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Abstract

Protoplasts of four Daucus carota subspecies and three wild Daucus species were isolated from 2-week-old shoot cultures during overnight incubation in an enzyme mixture composed of 1 % (w/v) cellulase Onozuka R-10 and 0.1 % (w/v) pectolyase Y-23. Before the culture, they were embedded in autoclave- or filter-sterilized alginate solution. Modified thin alginate layer (TAL) and extra thin alginate film (ETAF) techniques were applied for protoplast immobilization. A rich mineral-organic medium based on the formulation of Kao and Michayluk supplemented with 0.1 mg l−1 2,4-dichlorophenoxyacetic acid, 0.2 mg l−1 zeatin, and optionally 100 nM phytosulfokine (PSK), a peptidyl plant growth factor, was used for protoplast culture. Plating efficiency was genotype-dependent and in 40-day-old cultures, it varied from 10 % for Daucus pusillus to 73 % for D. carota subsp. sativus. A considerably higher ability in colony formation was observed in the modified TAL culture system using filter-sterilized alginate and in the presence of PSK in the protoplast culture medium. Plant regeneration through somatic embryogenesis stimulated by PSK application occurred for five out of the seven Daucus accessions used in the present study. We believe our data may facilitate the use of wild Daucus in somatic hybridization with cultivated carrot.

Details

Title
Plant regeneration from leaf-derived protoplasts within the Daucus genus: effect of different conditions in alginate embedding and phytosulfokine application
Author
Maćkowska, Katarzyna 1 ; Jarosz, Agata 1 ; Grzebelus, Ewa 1 

 Institute of Plant Biology and Biotechnology, Faculty of Horticulture, University of Agriculture in Krakow, Kraków, Poland 
Pages
241-252
Publication year
2014
Publication date
May 2014
Publisher
Springer Nature B.V.
ISSN
01676857
e-ISSN
15735044
Source type
Scholarly Journal
Language of publication
English
ProQuest document ID
2293083382
Copyright
Plant Cell, Tissue and Organ Culture (PCTOC) is a copyright of Springer, (2014). All Rights Reserved.