Sampling Sites

Five field sites were selected in the Finger Lakes region of New York State, near the city of Ithaca (Table 1). The sites represent early successional plant communities, with many having previous agricultural history. Sites included open fields or woodland edge containing areas both invaded (+) and uninvaded (−) by V. rossicum. Invaded sites contained >50% V. rossicum cover and uninvaded sites <1% V. rossicum cover by visual estimates. Field composited soil samples were kept in coolers and returned to the lab and sieved through 2-mm mesh to remove roots and organic debris within 24 h of collection. Subsamples of sieved soils were used for amplicon sequencing of bacterial and fungal composition, measurement of available soil N, and extracellular enzyme activities. The methods of the specific analyses are described in the subsequent sections. Field measurements of soil respiration were conducted once during this study. Due to limitations imposed by negotiated access to the research sites from private and public land owners, as well as equipment availability, sampling dates varied (Table 1).

Table 1 Names, abbreviations, locations, and sampling dates for Vincetoxicum rossicum research sites around Cayuga Lake, NY.

Description of Sites

Edwards Lake (EL) consists of Ovid (fine-loamy, mixed, active, mesic Aeric Endoaqualfs) & Rhinebeck (fine, illitic, mesic Aeric Endoaqualfs) silt loams (2% to 6% slope), which are well drained. Salt Point (SP) has well-drained Genesee (fine-loamy, mixed, superactive, mesic Fluventic Eutrudepts) silt loams (0% to 2% slope). Lansing Center Trail (LCT) has Ilion (fine-loamy, mixed, active, mesic Mollic Endoaqualfs) silty clay loams (0% to 2% slope) that tend to be poorly drained. At LCT, adjacent sites within 14 m are active agricultural fields, though sampling sites were in restored natural areas and along old field or woodland edges. Great Gully (GG) has well-drained Honeoye (fine-loamy, mixed, semiactive, mesic Glossic Hapludalfs) silt loams (2% to 8% slope). Cayuga Nature Center (CNC) has Hudson (fine, illitic, mesic Glossaquic Hapludalfs) silty clay loams (2% to 6% slope) that are moderately well drained (USDA-NRCS 2014). Sites were selected to have similar herbaceous cover common to postagricultural early successional sites for the region, including typical species of goldenrod (Solidago spp.), aster (Aster spp.), raspberry (Rubus spp.), milkweed (Asclepias spp.), Virginia-creeper [Parthenocissus quinquefolia (L.) Planch.], eastern poison-ivy [Toxicodendron radicans (L.) Kuntze], orchardgrass (Dactylis glomerata L.), multiflora rose (Rosa multiflora Thunb.), honeysuckle (Lonicera spp.), sugar maple (Acer saccharum Marshall), white ash (Fraxinus americana L.), white pine (Pinus strobus L.), and hickory species (Carya spp.). Vincetoxicum rossicum densities at EL were among the highest observed across all sites in this study, exceeding 90% cover by visual estimates.

Microbial Community 16S rRNA Gene and Internal Transcribed Spacer Sequencing

DNA was extracted from soil samples using the MoBio PowerSoil DNA Isolation Kit (Mo Bio Laboratories, Carlsbad, CA, USA). We amplified partial 16S rRNA genes (bacteria) and part of the fungal ITS (internal transcribed spacer) region using universal primers with the adapters required for two-step Nextera library preparation for Illumina MiSeq sequencing. For 16S rRNA gene amplification, we used the primers 341F (5′-CCTACGGGNGGCWGCAG-3′) and 805R (5′-GACTACHVGGGTATCTAATCC-3′) (Herlemann et al. Reference Herlemann, Labrenz, Jürgens, Bertilsson, Waniek and Andersson2011), and for ITS amplification, we used the primers ITS1F (5′-CTTGGTCATTTAGAGGAAGTAA-3′) and 58A2R (5′-CTGCGTTCTTCATCGAT-3′) (Gardes and Bruns Reference Gardes and Bruns1993; Martin and Rygiewicz Reference Martin and Rygiewicz2005). Amplification conditions and downstream preparation for sequencing are as described in Howard et al. (Reference Howard, Bell and Kao-Kniffin2017). For 16S rRNA gene sequencing, a 600-cycle MiSeq Reagent Kit v.3 was used, and for ITS sequencing, a 500-cycle MiSeq Reagent Kit v.2 was used (Illumina, San Diego, CA, USA). Sequencing was performed at the Cornell Genomics Facility (Ithaca, NY, USA).

