Exposure cassete k

Another aliquot of 0.1 mg of TL extract from radioactive samples was also applied to HPTLC plates to determine the esterification of [1-14 C]FA into LC. Lipid classes were separated as mention on 2.5. Developed HPTLC plates were placed for 1 week in closed exposure cassettes (Exposure Cassete-K, BioRad, Madrid, Spain) in contact with a radioactive-sensitive phosphorus screen (Imagen Screen-K, Biorad). The screens were then scanned with the Molecular Imager FX image acquisition system (BioRad), and the bands were quantified in percentage by Quantity One image analysis software (BioRad).

An aliquot of 0.1 mg of hatchlings TL was taken for determine the esterification pattern of [1-14 C]ARA into the different LC. Lipid classes were separated by one-dimensional double-development HPTLC as previously described 2.4. Developed HPTLC plates were placed for 2 weeks in closed exposure cassettes (Exposure Cassete-K, BioRad, Madrid, Spain) in contact with a radioactive-sensitive phosphorus screen (Imagen Screen-K, Biorad, Madrid, Spain). The screens were then scanned with Molecular Imager FX image acquisition system (BioRad, Madrid, Spain), and the bands were quantified using the Quantity One image analysis software (BioRad, Madrid, Spain). Identification of labelled bands was confirmed by radiolabelled standards simultaneously run on the same plate (Rodríguez et al., 2002) . andL-∝-1-palmitoyl-2-[1-14 C