Plant Material

The glyphosate-resistant (BR-R) Palmer amaranth population was collected from a field site in Ipiranga do Norte, Mato Grosso, Brazil. The glyphosate-susceptible (GA-S) Palmer amaranth population was originally collected in 2004 from the University of Georgia Ponder Farm Research Station (Culpepper et al. Reference Culpepper, Grey, Vencill, Kichler, Webster, Brown, York, Davis and Hanna2006). A known tall waterhemp population from Nebraska was used for species identification (Bernards et al. Reference Bernards, Crespo, Kruger, Gaussoin and Tranel2012).

Species-Diagnostic Marker

Tall waterhemp is another dioecious species in the Amaranthus genus but is not known to be present in Brazil. Additionally, a single-nucleotide polymorphism in the ALS gene has been used to genetically identify tall waterhemp and Palmer amaranth (Tranel et al. Reference Tranel, Wassom, Jeschke and Rayburn2002). To determine whether the dioecious Amaranthus individuals collected in Brazil were Palmer amaranth or tall waterhemp, a genotyping protocol was developed using the ALS polymorphism. Approximately 50 mg of young leaf tissue from three untreated GA-S individuals, six untreated BR-R individuals, and three known tall waterhemp individuals were used for DNA extraction using a modified cetyltrimethylammonium bromide (CTAB) extraction protocol (Doyle Reference Doyle1991). Samples were placed in tubes, a metal bead was added, and then the tubes were frozen in liquid nitrogen. The samples were ground using a Qiagen TissueLyser II (Qiagen, Valencia, CA) for 1 min at 30 oscillations s⁻¹. The ground tissue was incubated with 500 µl of 2×CTAB buffer with 4 µl of 2-mercaptoethanol at 50 C for 15 min. The suspension was then incubated for 15 min with 500 µl of 24:1 chloroform:isoamyl alcohol with gentle agitation and then centrifuged for 15 min at 15,000× g. The aqueous phase was removed and reseparated using another 500 µl of 24:1 chloroform:isoamyl alcohol and was centrifuged for 5 min at 15,000× g. The aqueous phase was once again removed and then precipitated with 50 µl sodium acetate (3M, pH 5.2) and 1,650 µl of 100% ethanol. After 15 min at room temperature, samples were centrifuged for 15,000 × g for 15 min. All liquid was removed, and the pellets were rinsed with 70% ethanol and allowed to dry. Dry pellets were resuspended in water. DNA concentration and quality were determined using a micro-spectrophotometer (NanoDrop 2000 Spectrophotometer, Thermo Fisher Scientific, Wilmington, DE).

Greenhouse Glyphosate Dose Response

A dose–response experiment was carried out in the greenhouse of the Weed Research Laboratory at Colorado State University in Fort Collins, CO, to quantify the level of glyphosate resistance. Seeds from the BR-R and GA-S Palmer amaranth populations were planted on 1% agar medium and placed in a refrigerator at 4 C for 7 d. They were then transferred to a germination bench at room temperature with 12/12 h of day/night to stimulate rapid and simultaneous germination. Germinated seedlings were then transplanted into commercial potting soil (Professional Growing Mix, Sun Gro^® Horticulture, Vancouver, Canada) in 5 by 5 cm inserts. They were treated with glyphosate at 8- to 10-cm height and kept in a greenhouse where they were maintained at 24±2 C temperatures and 15/9 h day/night photoperiods supplemented with metal-halide lamps (400 µmol m⁻² s⁻¹) and watered twice daily. The experiment was arranged in a randomized complete block design with three replicates. Each replicate contained six individuals for each population and dose, and four individuals for each population and dose when the experiment was repeated. A glyphosate dose response was conducted using 0, 0.05, 0.08, 0.2, 0.4, 0.8, 1.6, and 4.8 kg ae ha⁻¹ with commercially formulated glyphosate (potassium salt, Roundup WeatherMax^®, Monsanto, St. Louis, MO). When the experiment was repeated, an additional dose of 8 kg glyphosate ha⁻¹ was included. Applications were made using an overhead track sprayer (DeVries Manufacturing, Hollandale, MN) equipped with a flat-fan nozzle tip (TeeJet^® 8002EVS, Spraying System, Wheaton, IL) calibrated to deliver 187 L ha⁻¹ of spray solution at 172 kPa. Survival was recorded after 21 d, defined as any plant showing new growth. Dose–response analysis was conducted using the ‘drc’ package in R (Knezevic et al. Reference Knezevic, Streibig and Ritz2007; R Core Team 2015). Survival data (proportion) were analyzed using the three-parameter log-logistic model in the ‘drc’ package:

$$y\,{\equals}\,{D \over {\left[ {1{\plus}\left( {{x \over {{\rm LD50}}}} \right)^{b} } \right]}}$$

where y=survival; x=glyphosate dose (g ae ha⁻¹); D=upper limit; b=slope; and LD50=dose causing 50% reduction in survival.

