This method describes the determination of color of (Congress) wort using color discs.
Malt intended for use in beer brewing or elsewhere in the food industry
The determination of the color of the Congress wort is carried out under defined lighting conditions through a visual comparison of the wort color with the appropriate color discs. Please note that several individuals should perform the color measurement if possible.
The method describes how to determine the free amino nitrogen in the Congress wort by means of a color reaction using ninhydrin with amino acids.
Applicable for all (laboratory) worts
Low molecular weight nitrogenous substances, especially amino acids in the wort, have an influence on the course of fermentation and the formation of fermentation by-products. For a beer’s aroma profile, the concentration and composition of the amino acids are therefore of considerable significance due to their reactivity with reducing sugars (Maillard reaction), especially during kilning in the malthouse and during mashing and boiling in the brewhouse. The products from these reactions influence the redox potential, the color and the aroma of a beer.
Aside from the quantitative determination of the individual amino acids (methods using an ion exchanger, HPLC, GC), cumulative methods of determination are customary. However, these methods also measure NH4+ ions and amines to some degree.
With methods involving color reactions, the amino acids display color at different levels of intensity. Therefore, the reaction is based upon a “standard amino acid”; glycine usually serves as the standard amino acid for comparison.
With the ninhydrin method, the color yield varies with the individual amino acids between 70 and 105 %, based on glycine. Up to approx. 30 % of ammonium salts are quantified using this method and up to approx. 7 % of proline.
The ninhydrin reaction is the most well-known of the color reactions employed for use with amino acids. Ninhydrin is an oxidant and brings about the oxidative decarboxylation of amino acids, producing CO2, NH3 and the formation of an aldehyde. The aldehyde produced in this reaction possesses one less carbon atom than the original amino acid that served as the reactant. Reduced ninhydrin then reacts with non-reduced ninhydrin and the NH3 that was liberated to generate a blue pigment (all amino acids except for proline) or in the case of proline, a yellow pigment. Fructose also takes part in the color reaction as a reducing compound. Potassium iodide present in the solution used for dilution preserves the ninhydrin in an oxidized state and thus inhibits undesirable secondary reactions. The solution to be analyzed is heated together with ninhydrin at a pH of 6.7 and the resulting color is measured at 570 nm.
This method quantifies the amino acids, ammonia and also the terminal α-amino groups of the peptides and proteins. Proline is also measured in part at the wavelength employed in this method.
The method is non-specific for α-amino nitrogen, because γ-amino butyric acid found in wort also generates a color reaction in the presence of ninhydrin.
This method describes the spectrophotometric determination of the color of roasted malt beer/extract.
Roasted malt beer/extract intended for use in beer brewing or elsewhere in the food industry.
This method describes the visual determination of the color of roasted malt beer/extract.
Roasted malt beer/extract intended for use in beer brewing or elsewhere in the food industry.
The method describes the determination of the color of wort and beer by means of color discs.
Suitable for all beer worts and beers.
The colour is determined under defined lighting conditions by an optical colour comparison, whereby two halves of vision must be adjusted to the same colour intensity [1, 2].
Barley intended for the production of malt is to be evaluated on the basis of the characteristics described below.
visual assessment