Insect collection

Collection sites were divided into five regions (Central, South, West, East, and North) along two transects in the Midwest United States (Figure 1). A total of 25 samples were taken. All samples were collected from soybean fields by using sweep nets (Table 1). Two perpendicular transects were designed running from Minnesota/South Dakota to Missouri/ Kansas, and from Nebraska to Illinois/Ohio. Iowa was regarded as the central area for the two transects. The samples were collected from an area spanning about 960 miles (west to east: 1545 km) by about 790 miles (north to south: 1,271 km). The Mississippi River separated East samples from the others, the Missouri River separated the Center from West samples, and North from South samples were quite distant. The West samples were collected from Lincoln, Mead, Concord, and Clay Center areas of Nebraska in 2008 and 2010 (Table 1). The East samples were collected in 2003 (Waverly, Pemberville, and Hoytville in Ohio) and 2010 (Savoy, IL, and Logan, Richland, and Hancock in Ohio) (Table 1). All other samples were collected in 2010 (Table 1). The number of insects collected and used per location (sample) varied between 15 to more than 30. The collected C. trifurcata adults were stored in 95% alcohol until the samples reached the laboratory. The alcohol was then changed twice to avoid alcohol dilution by fluids from sampled adults, which can lead to DNA degradation, and then kept in the freezer at -80°C until processing for DNA isolation.

Figure 1.

Sampling sites of Midwest (USA) Cerotoma trifurcata subpopulations used in this study. *1-Brookings, 2-Becker, 3- Lamberton, 4-Sutherland, 5-Ames, 6-Lewis, 7-Chariton, 8-Concord, 9-Ithaca (Mead), 10-Lincoln, 11-Clay Center, 12-Manhattan, 13- Columbia, 14-Pemiscot, 15-Savoy, 16-Logan, 17-Waverly, 18-Richland, 19-Hancock, 20-Hoytville, 21-Pemberville. High quality figures are available online.

Table 1.

Code, collection site, collector, and date of collection of adult samples of Cerotoma trifurcata.

DNA extraction and quantification

DNA was extracted from the thorax of C. trifurcata adults using a hexadecyltrimethylammoniumbromide (CTAB; Sigma-Aldrich,  www.sigmaaldrich.com) extraction protocol as modified by Clark (2005). The frozen adults were first soaked and washed in a beaker of double distilled autoclaved water for 10 min. The adults were then prepared for DNA extraction by removing the gut, abdomen, and head, leaving only the thorax to use in the study. The thorax was homogenized in 500 µL of CTAB extraction buffer (100 mM Tris-HCL, 1.4 M NaCl, 0.02 M EDTA, 2% CTAB, and 0.2% β -mercapto ethanol) (Sigma- Aldrich). 10 µL Proteinase K (concentration of 200 µg/mL extraction buffer; Sigma-Aldrich) was added to the homogenate in each tube and then incubated for 1.5 hr at 65°C. RNase A (15 µL; 500 µg/mL concentration; Sigma-Aldrich) was added to the homogenates, and this was incubated for 2 hr at 37°C. After RNA and protein were removed from each sample, the homogenate was centrifuged at 14,000 rpm for 5 min at room temperature. The supernatant was then removed and placed in clean, 1.5-µL autoclaved micro-centrifuge tubes. This supernatant was further extracted with 500 µL of chloroform:isoamyl alcohol (24:1) (Sigma-Aldrich) by centrifugation at 14,000 rpm for 20 min to separate the phases. The top, aqueous phase was transferred into a clean, autoclaved, 1.5-mL micro-centrifuge tube, and the chloroform:isoamyl step was repeated. The aqueous phase was once again collected into another clean, autoclaved, 1.5-mL microcentrifuge tube. DNA was then precipitated by adding 400 µL chilled (-20°C) isopropanol to the aqueous phase and incubated at 4°C for at least 8 hr. After incubation, the precipitate was centrifuged at 12,000 rpm at 4°C for 30 min. The isopropanol was decanted; the DNA pellet was then rinsed with 500 µL 100% chilled ethanol (ETOH) and centrifuged at 12,000 rpm at 4°C for 5 min. The supernatant was poured off, the pellet was rinsed with 500 µL of 70% cold ETOH, and this was centrifuged for 5 min. The ETOH was decanted, and the pellet was then air dried at room temperature (24°C) for 50 min under the hood. After drying, the pellet, 80 µL of 1X TE buffer (10 mM Tris-HCL pH 8.0, 0.1 mM EDTA) was added into the micro-centrifuge tube with the DNA pellet and stored at 4°C for at least 8 hr; this was then transferred and kept at -20°C.

