The identification of numerous genes involved in the mitotic checkpoint and cell proliferation indicates that, with a more detailed time course experiment, this procedure represents a good model for understanding cell prolif eration and control within the constraints of whole ani mal physiology. The utilisation of starvation as a treatment emphasised not only the www.selleckchem.com/products/Gemcitabine-Hydrochloride(Gemzar).html essential processes underlying repair of the epithelia, but also the compet ing whole animal physiological requirements with regard to barrier repair, infection control and energy homeosta sis. Comparison with human disease genes has identified several putative candidates in fish for the maintenance of cytoskeletal structure, which are of potential use in aquaculture and fish husbandry studies.
Methods Fish Juvenile sea bream were maintained at the Centre of Marine Science field station in through flow seawater tanks at 17 21 C, 36% salinity and 12 h light and 12 h dark photoperiod for several weeks prior to the start of the experiments. The maintenance of fish and subsequent experiments complied with the Guide lines of the European Union Council and was covered by a group 1 licence. Behaviour and health of animals was monitored visually each day and no mortality occurred during the experiment. Experimental Design Sea bream were acclima Madrid, Spain and scales were removed by wiping fish with a wet paper towel in order to minimize damage. For sampling fish were anaesthe tised in 2 phenoxyethanol, as described above, weight and length was measured, blood collected and centri fuged and the plasma stored at 20 C.
Fish were sacrificed by sectioning the spinal cord and skin was collected from below the dorsal fin and carefully dissected free of mus cle and snap frozen in liquid nitrogen and stored at 80 tised for one week to the experimental circuit which consisted of 8 through flow seawater tanks, with water maintained at 19 21 C, 36% salinity and a 12 h light and 12 h dark photoperiod. Food was withheld from the fasted experimental groups for 1 week prior to removal of the scales which was consid ered day 0 of the trial. The experiment had 3 treatment groups, ST fasted for duration of experi ment, WS scales removed at time 0, STWS fasted for duration of the experiment with scales removed at time 0 and the control group with no treatment but subjected to the same anaesthesia handling as the treat ments groups.
Duplicate tanks for each treatment were prepared and 8 fish were sampled from one tank 3 days GSK-3 after the scales had been removed and from the second tank 7 days after the scales had been removed. Two tanks contained the control fish and were sampled at the same time as the experimental groups at day 3 and 7. To remove the scales, fish were lightly anaesthe tised in 2 phenoxyethanol, collected from 8 fish experimental group, 3 days after the removal of scales were measured.