Abstract
Tropical rainforests play important roles in carbon sequestration and are hot spots for biodiversity. Tropical forests are being replaced by rubber (Hevea brasiliensis) plantations, causing widespread concern of a crash in biodiversity. Such changes in aboveground vegetation might have stronger impacts on belowground biodiversity. We studied tropical rainforest fragments and derived rubber plantations at a network of sites in Xishuangbanna, China, hypothesizing a major decrease in diversity with conversion to plantations. We used metabarcoding of the 18S rRNA gene and recovered 2313 OTUs, with a total of 449 OTUs shared between the two land-use types. The most abundant phyla detected were Annelida (66.4% reads) followed by arthropods (15.5% reads) and nematodes (8.9% reads). Of these, only annelids were significantly more abundant in rubber plantation. Taken together, α- and β-diversity were significantly higher in forest than rubber plantation. Soil pH and spatial distance explained a significant portion of the variability in phylogenetic community structure for both land-use types. Community assembly was primarily influenced by stochastic processes. Overall it appears that forest replacement by rubber plantation results in an overall loss and extensive replacement of soil micro- and mesofaunal biodiversity, which should be regarded as an additional aspect of the impact of forest conversion.
Introduction
Tropical rainforests play important roles in biogeochemical cycling and climate regulation and act as reservoirs of global biodiversity by supporting around 50% of all described species1,2,3. Native forest areas are shrinking throughout the tropics, with rapid clearance for agriculture and plantations2,4,5,6. More than one million hectares of native forest have been converted to rubber plantation over the last few decades in the Mekong River Region alone7. This has led to a substantial reduction in structural and functional biodiversity5,8,9,10, a reduction in carbon sequestration11,12, and an increase in habitat fragmentation5,13 with noticeable alterations in the hydrological systems14,15,16. Forest conversion into plantations also drives changes in soil chemistry, for instance in pH, C: N ratio, P and Ca concentrations17,18. The resulting chemical degradation of tropical soils is fast and often results in a complete or partial loss of its productive capacity19.
Anthropogenic alteration of forests, through logging or replacement of native logged forest by plantation (which generally uses introduced species), may have various effects on alpha (α) and beta (β) diversity of the plants or animals being studied, but most of the studies suggest a decline in both measures of diversity3,5,9. In contrast to larger organisms, bacteria have been shown to undergo both an increase20 as well as a decrease21 in β-diversity following forest conversion to agriculture, with an increase or no effects on α-diversity20,21,22.
Soil microfauna (roughly defined as 5–120 µm) and mesofauna (somewhat inconsistently defined as 80 µm–2 mm), includes adults of various phyla (e.g., Nematoda, Tardigrada, Rotifera, small Annelida), and eggs/juvenile stages of some metazoan species23. These organisms have been often neglected from soil biodiversity surveys even though they are considered to play an important role in land ecosystem functioning. For example, nematodes play important roles in soil ecological processes such as nutrient cycling and plant growth24,25 and are sensitive enough to environmental changes to be used as bioindicators for ecotoxicological assessment of soil26.
In the past few years, DNA sequencing-based analyses of soil and sediment micro- and mesofaunal communities have revealed divergent lineages27,28,29, accompanied with large datasets of unknown sequences within known phyla that hint at a vast but poorly known diversity. Amongst Nematoda, for instance, it has been estimated that <4% of total species diversity is formally described30. This information gap is principally due to difficulty in studying these organisms because of their small size and hard-to-distinguish morphology at the species taxonomic level.
In this study, we focus on rainforests in the global biodiversity hotspot of the Xishuangbanna region of Yunnan, SW China. In Xishuangbanna, the original primary forest, as well as the derived logged forest, has been converted rapidly to rubber (Hevea brasiliensis Müll. Arg.) plantation. In 1992, rubber covered 87,000 ha, rising to 153,000 ha in 2002 and 424,000 ha in 201216. The impact of forest conversion to rubber plantation in southern China has already been explored with respect to soil nematodes, which is one aspect of micro- and mesofaunal diversity. Using traditional morphological methods, Xiao et al.31 compared nematode diversity in natural forests and rubber plantations, finding that conversion was associated with a decrease in both α- and β- diversity.
The present study goes further in encompassing the soil micro- and mesofauna and by including a larger number of sites than was sampled by Xiao et al.31. The present study also utilizes high-throughput sequencing interpreted with the help of biologically informative taxonomic resources covering alternate loci such as the 18S rRNA gene32. As such the technique is capable of recognizing cryptic biodiversity even within relatively well-studied groups (e.g., Nematoda), as well as undocumented biodiversity in relatively poorly studied groups (e.g., Tardigrada).
Our main hypotheses in this study were as follows:
-
(1)
We expected that forest conversion to rubber plantation would significantly alter the soil community composition, with each land-use type harboring a distinct soil metazoan community, with the forest conversion driving changes in soil chemistry which in turn modified the soil biota.
-
(2)
We predicted lower soil micro- and mesofaunal α- diversity in rubber plantation.
-
(3)
We also predicted lower β- diversity of micro- & mesofauna within rubber plantation compared to the native forest.
-
(4)
We predicted that the micro- & mesofaunal community assembly in both the native forest and derived rubber plantations would be strongly influenced by deterministic rather than stochastic/neutral processes, just as is the case for soil and sediment microbes from similar environments33,34,35.
Materials and Methods
Study location
The study was conducted around the Xishuangbanna Tropical Botanical Garden, XTBG (21°09′–22°33′N, 99°58′–101°34′E), in Xishuangbanna, Yunnan, China, concentrating on primary natural rainforests and adjacent monoculture rubber plantations. The mean annual temperature (MAT) and mean annual precipitation (MAP) were 21.7 °C and 1512 mm (1980–2008), respectively36.
Study area description
Xishuangbanna has a seasonal outer tropical climate, with hot, rainy summers and somewhat cooler and drier winters, which remain free of frost36. The tropical rainforests of Xishuangbanna are characterized by high species richness with up to 4180 species of vascular plants/2500 m2 plot and prevalence of epiphytes and epiphyllous mosses on the trees with the ubiquitous presence of woody lianas and strangling plants37. The tropical rainforest can be classified into two subtypes: tropical seasonal rain forest (in the lowlands; <900 m a.s.l., or meters above sea level) and tropical montane rain forest (900–1600 m a.s.l.)38, but with soil type differentiation within each of these (for soil types see Supplementary Table S1). For example, some areas of the lowland and montane forest are on limestone soils, with a distinctive plant community.