Shikimate Assay

Twenty individuals from each of the BR-R and the GA-S populations were grown in the greenhouse and tested for glyphosate resistance using an in vivo leaf-disk assay. Three technical replicates (5-mm leaf disks) from each individual per population were sampled, following the procedure described by Shaner et al. (Reference Shaner, Nadler-Hassar, Henry and Koger2005). The excised leaf disks were placed into 96-well microtiter plates containing 10 mM ammonium phosphate buffer and molecular grade glyphosate at the doses of 100, 500, and 1,000 µM. Shikimate levels were read at 380 nm on a fluorescence plate reader (BioTek^TM Synergy^TM 2 multi-mode microplate reader, Winooski, VT). A shikimate standard curve was used to quantify shikimate accumulation (ng shikimate µl⁻¹) in the samples. Data were analyzed using a t-test to compare shikimate accumulation between BR-R and GA-S.

EPSPS Gene Copy Number

Genomic DNA was used to determine 5-enolpyruvylshikimate-3-phosphate synthase (EPSPS) copy number using real-time quantitative PCR (qPCR). Twenty individuals from each of the GA-S and BR-R populations were grown in small pots, and young leaf tissue was collected from each individual for genomic DNA. The samples were immediately frozen in liquid nitrogen and stored at −80 C. Genomic DNA was extracted using the DNEasy Plant Mini Kit (Qiagen, Valencia, CA) and quantified using a NanoDrop spectrophotometer (Thermo Scientific, Wilmington, DE). DNA concentrations were adjusted to 5 ng µl⁻¹, and primer sets and qPCR conditions were used as previously described (primers ALSF2 and ALSR2, EPSF1 and EPSR8) (Gaines et al. Reference Gaines, Zhang, Wang, Bukun, Chisholm, Shaner, Nissen, Patzoldt, Tranel, Culpepper, Grey, Webster, Vencill, Sammons, Jiang, Preston, Leach and Westra2010). Threshold cycles (C_t) for EPSPS and ALS were recorded by a CFX Connect^TM Real-Time PCR Detection System thermal cycler (Bio-Rad Laboratories, Hercules, CA). Relative EPSPS gene copy number was calculated as 2^–ΔCt, with ΔCt=[(Ct, ALS) − (Ct, EPSPS)] (Gaines et al. Reference Gaines, Zhang, Wang, Bukun, Chisholm, Shaner, Nissen, Patzoldt, Tranel, Culpepper, Grey, Webster, Vencill, Sammons, Jiang, Preston, Leach and Westra2010). Triplicate technical replications were used to calculate the mean and standard error of the increase in EPSPS gene copy number relative to ALS.

Single-Dose ALS Testing

Single-dose experiments were conducted to assess resistance to the ALS inhibitors chlorsulfuron, sulfometuron-methyl (both sulfonylureas), and imazethapyr (imidazolinone). These experiments were conducted in the greenhouse at Colorado State University in Fort Collins, CO, under the same conditions as described in the glyphosate dose-response experiment. Individuals from BR-R and GA-S were treated at 8- to 10-cm height. The experiments with sulfonylureas used 28 individuals per population and treatment combination, and the experiments with imazethapyr used 36 individuals for each population. Chlorsulfuron (Glean, DuPont, Wilmington, DE) and sulfometuron-methyl (Oust, Bayer CropScience, Research Triangle Park, NC) were applied at 88 g ai ha⁻¹ and 315 g ai ha⁻¹, respectively. Imazethapyr (Pursuit, BASF, Research Triangle Park, NC) was applied at 61 g ai ha⁻¹ with 1.25% v/v crop oil concentrate. Height (cm), dry weight (g), and survival data were collected 21 d after treatment. The data were analyzed using ANOVA, and LSD with P=0.05 was used for multiple comparison adjustment.

ALS Gene Sequence

Approximately 50 mg of young leaf tissue was sampled from each of three untreated GA-S individuals, six untreated BR-R individuals, nine BR-R individuals that survived 315 g ai ha⁻¹ sulfometuron-methyl, and nine BR-R individuals that survived 88 g ai ha⁻¹ chlorsulfuron. DNA was extracted as described for the species-diagnostic marker. The full-length ALS gene was amplified by PCR using the forward primer: 5′-ATGGCGTCCACTTCAACAAACC-3′ and reverse primer 5′-CTAATAAGCCCTTCTTCCATCACCC -3′. Thirty microliter reactions were mixed following the standard protocol provided with Thermo Scientific Phusion polymerase and 20 ng of template genomic DNA. Reactions were cycled 32 times with the following three-step protocol: 98 C for 10 s, 62 C for 20 s, and 72 C for 90 s. PCR products were run on a 1% agarose gel to verify single band amplification. The expected bands at 2,010 bp were excised from the gel and purified following the standard protocol provided by the QIAquick Gel Extraction Kit from Qiagen. Purified PCR products were sequenced using both the amplification primers listed above and the following four sequencing primers: Seq_FP1 5′-AGTTTGTATTGCCACTTCTGGTCC-3′, Seq_FP2 5′-GAAATCCTCGCCAATGGCTGAC-3′, Seq_RP1 5′- GTCAGCCATTGGCGAGGATTTC-3′, Seq_RP2 5′-TGGACCAGAAGTGGCAATACAAAC-3′. Sanger sequencing reads were analyzed using A Plasmid Editor (aPe, version 2.0.49) and heterozygous base pairs were identified in the sequence trace files by manual inspection. Translated amino acid sequences obtained from BR-R and GA-S were compared with a known susceptible Palmer amaranth ALS amino acid sequence (Molin et al. Reference Molin, Nandula, Wright and Bond2016), GenBank protein accession AMS38337.1.