Field Dissipation

Field experiments were conducted in 2022 and 2023 at the East Tennessee Research and Education Center in Knoxville (35.53°N, 83.57°W). The soil type was a Sequatchie loam with sand, silt, and clay of 36%, 40%, and 24%, respectively; pH 6.3; and 1.9% organic matter. Cation-exchange capacity (CEC) of the soil was 7.1 meq 100 g⁻¹ (Midwest Labs, Omaha, NE, USA). Glufosinate-tolerant corn was planted into conventionally tilled plots at 76-cm row spacing, and each plot contained four rows of corn at 9 m length in both years. Plots were maintained free of weeds by post application of glufosinate. Three field experiments were conducted. In 2022, the field study included three treatments of amicarbazone, atrazine, and metribuzin applied individually. Two field studies were conducted in 2023, including the same three treatments as in 2022, with an additional treatment of amicarbazone and metribuzin applied to the same plot. The field corn was planted and the herbicides were applied on June 1, 2022, and May 4 and 19, 2023. Application rate was 494, 700, and 280 g ha⁻¹ for amicarbazone, atrazine, and metribuzin, respectively.

The herbicide applications were made during calm weather conditions (wind speed < 2 km hr⁻¹) to avoid off-target movement to adjacent plots. Herbicides were applied to the designated area within the plot using two passes with a handheld CO₂ pressurized backpack sprayer calibrated to spray 187 L ha⁻¹ at 276 kPa using AIXR 8002 nozzles (TeeJet^® Technologies, Wheaton, IL, USA). The sprayer boom had six nozzles spaced 50 cm apart. Sprayer nozzles were approximately 0.75 m above and vertically oriented to the soil surface to ensure proper overlap of the spray pattern. To further facilitate uniform application, herbicides were mixed at one-half the final rate and broadcast on each plot twice, spraying in opposite directions. The application technique of two applications per plot encouraged uniform distribution of test material and continuity of spray solution by thorough agitation of each mix. This technique directly addresses day 0 sampling error, a major challenge posed by herbicide dissipation field research. Day 0 sampling errors, where the total variation in observed herbicide concentration can be 2 to 5 times as great as other sampling times, are a common occurrence on these types of studies (Blumhorst and Mueller Reference Blumhorst and Mueller1997).

Field Sample Collection and Analysis

Field soil sample collection intervals were approximately 0, 3, 7, 14, 21, 28, 42, 84, and 150 DAT. Soil samples were collected using a golf cup cutter (Par Aide Products, St. Paul, MN, USA) and were 8 cm in depth and 10 cm in width, resulting in a soil sample of ∼800 cm³ (Mueller and Senseman Reference Mueller and Senseman2015). Samples were placed in freezer storage within 30 min of collection to minimize dissipation processes, and the samples remained frozen at −20 C until analysis. Soil sampling depth in these studies was limited to surface sampling, so there was the possibility that some herbicides could have leached below the sampling zone during the studies.

For extraction, collected samples were removed from the freezer and allowed to reach room temperature. Samples were thoroughly homogenized by mixing multiple times while still inside the plastic bag, and a portion (∼15 g) was weighed into a 50-ml conical centrifuge tube (Nunc™, Thermo Fisher Scientific, Waltham, MA, USA) for extraction. Methanol (30 ml) was added to the conical tube, placed on a shaker (∼1 h) (Harrison et al. Reference Harrison, Bull and Michaelides2013), filtered using 0.45-µl polytetrafluoroethylene (PTFE) filters, and analyzed via liquid chromatography–mass spectrometry (LC-MS) (6470 Triple Quadrupole, Agilent, Santa Clara, CA, USA). LC-MS peaks were converted to a concentration scale of nanograms of herbicide per gram of soil.

Herbicide concentrations were regressed as nanograms of herbicide per gram of soil against DAT using the first-order kinetics exponential decay model by SigmaPlot (version 14.0, Grafiti, Palo Alto, CA, USA). The herbicide concentration data were empirically fit to the equation

([1]) $$k = a \cdot {e^{( - b \cdot x)}}$$

where a is the y-intercept and represents the hypothetical initial herbicide concentration and b represents the first-order rate constant (k) empirically fitting the data of herbicide decline over time. This regression model is frequently used to describe herbicide dissipation in soils and is a major parameter input for use in computer simulation models used by the U.S. Environmental Protection Agency (2008). This two-parameter, single–exponential decay model fit most of the data curves relatively well, with some exceptions (most r ² > 0.90). Herbicide half-lives in days were calculated by the relationship

([2]) $${\rm{Half \hbox- life}}=0.693/k$$

Statistical evaluation of rate constants (and thus half-life values) was accomplished by comparing each rate constant (k) ± its standard error, with a nonoverlapping interval indicating a difference in herbicide half-life values for those two examined regression lines.

