Regeneration in Jatropha curcas: Factors affecting the efficiency of in vitro regeneration
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作者:
Sharma, Sweta
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Cent Salt & Marine Chem Res Inst CSIR, Discipline Wasteland Res, Bhavnagar 364002, Gujarat, IndiaKing Abdullah Univ Sci & Technol, Plant Stress Genom Res Ctr, Thuwal 239556900, Saudi Arabia
Sharma, Sweta
[2
]
Kumar, Nitish
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Cent Salt & Marine Chem Res Inst CSIR, Discipline Wasteland Res, Bhavnagar 364002, Gujarat, IndiaKing Abdullah Univ Sci & Technol, Plant Stress Genom Res Ctr, Thuwal 239556900, Saudi Arabia
Kumar, Nitish
[2
]
Reddy, Muppala P.
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King Abdullah Univ Sci & Technol, Plant Stress Genom Res Ctr, Thuwal 239556900, Saudi Arabia
Cent Salt & Marine Chem Res Inst CSIR, Discipline Wasteland Res, Bhavnagar 364002, Gujarat, IndiaKing Abdullah Univ Sci & Technol, Plant Stress Genom Res Ctr, Thuwal 239556900, Saudi Arabia
Reddy, Muppala P.
[1
,2
]
机构:
[1] King Abdullah Univ Sci & Technol, Plant Stress Genom Res Ctr, Thuwal 239556900, Saudi Arabia
[2] Cent Salt & Marine Chem Res Inst CSIR, Discipline Wasteland Res, Bhavnagar 364002, Gujarat, India
Factors influencing in vitro regeneration through direct shoot bud induction from hypocotyl explants of Jatropha curcas were studied in the present investigation. Regeneration in J. curcas was found to be genotype dependent and out of four toxic and one non-toxic genotype studied, non-toxic was least responsive. The best results irrespective of genotype were obtained on the medium containing 0.5 mg L-1 TDZ (Thidiazuron) and in vitro hypocotyl explants were observed to have higher regeneration efficiency as compared to ex vitro explain in both toxic and non-toxic genotypes. Adventitious shoot buds could be induced from the distal end of explants in all the genotypes. The number of shoot buds formed and not the number of explants responding to TDZ treatment were significantly affected by the position of the explant on the seedling axis. Explants from younger seedlings (<= 15 days) were still juvenile and formed callus easily, whereas the regeneration response declined with increase in age of seedlings after 30 days. Transient reduction of Ca2+ concentrations to 0.22 g L-1 in the germination medium increased the number of responding explants. Induced shoot buds, upon transfer to MS medium containing 2 mg L-1 Kn (Kinetin) and 1 mg L-1 BAP (6-benzylamino purine) elongated. These elongated shoots were further proliferated on MS medium supplemented with 1.5 mg L-1 IAA (indole-3-acetic acid) and 0.5 mg L-1 BAP and 3.01-3.91 cm elongation was achieved after 6 weeks. No genotype specific variance in shoot elongation was observed among the toxic genotypes except the CSMCRI-JC2, which showed reduced response. And for proliferation among the toxic genotypes, CSMCRI-JC4 showed highest number of shoots formed. Among the rest, no significant differences were observed. The elongated shoot could be rooted by pulse treatment on half-strength MS medium supplemented with 2% sucrose, 3 mg L-1 IBA (indole-3-butyric acid), 1 mg L-1 IAA, 1 mg L-1 NAA (alpha-naphthalene acetic acid) and subsequent transfer on 0.25 mg L-1 activated charcoal medium. The rooted plants could be established in soil with more than 90% success. No significant differences were observed in rooting of shoots in the different toxic genotypes. However, rooting response was reduced in non-toxic genotype as compared to toxic genotypes. (C) 2011 Elsevier B.V. All rights reserved.
VELASQUEZ, T. O. M. A. S. D. A. R. I. O. M. A. R. I. N.
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Univ Oriente, Dept Petr Engn, Av Univ, Maturin 6201, Monagas, VenezuelaUniv Oriente, Dept Petr Engn, Av Univ, Maturin 6201, Monagas, Venezuela
VELASQUEZ, T. O. M. A. S. D. A. R. I. O. M. A. R. I. N.
TOCUYO, D. A. N. Y. D. A. Y. J. O. S. E. F. I. N. A. A. R. R. I. O. J. A. S.
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Petr Venezuela, Data Anal Management, Punta de Mata 6217, Monagas, VenezuelaUniv Oriente, Dept Petr Engn, Av Univ, Maturin 6201, Monagas, Venezuela
TOCUYO, D. A. N. Y. D. A. Y. J. O. S. E. F. I. N. A. A. R. R. I. O. J. A. S.
机构:
Department of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, GhanaDepartment of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, Ghana
Danso, K.E.
Afful, N.T.
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Department of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, GhanaDepartment of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, Ghana
Afful, N.T.
Annor, C.
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Department of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, GhanaDepartment of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, Ghana
Annor, C.
Amoatey, H.M.
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Department of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, GhanaDepartment of Plant and Soil Sciences, Biotech and Nuclear Agriculture Research Institute, Ghana Atomic Energy Commission Legon, P.O. Box 80, Accra, Ghana