Field sampling
Sampling was carried out during the month of August 2013. Seven rainforest sampling sites were chosen within a 10 km radius of XTBG. Seven rubber plantation sites were chosen adjacent to each old-growth forest sampling site. In this study, there are fourteen sites in total (seven forests and seven rubber). At each sampling site, four quadrats (10 m × 10 m), were located >30 m apart along a linear transect. See SI Appendix Fig. S1 for sampling design; see Supplementary Table S1 for more details. Each 10 m × 10 m quadrat provided a single sample. This individual sample was the result of combining and mixing soil from 5 equal subsamples (each approximately 50 g) of soil from the top 10 cm, sampled using a small trowel marked to 10 cm depth starting down from the base of the litter layer. The five subsamples, one taken at each corner and one at the center, were gathered from each 0.01 ha area and mixed into a single soil sample bag39. Soil sample processing and DNA isolation were done one day after soil sampling. A list of the sampling sites and data on environmental parameters is provided as Supplementary Table S1. This study led to a total of 56 samples (7 sites × 4 biological replicate samples per site = 28 forest, and similarly 7 × 4 = 28 rubber plantation samples).
Soil micro- and mesofaunal DNA extraction and PCR amplification
To maximize capture of soil microfauna and mesofauna, 200 g of each soil sample was suspended in around 2 I distilled water (DW) and then gently sieved through a set of sieves.
For the combined micro- & mesofauna isolation under the Baermann funnel method, we used three different sieves in a vertical series. We placed a 2 mm sieve at the top and a 150 µm sieve below it. Below this was a 20 µm sieve (coarse to fine from top to bottom). 2 I of soil suspension was slowly poured onto the 2 mm sieve. We gently washed down all of the soil particles that would pass through the 2 mm sieve using more distilled water, so that stones, roots, and litter, etc., remained on the 2 mm sieve. We then collected accumulated particles – containing fauna - from both the remaining sieves below (150 µm & 20 µm) using a wash bottle to wash through finer particles. Mesofauna would be selectively accumulated on top of the 150 µm sieve, and microfauna on top of the 20 µm sieve. The accumulated material from each sieve was removed by spatula and placed together onto cotton gauze in a Baermann funnel for further extraction followed by sugar flotation40.
As well as removing stones, roots, etc., the 2 mm sieve ensured that the macrofauna (>2 mm) did not end up in the collected material. Smaller eukaryotes (e.g., smaller protists) and clays, along with water, would be able to pass through the 20 µm holes of the finest sieve.
In this manner, we could collect both the micro- & mesofauna from the soil while keeping the contamination from macrofauna to a minimum. This collected soil was then used for both Baermann funnel and sugar flotation extraction. The Baermann Funnel method is most often used to capture Nematoda, but will also capture most other types of motile micro- & mesofaunal populations, as it depends on organismal locomotion40,41.
After 24–36 hours, fauna that had moved down out of the soil-derived material, to the water at the bottom of the funnel were collected by draining the fluid into a Falcon tube. Tubes were then centrifuged for 10 min approximately at 5000 rpm (settling micro- & mesofaunal populations at the bottom), and the individual sediment pellet was collected from each for DNA extraction42. Less active/dead components remaining in the soil material within the funnel were then captured by sugar flotation and centrifugation using a 40% (w/v) sugar solution, to yield a pellet in each tube43. This combined procedure was intended to increase the efficiency of capture of a range of micro- and mesofauna by capturing both active (funnel) and less active or dead components (flotation).
The extracted pellets from both methods were combined before DNA extraction at the tropical forest ecology lab in XTBG, China, using the MoBio Power Soil DNA isolation kit (MoBio Laboratories, Carlsbad, CA) according to the manufacturer’s instructions.
The isolated DNA was stored at −80 °C, and was later used as a template to amplify a ~400 bp diagnostic region, defined by primers NF1 (C. elegans 1226–1250 bp position) and 18Sr2b (C. elegans 1567–1588 bp position) towards the 3′ end of the 18S rDNA with PCR reaction conditions as described by Porazinska et al.44. Detailed PCR procedure is described in SI Appendix, Section 1b. This primer pair was originally designed for nematodes, but we were able to test its suitability in coverage for the whole of subkingdom Metazoa. We used the Ecotaxaspecificity module (http://pythonhosted.org/OBITools/scripts/ecotaxspecificity.html) under the ecoPrimers platform (http://pythonhosted.org/OBITools/scripts/ecoPrimers.html) which evaluates barcode resolution at different taxonomic ranks45. For the primer pair tested, ecoPrimers calculates a taxonomic coverage, which is the number of amplified target species relative to the total number of target species in the input database. Taxonomic coverage rates of 100% (SI Appendix: Section 1c,d) across all metazoan sequences for phyla in the SILVA SSU database suggest that the barcode designed for nematodes is degenerate enough to be used as a general primer for subkingdom Metazoa. All metazoan sequences across all phyla in the SILVA SSU database are predicted to amplify with this primer pair (Complete details can be found in SI Appendix: Section 1c,d).
Data analysis
Sequence processing
Generated sequences were processed following Mothur’s 454 SOP46. All sequences shorter than 150 nucleotides, with homopolymers longer than eight nucleotides and all reads containing ambiguous base calls or incorrect primer sequences, were removed. Remaining sequences were aligned against the SILVA SSU eukaryotic aligned database. The sequences were further filtered to remove gaps generated after alignment, then preclustered using the Mothur implementation of pseudo-single linkage preclustering algorithm from Huse and colleagues47. Putative chimeric sequences were detected and removed via the Chimera Uchime algorithm contained within Mothur48 in de novo mode, which first splits sequences into groups and then checks each sequence within a group using the more abundant groups as a reference. Taxonomic classification of Metazoa was performed at a Bayesian cut-off of 55% with 1000 iterations against SILVA-ARB (database containing aligned 18S ribosomal RNA sequences with a minimum length of 1200 bases for Eukarya~ http://www.arb-silva.de/download/arb-files/; August 23, 2013). The remaining reads were then clustered using Mothur’s average algorithm. All samples were standardized by random subsampling to 1885 reads per sample (based on the smallest sample size by default), using the sub.sample command (http://www.mothur.org/wiki/Sub.sample), for calculating richness (OTUs at ≥99% sequence similarity), rarefaction curves, diversity and community compositional indices and matrices to be used later for the statistical analyses.
Statistical analyses
All data were analyzed using R 3.3.049 except for NMDS analysis which was performed in Primer-6 Software. To test for differences in richness (OTUs), abundance (read counts), diversity indices (Shannon, and Faith Phylogenetic diversity; PD) and soil physicochemical parameters i.e., TOC (Total Organic Carbon), TN (Total Nitrogen), pH, SX (Soil Texture), ST (Soil Temperature), Ele (Elevation), GSW (Gravimetric Soil Water) & AP (Available Phosphorus), (SI Appendix: Section 1a) between forest and rubber plantation, we used GLMM with a Poisson distribution in package lme4 & nlme and site as a random term (for integer dataset: OTUs) and glmmPQL with a Quasi-Poisson distribution in package MASS as this allows quasi distributions with cluster as a blocking term (for non-integer data-set: abundance, Shannon, and PD etc.)50. The functions glmm and lmer do not work with a quasi-Poisson distribution51.
