The biological half-life and final residue levels of indoxacarb and pyridalyl were determined in cauliflower over a 10-day cultivation period following applications of a standard (100 g a.i.ha–1 and 200 g a.i.·ha–1, respectively) and double dose (200 g a.i.·ha–1 and 400 g a.i.·ha–1, respectively). The residue levels were analyzed by gas chromatography with recovery ranging from 92.1% to 109.7%. The biological half-lives of indoxacarb and pyridalyl were 6.33 and 7.74 days for the standard dose, and 6.26 and 7.44 days for the double dose, respectively. The initial and persisting concentrations of indoxacarb and pyridalyl were all below the Korean maximum residue limits for broccoli of 1.0 mgkg–1 and 3.0 mgkg–1, respectively.
Cauliflower (Brassica oleracea var. botrytis L.) is an important vegetable crop grown extensively in Asia, Europe, and America. It is low in fat and high in dietary fiber, folate, water, and vitamin C, has a very high nutritional density, and contains glucosinolates (including sulfurophane), which may improve the liver’s ability to detoxify carcinogenic substances. A high intake of cauliflower has been found to reduce the risk of aggressive prostate cancer [
Indoxacarb, methyl (S)-N-[7-chloro-2,3,4a,5-tetrahydro- 4a-methoxycarbonyl)indeno[1,2-e][1,3,4]oxadiazin-2ylcarbonyl]-4’-(trifluoromethoxy)carbanilate (
Pyridalyl, 2,6-dichloro-4-(3,3-dichloroallyloxy)phenyl 3-[5-9trifluoromethyl]-2-pyridyloxy]propyl ether (
As cauliflower is not a popular food item in Korea, good agricultural practice (GAP) standards and maximum residue limit (MRL) values for cauliflower were not available. For this reason, field treatments were carried out according to GAP standards for broccoli. The aim of this study was to determine the biological half-life and residue patterns of two pesticides, indoxacarb and pyridalyl, in cauliflower during cultivation. The final residue levels at harvest were predicted after both pesticides were sprayed two and three times, at 7- and 10-day spray intervals, to determine the exact dose, preharvest interval (PHI), and harvest time that minimized the effects of the residues.
Analytical standard indoxacarb (99.5% pure) and pyridalyl (98.5% pure) were purchased from Dr. Ehrenstorfer
GmbH (Augsburg, Germany). Stock (1000 mg∙L–1) and working standard solutions were prepared in acetone and used as external standards throughout the study. A florisil solid-phase extraction (SPE) cartridge (1000 mg/6mL) was purchased from Phenomenex (Torrance, CA, USA). All solvents were of pesticide residue grade and obtained from Merck (Darmstadt, Germany).
The experimental field was located under a greenhouse in Yesan-eup, Yesan-gun, Chungcheongnam-do, Korea. Field-grown cauliflower was divided into 15 of 10-m2 plots, including three experimental replicates with a randomized complete block design. Treatments were carried out with the following commercial products according to the GAP standard for broccoli in Korea: Ammate WP (10% indoxacarb) at a standard single dose of 100 g a.i.∙ha–1 and a double dose of 200 g a.i.∙ha–1, and Pleo EW (10% pyridalyl) at a standard single dose of 200 g a.i.∙ha–1 and a double dose of 400 g a.i.∙ha–1. Pesticides were applied at 7-day intervals using a rechargeable battery sprayer (KS-PK 2000; Kwang Sung, Daejeon, Korea) with a spray volume of 0.4 L∙m–2. The control plot was maintained at a safe distance. After the final spraying, representative samples (8 - 9 cauliflower heads) were collected at 0 (2 h), 1, 2, 3, 5, 7, 9, and 10 days, and brought to the laboratory in polyethylene bags with minimal finger contact. Samples of chopped cauliflower heads were mixed and quartered and then blended and stored in a freezer at –20˚C until analysis.
Meteorological data were continuously recorded with a DT-172 temperature and humidity datalogger (CEM, Guangdong, China). During the experimental period, the average relative humidity ranged from 53.9% to 84.5%, with maximum and minimum average daily temperatures of 17.3˚C and 5.6˚C, respectively.