Each DNA sample was quantified by using both a 1% agarose gel and Nanodrop spectrophotometer (ND 1000 V3.5.1) (Thermo Scientific,  www.thermoscientific.com). The Nanodrop spectrophotometer provides both the quality and quantity measurements based on the 280/260 ratio readings. However, this does not show fully the DNA quality, that is, if it is degraded or not. So, a 1% agarose gel with a λ DNA marker (22.2 ng/µL) was run at 60 volts for 20 min to further quantify the DNA. The agarose gels were visualized under the UV light using Genomic Solution software (Genomic Solutions, Harvard Bioscience,  www.harvardbioscience.com). After quantification, the DNA samples were diluted to 23 ng/µL concentration by adding 1 X TE buffer. These diluted DNA samples were then kept at -20°C until they were used, after which the samples were kept at -80°C as vouchers.

Table 2.

The sequences of oligonucleotide adapters, and primers used for AFLP analysis of Cerotoma trifurcata.

Table 3.

Selective AFLP primer combinations, number of markers, and fragment size for the primer pair combinations for Cerotoma trifurcata study.

AFLP process

A modified AFLP protocol (Vos et al. 1995) was used to assess the genetic variability within and among C. trifurcata samples. DNA extracted from individual samples of C. trifurcata was used. The AFLP procedure consists of three basic steps: 1) DNA template preparation; 2) DNA template pre-amplification; and 3) selective amplification of the pre-amplified product. The DNA extracts were digested with EcoR1 and Mse1 restriction enzymes and ligated with specific adapters (Table 2). The ligation product was diluted 1:10 with 1X TE buffer. This was then used as a template for the preamplification and selective amplification. Three combinations of two IRD-labeled ECOR1 primers (ACA and AAC) and two unlabelled MSe1 primers (CAA and CAG) (LI-COR,  www.licor.com) were used in this study to determine the genetic variability within and between the C. trifurcata samples (Table 3). A control (all the AFLP reagents except DNA) was also run with the insect samples. AFLP products were separated in 6.5% denaturing polyacrilamide gels (LICOR) and visualized in a Li-COR Gene Read IR 4200 DNA sequencer (LI-COR) for 2.5 hr at 45°C and 1500 volts. First and last lanes of the gel were loaded with 1 µL of IRD-labeled 50–700 base pair size standard marker (LICOR).

AFLP gel scoring

The AFLP bands were scored, using IRD-700 labeled 50–700 bp marker as a size reference with the SAGA Generation 2 software, version 3.2 (LI-COR). The visibility, sharpness, and repeatability of the bands were guiding criteria in marker selection for scoring. Profiles from multiple individuals were aligned and scored based on the presence (1) or absence (0) of a band on the AFLP gel, producing a binary data matrix.

