Cells were maintained in a tissue culture flask and kept in a humidified incubator (5% CO2 in air at 37 °C)
with a medium change every 2–3 days. When the cells reached 70–80% confluence, they were harvested with trypsin – EDTA (ethylene diamine tetra acetate) and seeded into a new tissue culture flask. W. fruticosa flowers were collected from natural habitat during November–January. Plant material was identified by Dr. V.T Antony and a voucher specimen (Acc. No. 7566) was deposited at the herbarium of the Department of Botany, S.B College, Changanassery, Kottayam, Kerala. Flowers were shade-dried, powdered and 50 g of dried powder was soxhlet extracted with 400 mL of methanol for 48 h. The extract was concentrated under reduced pressure using a Selleckchem CX5461 rotary evaporator and was kept under refrigeration. The yield of methanolic extract of Woodfordia fruticosa (MEWF) was 12.5% (w/w). The concentrate was suspended
in 5% Tween 80 for in vivo study and in DMSO for in vitro antiproliferative study. For in vitro antiproliferative study, MEWF was dissolved R428 in DMSO at a concentration of 25 mg/ml. The test solution was prepared freshly on the day of use, diluted to two different concentrations of MEWF (100 μg/ml, 50 μg/ml) and 5-flourouracil, the standard control (50 μg/ml) with DMEM medium containing 10% (v/v) FBS and 1x antibiotic-antimycotics. Male Wistar rats weighing 160–180 g were used for this study. The animals were housed in polypropylene cages and had free access to standard pellet diet (Sai Durga Feeds, Bangalore, India) and drinking water. The animals were maintained at a controlled condition of temperature of 26–28 °C with a 12 h light: 12 h dark cycle. Animal studies were followed according to Institute Animal Ethics Committee regulations approved by the Committee for the Purpose of Control and Supervision of Experiments on Animals (CPCSEA Reg. No. B 2442009/4) and conducted humanely. HCC was induced by oral administration from of 0.02% NDEA (2 ml, 5 days/week for 20 weeks).3 Silymarin at an oral dose of 100 mg/kg body weight was used as standard control.8
Two different doses of MEWF (100 mg/kg and 200 mg/kg) were also prepared for oral administration to the animals. The lethal dose of W. fruticosa was found to be more than 2000 mg/kg p.o. 7 Thirty six rats were divided into six groups, Group I – Normal control Daily doses of Silymarin and MEWF treatments were started in group III–V animals 1 week before the onset of NDEA administration and continued up to 20 weeks. Group VI served as drug control received MEWF alone for the entire period. The rats were sacrificed 48 h after the last dose of NDEA administration. Rat livers were blotted dry and examined on the surface for visible macroscopic liver lesions (neoplastic nodules). The grayish white lesions were easily recognized and distinguished from the surrounding non- nodular reddish brown liver parenchyma. The nodules were spherical in shape.