Study Area

The study area is represented by the Magadino plain, the largest alluvial plain of the Ticino River located in southern Switzerland (Figure 1). The plain is characterized by an Insubric climate, i.e., mild and dry winters and warm, but stormy summers (Klötzli Reference Klötzli1988; Spinedi and Isotta Reference Spinedi and Isotta2004). The mean annual precipitation and the mean annual temperature are 1,806 mm and 11.9 C, respectively (climate normal 1991 to 2020, Meteoswiss climatological station of Magadino/Cadenazzo). In Canton Ticino, the geological and soil substrate mainly consists of metamorphic crystalline rock (Labhart Reference Labhart1992), giving way to sandy deposits with pebbles and gravel in the floodplains, with an intermediate sandy loam soil composition at the superficial soil level (Czerski et al. Reference Czerski, Giacomazzi and Scapozza2022; Scapozza Reference Scapozza2013). The plain is particularly rich in exotic flora and invasive neophytes (Schoenenberger et al. Reference Schoenenberger, Rötlisberger and Carraro2014), and among the taxa of the P. cuspidatum aggregate, P. ×bohemicum is the most widely distributed and displays the highest colonization potential.

Figure 1. Study area with the location of two wild populations in Canton Ticino (Switzerland) of Polygonum ×bohemicum (white circles), the nearby research campus (black triangle), and the two urban centers of Locarno and Bellinzona (yellow squares). (A) Map of Switzerland and (B) map of the study area (Magadino plain).

Study Design and Workflow

As reported in Figure 2, the study was developed with two subsequent phases (i.e., Phase I in autumn 2021 and Phase II in spring 2022) and on two different sites (i.e., Gudo and Cadenazzo; see Figure 1 for location details). Both sites consist of historically important naturalized populations of P. ×bohemicum not subjected to control measures and currently covering more than 500 m² in an open area surrounded by cultivated fields. The hybrid P. ×bohemicum can reach 4.5 m height and is characterized by morphological intermediate characteristics between the two parent taxa (Alberternst and Böhmer Reference Alberternst and Böhmer2011; InfoFlora 2023). The stems are partially spotted with reddish spots, and the leaves are slightly heart-shaped and can measure up to 25-cm long and 18-cm wide with trichomes situated on the veins of the abaxial side of the leaves. Preliminary field examinations using a field lens identified 0.5-mm-long trichomes (Alberternst and Böhmer Reference Alberternst and Böhmer2011), which allowed us to confirm the exclusive presence of P. ×bohemicum at both sites.

Figure 2. Research workflow for the present study on anatomical characteristics and resprouting capacity of the underground organs of Polygonum ×bohemicum. RH, relative humidity.

In a first step (Phase I; Figure 2), we focused on the description of the anatomical features of the underground organs with the aim of developing a field-ready identification method to unambiguously discriminate between rhizomes and roots based on morpho-anatomical characteristics. For this purpose, at the beginning of November 2021, a 1-m-deep trench was dug with a mechanical excavator at the Gudo site. All underground organs were manually sieved from the excavated soil. Specimens of presumed rhizomes and roots were then sampled, transported to the lab facilities at the nearby research campus in Cadenazzo, cleaned of soil residuals, and processed as described in the section “Morpho-anatomical Analysis”. Once the morpho-anatomical analysis of the collected specimens was concluded, a partial validation of the developed field method was made by returning to the trench dug in Gudo. The trench excavation was continued, collecting new fresh underground organs with a total diameter ranging from 0.75 to 1.5 cm and preliminarily separating rhizomes and roots using the proposed protocol (pith test development in Figure 2). Based on the assumption that specimens classified as roots are not able to resprout, collected rhizomes and roots organs were first cut into 3-cm segments and subjected to a resprouting test at the greenhouse facilities of the research campus to confirm the correct distinction of rhizomes and roots (see Figure 2 and the section “Resprouting Tests”).