We employed the methods of Jost52 to multiplicatively partition γ-diversity into independent α- and β- components for each management type. We used the “multipart” function in Vegan package and ran 1000 simulations to compare values against a null model. Following Jost52, we partitioned species richness using a multiplicative framework, in which γ = α × β. We assessed α- & β- diversity at three spatial scales, such that overall γ- diversity within each forest was expressed as:
where α.1 & β.1 denote species richness and β- diversity between sites, respectively; α.2 & β.2 denote species richness and β- diversity between forest and rubber plantation, respectively; α.3 & β.3, denote species richness and β- diversity within sites, respectively. We then assessed whether forest clearance and conversion to plantation had influenced the β- diversity, by partitioning γ- diversity, separately for the forest samples and samples from rubber plantation, respectively.
We performed Non-metric Multi Dimensional Scaling (NMDS) to explore patterns in phylogenetic community composition using both the unweighted UniFrac & β-MNTD (β-mean nearest taxon distance) distance matrix with Primer-6 software53. The unweighted UniFrac measures the distance between two communities by calculating the fraction of the branch length in a phylogenetic tree that leads to descendants in either, but not both, of the two communities54. β-MNTD is the mean phylogenetic distance to the closest relative in a paired community for all taxa and is sensitive to the changes of lineages close to the phylogenetic tips55. We used an analysis of similarity (ANOSIM) with 999 permutations to test if community composition was significantly different between the forest and samples from rubber plantation. To test whether the taxonomic composition results may have been influenced by pseudoreplication or spatial arrangement of study sites (Ramage et al. 2013), we used a Mantel test under the function mantel (999 permutations/analysis) in package Vegan in R56 to compare the taxonomic composition to geographic distance between pairs of transects within a land-use type.
We performed a redundancy analysis (RDA) based variation partitioning analysis57 to assess the relative effects of environmental and spatial variables on community composition. We used Hellinger transformed OTU abundance data as the response variable and two sets of explanatory variables which included environmental variables (pH, Ele, TOC, AP, GSW, SX, TN, and ST) and spatial variables (geographical co-ordinates for sampling sites), respectively. Before the RDA, the environmental variables with high variance inflation factor (VIF) >10 were eliminated to avoid collinearity among factors. The importance of environmental and spatial variables in explaining species composition was determined by an RDA analysis using Monte Carlo permutation tests (999 unrestricted permutations) followed by forward selection to remove the non-significant variables from each of the explanatory sets.
To further evaluate the relative importance of each environmental variable and spatial distance on the community phylogenetic dissimilarity, we used a multiple regression on matrices (MRM) approach58. Before applying MRM to the dataset, we looked for redundant environmental factors using the VARCLUS procedure59 in the Hmisc R package60 and removed TN as it was highly correlated with TOC (Spearman’s ρ2 = 0.80). In MRM, non-significant factors were removed sequentially, and the analysis was repeated until only significant factors were left in the model. Significance was tested by permutations (9999), and P-values of the two-tailed tests are reported for this analysis.
Phylogenetic analysis
Phylogenetic analyses were performed to answer whether the community assembly in both the native forest and derived rubber plantations is influenced by deterministic or neutral processes (stochastic). A maximum-likelihood tree was constructed using aligned 18S rRNA gene sequences of representative OTUs in FastTree61. To evaluate the phylogenetic signal, an environmental optimum for each OTU was calculated for each environmental variable as in Stegen et al.62. Between-OTU environmental optimum differences were calculated as Euclidean distances using optima for all the environmental variables. The correlation coefficients between differences in environmental optima and phylogenetic distances were measured using Mantel correlogram with 999 random permutations34,35.
To calculate the turnover in phylogenetic community composition, we calculated the βMNTD55,63 using ‘comdistnt’ function (abundance.weighted = TRUE) of Picante R package64. Further, to investigate the influence of deterministic and stochastic processes on community assembly of soil micro- and mesofauna, a null modeling approach was implemented34,35. First, we calculated the β-nearest taxon index or βNTI, which is the difference between observed βMNTD and the null distribution (999 times) of βMNTD measured in units of its standard deviation. Values of βNTI < −2 and >+2 indicate significantly less and more than expected phylogenetic turnover (deterministic assembly), respectively. However, comparisons falling within the null distribution of βMNTD (|βNTI|<+2) indicate that the observed difference in community composition is not the result of deterministic selection and are instead attributable to stochastic assembly63.
Results
The 18S rRNA gene metagenomic data (SI Appendix Fig. S2) gives details of both taxonomic identity and relative abundances of reads within each taxonomic category. It would be unrealistic to try to assign relative abundances of individuals to each taxonomic category since even closely related species of Metazoa from the same class or phylum can differ dramatically in size – and the samples pick up a great diversity of Metazoan taxa. For multicellular organisms, the number of cells and thus the number of copies of phylogenetic markers (such as 18S rRNA here) per individual are influenced by their size and their biomass. Consequently, under the premise that there was no technical bias, the number of reads obtained after PCR and NGS will probably be more closely correlated to their fractional biomass than abundance in terms of individuals.
Land-use and community composition
The 56 soil samples from forest and rubber plantation yielded 4127 micro- and mesofaunal OTUs at ≥99% similarity from a total of 314,743 quality sequences. Out of the 4127 OTUs (without subsampling), 449 OTUs were shared between both land-use types (SI Appendix Fig. S3). Forest samples yielded 1864 unique OTUs and samples from rubber plantation had 1814 unique OTUs. At a subsampling size of 1885 reads, the mean number of OTUs per sample was 96 ± 31 (SD), ranging from 49 to 180 OTUs per sample.
In total, and for each of the two land-use types separately, the most abundant phylum was Annelida with 66.4% of all reads, followed by Arthropoda (15.5%), Nematoda (8.9%), Platyhelminthes (6.6%), Rotifera (1.3%), Tardigrada (0.25%) and Gastrotricha (0.16%). Of these, only annelids were significantly more abundant (as a proportion of reads) in rubber plantation than in forest (glmm PQL; t = 2.85, ρ < 0.05; SI Appendix Fig. S2).
The NMDS results revealed that phylogenetic community composition of both land-use types, based on both unweighted UniFrac and β-MNTD, was driven by forest conversion to rubber plantation, with samples from rubber plantation forming separate clusters apart from forest samples (Fig. 1; ANOSIM results, R = 0.3, ρ = 0.001). These results show clearly that the micro- and mesofaunal community composition of the rubber plantation differed from the original native forest. We did not find any significant effect of distance on taxonomic composition, by testing for phylogenetic signal using Mantel correlograms of soil microbiome within land-use types for forest samples (Mantel test, P > 0.05). However, we did find a significant effect of distance on composition matrices for samples from rubber plantation (Mantel test, R = 0.22, P < 0.05). As the correlation was weak, most of the variation observed in community composition may be explicable by land use change with a small fraction as a result of pseudoreplication. According to Oksanen65, true treatment replication is sometimes impossible to achieve in a study, and thus its absence need not weaken the value of a study, provided that the results are judged properly.
