DIN EN 14123-2008 Foodstuffs - Determination of aflatoxin B and the sum of aflatoxin B B G and G in hazelnuts peanuts pistachios figs and paprika powder - High performance liquid ca.pdf
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1、March 2008DEUTSCHE NORM English price group 13No part of this standard may be reproduced without prior permission ofDIN Deutsches Institut fr Normung e. V., Berlin. Beuth Verlag GmbH, 10772 Berlin, Germany,has the exclusive right of sale for German Standards (DIN-Normen).ICS 67.050!$LV Miis the mola
2、r mass of each aflatoxin, in grams per mol; DIN EN 14123:2008-03 EN 14123:2007 (E) 6 iis the molar absorption coefficient of each aflatoxin in toluene and acetonitrile (4.18), in square metres per mol; b is the optical path length of the cell, in centimetres. Miand iof aflatoxins B1, B2, G1and G2are
3、 given in Table 1. Table 1 Molar mass and molar absorption coefficient of aflatoxins B1, B2, G1and G2(In mixture of toluene and acetonitrile (4.18) Aflatoxin Mig/mol im2/mol B1312 1930 B2314 2040 G1328 1660 G2330 1790 4.21 Mixed aflatoxins stock solution Prepare a mixed aflatoxins stock solution con
4、taining 1000 ng/ml of aflatoxin B1and G1, 200 ng/ml of aflatoxin B2and G2in the toluene and acetonitrile mixture (4.18) by appropriate dilution of aflatoxins (B1, B2, G1and G2) stock solutions (4.20). NOTE A commercial total aflatoxins standard solution which is ready to use in a vial containing 100
5、0 ng/ml of total aflatoxin may be used as an alternative. 4.22 Diluted mixed aflatoxins stock solution Prepare a diluted mixed aflatoxins stock solution containing 100 ng/ml of aflatoxin B1and G1, 20 ng/ml of aflatoxin B2and G2in the toluene and acetonitrile mixture (4.18) by pipetting exactly 1,0 m
6、l of the mixed aflatoxins stock solution (4.21) into a 10 ml calibrated volumetric flask (5.10), fill to the mark with the toluene and acetonitrile mixture (4.18) and mix well. Wrap the flask tightly in aluminium foil and store it at less than 4 C or in a freezer. Before use, do not open the flask u
7、ntil the contents have reached room temperature to avoid incorporation of water by condensation. 4.23 Mixed aflatoxins calibration solutions Use the diluted mixed aflatoxins stock solution containing 100 ng/ml of aflatoxin B1and G1, 20 ng/ml of aflatoxin B2and G2(see 4.22) for pipetting the volumes
8、as given in Table 2 into a set of 10 ml volumetric flasks (5.10). Evaporate the toluene/acetonitrile solution just to dryness under a stream of nitrogen at room temperature. To each flask, add 4 ml of methanol, let aflatoxins dissolve, dilute to 10 ml with water, and shake well. Methanol and water a
9、re subject to volume contraction when mixed, so adjust the volume again to the given volume. DIN EN 14123:2008-03 EN 14123:2007 (E) 7 Table 2 Preparation of mixed aflatoxins calibration solutions Calibration solution Mass concentration of calibration solution ng/ml Taken from diluted stock solution
10、(4.22) l B1B2G1G21 40 0,400 0,080 0,400 0,080 2 120 1,200 0,240 1,200 0,240 3 200 2,000 0,400 2,000 0,400 4 280 2,800 0,560 2,800 0,560 5 360 3,600 0,720 3,600 0,720 4.24 Spiking solution Prepare a spiking solution by pipetting 2 ml of the mixed aflatoxins stock solution (containing 1000 ng/ml of af
11、latoxin B1and G1, 200 ng/ml of aflatoxin B2and G2, see 4.21) into a 10 ml calibrated volumetric flask. Evaporate the toluene/acetonitrile solution just to dryness under a stream of nitrogen at room temperature. Dilute to the mark with methanol and shake well. The concentration of this spiking soluti
12、on is 200 ng/ml of aflatoxin B1and G1, and 40 ng/ml of aflatoxin B2and G2. Wrap the flask tightly in aluminium foil and store it at less than 4 C. Before use, do not open the flask until the contents have reached room temperature to avoid incorporation of water by condensation. 5 Apparatus 5.1 Gener