In a second step (Phase II; Figure 2), we focused on the morpho-anatomical features of rhizomes that increase their ability to resprout. In spring 2022 (mid-March to mid-April), we collected rhizomes ranging from 0.25 to 3 cm in total diameter from twelve 20 by 20 by 20 cm cubic soil samples excavated by hand with a shovel in Gudo and in Cadenazzo (i.e., six soil cubes at each site). Collected rhizomes were first checked for correct identification using the developed pith-test method and then cut into 3-cm segments taking care to have exactly one node in each segment. Each obtained segment was first characterized by different measurements (e.g., weight, total diameter, pith diameter, pith brightness, and pith color) and then subjected to a resprouting test at the greenhouse facilities of the research campus (see Figure 2 and the sections “Rhizome Measurements” and “Resprouting Tests”).

Morpho-anatomical Analysis

Cleaned underground organs sampled in Gudo were subjected to a preliminary visual classification into rhizomes and roots based on the external habit (Fuchs Reference Fuchs1957; Martin et al. Reference Martin, Dommanget, Lavallée and Evette2020) until ca. 25 specimens of presumed rhizomes and 25 of presumed roots were obtained. For a detailed analysis of the morpho-anatomical features, we first produced high-resolution color images depicting the external appearance and transversal sections of a selection of rhizomes and roots by using a stereo microscope (Olympus SZX16 with a Plan Apochromat 1× PF objective) equipped with a DP28 digital camera and stitching the obtained images with the software CellSens v. 1.16 (Olympus Corporation, 3-1 Nishi-Shinjuku 2-chome, Shinjuku-ku, Tokyo 163-0914, Japan). In the second step, samples were first put in small plastic bottles filled with 40% ethanol that was then replaced with 70% ethanol (at least four washes) for long-term conservation. Microanatomical differences between rhizomes and roots were further investigated by producing 20-μm thin slides from 10 samples of young and old rhizomes and roots. To perform thin sections, the samples were sectioned with the WSL Lab-Microtome (Swiss Federal Institute for Forest, Snow and Landscape Research, Zürcherstrasse 111, 8903 Birmensdorf, Switzerland; see also Gärtner and Schweingruber Reference Gärtner and Schweingruber2013). Obtained microslides were transferred onto glass slides and stained with a water solution of safranine (10 g L^-1) and astrablue (5 g L^-1) to highlight the tissues containing lignin and cellulose, respectively. Thin sections were finally fixed on slides with EUKITT mounting resins (ORSAtec GmbH, Max-Fischer-Strasse 11, 86399 Bobingen, Germany) and observed under a compound upright microscope (Olympus BX53 with 5× and 10× objectives; Olympus Corporation, Tokyo 163-0914, Japan). Selected anatomical details were then photographed with the connected DP28 digital camera combined with CellSens software, and further processed with Photoshop (v. 23.5.3; Adobe Corporation, 345 Park Avenue San Jose, CA 95110-2704, USA) for cleaning or feature selection purposes.

Rhizome Measurements

Each collected 3-cm rhizome segment for the main resprouting test was subjected to different measurements (Figure 2; Table 1). We first measured the weight with a Mettler Toledo laboratory balance (precision at 10⁻² g; Mettler-Toledo, 1900 Polaris Parkway Columbus, OH 43240, USA). We then used the stereo microscope to take high-resolution color images with fixed parameters (magnification 0.7×, diaphragm 3.5, light source 0.9, exposure time 20 ms, and gain 3.36×) and stitched the obtained images with the CellSens software. For large diameters, the images were captured using the Instant Multiple Image Alignment function. On the images obtained, we measured the rhizome total diameter and pith diameter by calculating the mean between two measurements (horizontal and vertical line options of the CellSens software, precision at 10⁻⁶ mm).

Table 1. Rhizome measurements in Polygonum ×bohemicum.