NMDS of metazoan community composition using the unweighted UniFrac (left); (2D stress: 0.23, 3D: stress 0.17) and β-MNTD index (right); (2D stress: 0.22, 3D: stress 0.16) in relation to land-use type.
Testing for phylogenetic signal using Mantel correlograms showed significant correlations between differences in OTU environmental optima and OTU phylogenetic distances but only across relatively short phylogenetic distances (ρ < 0.05, SI Appendix Fig. S4). We examined the relationship between βNTI and land-use type to infer changes in the relative influences of deterministic and stochastic assembly processes on the micro- and mesofaunal community. The pairwise comparisons of βNTI values within each land-use indicated similar patterns (Fig. 2). In forest and rubber plantation, the mean of pairwise βNTI values fell between the null distribution of βMNTD (|βNTI| <+2) indicating that community assembly is primarily influenced by stochastic processes.
Patterns of βNTI across both land-use types. Horizontal dashed blue line indicate upper and lower significance thresholds at βNTI = +2 and −2, respectively.
Land-use and diversity
The rarefaction analysis showed that both richness and sample heterogeneity of OTUs were higher in the forest than in rubber plantation (Fig. 3). The α-diversity of 18S rRNA gene-based OTUs was significantly altered by forest conversion to rubber plantation. At a depth of 1885 reads, micro- and mesofaunal richness (OTUs) was significantly higher in the forest than in rubber plantation (GLMM; t = −2.28, p < 0.05). When measured separately for each of the three most abundant phyla (Table 1), only arthropods yielded significant results with OTU richness being higher in native forest (GLMM; t = −2.62, p < 0.01).
Rarefaction curve showing taxon richness of the operational taxonomic units (OTUs: ≥ 99% sequence similarity) of the 18S rRNA gene. OTUs average ± standard error (n = 28 for each forest and rubber plantation) at each rarefaction level is represented with triangles and squares respectively for the forest and samples from rubber plantation, respectively.
Other α-diversity indices also showed that diversity was significantly higher in native forests (glmm PQL results: Shannon; t = −4.7, p < 0.001, Faith’s PD; t = −3.5, p < 0.01), compared to the rubber plantations. Similar results were found when tested separately for each of the three major phyla present except for nematodes which did not yield any significant difference between the two land use types (Table 1).
Multiplicative diversity partitioning indicated that the native forest had significantly higher (p < 0.001) metazoan α- and β-diversity than rubber plantation at all levels in the hierarchy (Table 2). Multiplicative partitioning yielded similar results for analyses done separately for each of the three most abundant phyla (Table 2). Annelids, when taken separately, showed exactly the same patterns of diversity as observed for the total metazoan community. Nematodes and arthropods, however, showed a different pattern, with higher diversity in rubber plantation at some (but not all) hierarchal scales. For arthropods, α-diversity when measured between forest sites and for forest overall emerged as significantly higher than for rubber plantation. By contrast, beta diversity when calculated between rubber plantation sites, and for the total rubber plantation dataset, was significantly higher than for forest samples. For nematodes, at all levels in the taxonomic hierarchy, the diversity was higher in samples from rubber plantation - except for total beta diversity.
Variation partitioning & RDA results revealed that in forest samples, environmental variables (i.e., pH, TOC & GSW) and Ele explained 25.3% of the total variation (ρ < 0.005) of metazoan communities, of which 21.9% of the total variation (ρ < 0.005) could be explained by soil variables alone (Fig. 4; top). In isolation, spatial variables were insignificant and could not explain any of the variation observed (ρ > 0.5). Likewise, within the rubber plantation metazoan community, environmental variables (pH & ST) and Ele explained the largest proportion (9.9%) of the total variation (ρ < 0.01) (Fig. 4; bottom). Unlike the forest, around 3.3% of total metazoan community variation in the rubber plantation could be explained by spatial variables (ρ < 0.05), while abiotic and spatial variables together explained around 14.1% of the variation (ρ < 0.01). Similar results were found for each of the three most abundant phyla (SI Appendix Fig. S5).
Variation partition analysis explaining the percentage of variation explained by abiotic (environmental distance) and spatial variables (geographical distance) of forest community and rubber monoculture community based on 18SrRNA gene sequences; see Materials & Methods section. Unique fractions of each explanatory set were evaluated by 999 permutations. Variation explained by abiotic variables were significant for both land-use types (forest: P < 0.005; rubber plantation: P < 0.01) whereas spatial variables were able to explain a significant part of variation for forest only (forest: P < 0.05).
The MRM model explained a significant proportion of the variability in total phylogenetic community structure, with most of the environmental parameters in both land-use types (Table 3). Among the environmental variables measured, soil pH and TOC were correlated to UniFrac distance and β-MNTD for the total phylogenetic community for the forest whereas only soil pH was correlated to β-MNTD for the samples from rubber plantation. Spatial distance was significantly correlated to the unweighted UniFrac for both the forest and rubber plantation samples, but to β-MNTD only for samples from rubber plantation (Table 3).
When checked for differences between the two land-use types for major soil variables, a significant difference in TOC (glmm PQL; t = −2.8, p < 0.05) and a marginally significant difference in TN (glmm PQL; t = −2.0, p = 0.051), was present. Soil C: N ratio was also lower in samples from rubber plantation (p < 0.05).
Discussion
Impacts of conversion to plantation on community composition
Conversion of the forest to rubber plantation results in consistent changes in soil micro- & mesofaunal community composition. In comparison to rubber plantation, a larger proportion of variation for forest can be explained using abiotic parameters (Fig. 4, Variation Partitioning Results). Similarly, MRM results (Table 3) suggest that soil pH and TOC delimit the community composition to a certain extent, mostly for forest sites. It seems that for forest samples, environmental variables are a major force in structuring communities. There may be some analogy with a recent soil microfaunal study from Antarctica where microfaunal distribution was controlled by nutrients such as pH, organic matter and soil moisture66.
The phylogenetic signal55,67, detected across relatively short phylogenetic distances, indicates that closely related micro- and mesofaunal OTUs tend to occupy similar niches (ρ < 0.05, SI Appendix Fig. S4). Similar patterns have been observed in other studies of both prokaryotic and eukaryotic microbial communities[62,68,69. From phylogenetic null modeling34 we found a strong impact of stochastic processes on the assembly of micro- and mesofaunal communities in soils of both forest and rubber plantation, suggesting that despite its other evident effects, the shift to a highly altered rubber plantation environment has not altered the role of stochasticity in community structure.
According to other studies, conversion from forest to rubber plantation is also accompanied by a progressive increase in soil bulk density and continuous decrease in pore space (soil compaction) in the 0–10 cm soil layer70,71, which may decrease the niche availability for many small soil animals. There are also significant changes in the other soil properties70,71, which may affect the microbial community which is, in turn, grazed upon by many soil metazoans. Physical disturbance in rubber plantation sites at XTBG also results from the prevalent management practices, which might suppress metazoan abundances. Reports have shown positive effects of limiting physical disturbance on metazoan abundance, especially the nematode fauna72.