For processing of the ITS sequences, we followed the modified Brazilian Microbiome Project pipeline (Pylro et al. Reference Pylro, Roesch, Morais, Clark, Hirsch and Tótola2014) described in Howard et al. (Reference Howard, Bell and Kao-Kniffin2017). Due to low sequencing efficiency in our 16S rRNA gene run (leading to fewer recovered sequences), we processed all 16S rRNA gene sequences in Mothur (Schloss et al. Reference Schloss, Westcott, Ryabin, Hall, Hartmann, Hollister, Lesniewski, Oakley, Parks and Robinson2009) to retain at least several hundred sequences per sample. Reads were merged with make.contigs, primers removed with trim.seqs (pdiffs=2, maxambig=0), and sequences were aligned using align.seqs followed by screen.seqs and filter.seqs. The data set was reduced to only unique sequences with unique.seqs, and sequences with only one base pair different per 100 bp were classified as identical using pre.cluster. Chimeras were removed using chimera.uchime (dereplicate=t) followed by remove.seqs. Sequences were then classified with classify.seqs (greengenes v13_8_99), and those classified as ‘Chloroplast’, ‘Mitochondria’, ‘Archaea’, ‘Eukaryota’, or ‘unknown’ were removed. Operational taxonomic units (OTUs) were created at 97% sequence similarity using cluster.split, singletons were removed with split.abund, and OTUs were classified with classify.otu. MiSeq data have been deposited in the NCBI Sequence Read Archive and are available under the project number SRP154002.

Soil Nitrogen Availability

Soil samples were measured for extractable soil ammonium (NH₄ ⁺) and nitrate (NO₃ ⁻), determined as the sum of nitrite and nitrate (i.e., NO₂ ⁻ + NO₃ ⁻), hereafter referred to as “nitrate.” Extractable NH₄ ⁺ and NO₃ ⁻ were determined using a potassium chloride (KCl) extraction method described in Drinkwater et al. (Reference Drinkwater, Cambardella, Reeder and Rice1996) with the following modifications. Following shaking with KCl, samples were filtered using an acid-washed 125-ml erlenmeyer flask, topped with a funnel and folded filter paper (Whatman No. 1, 150-mm diameter). Filtered samples were poured into 20-ml scintillation vials and stored at −20 C before analysis. Extracted samples were analyzed using a SEAL AQ2 discrete analyzer (SEAL Analytical, Mequon, WI, USA), following the EPA-150-A Rev. 2 and EPA-114-A Rev.8 protocols for measuring NH₄ ⁺ and NO₃ ⁻, respectively. Extractions were performed in triplicate and averaged for subsequent statistical analysis.

Soil Respiration

A CIRAS-1 portable infrared gas autoanalyzer, equipped with an SRC-1 soil respiration chamber and STP-1 soil temperature probe (PP Systems, Amesbury, MA, USA) was used to measure soil respiration. PVC rings were installed at 10 randomly selected locations at each site where V. rossicum was present or absent at least 72 h before sampling at each site, leaving ~10 cm of the top of the ring exposed above the soil surface [n=100, 10 replicates by 2 treatments (present or absent) by 5 sites]. A flexible rubber coupling was attached to the SRC-1 and connected to each PVC ring for sampling. The headspace volume was determined and entered into the CIRAS-1 unit before sampling.

