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A specified quantity of water is evaporated, and any remaining moisture is subsequently eliminated in a drying oven. The dry residue is then weighed.

The onset of germination is accompanied by the synthesis of enzymes, which can be made visible using fluorescein dibutyrate (FDB). The reagent fluoresces in the presence of lipases.

In order to make the enzyme activity visible, the kernels are first split in half and coated with the FDB reagent after which they are examined in a suitable measuring device under UV light. An intense yellow fluorescence can be seen in the parts of the kernels where enzyme activity is present.

The sample is combusted in a pure oxygen atmosphere at approx. 1000 °C. The resulting mix of gases comes into contact with a CuO/Pt catalyst and is thereby completely oxidized and subsequently freed of all by-products which could potentially interfere with analysis.

After the nitrogen oxides formed in the combustion process are reduced upon contact with tungsten, all nitrogen compounds in the sample are reduced to elemental nitrogen (N₂). The elemental nitrogen is then detected by means of a thermal conductivity detector (TCD), the signal of which is quantitatively evaluated by a dedicated integrator.

The extract content of malt refers to the compounds from finely ground malt (fine grind), which are brought into solution during a standardized mashing process.

The extract content is determined by the weight ratio sL 20/20 of the wort on the basis of the official sugar tables (Plato tables) at 20 °C. sL 20/20 stands for the weight ratio of a volume of wort at 20 °C to the same volume of water at the same temperature. 

Wort is produced using a laboratory mash method (fine grind) after which the nitrogen content of the wort is determined.