Reduction in soil carbon on conversion to rubber plantation may also be an important factor. Soil carbon provides a resource for fungi and bacteria, on which many soil micro- and mesofaunal community feeds, and thus changes in this food source could adversely affect their diversity. Also possibly important in producing lower soil micro- and mesofaunal diversity is the dominance of a non-native tree species (rubber) which fewer soil micro- and mesofauna may be adapted to feeding off.
Considering the phyla individually, annelids were significantly more abundant in the rubber plantation (p < 0.05, Table 1). We did not find any indication of invasive earthworm species such as Pontoscolex corethrurus73, and most reads belonged to highly diverse small annelid families (Enchytraeidae or potworms, Naididae & Tubificidae). Arthropoda, which comprises the vast majority of the described tropical rainforest fauna and is estimated in total at around 2.5–3.7 million species74,75 was represented by more OTUs in the forest (p < 0.01, Table 1). Soil calcium concentration is a limiting factor for terrestrial ostracods (Crustacea)76 and millipedes (Diplopoda)77.
Nematoda showed no significant changes in relative abundance with land-use change, although the family level feeding guild structure of the nematode community showed striking differences in relation to the land-use type (SI Appendix Fig. S6). An increase in Bacteria Feeding (BF) along with Fungi Feeding (FF) guilds in rubber plantation could be because the Omnivore Predator (OP) guild are sensitive to land use change and need more time to establish compared to more rapidly growing BF and FF nematodes78,79. The Plant-Feeding (PF) guild was significantly reduced in the rubber plantation soils, which is unsurprising as their abundance has been found to be directly correlated to plant community richness and soil C: N ratio80.
Impacts of plantations on alpha-diversity
We predicted a substantial impact of forest conversion on soil micro- and mesofaunal α-diversity, and the results of this study suggest that indeed the conversion of the tropical forest of southern Yunnan to rubber plantation has resulted in a consistent decrease in α-diversity for soil micro- and mesofaunal community, except for nematodes, when these are considered separately. Possible reasons why α-diversity is lower in rubber plantations than in forest environments include: lack of small-scale heterogeneity in terms of various sizes/types of trees and shrubs, lower diversity of plants giving fewer organic substrates for niche differentiation in feeding, and a relative lack of carbon in litter and coarse debris flux resulting in fewer niches81,82.
Pesticides are generally used on rubber plantations, for example, to kill weeds, and are a possible factor producing the observed differences in soil metazoan diversity, as they are toxic to non-target species including soil animals83,84. A prevalent management practice in rubber plantations is repeated application of glyphosate, (alone or in a mixture with other pesticides)31 which increases the presence of glyphosate residues in soils85,86,87,88 and can be detected in top soils even after two years since the last spraying86. Glyphosate is reportedly a potent microbiocide89,90 and has been reported to severely affect the casting activities and reproduction of earthworms91.
Another conventional control practice used for powdery mildew and anthracnose diseases of rubber plantations is annual spraying of sulfur powder during the leaf expansion period of the rubber tree. This application over a period of time has been reported to reduce soil pH92, and it could be one of the reasons behind the lower pH observed in our samples from rubber plantation. However, in a study Li et al.92 sulfur spraying did not significantly alter the soil microbial community composition and function over the long term (48 years) some specific microorganisms, such as acidophilic bacteria, in the soil can use sulfur as an energy source and oxidize sulfur to SO42− accompanied with a decrease in soil pH which will persist over the years93. Changes in soil physicochemical characteristics and microbial community with the use of pesticides - as shown by these two examples - may eventually have effects on the micro- and mesofaunal populations of the rubber plantation soils.
Ecosystem engineers, such as earthworms, have been found to show a drastic decrease in abundance under rubber monoculture (possibly due to decline in soil exchangeable Ca94 and glyphosate herbicide91 in soil from rubber plantations). This may influence the diversity of other soil animals by regulating the availability, diversity, and spatial distribution of resources available to them95,96, and may help to explain the lower α-diversity in samples from rubber plantation.
Impact of conversion to plantations on beta-diversity
As anticipated, and consistent with earlier studies of larger organisms, a decrease in micro- and mesofaunal β-diversity with the conversion from forest to rubber plantation was observed97,98 except for arthropods and nematodes. Still, total β-diversity for nematodes in samples from rubber plantation was marginally lower than forest samples (Table 2).
The uncoupling of α- and β-diversity after ecosystem conversion that is observed here for arthropods is generally not seen in examples from plants and larger animals98: conversion usually results in decreases in both α- and β-diversity in parallel as observed above for the total population. Although rarely found in higher organisms99 the converse situation – a decrease in β-diversity along with an increase in α-diversity in response to human disturbances has been reported elsewhere100,101. Similar uncoupling between α- and β-diversity has also been previously reported for bacterial communities, where the natural vegetation was either converted to agriculture20 or plantation21.
Various ecological mechanisms could be behind the greater arthropod β-diversity we observed in rubber plantations. With a random loss of the species present in the original rainforest (associated here with deforestation and initial and continuous human disturbance) and limited dispersal, species richness at the α-diversity level will be low and few species will be shared between disturbed plots. This will lead to an increased β-diversity between rubber plantation plots. Apart from the effects of dispersal limitation102,103, the increased arthropod β-diversity in rubber plantations might be a consequence of some unknown aspect of habitat heterogeneity that leads to species sorting by environmental selection103,104.
The diversity of a plant community is likely to be one of the major environmental factors that influences the diversity of the soil micro- and mesofaunal community, through shaping the resource availability to the soil community105. Although soil micro- and mesofauna need very small patch sizes and comparatively smaller sources of energy and nutrients to maintain their diversity, soil animal diversity is expected to increase with greater plant diversity due to enhanced opportunities for niche differentiation with respect to habitat use and sources of energy and nutrients106,107,108. However, the patterns are not consistent, and it has been often shown that the effect of plant species identity is greater than that of plant species richness107,109,110,111. The effect of plants on soil animal diversity is generally regulated in two different ways, i.e., availability of a resource and diversity of a resource107,112. Plants not only play a role in the availability of metabolic resources, but also have effects on other ecological factors that further shape soil habitats and niche space, including the presence and abundance of ecosystem engineers95,96, microclimatic conditions, and general soil properties.
Conclusion
It is clear that conversion of forest to rubber plantation involves a major turnover of lower level taxa (expressed as OTUs) of micro- and mesofauna, and an overall loss of diversity. Hypothetically, this loss of micro- and mesofaunal diversity could result in lower soil and ecosystem resilience, by analogy with other systems where removal of diversity has resulted in decreased stability112. It is also relevant to consider whether the loss of the original rainforest soil micro- and mesofauna might make it more difficult to re-establish tropical rainforest on former rubber plantations, as these organisms have important and specialized roles in nutrient cycling in tropical forests. Such questions should be investigated in further studies of this and other analogous systems.
