4.5 Article

In vitro regeneration using twin scales for restoration of critically endangered aquatic plant Crinum malabaricum Lekhak & Yadav: a promising source of galanthamine

Journal

PLANT CELL TISSUE AND ORGAN CULTURE
Volume 141, Issue 3, Pages 593-604

Publisher

SPRINGER
DOI: 10.1007/s11240-020-01818-1

Keywords

Crinum malabaricum; Critically endangered; Twin scales; In vitro regeneration; Galanthamine

Funding

  1. Science and Engineering Research Board, Department of Science and Technology, Government of India [EMR/2016/007795]

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Key message Crinum malabaricum is a critically endangered aquatic plant species and natural source of galanthamine. It is endemic to India and about 1000 plants only available in a private estate in the Western Ghats of India. In vitro regeneration protocol has been developed utilizing twin scales for conservation of this plant. It is the first report on effective in vitro propagation and bulblets formation in C. malabaricum. This study intended to develop a significant in vitro regeneration protocol for sustainable propagation, conservation and re-establishment of critically endangered aquatic plant species Crinum malabaricum Lekhak & Yadav (Malabar river lily). This plant is the natural source of galanthamine, the drug to treat Alzheimer's disease. We present a scientific understanding, emphasizing the use of twin scales (separated from the large parent bulb) in direct regeneration of new shoots and proliferation of bulblets assisted by nutrients supply. The meristematic region of the bulb plate, present between the scales was activated using cytokinins to produce shoots (maximum 12 shoots per twin scale) on full strength Murashige and Skoog's (MS) medium augmented singularly with 2.0 mg L-1 6-benzylaminopurine (BAP). Upon subculturing of shoots on diverse concentrations of plant growth regulators (BAP and IAA/NAA), BAP alone at 2.0 mg L-1 was served optimum for the better proliferation of shoots (53 shoots). The regenerated shoots were rooted in vitro on half strength MS medium fortified with various types of auxins. Highest number of roots (11.6 within 4 weeks) and bulblets (after 3 months) resulted with 1.0 mg L-1 Indole-3-butyric acid (IBA) under in vitro conditions. The rooted plants were hardened in the greenhouse and finally transferred to the natural stream with 83% survival rate. The SCoT (start codon targeted) and ISSR (inter simple sequence repeats) marker analysis of in vitro raised and mother plants confirmed the genetic stability of tissue cultured plants and the reliability of present protocol for C. malabaricum. It is the foremost report on in vitro regeneration and genetic fidelity analysis for restoration of this critically endangered aquatic plant using twin scale technique. The study could help in ex situ conservation, reintroduction and restoration of C. malabaricum population in its natural habitat.

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