Soil preparation
Soil (the top 10 cm below the easily removed litter layer) was collected from a forested area of Point Reyes National Seashore (PRNS), California, USA, see (Branco et al. 2013) for site details. GPS location: N38 05.087 W122 52.253. After the removal of stones and larger material, the soil was air dried for 48 h prior to being sieved to 2 mm in the laboratory. Sterile sand (autoclaved for 30 min on three successive days) was added to the soil to 30 % v/v to improve aeration during the experiment. AgNP (20 nm diameter, 99.8 % purity, obtained from US Research Nanomaterials Inc, Texas 77084, USA) were added to a smaller portion of the soil (~100 g) and mixed thoroughly (for 10 min using a metal spatula) to obtain a homogenous dispersion of AgNP. This 100 g of soil was then thoroughly mixed into larger soil volume in ‘zip-loc’ bags to obtain final AgNP levels of 350 and 790 mg Ag/kg (see below). These AgNP levels were chosen as they were similar to those used in previous work (Kumar et al. 2011) and represent a high level of AgNP contamination. Non-contaminated control soil was also prepared in the same way but without the addition of AgNP. The soil:sand mix (65 ml volume) was then added to individual ‘cone-tainers’ (Steuwe and Sons, Corvallis, USA) and covered with a 1 cm depth of sterile sand. Altogether 14 replicates of each treatment (0, 350 and 790 mg Ag/kg) were prepared.
Soil analysis
Dried soil (40 °C) was analysed by the UC Davis College of Agricultural and Environmental Sciences Analytical Laboratory using standard methods (prior to experimental set-up). Soil texture pH, organic C, total N, total P (Olsen), total silver and extractable silver were determined and results reported in Tables 1, 2 and 3.
Table 2 Ectomycorrhizal genera fund on roots from soils containing 0, 350 and 790 mg Ag/kg
Table 3 Total and extractable Ag levels in contaminated soil samples
Analysis of total silver in soil
Soil samples were digested by nitric acid/hydrogen peroxide closed vessel microwave digestion and the total amount of silver in the digest analysed by ICP-AES (UC Davis standard method 590.02).
Extractable silver analysis of soil
The level of extractable silver in triplicate samples obtained from each treatment at the end of the plant growth period (4 months: see below) was determined by the method of Hou et al. (2005). Briefly 1 g soil was added to 10 ml of 1 M NH4NO3 (pH 7) and shaken at 100 rpm in an orbital shaker for 4 h at 25 °C. The extract was collected by centrifugation at 3000 rpm×g for 10 min. Extracts were stored at −20 °C until analysis by ICP-AES using standard methods at UC Davis.
Preparation and growth of Pinus muricata D. Don (Bishop pine) seedlings
Pinus muricata cones were collected from different trees in PRNS and dried in the laboratory to allow collection of seeds. Wings were removed from seeds and stored at 4 °C until required. To start germination, seeds were placed in 15 % (v/v) H2O2 solution plus tween 80 (one drop per 500 ml) and stirred for 15 min. Seeds were then collected in a sieve, rinsed with deionised water and finally soaked in deionised water for 24 h prior to planting in soil. Three seeds were planted in each cone-tainer (prepared as described above) and distilled water added until saturated soil moisture conditions were achieved (maintained throughout the experiment). Cone-tainers were incubated at 20 °C in a growth chamber set at a constant light intensity of ~220 µmol m−2s−1.
Sampling of plants and soil
Seedlings were thinned to one per cone-tainer after a period of 1 month, and the thinned seedlings used for initial experimental observations of root length, root and shoot fresh weight. The remaining seedlings were grown for a further 4 months and destructively harvested for measurement of shoot and root fresh weight and ectomycorrhizal diversity on roots. Soil was also analysed for extractable silver levels after 4 months (see above).
Collection of ectomycorrhizal roots, DNA extraction and PCR
Root tips were collected from a random subsample (from five cone-tainers) of the different AgNP-treated pine seedlings. The aim of the experiment was to observe the total diversity of ECM present. So roots that displayed different ectomycorrhizal root morphology (such as variations in colour, diameter and tissue density (Comas et al. 2014) were preferentially collected. Most of the AgNP-treated plants showed no obvious visual ECM colonisation so ‘normal’ roots were collected in an attempt to discover if any ectomycorrhizal colonisation was present. Overall, a total of 10 root tip samples were collected from each treatment and were subjected to immediate extraction using the REDExtract-N-Amp Tissue PCR Kit (Sigma-Aldrich, Saint Louis, MO, USA). Each root tip was added to 20 μL of extraction buffer and incubated at 95 °C for 10 min. Then 20 μL neutralisation buffer was immediately added and the extracts stored at −20 °C prior to PCR. PCR was carried under using standard conditions with the fungal specific primer pair ITS1f and ITS4 (Gardes and Bruns 1993; White et al. 1990). PCR products were cleaned using AmPURE magnetic beads following manufacturers recommendations. PCR products were sequenced in forward and reverse directions using an ABI3170 Genetic Analyser (Applied Biosystems, Foster City, CA, USA). Fungi were defined using a 97 % sequence similarity cut-off and named according to the nearest BLAST match.
Statistical analysis
All data were analysed by one-way ANOVA and differences between individual means were determined by post hoc least significance difference analysis using SPSS version 21.