13、al All glassware coming into contact with aqueous solutions of aflatoxins shall be washed with acid solution before use. Many laboratory washing machines do this as part of the washing program. Otherwise soak such laboratory glassware in sulfuric acid (2 mol/l) for several hours (e.g. 15 h overnight
14、), then rinse well (e.g. three times) with water to remove all traces of acid. Check the absence of acid with pH paper. This treatment is necessary, because the use of non-acid washed glassware may cause losses of aflatoxins. In practice, the treatment is necessary for round bottomed flasks, volumet
15、ric flasks, measuring cylinders, vials or tubes used for calibration solutions and final extracts (particularly autosampler vials), and Pasteur pipettes, if these are used to transfer calibration solutions or extracts. 5.2 Usual laboratory apparatus and, in particular, the following 5.3 Laboratory m
16、ill, or explosion proof high speed blender1) , necessary for the production and extraction of pastes from hazelnuts, peanuts, pistachios and figs, with suitable blender jar 5.4 Adjustable vertical or horizontal shaker, needed for the analysis of paprika powder 5.5 Paper filter, e.g. 24 cm diameter,
17、prefolded 5.6 Conical flask, with screw top or glass stopper 1) Contact your National Standardization Institute for appropriate high speed blenders. DIN EN 14123:2008-03 EN 14123:2007 (E) 8 5.7 Glass microfiber filter paper, retention size 1,6 m or smaller 5.8 Reservoir, 75 ml with luer tip connecto
18、r for immunoaffinity column (IAC) 5.9 Hand pump, 20 ml syringe with luer lock or rubber stopper for IAC 5.10 Volumetric glassware, flasks of e.g. 3 ml, 5 ml, 10 ml and 20 ml, with an accuracy of at least 0,5 % 5.11 HPLC system, consisting of 5.11.1 HPLC pump, suitable for flow rate at 1,0 ml/min 5.1
19、1.2 Injection system, capable for total loop injection. A 100 l loop is recommended. In the case that a different loop size than recommended is used it shall be guaranteed that the limit of detection (LOD) for the system is 0,2 ng/g (signal-to-noise-ratio = 3) and the limit of quantification (LOQ) i
20、s 0,5 ng/g (signal-to-noise-ratio = 6) for each aflatoxin (using the standard solutions). 5.11.3 RP-HPLC column, e.g. C18or ODS-2 (length of 25 cm, inner diameter of 4,6 mm and particle size of 5 m), which ensures a baseline resolution of the aflatoxin B1, B2, G1and G2peaks from all other peaks. The
21、 maximum overlapping of peaks shall be less than 10 %. It could be necessary to adjust the mobile phase for a sufficient baseline resolution. A suitable pre-column should be used. 5.11.4 Post-column derivatisation system, with PBPB (only to be used with mobile phase A (4.15) Consisting of an HPLC pu
22、lseless pump, zero-dead volume T-piece, reaction tubing min. 45 cm x 0,5 mm internal diameter PTFE. 5.11.5 System for derivatisation with electrochemically generated bromine, e.g. KOBRA cell2)(only to be used with mobile phase B (4.16). 5.11.6 Fluorescence detector, with a wavelength of = 360 nm exc
23、itation filter and a wavelength of = 420 nm cut-off emission filter, or equivalent (e.g. a detector with an adjustable monochromator). Recommended settings for adjustable detectors are 365 nm (excitation wavelength), 435 nm (emission wavelength) and a bandwidth of 18 nm. 5.12 Disposable filter unit,
24、 of pore size 0,45 m Prior to usage, verify that no aflatoxin losses occur during filtration (recovery testing). NOTE There is a possibility that various filter materials can retain aflatoxins. 5.13 Pipettes, 2 ml, 5 ml and 10 ml capacity, with an accuracy of at least 0,5 % 5.14 Analytical balance,
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