Abstract:
In Sri Lanka, Orchids (orchidaceae) are among prominent flora, which is adapted to a wide
range of eco-climatological zones. However their existence has been endangered due to
various pressures on the environment imposed by man. Orchids with showy flowers
encounter an added disadvantage due to over-collection from the wild. Although, legislative
measures play an important role the most effective measure to conserve orchids is to make
available the species in the required amounts and reintroduce them to their natural
habitats.
Ipsea speciosa, Rhynchostylis retusa, Dendrobium maccarthiae and Vanda spathulata
were identified as endangered species. The suggested approach to preserve these orchids
requires high capacity multiplication techniques to generate the required plants. The
present studies investigate two methods in generating the required plants for the proposed
conservation plan, by tissue culture multiplication techniques such as in-vitro vegetative
propagation and embryo culture.
Experiments were carried out to identify the correct maturity stage for in-vitro seed
germination of ipsea and Rhynchostylis. Results showed that 2 months after pollination
was the best stage for Ipsea and 2-month-old-pods took 20 days to germinate. 100%
germination was observed in basal MS medium with charcoal (2g/l) and PVP (2g/l), V&W
with banana extracts (75g/l) and coconut water (1 OOml/l) and KNC with banana extracts
(75g/l). 6 months after pollination was the correct maturity stage for Rhynchostylis and 6-
month-old-pods took 20 days to germinate. 100% germination was observed in KNC
medium with banana extracts (75g/l), coconut water (1 OOml/l), and V& W with banana
extracts (75g/l), coconut water (1 OOml/l). 100% germination was observed in basal MS,
KNC and V&W with banana extracts and coconut water in Dendrobium and Vanda 70%
germination was successful in V&W medium.
In in- vitro vegetative propagation experiments growing rhizome tips on Ms medium with
charcoal (2g/l) showed the better establishment (60%) for Ipsea and 5mg/l NAA and
0.5mg/l BAP gave the highest proliferation (1:6). Nodal segments of Dendrobium took 4
weeks for bud break on MS medium. Addition of GA3 (0.3mg/l) to the medium did not
accelerate the bud break of Dendrobium.
Key words: Conservation, Embryo rescue, Endangered orchids, Multiplication techniques,
Showy flowered orchids, Tissue culture, and