Soil Extracellular Enzyme Activity

Soil extracellular enzymes, primarily produced by microorganisms, facilitate the decomposition of plant residues and soil organic matter (SOM), such that products become available for microbial and plant assimilation or further transformations. The potential activities of extracellular enzymes can be an indicator of the ability of a soil microbiome to transform different classes of compounds and the overall activity of microorganisms in the soil environment. Measurements of potential soil extracellular enzyme activities were performed on fresh soil within 48 h of field sampling. Refer to Table 2 for the full list of targeted extracellular enzymes and their relevance to C, N, or P cycling. The protocol was developed from German et al. (Reference German, Weintraub, Grandy, Lauber, Rinkes and Allison2011) and Saiya-Cork et al. (Reference Saiya-Cork, Sinsabaugh and Zak2002). Briefly, a 2- to 3-g subsample of each soil was weighed, recorded, and blended for 30 s with 150 ml 50 mM sodium bicarbonate buffer (pH 8) to achieve a suspended soil slurry. For hydrolytic enzymes, a 200-μl aliquot of slurry was added to a black 96-well, solid, flat-bottom plate (Greiner Bio-One, Monroe, NC, USA); four replicates were run for each sample per enzyme, and a separate plate was prepared for 100 mM AMC and MUB standards, respectively. A 50-μl aliquot of 200 μM fluorescently labeled enzyme substrate (Sigma-Aldrich, St Louis, MO, USA) was added to each sample. A full list of extracellular enzyme substrates is listed in Table 2. For oxidative enzymes, soil slurries were added as above to 20 wells of a white, clear-bottom 96-well plate (Greiner Bio-One, Monroe, NC, USA). Ten wells received an additional 50 μl of 50 mM buffer, while 50 μl 3,4-dihydroxy-L-phenylalanine (DOPA) was added to the remaining 10 wells. An additional 10 μl 0.3% H₂O₂ was added to half of the +buffer and +DOPA wells. Five internal standards of buffer, buffer and DOPA, and each with H₂O₂ were run on each plate. All plates were incubated at room temperature (25 C) for 3 h. With 15 min before the end of incubation, 150 μl from each oxidative well was transferred to a new plate, leaving settled sediments behind. Plates were read on a BioTek, Synergy HT Multi-Mode Microplate Reader, with Gen5 software (BioTek Industries, Winooski, VT, USA). Hydrolytic plates were read at 365-nm excitation and 450-nm emission, while oxidative plates were read at 460-nm absorbance.

Table 2 Soil extracellular enzymes, substrates, enzyme targets, and standards measured during analysis.Footnote ^a

^a Table adapted from (German et al. 2011).

^b Specific nutrients associated with enzyme targets are listed in parentheses: C, carbon; N, nitrogen; and P, phosphorous.

Statistical Analyses

Statistical analyses were performed on the data using JMP Pro 10 (SAS, Cary, NC, USA). Data were transformed as needed to fit the assumptions of normality and homogeneity of variance; however, back-transformed means and confidence intervals are reported here. For soil extracellular enzyme activities data, outliers were removed using a Dixon’s Q-test, then analytical replicates were averaged before further analysis. Results were analyzed using a two-level mixed model, where site is a random effect and the effect of V. rossicum is a fixed effect. Site is treated as random, because the sites used for this study are a sampling of sites that contain V. rossicum; therefore, inferences specific to each site are not of interest. Instead, the restricted maximum likelihood (REML) variance component of site indicates the percentage of unexplained variance in the model attributed to the site random effect.

([1]) $${\rm Response}{\equals}{\rbeta }_{0} {\plus}{\rbeta }_{1} \left( {{\rm site}_{{{\rm random}}} } \right){\plus}{\rbeta }_{2} \left( {{\rm treatment}_{{{\rm fixed}}} } \right){\plus} {\rm {\repsilon}}$$

The number of sequences per sample was rarefied to the lowest number available in a single sample, excluding samples in which amplification/sequencing was unsuccessful (one replicate each of ‘Cayuga - V. rossicum absent’, ‘Lansing - V. rossicum absent’, and ‘Lansing - V. rossicum present’ for 16S rRNA gene sequences, and two replicates of ‘Salt Point - V. rossicum present’ and 1 replicate of ‘Gully - V. rossicum present’ for ITS sequences). For 16S rRNA gene sequences, we rarefied to 376 sequences sample⁻¹, and for ITS sequences, we rarefied to 3,126 sequences sample⁻¹.

All downstream analyses of 16S rRNA gene and ITS sequences were performed in R. We created principal coordinate analysis (PCoA) plots of Bray-Curtis distances between sites using vegdist (package ‘vegan’) and cmdscale (package ‘stats’). We used permutational multivariate analysis of variance (PERMANOVA) to test for significant differences in bacterial and fungal community composition by location and V. rossicum treatment with adonis (package ‘vegan’). We calculated fungal and bacterial Shannon diversity for each site using diversity (package ‘vegan’), and tested for differences based on V. rossicum presence or absence using t.test (package ‘stats’). We created 100% bar plots of taxonomy by site by V. rossicum treatment using phyloseq and barplot (package ‘graphics’). We created a heat map of Ascomycota OTUs using average clustering of Bray-Curtis distances for both sites and OTUs, and this was visualized with heatmap.2 (package ‘gplots’). OTUs with a relative abundance less than 0.5% were not visualized, but were included in distance calculations.