition to the endemism present in many species, there are few works related to conservation of the genus and more research is needed to elucidate potential methods for its preservation. The objective of this research was the in vitro conservation of the species Hyptis ramosa. In addition to adjusting the protocols of cryopreservation of axillary guides and shoots, we aimed to contribute to the conservation of germplasm of this species. The microplants used came from the germination of seeds in MS1/2 medium. For the in vitro conservation, 10 treatments were evaluated, with different combinations between sucrose, mannitol, and sorbitol. After inoculation, the plants were maintained in a growth room for 240 days and evaluated at 60, 120, 180, and 240 days. Each evaluation quantified the number of shoots, shoot length, root number, and root length. For cryopreservation, the techniques of vitrification for axillary calluses and buds and for encapsulation of axillary shoots were evaluated. The tests were carried out in the Laboratory of Germination (LAGER) and Vegetable Tissue Culture (LCTV) of the Horto Florestal Experimental Unit da Universidade Estadual de Feira de Santana. With the results obtained, we concluded that in vitro conservation of microplants of this species is possible using the combination of 87.64 mM sucrose combined with 87.64 mM mannitol in MS medium (MURASHIGE; SKOOG, 1969). With the methodology used, cryopreservation of calluses and shoots of the species was not possible. Cell death occurred in the first stages of the callus vitrification process and in the cryogenic stage for the shoots.
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spelling Oliveira, Lenaldo Muniz de3431450458100109014502http://lattes.cnpq.br/1834182442036222Santos, Suzivany Almeida dos2018-09-17T22:21:01Z2017-09-29SANTOS, Suzivany Almeida dos. Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE). 2017. 67 f. Dissertação (Mestrado Acadêmico em Recursos Genéticos Vegetais)- Universidade Estadual de Feira de Santana, Feira de Santana, 2017.http://tede2.uefs.br:8080/handle/tede/710The genus Hyptis is composed of about 400 species distributed throughout several countries, the majority being in a native and non-domesticated state. The genus has great importance for the pharmaceutical industry because of the high diversity found in its species. It has excellent pharmacological potential and is of great economic interest. Biological properties like it’s antimicrobial, anti - inflammatory, anesthetic, and insecticidal potential have already been demonstrated. However, in addition to the endemism present in many species, there are few works related to conservation of the genus and more research is needed to elucidate potential methods for its preservation. The objective of this research was the in vitro conservation of the species Hyptis ramosa. In addition to adjusting the protocols of cryopreservation of axillary guides and shoots, we aimed to contribute to the conservation of germplasm of this species. The microplants used came from the germination of seeds in MS1/2 medium. For the in vitro conservation, 10 treatments were evaluated, with different combinations between sucrose, mannitol, and sorbitol. After inoculation, the plants were maintained in a growth room for 240 days and evaluated at 60, 120, 180, and 240 days. Each evaluation quantified the number of shoots, shoot length, root number, and root length. For cryopreservation, the techniques of vitrification for axillary calluses and buds and for encapsulation of axillary shoots were evaluated. The tests were carried out in the Laboratory of Germination (LAGER) and Vegetable Tissue Culture (LCTV) of the Horto Florestal Experimental Unit da Universidade Estadual de Feira de Santana. With the results obtained, we concluded that in vitro conservation of microplants of this species is possible using the combination of 87.64 mM sucrose combined with 87.64 mM mannitol in MS medium (MURASHIGE; SKOOG, 1969). With the methodology used, cryopreservation of calluses and shoots of the species was not possible. Cell death occurred in the first stages of the callus vitrification process and in the cryogenic stage for the shoots.O gênero Hyptis abrange cerca de 400 espécies distribuídas em vários países, sendo a grande maioria ainda encontrada em estado nativo e não domesticado. O gênero apresenta grande importância para a indústria farmacêutica por apresentar uma grande diversidade de espécies com grande potencial farmacológico e de interesse econômico, com diversas atividades biológicas já comprovadas, como antimicrobiana, anti-inflamatória, anestésica e inseticida. Contudo, além do endemismo presente em muitas espécies existem poucos trabalhos relacionados com a sua conservação, havendo a necessidade de mais pesquisas. No presente trabalho objetivou-se a conservação in vitro de plantas de Hyptis ramosa, além de ajustar protocolos para crioconservação de calos e gemas axilares, visando contribuir para a conservação de germoplasma desta espécie. As microplantas utilizadas foram provenientes da germinação de sementes em meio MS1/2. Para conservação in vitro foram avaliados 10 tratamentos, com diferentes combinações entre sacarose, manitol e sorbitol. Após a inoculação as plantas foram mantidas em sala de crescimento por 240 dias, com avaliações aos 60, 120, 180 e 240 dias, quantificando-se o número de brotos, comprimento da parte aérea, número de raiz e comprimento da raiz. Para a crioconservação foram avaliadas as técnicas de vitrificação para calos e gemas axilares e de encapsulamento de gemas axilares. Os ensaios foram realizados nos Laboratórios de Germinação (LAGER) e de Cultura de Tecidos Vegetais (LCTV) da Unidade Experimental Horto Florestal da Universidade Estadual de Feira de Santana. Com os resultados obtidos pôde-se concluir que é possível a conservação in vitro de microplantas dessa espécie, utilizando-se a combinação de 87,64mM de