- Indirect shoot organogenesis from leaf explants of Adhatoda vasica Nees.
Indirect shoot organogenesis from leaf explants of Adhatoda vasica Nees.
A novel protocol for indirect shoot organogenesis of Adhatoda vasica was developed using petiole explants derived from mature shrubby plants. Media with concentrations of cytokinins in combination with auxins were used to induce callus formation in two explants types: petiole and leaf segment. The frequency of callus formation from petiole and leaf segment explants on Murashige and Skoog (MS) basal medium supplemented with 0.25Ā mgĀ l(-1) thidiazuron (TDZ) and 0.25Ā mgĀ l(-1) Ī±-naphthaleneacetic acid (NAA) was 100āĀ±ā0.0 and 83.70āĀ±ā0.52% respectively, while on this medium supplemented with 0.25Ā mgĀ l(-1) 6-(Ī³-Ī³, dimethylallyamino purine) (2iP) and 0.25Ā mgĀ l(-1) NAA, the callus frequency was 100āĀ±ā0.0 and 96.70āĀ±ā0.67% respectively. The highest shoot regeneration (90.60āĀ±ā0.52%) response and the maximum shoots (8.10āĀ±ā0.28) per callus were achieved from petiole explants on MS medium containing 0.25Ā mgĀ l(-1) TDZ and 0.25Ā mgĀ l(-1) NAA. On the contrary, on Schenk & Hildebrandt (SH) basal medium supplemented with 0.25Ā mgĀ l(-1) TDZ and 0.25Ā mgĀ l(-1) NAA, the frequency of callus formation from petiole and leaf segment explants was 100āĀ±ā0.0 and 90.50āĀ±ā0.89% respectively while the callus frequency on this medium containing 0.25Ā mgĀ l(-1) 2iP and 0.25Ā mgĀ l(-1) NAA was 100āĀ±ā0.0 and 89.90āĀ±ā0.72% respectively. The shoot regeneration frequency for petiole explants was 89.90āĀ±ā0.46% producing 6.00āĀ±ā0.21 shoots per callus on SH basal medium supplemented with 0.25Ā mgĀ l(-1) TDZ and 0.25Ā mgĀ l(-1) NAA. Whereas petiole explants could induce 83.70āĀ±ā0.50% shoot regeneration and 7.3āĀ±ā1.05 shoots per callus on SH medium containing 0.25Ā mgĀ l(-1) indole-3-butyric acid (IBA), 0.5Ā mgĀ l(-1) 6-benzyladenine (BA) and 0.5Ā mgĀ l(-1) 2iP. Elongation of regenerated shoot was obtained on MS basal medium supplemented with 0.25Ā mgĀ l(-1) TDZ. All regenerated shoots developed adventitious roots within 4Ā weeks when transferred to rooting medium containing SH medium supplemented with 0.5Ā mgĀ l(-1) IBA. Total nine rooted plantlets were transferred from in vitro to in vivo conditions and eight plants survived and successfully acclimatized in the shaded greenhouse 12Ā weeks after transplanting.