DBOOD (Coelho 2001) was used to evaluate the correlation between the coefficient of variation and the number of molecular markers observed, thus providing an estimate of the robustness of the data (Hoelzel 1995). The binary data matrix was then used to estimate genetic similarity using the Jaccard index through the SIMQUAL procedure using NTSYSpc (Rohlf 2000). Dendrograms were constructed to illustrate genetic similarity, following the methodology described by Sneath and Sokal (1973). Bootstrap analysis was used (10,000 resamples), using BOOD-P software version 3.1 (Coelho 2001) as a way of testing the reliability of the dataset for further analysis. The software package Arlequin version 3.1 (Excoffier et al. 2005) was used to conduct the analysis of molecular variance (AMOVA). The AMOVA tests for genetic structure and genetic variability among groups, within groups, and within locations (Schneider et al. 2000). ARLEQUIN (version 3.1) was also used for pair-wise comparisons to test genetic divergence (F_ST - Wright's inbreeding coefficient; Slatkin 1995). Genetic isolation was tested, comparing geographic distance and genetic dissimilarity, using the Mantel test (Mantel 1967; Smouse et al. 1986) with 1000 permutations using ARLEQUIN version 3.1. POPGENE version 1.32 (Yeh and Boyle 1997) was used to determine the degree of polymorphisms both within and between samples of C. trifurcata. Genetic differentiation between samples was assessed using Nei's gene diversity index (G_ST) in POPGENE; gene flow was estimated from G_ST, expressed as (N_m) = 0.5 (1- G_ST)/G_ST (McDermott and McDonald 1993, Bonin et al. 2007, Ryman and Leimar 2009). West (Nebraska) samples from 2008 and 2010 and East (Illinois/Ohio) samples from 2003 and 2010 were used to test for temporal genetic variation of C. trifurcata using total genetic diversity (H_T), the Mantel test, and gene flow. Fall armyworm larvae, Spodoptera frugiperda (J.E. Smith) (Lepidoptera: Noctuidae) were used as the outlier group to test the robustness of the analytical tool in the POPGENE analysis.

The effectiveness of AFLP markers

Each primer combination was used with 24 randomly selected individuals from the samples for assessing the genotyping error. Each primer combination was replicated three times, with these same 24 individuals, and the AFLP processes as initially done for the main experiment. The individual loci were then examined for mismatches among the three replicates. The error rate was calculated as the ratio of the total number of mismatches (presence or absence of a band) at a particular locus to the number of the replicated individuals (Pompanon et al. 2005; Bonin et al. 2007). Loci with an error rate greater than 0.1 were rejected and not used in the study.

The polymorphism and robustness of AFLP primers analyzed

A total of 175 loci ranging in size from 50 to 400 bp were observed using the three primer combinations (Table 3). About 96.5% of the genetic variability was accounted for, indicating that there was sufficient number of markers for further robust analysis (Coelho 2001).

The number of loci that were polymorphic for all the samples examined ranged between 124 and 168, with an average of 143 loci. The average loci polymorphism was 82% and ranged from 70.86% to 96% for Ames (Iowa) and Concord (Nebraska), respectively (Table 4).

Temporal variation of C. trifurcata for Nebraska and Ohio samples

The total genetic diversity (H_T), when comparing the 2008 and 2010 Nebraska samples, was 0.400, 0.410, 0.440, and 0.296 for Lincoln, Mead, Concord, and Clay Center, respectively. The proportion of total diversity among these samples (G_ST) was 0.136, 0.124, 0.089, and 0.032 for Lincoln, Mead, Concord, and Clay Center, respectively. Gene flow (N_m) for Lincoln, Mead, Concord, and Clay Center were 3.189, 3.527, 5.109, and 5.250, respectively, which indicates a high gene flow between the 2008 and 2010 samples. The total genetic diversity of the East samples taken in 2003 and 2010 was 0.385. The proportion of total diversity among samples was 0.175, and gene flow was found to be 2.362 for East samples. Mantel tests revealed no correlation between genetic and geographic distance for the western Midwest (Nebraska) region samples (r = 0.217; P = 0.181); the regression supported this finding (F_1,26 = 3.07; P = 0.079; R² =0.003). Similarly, results from the eastern Midwest (Illinois/Ohio) also showed no significant dependency of genetic distance on geographic distance (F_1,26 = 2.86; P = 0.103; R² = 0.099). Therefore, these samples (2003 and 2008) were used as part of the overall analyses.

Table 4.