sacarose combinado com 87,64mM de manitol, em meio MS (MURASHIGE; SKOOG, 1969). Com a metodologia utilizada não foi possível a crioconservação de calos e gemas da espécie, havendo a morte celular nas primeiras etapas do processo de vitrificação dos calos e na etapa criogênica para as gemas.Submitted by Ricardo Cedraz Duque Moliterno (ricardo.moliterno@uefs.br) on 2018-09-17T22:21:01Z No. of bitstreams: 1 SUZIVANY-Dissertação final_Pós defesa pronta.pdf: 1092823 bytes, checksum: d04950266649fc7c286bacbc00d0e7ed (MD5)Made available in DSpace on 2018-09-17T22:21:01Z (GMT). No. of bitstreams: 1 SUZIVANY-Dissertação final_Pós defesa pronta.pdf: 1092823 bytes, checksum: d04950266649fc7c286bacbc00d0e7ed (MD5) Previous issue date: 2017-09-29Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPESapplication/pdfporUniversidade Estadual de Feira de SantanaMestrado Acadêmico em Recursos Genéticos VegetaisUEFSBrasilDEPARTAMENTO DE CIÊNCIAS BIOLÓGICASCalogêneseCultivo in vitroEspécies medicinais nativasCallogenesisIn vitro cultureNative medicinal speciesCIENCIAS AGRARIASConservação in vitro DE Hyptis ramosa Pohl ex Benth. 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dc.title.por.fl_str_mv Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
title Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
spellingShingle Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
Santos, Suzivany Almeida dos
Calogênese
Cultivo in vitro
Espécies medicinais nativas
Callogenesis
In vitro culture
Native medicinal species
CIENCIAS AGRARIAS
title_short Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
title_full Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
title_fullStr Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
title_full_unstemmed Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
title_sort Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE)
author Santos, Suzivany Almeida dos
author_facet Santos, Suzivany Almeida dos
author_role author
dc.contributor.advisor1.fl_str_mv Oliveira, Lenaldo Muniz de
dc.contributor.advisor1ID.fl_str_mv 34314504581
dc.contributor.authorID.fl_str_mv 00109014502
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/1834182442036222
dc.contributor.author.fl_str_mv Santos, Suzivany Almeida dos
contributor_str_mv Oliveira, Lenaldo Muniz de
dc.subject.por.fl_str_mv Calogênese
Cultivo in vitro
Espécies medicinais nativas
topic Calogênese
Cultivo in vitro
Espécies medicinais nativas
Callogenesis
In vitro culture
Native medicinal species
CIENCIAS AGRARIAS
dc.subject.eng.fl_str_mv Callogenesis
In vitro culture
Native medicinal species
dc.subject.cnpq.fl_str_mv CIENCIAS AGRARIAS
description The genus Hyptis is composed of about 400 species distributed throughout several countries, the majority being in a native and non-domesticated state. The genus has great importance for the pharmaceutical industry because of the high diversity found in its species. It has excellent pharmacological potential and is of great economic interest. Biological properties like it’s antimicrobial, anti - inflammatory, anesthetic, and insecticidal potential have already been demonstrated. However, in addition to the endemism present in many species, there are few works related to conservation of the genus and more research is needed to elucidate potential methods for its preservation. The objective of this research was the in vitro conservation of the species Hyptis ramosa. In addition to adjusting the protocols of cryopreservation of axillary guides and shoots, we aimed to contribute to the conservation of germplasm of this species. The microplants used came from the germination of seeds in MS1/2 medium. For the in vitro conservation, 10 treatments were evaluated, with different combinations between sucrose, mannitol, and sorbitol. After inoculation, the plants were maintained in a growth room for 240 days and evaluated at 60, 120, 180, and 240 days. Each evaluation quantified the number of shoots, shoot length, root number, and root length. For cryopreservation, the techniques of vitrification for axillary calluses and buds and for encapsulation of axillary shoots were evaluated. The tests were carried out in the Laboratory of Germination (LAGER) and Vegetable Tissue Culture (LCTV) of the Horto Florestal Experimental Unit da Universidade Estadual de Feira de Santana. With the results obtained, we concluded that in vitro conservation of microplants of this species is possible using the combination of 87.64 mM sucrose combined with 87.64 mM mannitol in MS medium (MURASHIGE; SKOOG, 1969). With the methodology used, cryopreservation of calluses and shoots of the species was not possible. Cell death occurred in the first stages of the callus vitrification process and in the cryogenic stage for the shoots.
publishDate 2017
dc.date.issued.fl_str_mv 2017-09-29
dc.date.accessioned.fl_str_mv 2018-09-17T22:21:01Z
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dc.identifier.citation.fl_str_mv SANTOS, Suzivany Almeida dos. Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE). 2017. 67 f. Dissertação (Mestrado Acadêmico em Recursos Genéticos Vegetais)- Universidade Estadual de Feira de Santana, Feira de Santana, 2017.
dc.identifier.uri.fl_str_mv http://tede2.uefs.br:8080/handle/tede/710
identifier_str_mv SANTOS, Suzivany Almeida dos. Conservação in vitro DE Hyptis ramosa Pohl ex Benth. (LAMIACEAE). 2017. 67 f. Dissertação (Mestrado Acadêmico em Recursos Genéticos Vegetais)- Universidade Estadual de Feira de Santana, Feira de Santana, 2017.
url http://tede2.uefs.br:8080/handle/tede/710
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dc.publisher.none.fl_str_mv Universidade Estadual de Feira de Santana
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dc.publisher.country.fl_str_mv Brasil
dc.publisher.department.fl_str_mv DEPARTAMENTO DE CIÊNCIAS BIOLÓGICAS
publisher.none.fl_str_mv Universidade Estadual de Feira de Santana
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