Íslenskar landbúnaðarrannsóknir - 01.09.1982, Qupperneq 9

Íslenskar landbúnaðarrannsóknir - 01.09.1982, Qupperneq 9
RESIDUE OF LINURON IN SOILS 7 tion into petroleum ether. The extract was again evaporated to dryness and the linuron residue hydrolysed in hydrochloric acid to form 3,4—dichloroaniline. This aniline was then measured by application of an auto- mated diazotization and coupling proce- dure (Friestad 1967, 1974, 1978). Soil analysis The procedure as described by Friestad (1978) was followed closely. A preliminary investigation of the soil extraction proce- dure indicated that a 24 hour delay was necessary after shaking a soil sample in dichloromethane, before removal of an aliquot for analysis. Higher recoveries of linuron were obtained after a delay of 24 hours (mean recovery 78%) or 48 hours (mean recovery 79%) than if the aliquot was taken immediately (mean recovery 59%). On the basis of these findings, each sample was allowed to settle for 24 hours in the dichloromethane extractant. After this interval, an aliquot ofthe clear supernatent was removed for clean-up by dimethyl sulphoxide extraction. All evaporation of solvents was performed in a water bath at 70°C. Some minor changes were made to the Autoanalyser module as presented by Friestad (1974). In particular, it was found to be beneficial to the flow pattern to omit the Brij 35 from the sodium nitrite reagent. The manifold flow diagram is shown in figure 2. In order to assess recovery of linuron from soil the following experiment was done on 4 test soil samples. One mg of linuron, dissolved in 5-10 ml diluted ethanol was pipetted over 100.00 g of each ofthe undried, sieved test soils which were Flow diagram of Autoanalyser module. FUðirit fyrir hina sjálfoirku efnagreiningu á linuron.
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