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DETERMINATION OF CAROTENOIDS


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2.6. DETERMINATION OF CAROTENOIDS



  1. 2.6.1. Extraction




  1. The lipophilic fraction was extracted according to the procedure described by




  1. Rodríguez-Roque and others (2013) with slight modifications.




  1. First, 1 g of lyophilized non-digested or digested samples was mixed with 0.01 g of




  1. magnesium hydroxide carbonate, 0.01 g of butylhydroxytolune (BHT) and 15 mL of




  1. ethanol:hexane (4:3 v/v) in an Ultraturrax (T-25 Basic, IKA®-Werke GmbH & Co.,




  1. Staufen, Germany) for 2 min in an ice-bath. Then, the mixture was filtered once under




  1. reduced pressure using a Whatman no.1 filter paper. The residue was re-extracted with a




  1. second volume of 10 mL of ethanol:hexane (4:3 v/v) and again filtered. The pellet was




  1. washed twice with 5 mL of ethanol and once with 5 mL of hexane, until the residue was




  1. colourless. All the extracts were combined and washed twice with 10 mL of sodium




  1. chloride (100 g L-1) and thrice with 10 mL of distilled water to remove unwanted water-




  1. soluble substances. The aqueous layer was discarded and the organic phase was




  1. collected. All the procedures were carried out under dim lighting using amber glassware




  1. in order to prevent carotenoid oxidation and isomerization.


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