Genetic diversity estimates for all Cerotoma trifurcata subpopulations : number of polymorphic loci, percent loci polymorphism, heterozygosity (genetic variation) for a subpopulation (H_S), heterozygosity for all C. trifurcata subpopulations (H_T), gene flow among all subpopulations (N_m) and genetic variation between subpopulations (G_st).

Table 5.

Analysis of molecular variance (AMOVA) for 25 subpopulations of Cerotoma trifurcata collected from five different regions of the Midwestern USA (North, South, East, West, and Central).

Genetic diversity, G_ST values, and gene flow

The average heterozygosity (H_S) for individual samples was 0.335; the highest H_S (0.425) was recorded at Concord, NE, and the lowest (0.229) was recorded at Lewis, IA (Table 4). The average total heterozygosity (H_T) for all the C. trifurcata samples (0.426) was high. This indicates that the overall heterozygosity of the C. trifurcata population is higher than that seen in individual samples. Analysis of multiple locations in POPGENE (Nei 1973; McDermott and McDonald 1993) for genetic diversity estimate (G_ST) for all the samples revealed a moderate level of differentiation (G_ST = 0.215) (Table 4). The average gene flow (N_m) among the C. trifurcata samples was <1 (1.83) (Table 4).

Figure 2.

Genetic (dissimilarity) and geographic distance correlation among the Cerotoma trifurcata subpopulations sampled from western-Midwest USA (Nebraska), southern-Midwest USA (Missouri and Kansas), northern-Midwest USA (Minnesota and South Dakota), central-Midwest USA (Iowa), and eastern-Midwest USA (Ohio and Illinois). High quality figures are available online.

Figure 3.

Dendogram illustrating the relationships among all the 25 Cerotoma trifurcata subpopulations collected from the Midwest USA, and an out group population of fall armyworm (FAW) collected from Iowa. Bootstrap values, when < 50%, are given at each of the forks (1000 replicates). High quality figures are available online.

Comparing genetic distance and geographical distance

The results of the Mantel test for the entire data set revealed no significant correlation between geographic and genetic distance (r = 0.077, P = 0.180) in the C. trifurcata samples. This implied that there was no structure in the genetic variation among the samples in relation to either an increase or decrease in geographical distance. The majority of the dissimilarity matrixes had values between 0.1 and 0.25 (Figure 2). In addition, the analysis of dissimilarity by geographic distance scatter plots revealed random dispersion of the matrices for all C. trifurcata samples (Figure 2).

Analysis of molecular variance

Results from the AMOVA revealed the highest percentage of the variation (81.8%) from the total variation was from within C. trifurcata sample locations; 12.6% of the total genetic variation was from among samples within groups; and the variability among the groups accounted for 5.60% of the total C. trifurcata samples' variation (Table 5). The genetic divergence (0.182), which was measured by the fixation index (F_ST) as calculated by Arlequin (Excoffier et al. 1992), showed a moderate degree of genetic differentiation among C. trifurcata samples. The dendrogram clustering for the entire C. trifurcata samples of all locations did not show any distinctly defined groups or clustering that could separate the samples of C. trifurcata into geographic locations as defined for the Midwest USA in this study (Figure 3). Moreover, the S. frugiperda larvae samples used as the outlier group to test the robustness of the analytical tool clearly separated from the C. trifurcata samples, indicating the reliability of the cluster analysis (Figure 3).

The AFLP markers reproducibility

The reproducibility of the results by the three primer pairs, tested on 24 samples randomly selected from various samples, indicated that the AFLP approach was accurate and reliable. The average error rate found in this study was 5.85% (Table 3). The maximum error rate acceptable varies with the scope of the study, but in most cases it should never exceed 10% (Bonin et al. 2007). This implies that the error rate for this study was within the acceptable range; hence, the findings have at least 90% repeatability. Pompanon et al. (2005) emphasized that estimation of error rate should be a priority in AFLP studies. This study has revealed that AFLP is reproducible with an error rate of 5.85%. It is difficult to eradicate the genotyping errors because molecular assays and sample handling manually are not 100% (Bonin et al. 2004).