Data Availability
DNA sequences: All data are available from Figshare (Metadata: https://doi.org/10.6084/m9.figshare.3506822.v2; Sequence data: https://doi.org/10.6084/m9.figshare.7842029). Datasets and metadata are published under the CCo license. R scripts: available upon request; please email singhdharmesh24@gmail.com for R scripts derived from freely available R packages online: see material and methods for more details. Site information such sample locations with coordinates, vegetation types and other physiochemical properties of the soils used in this study: supplied as a supporting document with the manuscript; see Supplementary Table 1 for more details.
References
Dirzo, R. & Raven, P. H. Global state of biodiversity and loss. Annu. Rev. Env. Resour. 28, 137–167 (2003).
Wright, S. J. Tropical forests in a changing environment. Trends Ecol. Evol. 20, 553–560 (2005).
Gibson, L. et al. Primary forests are irreplaceable for sustaining tropical biodiversity. Nature 478, 378 (2011).
Gibbs, H. K. et al. Tropical forests were the primary sources of new agricultural land in the 1980s and 1990s. P. Natl. Acad. Sci. USA 107, 16732–16737 (2010).
Sodhi, N. S., Koh, L. P., Brook, B. W. & Ng, P. K. L. Southeast Asian biodiversity: an impending disaster. Trends Ecol. Evol. 19, 654–660 (2004).
FAO. Forests for improved nutrition and food security. Rome. www.fao.org/forestry/27976-02c09ef000fa99932eefa37c22f76a055.pdf (2010).
Li, Z. & Fox, J. M. Mapping rubber tree growth in mainland Southeast Asia using time-series MODIS 250 m NDVI and statistical data. Appl. Geogr. 32, 420–432 (2012).
Danielsen, F. & Heegaard, M. In Management of Tropical Forests: Towards an Integrated Perspective (ed. Øyvind, Sandbukt) 73–92 (Centre for Development and the Environment, University of Oslo, 1995).
Aratrakorn, S., Thunhikorn, S. & Donald, P. F. Changes in bird communities following conversion of lowland forest to oil palm and rubber plantations in southern Thailand. Bird Conserv. Int. 16, 71–82 (2006).
Wu, Z.-L., Liu, H.-M. & Liu, L.-Y. Rubber cultivation and sustainable development in Xishuangbanna, China. Int. J. Sust. Dev. World 8, 337–345 (2001).
Zhang, M., Fu, X. H., Feng, W. T. & Zou, X. Soil organic carbon in pure rubber and tea-rubber plantations in South-western China. Trop. Ecol. 48, 201–207 (2007).
Ziegler, A. D. et al. Carbon outcomes of major land-cover transitions in SE Asia: great uncertainties and REDD plus policy implications. Global Change Biol. 18, 3087–3099 (2012).
Li, H. M., Ma, Y. X., Liu, W. J. & Liu, W. J. Clearance and fragmentation of tropical rain forest in Xishuangbanna, SW, China. Biodivers. Conserv. 18, 3421–3440 (2009).
Guardiola-Claramonte, M. et al. Local hydrologic effects of introducing non-native vegetation in a tropical catchment. Ecohydrology 1, 13–22 (2008).
Tan, Z. H. et al. Rubber plantations act as water pumps in tropical China. Geophys. Res. Lett. 38 (2011).
Xu, J. C., Grumbine, R. E. & Beckschafer, P. Landscape transformation through the use of ecological and socioeconomic indicators in Xishuangbanna, Southwest China, Mekong Region. Ecol. Indic. 36, 749–756 (2014).
McGrath, D. A., Smith, C. K., Gholz, H. L. & Oliveira, F. D. Effects of land-use change on soil nutrient dynamics in Amazonia. Ecosystems 4, 625–645 (2001).
Murty, D., Kirschbaum, M. U. F., McMurtrie, R. E. & McGilvray, A. Does conversion of forest to agricultural land change soil carbon and nitrogen? A review of the literature. Global Change Biol. 8 (2002).
Stocking, M. A. Tropical soils and food security: The next 50 years. Science 302, 1356–1359 (2003).
Rodrigues, J. L. M. et al. Conversion of the Amazon rainforest to agriculture results in biotic homogenization of soil bacterial communities. P. Natl. Acad. Sci. USA 110, 988–993 (2013).
Lee-Cruz, L., Edwards, D. P., Tripathi, B. M. & Adams, J. M. Impact of Logging and Forest Conversion to Oil Palm Plantations on Soil Bacterial Communities in Borneo. Appl. Environ. Microb. 79, 7290–7297 (2013).
Lan, G. Y. et al. Change in Soil Microbial Community Compositions and Diversity Following the Conversion of Tropical Forest to Rubber Plantations in Xishuangbanna, Southwest China. Trop. Conserv. Sci. 10, 1–14 (2017).
Barrios, E. Soil biota, ecosystem services and land productivity. Ecol. Econ. 64, 269–285 (2007).
Danovaro, R. et al. Exponential decline of deep-sea ecosystem functioning linked to benthic biodiversity loss. Curr. Biol. 18, 1–8 (2008).
Wardle, D. A. The influence of biotic interactions on soil biodiversity. Ecol. Lett. 9, 870–886 (2006).
Neher, D. A. Role of nematodes in soil health and their use as indicators. J. Nematol. 33, 161–168 (2001).
Behnke, A. et al. Microeukaryote community patterns along an O-2/H2S gradient in a supersulfidic anoxic Fjord (Framvaren, Norway). Appl. Environ. Microb. 72, 3626–3636 (2006).
Richards, T. A. & Bass, D. Molecular screening of free-living microbial eukaryotes: diversity and distribution using a meta-analysis. Curr. Opin. Microbiol. 8, 240–252 (2005).
Groisillier, A., Massana, R., Valentin, K., Vaulotl, D. & Guilloul, L. Genetic diversity and habitats of two enigmatic marine alveolate lineages. Aquat. Microb. Ecol. 42, 277–291 (2006).
Creer, S. et al. Ultrasequencing of the meiofaunal biosphere: practice, pitfalls and promises. Mol. Ecol. 19, 4–20 (2010).
Xiao, H. F. et al. Intensive rubber cultivation degrades soil nematode communities in Xishuangbanna, southwest China. Soil Biol. & Biochem. 76, 161–169 (2014).
Bik, H. M. et al. Sequencing our way towards understanding global eukaryotic biodiversity. Trends Ecol. Evol. 27, 233–243 (2012).
Ofiteru, I. D. et al. Combined niche and neutral effects in a microbial wastewater treatment community. P. Natl. Acad. Sci. USA 107, 15345–15350 (2010).
Stegen, J. C. et al. Quantifying community assembly processes and identifying features that impose them. Isme J. 7, 2069–2079 (2013).
Wang, J. J. et al. Phylogenetic beta diversity in bacterial assemblages across ecosystems: deterministic versus stochastic processes. Isme J. 7, 1310–1321 (2013).
Li, Y. W., Deng, X. B., Cao, M., Lei, Y. B. & Xia, Y. J. Soil restoration potential with corridor replanting engineering in the monoculture rubber plantations of Southwest China. Ecol. Eng. 51, 169–177 (2013).