Lab Degradation

Lab studies were conducted using previously described methods (Mueller et al. Reference Mueller, Parker, Steckel, Clay, Owen, Curran, Currie, Scott, Sprague, Stephenson, Miller, Prostko, Grichar, Martin, Kruz, Bradley, Bernards, Dotray, Knezevic, Davis and Klein2017). Laboratory studies examined the three herbicides in four different soil scenarios. The soil scenarios were a 2 × 2 factorial of location (Illinois or Tennessee) and previous atrazine history being confirmed (yes or no) (Mueller et al. Reference Mueller, Parker, Steckel, Clay, Owen, Curran, Currie, Scott, Sprague, Stephenson, Miller, Prostko, Grichar, Martin, Kruz, Bradley, Bernards, Dotray, Knezevic, Davis and Klein2017). Soils were collected from the field location previously described in Tennessee (35.53°N, 83.57°W) and also from Washington County, IL, near 38.36°N, 89.71°W. Surface soils (0 to 10 cm) were from areas with documented histories of being atrazine-free for at least 20 yr and from a nearby field with documented, continuous atrazine use for 10 yr or longer. Soils from Illinois were a silt loam with pH 6.6, CEC 21 meq 100 g⁻¹, and OM content of 3.2%. Soils used in the lab research were stored at ambient temperature, and containers were opened periodically to ensure that the aerobic processes of the soil microorganisms were not inhibited. Soils were analyzed using the described lab methods and analysis to ensure no detectable residues of herbicides before lab study initiation (data not shown).

Fortifying stock solutions (all ∼140 mg ml⁻¹) were prepared for each herbicide from a separate analytical standard for amicarbazone, atrazine, and metribuzin (all > 98% purity) (ChemService, West Chester, PA, USA). Stock solutions were made by dissolving analytical herbicide in water by stirring overnight (∼14 h) and using gentle heat (<45 C) when needed. Stock solutions were filtered to remove any undissolved particles that would increase precision in the fortifying solutions. Organic solvents have been reported to allow higher concentrations of herbicides to be dissolved (Shaner Reference Shaner2014), but these were not used in these experiments to avoid negative impacts on the soil microbial communities. Final solutions were prepared by diluting the stock solution with water to the desired concentrations. Each herbicide + soil combination was examined in 20 individual vials.

Dry soils were sieved using a 2.0-mm sieve (Gilson, Lewis Center, OH, USA) to remove rocks and large debris; soils were then saturated to field capacity and allowed to drain overnight. Soil (∼5 g soil of each individual soil) was added to a 20-ml vial (Wheaton, Millville, NJ, USA). Each vial was then fortified with a single analytical herbicide dissolved in 500 µl water. The combined herbicide treatments (mixed) were fortified using 250 µl of each herbicide. Similar soil moisture was maintained inside each vial by not allowing evaporation, as soil moisture differences can affect herbicide dissipation (Beestman and Deming Reference Beestman and Deming1974; Savage Reference Savage1978; Taylor-Lovell et al. Reference Taylor-Lovell, Sims and Wax2002). Duplicate vials of each treatment in each soil were removed from the incubator at −1 (prior to fortification), 0, 4, 7, 14, 21, 28, 42, 63, and 84 DAT and placed into storage at −20 C until extraction. The extraction of lab samples was similar to field-collected samples. Methanol (12 ml) was added to vials, placed on a shaker (∼1 h), filtered using 0.45-µl PTFE filters, and analyzed via LC-MS. LC-MS methods were the same as the field trials.

Analytical Methods

A previously published method for amicarbazone utilized LC for herbicide quantification (Chermenskaya and Alekseev Reference Chermenskaya and Alekseev2021). Lab analysis in this research used an Agilent 1260 liquid chromatograph coupled with an Agilent 6470 mass spectrometer. All separations used a gradient of water + 0.1% formic acid and acetonitrile + 0.1% formic acid (all reagents MS-MS grade). The gradient used was similar for each herbicide, including initial conditions of 50% to 80% aqueous phase, changing to ∼90% organic phase in 3 to 4 min. Retention time for amicarbazone, metribuzin, and atrazine was 1.3, 3.9, and 7.2 min, respectively. Extraction efficiencies were >82% for all herbicides and soils (data not shown). The lower limit of quantitation for amicarbazone, atrazine, and metribuzin was 5 ng g⁻¹ soil. Analysis blanks and quality assurance samples were distributed throughout each batch of soil sample analyses.