[Analysis of phenmedipham in agricultural products by HPLC].

An analytical method was developed for the determination of phenmedipham (PM) in agricultural products using reversed-phase high-performance liquid chromatography with UV detection. A sample was extracted with acetonitrile, and the acetonitrile layer was separated by salting-out. The acetonitrile phase was isolated and evaporated. The extract was dissolved in diethyl ether-hexane (1 : 1), and then cleaned up on a Florisil column. The column was washed with diethyl ether-hexane (1 : 1), and PM was eluted with acetone-hexane (3 : 7), and the eluate was evaporated. The residue was dissolved in acetone-hexane (2 : 8), and the sample solution was cleaned up on SAX/PSA cartridge. The SAX/PSA cartridge was washed with acetone-hexane (2 : 8), and PM was eluted with acetone-hexane (3 : 7). If required, the eluate of the Florisil column was cleaned up with SAX/PSA and ENVI-Carb/ NH2 cartridges. The SAX/PSA cartridge was washed with acetone-hexane (2 : 8), and connected to be ENVI-Carb/NH2 cartridge. The cartridges were washed with acetone-hexane (3 : 7), and then the SAX/PSA cartridge was removed. PM was eluted with acetonitrile-toluene (3 : 1) from the ENVI-Carb/NH2 cartridge. PM in the eluate was separated isocratically on an ODS column (4.6 mm i.d. x 150 mm, 5 microm) using acetonitrile-water (6 : 4) as a mobile phase (flow-rate 1.0 mL/min, temp. 40 degrees C), with monitoring at 235 nm. The calibration curve was linear from 0.005 microg/mL to 10 microg/mL of PM. The recoveries of PM from eight kinds of agricultural products spiked at levels of 0.1 and 0.02 microg/g were 80.8-98.7%. The determination limit was 0.01 microg/g.

[Performance study of analytical method for ethoxyquin in fruit].

A performance study of an analytical method of ethoxyquin (ET) in apples and pears was conducted. In the proposed method, the sample was homogenized with thiourea and ET was extracted with acetone instead of hexane used in the official analytical method for ET, in order to improve the extraction efficiency. Furthermore, dibutyl hydroxytoluene was added in the test solution to prevent the decomposition of ET. For evaluation of the method. ET spiked into apples and pears at the level of 0.2 microgram/g was determined in replicate in six laboratories. Mean recoveries from apple, pear and Japanese pear were 85.3, 83.0 and 83.9%, respectively. Repeatability relative standard deviation values were 3.8-4.7% and reproducibility relative standard deviation values were 7.8-11.3%. The detection limits were 0.001-0.025 microgram/g in the six laboratories; this value may reflect instrument performance. ET spiked into apples and pears at the level of 0.2 microgram/g was detected by both LC/MS and GC/MS.