Determination of genetic stability in long-term somatic embryogenic cultures and derived plantlets of cork oak using microsatellite markers

Determination of genetic stability in long-term somatic embryogenic cultures and derived plantlets of cork oak using microsatellite markers

Microsatellites were used to test genetic stability in somatic embryos (SE) of Quercus suber L. The SE were obtained by a simple somatic embryogenesis protocol: leaf explants from two adult plants (QsG0, QsG5) and from two juvenile plants (QsGM1, QsGM2) were inoculated on Murashige and Skoog (MS) me...

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Veröffentlicht in:Tree physiology 2006-09, Vol.26 (9), p.1145-1152
Hauptverfasser: Lopes, T, Pinto, G, Loureiro, J, Costa, A, Santos, C
Format: Artikel
Sprache:eng
Schlagworte:
2,4-D
Alleles
callus
Cell Culture Techniques
Cells, Cultured
clones
culture media
DNA fingerprinting
dose response
explants
forest trees
Genes, Plant
genetic markers
genetic stability
genetic variation
in vitro culture
in vitro regeneration
leaves
methodology
micropropagation
microsatellite repeats
Microsatellite Repeats - genetics
molecular sequence data
Quercus - cytology
Quercus - embryology
Quercus - genetics
Quercus suber
somatic embryogenesis
somatic embryos
Time Factors
zeatin
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container_end_page 1152
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container_title Tree physiology
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creator Lopes, T
Pinto, G
Loureiro, J
Costa, A
Santos, C
description Microsatellites were used to test genetic stability in somatic embryos (SE) of Quercus suber L. The SE were obtained by a simple somatic embryogenesis protocol: leaf explants from two adult plants (QsG0, QsG5) and from two juvenile plants (QsGM1, QsGM2) were inoculated on Murashige and Skoog (MS) medium with 2,4-dichlorophenoxyacetic acid and zeatin. Calluses with primary embryogenic structures were transferred to MSWH (MS medium without growth regulators) and SE proliferated by secondary somatic embryogenesis. High morphological heterogeneity was found among cotyledonary SE. However, converted plants looked morphologically normal with well-developed rooting systems and shoots. The genetic stability of the plant material during the somatic embryogenesis process was evaluated by using six to eight nuclear microsatellites transferred from Q. myrsinifolia Blume, Q. petraea (Matts.) Liebl. and Q. robur L. Five of eight microsatellites distinguished among the genotypes analyzed, and for QsG0, QsGM1 and QsGM2, uniform microsatellite patterns were generally observed within and between SE and the respective donor genotypes. For genotype QsG5, the same pattern was observed in all samples analyzed except one, where the mutation percentage was 2.5%. We conclude that microsatellite markers can be used to assess genetic stability of clonal materials and to determine genetic stability throughout the process of somatic embryogenesis. The simple somatic embryogenesis protocol described has potential for the commercial propagation of Q. suber because it results in a low percentage of mutations.
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source MEDLINE; Oxford University Press Journals All Titles (1996-Current)
subjects 2,4-D
Alleles
callus
Cell Culture Techniques
Cells, Cultured
clones
culture media
DNA fingerprinting
dose response
explants
forest trees
Genes, Plant
genetic markers
genetic stability
genetic variation
in vitro culture
in vitro regeneration
leaves
methodology
micropropagation
microsatellite repeats
Microsatellite Repeats - genetics
molecular sequence data
Quercus - cytology
Quercus - embryology
Quercus - genetics
Quercus suber
somatic embryogenesis
somatic embryos
Time Factors
zeatin
title Determination of genetic stability in long-term somatic embryogenic cultures and derived plantlets of cork oak using microsatellite markers
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