Somatic Embryogenesis and Plant Regeneration in Diploid Banana Cultivars (Musa acuminata cv. Chingan and Musa acuminata cv. njalipoovan) from Kerala
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Abstract
Plant regeneration by somatic embryogenesis was attempted with diploid banana cultivars Musa acuminata cv.
Chingan (AA) and Musa acuminata cv. Njalipoovan (AB). In vitro plants grown on solid MS medium supplemented
with BA (4.4-17.6 μM) and TDZ (0.45-9 μM) were used as explant source. The basal meristem including 3-4
leaf primordial and excised apices were inoculated on MS medium supplemented with 2,4-D (0.225-9 μM) and
BA (0.044-8.8 μM) for callus induction. Pale yellow embryogenic callus initiated after three weeks of inoculation
and subsequent subculture were done in the same medium to enhance callus proliferation. Maximum callus
proliferation was observed in 2,4-D (4.5 μM) along with BA (2.2 μM). Embryogenic calli were isolated and transferred
to 100 ml erlenmeyer flask with 20 ml of liquid MS medium with zeatin (0.46-4.56 μM) and malt extract
(100 mg/l) or malt extract and ascorbic acid (0.01-0.5 mg/l). The culture medium was refreshed every third week,
embryogenic complexes and compact structures were removed. Small embryo-like structures and embryogenic calli
were transferred to fresh medium. After 4-5 subculture the embryos were isolated and inoculated on petridish
containing MS basal medium. Leaf and root initials were developed after 2-3 weeks. These were then transferred
to same medium in culture bottles. After 3 weeks, plants of 4-5 cm height were transferred to vermiculate with
100 per cent survival rate.