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Effective callus induction and plant regeneration in callus and protoplast cultures of Nigella damascena L.

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TLDR
The main objective of this study was to develop in vitro systems utilizing N. damascena seedlings, as an easily accessible explant source, for efficient callus induction and proliferation, and plant regeneration via somatic embryogenesis, and to validate the usefulness of the obtained callus as a source of protoplasts and their capability to develop into plants.
Abstract
In this study we report the development of effective in vitro systems for a medicinal plant Nigella damascena L. comprising: (1) callus induction, (2) somatic embryogenesis in callus cultures with subsequent plant regeneration, and (3) isolation and regeneration of callus-derived protoplasts. Callus development was achieved on 83–100% of hypocotyl and cotyledon explants, whereby Murashige and Skoog medium (MS) supplemented with 3 mg L−1 6-benzylaminopurine and 0.5 mg L−1 α-naphthaleneacetic acid (NAA; BN medium) was more advantageous than MS with kinetin and NAA (KN medium). Histological observations of calli revealed the presence of embryogenic zones from which somatic embryos developed on the hormone-free medium. Plant regeneration was observed on 76–95% of calli. A high capacity to form somatic embryos and regeneration was maintained in long-lasting cultures, i.e. even in 2 year old callus. The obtained callus was also a good source tissue for protoplast isolation. By applying a mixture of cellulase and pectolyase, the acceptable yield of viable protoplasts was achieved, especially from hypocotyl-derived callus maintained on BN medium. Protoplasts embedded in an alginate matrix and cultured in modified Kao and Michayluk media re-constructed their cell wall and re-entered mitotic divisions. About 30% of small cell aggregates formed microcalli, which, after the release from alginate, proliferated continuously on KN and BN media, irrespective of the tissue variant used as the protoplast source. Somatic embryo formation and plant regeneration were successful on hormone-free media. An effective plant regeneration system of N. damascena protoplast cultures has been developed and is being reported for the first time. The main objective of this study was to develop in vitro systems utilizing N. damascena seedlings, as an easily accessible explant source, for efficient callus induction and proliferation, and plant regeneration via somatic embryogenesis. Moreover, we attempted to validate the usefulness of the obtained callus as a source of protoplasts and their capability to develop into plants.

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Journal ArticleDOI

Protoplast Regeneration and Its Use in New Plant Breeding Technologies.

TL;DR: In this article, the use of transient transformation and regeneration of plant protoplasts is discussed in the application of new plant breeding technologies and review pertinent literature on successful protoplast regeneration.
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Efficient in vitro plant regeneration from leaf-derived callus and genetic fidelity assessment of an endemic medicinal plant Ranunculus wallichianus Wight & Arnn by using RAPD and ISSR markers

TL;DR: A protocol for mass multiplication of Ranunuculus wallichianus through indirect organogenesis and evaluates the clonal fidelity of regenerants by using RAPD and ISSR markers is developed and could be effective for the conservation of R. wallichanus.
Journal ArticleDOI

Elicitation Effects on Some Secondary Metabolites and Antioxidant Activity in Callus Cultures of Allium jesdianum Boiss. & Buhse.: Methyl Jasmonate and Putrescine.

TL;DR: The results showed the superiority of MeJ over Pu for increasing the secondary metabolites and antioxidant activity in calluses of Allium jesdianum, compared to the control as mentioned in this paper.
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Medium composition affects the tissue culture-induced variation in triticale regenerants

TL;DR: A relationship between medium composition and the changes observed between triticale donor plants and their regenerants is revealed and may give rise to studies aimed at obtaining regenerants with the desired direction of variation generated by plant tissue culture.
Journal ArticleDOI

Optimization of Isolation and Transformation of Protoplasts from Uncaria rhynchophylla and Its Application to Transient Gene Expression Analysis

TL;DR: In this paper , an optimized protocol for U. rhynchophylla protoplast isolation, purification, and transient gene expression was developed, which was used for subcellular localization of transcription factor UrWRKY37.
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Journal ArticleDOI

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Journal ArticleDOI

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