Zhu, H. The tropical rainforest vegetation in Xishuangbanna. Chin. Geogr. Sci 2, 64–73 (1992).
Zhu, H., Cao, M. & Hu, H. B. Geological history, flora, and vegetation of Xishuangbanna, southern Yunnan, China. Biotropica 38, 310–317 (2006).
Fulthorpe, R. R., Roesch, L. F. W., Riva, A. & Triplett, E. W. Distantly sampled soils carry few species in common. Isme J. 2, 901–910 (2008).
Baermann, G. Eine einfache Methode zur Auffindung von Ancyclostomum (Nematode) Larven in Erdproben. Nederlands Tijdscrift Voor Geneeskunde. 57, 131–137 (1917).
Whitehead, A. G. & Hemming, J. R. A Comparison of Some Quantitative Methods of Extracting Small Vermiform Nematodes from Soil. Ann. Appl. Biol. 55, 25–38 (1965).
Viglierchio, D. R. & Schmitt, R. V. On the Methodology of Nematode Extraction from Field Samples - Baermann Funnel Modifications. J. Nematol. 15, 438–444 (1983).
Jenkins, W. R. A rapid centrifugal-flotation technique for separating nematodes from soil. Plant Dis. Rep. 48, 692 (1964).
Porazinska, D. L. et al. Evaluating high-throughput sequencing as a method for metagenomic analysis of nematode diversity. Mol. Ecol. Resour. 9, 1439–1450 (2009).
Riaz, T. et al. EcoPrimers: inference of new DNA barcode markers from whole genome sequence analysis. Nucleic Acids. Res. 39, e145, https://doi.org/10.1093/nar/gkr732 (2011).
Schloss, P. D., Gevers, D. & Westcott, S. L. Reducing the Effects of PCR Amplification and Sequencing Artifacts on 16S rRNA-Based Studies. Plos One 6, e27310, https://doi.org/10.1371/journal.pone.0027310 (2011).
Huse, S. M., Welch, D. M., Morrison, H. G. & Sogin, M. L. Ironing out the wrinkles in the rare biosphere through improved OTU clustering. Environ. Microbiol. 12, 1889–1898 (2010).
Edgar, R. C., Haas, B. J., Clemente, J. C., Quince, C. & Knight, R. UCHIME improves sensitivity and speed of chimera detection. Bioinformatics 27, 2194–2200 (2011).
R: A language and environment for statistical computing (R Foundation for Statistical Computing, Vienna, Austria, 2016).
Zuur, A. F., Ieno, E. N., Walker, N. J., Saveliev, A. A. & Smith, G. M. Mixed effects models and extensions in ecology with R. (Springer, New York, 2009).
Bates, D., Machler, M., Bolker, B. M. & Walker, S. C. Fitting Linear Mixed-Effects Models Using lme4. J. Stat. Softw. 67, 1–48 (2015).
Jost, L. Partitioning diversity into independent alpha and beta components. Ecology 88, 2427–2439 (2007).
Clarke, K. R. & Gorley, R. N. Primer v6: User Manual/Tutorials (Primer-E Ltd.: Plymouth, UK., 2006).
Lozupone, C. & Knight, R. UniFrac: a new phylogenetic method for comparing microbial communities. Appl. Environ. Microb. 71, 8228–8235 (2005).
Fine, P. V. & Kembel, S. W. Phylogenetic community structure and phylogenetic turnover across space and edaphic gradients in western Amazonian tree communities. Ecography 34, 552–565, https://doi.org/10.1111/j.1600-0587.2010.06548.x (2011).
Oksanen, J. et al. Package ‘vegan’. R Packag ver 254, 20–28 (2013).
Peres-Neto, P. R., Legendre, P., Dray, S. & Borcard, D. Variation partitioning of species data matrices: Estimation and comparison of fractions. Ecology 87, 2614–2625 (2006).
Legendre, P., Lapointe, F. J. & Casgrain, P. Modeling brain evolution from behavior: A permutational regression approach. Evolution 48, 1487–1499 (1994).
Sarle, W. S. The VARCLUS Procedure. SAS/STAT User’s Guide. 4th edn, (Cary NC: SAS Institute, Inc., 1990).
Harrell, F. E. & Dupont, C. Hmisc: Harrell miscellaneous. R package version 3.9-3. Available at http://CRAN.R-project.org/package=Hmisc (2012).
Price, M. N., Dehal, P. S. & Arkin, A. P. FastTree 2-Approximately Maximum-Likelihood Trees for Large Alignments. Plos One 5, e9490, https://doi.org/10.1371/Journal.Pone.0009490 (2010).
Stegen, J. C., Lin, X., Konopka, A. E. & Fredrickson, J. K. Stochastic and deterministic assembly processes in subsurface microbial communities. Isme J. 6, 1653–1664 (2012).
Kembel, S. W. et al. Picante: R tools for integrating phylogenies and ecology. Bioinformatics 26, 1463–1464 (2010).
Oksanen, L. The devil lies in details: reply to Stuart Hurlbert. Oikos 104, 598–605 (2004).
Smykla, J. et al. Geochemical and biotic factors influencing the diversity and distribution of soil microfauna across ice-free coastal habitats in Victoria Land, Antarctica. Soil Biol. & Biochem. 116, 265–276 (2018).
Cavender-Bares, J., Kozak, K. H., Fine, P. V. A. & Kembel, S. W. The merging of community ecology and phylogenetic biology. Ecol. Lett. 12, 693–715 (2009).
Moroenyane, I., Chimphango, S. B. M., Wang, J., Kim, H. K. & Adams, J. M. Deterministic assembly processes govern bacterial community structure in the Fynbos, South Africa. Microb. Ecol. 72, 313–323 (2016).
Tripathi, B. M. et al. Soil pH mediates the balance between stochastic and deterministic assembly of bacteria. Isme J. 12, 1072–1083 (2018).
Dawoe, E. K., Quashie-Sam, J. S. & Oppong, S. K. Effect of land-use conversion from forest to cocoa agroforest on soil characteristics and quality of a Ferric Lixisol in lowland humid Ghana. Agroforest. Syst. 88, 87–99 (2014).
Li, H. M., Ma, Y. X., Liu, W. J. & Liu, W. J. Soil Changes Induced by Rubber and Tea Plantation Establishment: Comparison with Tropical Rain Forest Soil in Xishuangbanna, SW China. Environ Manage 50, 837–848 (2012).
Nakamoto, T., Yamagishi, J. & Miura, E. Effect of reduced tillage on weeds and soil organisms in winter wheat and summer maize cropping on Humic Andosols in Central Japan. Soil Till. Res. 85 (2006).
Gonzalez, G., Huang, C. Y., Zou, X. M. & Rodriguez, C. Earthworm invasions in the tropics. Biol. Invasions 8, 1247–1256 (2006).