To assess the rhizome pith main color, we first removed all peripheral vascular bundles and cortex from the image of each segment section using Photoshop, keeping only the pith and converting it in Tag Image File Format (.TIFF). To remove impurities and stains from the images, pith colors were clustered for each image with R (RStudio Core Team 2023) using the Colordistance (Weller and Westneat Reference Weller and Westneat2019) and Countcolors (Hooper et al. Reference Hooper, Weller and Amelon2020) packages. The clusters were built on all pith pixels, and the frequencies of the five most frequent RGB clusters were calculated using getKMeanColors and extractClusters functions in Colordistance package (Weller and Westneat Reference Weller and Westneat2019). Finally, only the first or two most frequent color clusters (at least 20% frequency) were retained and, if applicable, averaged.

From the obtained pith main RGB colors, we calculated the corresponding pith brightness along a continuous grayscale ranging from 0 (black) to 1 (white) using the rgb2gray.luminosity function of the plotteR package (Weise Reference Weise2019). To enhance visualization and define ordered color scales that are simple and easy to use in the field, we calculated six pith brightness classes and six color classes. Brightness classes were obtained by dividing the value range into six regular intervals. RGB color values were also clustered into six color classes by using the kmeans function on the RGB values matrix.

Resprouting Tests

The resprouting tests took place in the greenhouse facilities of the research campus in Cadenazzo. For this purpose, the 3-cm segments of the underground organs were buried 1.5-cm deep in a 5-cm-deep mixture of sand and loam (soil composition: 1 part silt loam, 1 part sand, 1 part manure, and 1 part expanded shale) in plastic trays (Cindy Seed trays with sieve bottom; Caminada Sementi SA, Via Pré d’Là, 6814 Lamone, Switzerland), into which water was added daily to maintain soil moisture. In both preliminary and main resprouting experiments (see Figure 2), trays were inspected for resprouting specimens every 2 to 3 d for a total experimental period of 70 d. The preliminary resprouting test took place late November 2021 with 103 rhizome and 43 root segments which were kept at a mean temperature of 16 ± 4 C and at 50% relative air humidity. The main resprouting test took place in April 2022 with 201 rhizome segments in total (106 from Gudo and 95 from Cadenazzo), which were kept at 22 ± 5 C with 52% relative air humidity.

Statistical Analysis

To identify the features enhancing the rhizomes’ resprouting ability, we tested whether relationships between the continuous variables and resprouting capacity encoded as a binary response were significant. The glmer function in lme4 package (Bates et al. Reference Bates, Mächler, Bolker and Walker2015) was used to perform a binomial model (fitting generalized linear models, binomial multivariate), assessing all morphological rhizome patterns. A mixed-modeling approach was applied, as we were not interested in the effect provided by the site (random factor). To avoid multicollinearity, the variance inflation factor (vif) was calculated, and the model was adapted. We then calculated the model R squared using the MuMln package (Bartoń Reference Bartoń2023), as well as the estimates of the retained variables, their confidence intervals (2.5% and 97.5%), their P-values in the model, and their respective vif values (Table 2).

Table 2. Estimate statistics of the fitted generalized linear mixed model for resprouting ability (logistic) in Polygonum ×bohemicum (n _tot = 201).

^a Weight was removed to avoid multicollinearity with total diameter.

^b Pith brightness corresponding to the continuous grayscale (0–1).

To assess the informative and diagnostic value of pith chromatic characteristics, curves representing the resprouting capacity for all pith brightness and color classes were calculated. Differences in resprouting capacity among classes were tested using Pearson’s chi-square tests (Hope Reference Hope1968). To provide easily usable color scales to assess rhizome resprouting capacity in the field, we analyzed the differences among pith color classes (Supplementary Figure S1). Differences in pith brightness values (i.e., continuous grayscale) were visualized as box plots among pith color classes. Significant mean differences were tested with Kruskal-Wallis for general mean comparison and Wilcoxon tests for pairwise comparisons (Hollander and Wolfe Reference Hollander and Wolfe1973) using a false discovery rate correction (Benjamini and Yekutieli Reference Benjamini and Yekutieli2001). Significant nominal levels of 1% and 5% were used for general and pairwise comparisons, respectively. In addition, a practical fact sheet with reference color scales representing the pith brightness and color classes was developed (Supplementary Figure S2). All analyses were performed in R (RStudio Core Team 2023).