An improved protocol for plant regeneration from leaf- and hypocotyl-derived protoplasts of carrot

Grzebelus, Ewa; Szklarczyk, Marek; Barański, Rafał

doi:10.1007/s11240-011-0078-5

Cited by 55 publications

(52 citation statements)

References 39 publications

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“…1a), respectively. All steps of protoplast isolation were performed according to a previously described protocol (Grzebelus et al 2012a). Briefly, about 1 g of source tissue was cut in 9 9 1.5 cm glass Petri dish into small pieces in the presence of a 0.5 M mannitol solution (pH = 5.6-5.8), and incubated for 1 h at 26 ± 2°C in the dark to plasmolyze the cells.…”

Section: Protoplast Isolationmentioning

confidence: 99%

“…Therefore, before applying this procedure to plant breeding programs, successful protocols for plant regeneration from protoplasts of both partners should be elaborated. For carrot, well known as a model species for plant tissue culture systems, efficient procedures for protoplast isolation and plant regeneration from different types of source tissue, such as suspension cultures, petioles, leaves, and hypocotyls have been presented (Grambow et al 1972;Dirks et al 1996;Grzebelus et al 2012a). However, to our knowledge, similar studies with regard to wild Daucus species do not exist.…”

Section: Introductionmentioning

confidence: 99%

“…Protoplasts embedded in alginate matrix can be dispensed as beads (Damm and Willmitzer 1988), blocks (Pan et al 2003), or layers with different thickness such as thin alginate layers (TAL, Damm et al 1989) and extra thin alginate films (ETAF, Pati et al 2005), and then cultured in liquid media. Alginate has been successfully used as a gelling agent in protoplast cultures of many species; among others, in Lotus covniculatus and Nicotiana tabacum (Pati et al 2005), Citrus sinensis (Niedz 2006), Helianthus annuus (Rákosy-Tican et al 2007), D. carota (Grzebelus et al 2012a), Beta vulgaris (Grzebelus et al 2012b), and Brassica oleracea (Kiełkowska and Adamus 2012).…”

Section: Introductionmentioning

confidence: 99%

“…Protoplasts were isolated from in vitro grown shoots produced from seeds. In order to obtain aseptic material, donor seeds were disinfected using a three-step procedure, as described by Grzebelus et al (2012a). To make the germination of wild accessions possible, decontaminated seeds were left to swell in sterile water.…”

Section: Introductionmentioning

confidence: 99%

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Plant regeneration from leaf-derived protoplasts within the Daucus genus: effect of different conditions in alginate embedding and phytosulfokine application

Maćkowska

Jarosz

Grzebelus

2014

Plant Cell Tiss Organ Cult

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Protoplasts of four Daucus carota subspecies and three wild Daucus species were isolated from 2-weekold 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.

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Section: Protoplast Isolationmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Plant regeneration from leaf-derived protoplasts within the Daucus genus: effect of different conditions in alginate embedding and phytosulfokine application

Maćkowska

Jarosz

Grzebelus

2014

Plant Cell Tiss Organ Cult

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“…These species are considered to be recalcitrant to DH technologies, although carrot is a model plant for tissue culture and regeneration protocols are available for several species Grzebelus et al 2012). Practical utilization of the DH technique is hindered by the low efficiency of embryogenesis in carrot anther cultures.…”

Section: Introductionmentioning

confidence: 99%

Microspore embryogenesis and production of haploid and doubled haploid plants in carrot (Daucus carota L.)

Zhuang

et al. 2012

Plant Cell Tiss Organ Cult

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Protocols were developed for the generation of haploid and doubled haploid plants from isolated microspores of carrot (Daucus carota L.). Forty-seven carrot accessions, including six inbred lines, 11 cultivars, 20 F 1 s, two BC 1 F 1 s, four F 2 s, one F 3 , and three F 4 s, were screened to evaluate the genotype influence on isolated microspore embryogenesis over 4 years. Twenty-eight accessions responded by producing embryos and/or calli. A cytological analysis showed that two modes of carrot microspore embryogenesis exist: an indirect route via calli (C mode), and a direct route via embryos (E mode). Eleven accessions were in the C mode, and 17 were in both modes. The highest production rates were in 10Y25 (a European Nantes cultivar) with 27 calli and 307 embryos, and 100Q6 (a semi-Nantes F 1 hybrid) with 176 calli and 114 embryos. The time period to produce embryos or calli differed significantly between 2 and 6 months. Cold and heat pretreatment generally had a negative impact on the induction of microspore embryogenesis, but a short pretreatment showed a positive influence on some accessions. Twentyeight lines regenerated plants from the primary individual embryos or calli of three accessions were established to analyze the ploidy level. The percentage of spontaneous diploidization showed very wide differences among the accessions and lines. Differences in leaf color intensity, leaf size, and leaf dissection were found among haploid, doubled haploid, and triploid plants.

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Tissue Culture and Regeneration: A Prerequisite for Alien Gene Transfer

Wędzony

Szechyńska‐Hebda

Żur

et al. 2013

Alien Gene Transfer in Crop Plants, Volume 1

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An improved protocol for plant regeneration from leaf- and hypocotyl-derived protoplasts of carrot

Cited by 55 publications

References 39 publications

Plant regeneration from leaf-derived protoplasts within the Daucus genus: effect of different conditions in alginate embedding and phytosulfokine application

Plant regeneration from leaf-derived protoplasts within the Daucus genus: effect of different conditions in alginate embedding and phytosulfokine application

Microspore embryogenesis and production of haploid and doubled haploid plants in carrot (Daucus carota L.)

Tissue Culture and Regeneration: A Prerequisite for Alien Gene Transfer

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