A 20-g sample was placed into an Erlenmeyer flask with 100 mL acetone and shaken for 30 min on a mechanical shaker (Vision Scientific Co., Ltd., Daejeon, Korea). The sample was then filtered under vacuum through a Buchner funnel. The container and filter cakes were washed with 30 mL acetone and the rinsate was combined with the previous filtrate. The filtrate was concentrated to about 20 mL using a vacuum rotary evaporator and transferred to a 1-L separatory funnel. After adding 300 mL distilled water and 50 mL saturated sodium chloride solution to the above extract, partitioning was carried out twice with 70-mL portions of n-hexane. The hexane layer was collected over 30 g of anhydrous sodium sulfate and evaporated to dryness on a vacuum rotary evaporator at 40˚C. The dried extract was dissolved in 3 mL n-hexane for cleanup.
The florisil SPE cartridge was preconditioned with 5 mL n-hexane and the sample extract from the partitioning step was then added. To remove impurities, the SPE cartridge was washed with 5 mL n-hexane and eluted with 15 mL acetone/n-hexane (20:80, v/v) for indoxacarb and 30 mL acetone/n-hexane (20:80, v/v) for pyridalyl. The eluate was evaporated to dryness in a vacuum rotary evaporator at 40˚C and the residue was redissolved in 4 mL acetone for gas chromatography with an electron capture detector (ECD).
A gas chromatograph (model 6890; Agilent, Santa Clara, CA, USA) equipped with an ECD and DB-5 column (30 m × 0.25 mm i.d., 0.25 μm film thickness) was used to determine the level of pesticide residue. A 1-μL sample was injected in split mode (28:1) and the injector and detector temperatures were 250˚C and 320˚C, respectively. Oven temperature programming was initialized with a 2 min hold at 190˚C, and then the temperature was increased at 10˚C∙min–1 to 300˚C, where it was finally held for 10 min, giving a total run time of 22 min. Ultrapure nitrogen was used as the carrier gas with a flow rate of 1 mL∙min–1, and the retention times of indoxacarb and pyridalyl were 15.87 and 14.28 min, respectively.
Recovery studies were performed with fortification levels of 0.02 mg∙kg–1 [10 × limit of quantification (LOQ)] and 0.1 mg∙kg–1 (50 × LOQ), obtained from control samples. Three replicates were analyzed at each fortification level. Average recoveries were 92.1% - 109.7%, whereby the coefficient of variation was within 10%, which is generally considered satisfactory for residue quantification. Results of the recovery studies are presented in
The residue results were the means from three replicates of each treatment and all data were analyzed applying simple descriptive statistics such as the mean and standard deviation using Microsoft Excel.
Residues of the pesticides were determined in samples by comparing the area of the concentration peak with that of the external standard method. A six-point calibration curve from 0.01 to 2 mg∙kg–1 was constructed for quantitative analysis. The detector responses of two pesticides were linear throughout the entire range of concentrations, with a correlation coefficient (R2) of 0.999*** shown in
CV, coefficient of variation; LOQ, limit of quantification.
Initial (2 h) deposits of indoxacarb on cauliflower were 0.29 and 0.58 mg∙kg–1 for the recommended and double doses, respectively. Ten days after application, the remaining residues were 0.07 and 0.16 mg∙kg–1, respectively. Hence, 75.86% and 72.41% of the initial residue levels, respectively, had dissipated.
surrounded the head were discarded in this study, while the whole plant of the Chinese cabbage was used by Lee et al. [
The final residue levels were compared when indoxacarb was sprayed two and three times at 100 g a.i.∙ha–1 with a spray interval of 7 and 10 days. Indoxacarb residues according to the level of application are shown in
Initial (2 h) deposits were 0.43 and 0.84 mg∙kg–1 for the recommended and double doses, respectively. Ten days after application, the remaining residues were 0.12 and 0.30 mg∙kg–1; i.e., 72.09% and 64.29% of the initial residue levels had dissipated.
residue levels can only be compared with MRLs set by individual countries’ due to the absence of MRLs set by bodies such as the European Union or Food and Agriculture Organization/World Health Organization. Japan has set a level of 2 mg∙kg–1 as the MRL for broccoli, which is higher than the levels of pyridalyl residues on cauliflower measured in this study. The biological halflives of pyridalyl in cauliflower for the recommended and double doses were 7.74 and 7.44 days, respectively. To the best of our knowledge, no other information regarding pyridalyl residues on cauliflower has been published. However, Svetlana et al. [
The final residue levels were compared after pyridalyl has been applied two and three times at a spray interval of 7 and 10 days; the predicted residues are given in
This study was financially supported by the National Agricultural Products Quality Management Services, Republic of Korea.