2009
DOI: 10.21273/hortsci.44.5.1400
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Optimizing Initiation and Maintenance of Vitis Embryogenic Cultures

Abstract: Stamens and pistils from mature grapevines and leaves from in vitro micropropagation cultures were used to optimize parameters influencing somatic embryogenesis in Vitis. Embryogenic competence was dependent on species/variety, explant type and developmental stage, medium composition, and growth regulator concentration. Of varieties evaluated, a greater number produced embryogenic cultures from stamens and pistils (26) compared with leaves (six). Among the different stamen an… Show more

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Cited by 43 publications
(35 citation statements)
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“…The highest embryogenic response was observed from 'Supreme' leaves (12.3%) and 'Delicious' petioles (12.2%) and unopened leaves (11%). Such variations in embryogenic response from leaves were previously reported with Vitis vinifera varieties (Dhekney et al 2009a). Robacker (1993) obtained embryogenic cultures from petioles of two of the five varieties tested, but the size of explants from which petioles were obtained was much greater than some of the explant types used in this study.…”
Section: Induction Of Embryogenic Culturessupporting
confidence: 80%
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“…The highest embryogenic response was observed from 'Supreme' leaves (12.3%) and 'Delicious' petioles (12.2%) and unopened leaves (11%). Such variations in embryogenic response from leaves were previously reported with Vitis vinifera varieties (Dhekney et al 2009a). Robacker (1993) obtained embryogenic cultures from petioles of two of the five varieties tested, but the size of explants from which petioles were obtained was much greater than some of the explant types used in this study.…”
Section: Induction Of Embryogenic Culturessupporting
confidence: 80%
“…Proliferating embryogenic material from solid or liquid medium were transferred to X6 medium for development of somatic embryos (SE). X6 medium consisted of a modified MS medium lacking glycine and supplemented with 3.033 g l -1 KNO 3 and 0.364 g l -1 NH 4 Cl (as the sole nitrogen source), 60.0 g l -1 sucrose, 1.0 g l -1 myo-inositol, 7.0 g l -1 TC agar (Phytotechnology laboratories, LLC, Shawnee Mission, KS, USA), 0.5 g l -1 activated charcoal and a pH value adjusted to 5.8 prior to autoclaving (Dhekney et al 2009a). After the first transfer, 0.2 g of embryogenic culture from each variety was transferred to fresh X6 medium.…”
Section: Maintenance Of Embryogenic Culturesmentioning
confidence: 99%
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“…The development of fungal disease-resistant transgenic grapevines that would greatly reduce or eliminate the need for fungicide sprays was envisioned at a time when genetic transformation and regeneration of this recalcitrant woody species was deemed difficult (Walker 1996). Recent advances in grapevine genetic engineering now make it possible to insert an array of genes for Vitis crop improvement (Dhekney et al , 2009a(Dhekney et al , b, 2010Li et al 2006Li et al , 2008.…”
Section: Introductionmentioning
confidence: 99%