Hamilton, A. J. et al. Quantifying Uncertainty in Estimation of Tropical Arthropod Species Richness. Am. Nat. 176, 90–95 (2010).
Basset, Y. et al. Arthropod Diversity in a Tropical Forest. Science 338, 1481–1484 (2012).
Ohta, T., Niwa, S., Agetsuma, N. & Hiura, T. Calcium concentration in leaf litter alters the community composition of soil invertebrates in warm-temperate forests. Pedobiologia 57, 257–262 (2014).
Golovatch, S. I. & Kime, R. D. Millipede (Diplopoda) distributions: A review. Soil Organisms 81, 565–597 (2009).
Ferris, H., Bongers, T. & de Goede, R. G. M. A framework for soil food web diagnostics: extension of the nematode faunal analysis concept. Appl. Soil. Ecol. 18, 13–29 (2001).
Liang, W. J. et al. Nematode faunal response to long-term application of nitrogen fertilizer and organic manure in Northeast China. Soil Biol. & Biochem. 41, 883–890 (2009).
Cortois, R. et al. Possible mechanisms underlying abundance and diversity responses of nematode communities to plant diversity. Ecosphere 8, e01719, https://doi.org/10.1002/ecs2.1719 (2017).
Zak, D. R., Holmes, W. E., White, D. C., Peacock, A. D. & Tilman, D. Plant diversity, soil microbial communities, and ecosystem function: Are there any links. Ecology 84, 2042–2050 (2003).
Bezemer, T. M. et al. Divergent composition but similar function of soil food webs of individual plants: plant species and community effects. Ecology 91, 3027–3036 (2010).
Relyea, R. A. The impact of insecticides and herbicides on the biodiversity and productivity of aquatic communities. Ecol. Appl. 15, 618–627 (2005).
Rahman, P. M., Varma, R. V. & Sileshi, G. W. Abundance and diversity of soil invertebrates in annual crops, agroforestry and forest ecosystems in the Nilgiri biosphere reserve of Western Ghats, India. Agroforest. Syst. 85, 165–177 (2012).
Al-Rajab, A. J., Amellal, S. & Schiavon, M. Sorption and leaching of (14)C-glyphosate in agricultural soils. Agron. Sustain. Dev. 28, 419–428 (2008).
Bergstrom, L., Borjesson, E. & Stenstrom, J. Laboratory and Lysimeter Studies of Glyphosate and Aminomethylphosphonic Acid in a Sand and a Clay Soil. J. Environ. Qual. 40, 98–108 (2011).
Borggaard, O. K. & Gimsing, A. L. Fate of glyphosate in soil and the possibility of leaching to ground and surface waters: a review. Pest. Manag. Sci. 64, 441–456 (2008).
Simonsen, L., Fomsgaard, I. S., Svensmark, B. & Spliid, N. H. Fate and availability of glyphosate and AMPA in agricultural soil. J. Environ. Sci. Heal. B. 43, 365–375 (2008).
Zobiole, L. H. S., Kremer, R. J., Oliveira, R. S. & Constantin, J. Glyphosate affects micro-organisms in rhizospheres of glyphosate-resistant soybeans. J. Appl. Microbiol. 110, 118–127 (2011).
Druille, M., Cabello, M. N., Omacini, M. & Golluscio, R. A. Glyphosate reduces spore viability and root colonization of arbuscular mycorrhizal fungi. Appl. Soil. Ecol. 64, 99–103 (2013).
Gaupp-Berghausen, M., Hofer, M., Rewald, B. & Zaller, J. G. Glyphosate-based herbicides reduce the activity and reproduction of earthworms and lead to increased soil nutrient concentrations. Sci. Rep.-UK 5, 12886, https://doi.org/10.1038/Srep12886 (2015).
Li, Y. W. et al. Accumulated Impacts of Sulfur Spraying on Soil Nutrient Availability and Microbial Biomass in Rubber Plantations. Clean-Soil Air Water 44, 1001–1010 (2016).
Wang, Y. P. et al. Effect of sulphur on soil Cu/Zn availability and microbial community composition. J. Hazard. Mater. 159, 385–389 (2008).
Aweto, A. O. Physical and Nutrient Status of Soils under Rubber (Hevea-Brasiliensis) of Different Ages in Southwestern Nigeria. Agr. Syst. 23, 63–72 (1987).
Lavelle, P. et al. Soil function in a changing world: the role of invertebrate ecosystem engineers. Eur. J. Soil Biol. 33, 159–193 (1997).
Eisenhauer, N. The action of an animal ecosystem engineer: Identification of the main mechanisms of earthworm impacts on soil microarthropods. Pedobiologia 53, 343–352 (2010).
Philpott, S. M. et al. Biodiversity Loss in Latin American Coffee Landscapes: Review of the Evidence on Ants, Birds, and Trees. Conserv. Biol. 22, 1093–1105 (2008).
Bierregaard, R. O. Jr., Gascon, C., Lovejoy, T. E. & Mesquita, R. C. G. 496 (Yale University Press, New Haven & London, 2001).
Olden, J. D. & Poff, N. L. Toward a mechanistic understanding and prediction of biotic homogenization. Am. Nat. 162, 442–460 (2003).
Hewitt, J., Thrush, S., Lohrer, A. & Townsend, M. A latent threat to biodiversity: consequences of small-scale heterogeneity loss. Biodivers. Conserv. 19, 1315–1323 (2010).
Smart, S. M. et al. Biotic homogenization and changes in species diversity across human-modified ecosystems. P. R. Soc. B. 273, 2659–2665 (2006).
Chase, J. M. & Myers, J. A. Disentangling the importance of ecological niches from stochastic processes across scales. Philos. T. R. Soc. B. 366, 2351–2363 (2011).
Hanson, C. A., Fuhrman, J. A., Horner-Devine, M. C. & Martiny, J. B. H. Beyond biogeographic patterns: processes shaping the microbial landscape. Nat. Rev. Microbiol. 10, 497–506 (2012).
Kallimanis, A. S. et al. How does habitat diversity affect the species-area relationship? Global Ecol. Biogeogr. 17, 532–538 (2008).
Sylvain, Z. A. & Wall, D. H. Linking Soil Biodiversity and Vegetation: Implications for a Changing Planet. Am. J. Bot. 98, 517–527 (2011).
Anderson, J. M. Inter-Habitat and Intra-Habitat Relationships between Woodland Cryptostigmata Species-Diversity and Diversity of Soil and Litter Microhabitats. Oecologia 32, 341–348 (1978).
Wardle, D. A., Yeates, G. W., Barker, G. M. & Bonner, K. I. The influence of plant litter diversity on decomposer abundance and diversity. Soil Biol. & Biochem. 38, 1052–1062 (2006).
Coleman, D. C. From peds to paradoxes: Linkages between soil biota and their influences on ecological processes. Soil Biol. & Biochem. 40, 271–289 (2008).
Wardle, D. A., Yeates, G. W., Williamson, W. & Bonner, K. I. The response of a three trophic level soil food web to the identity and diversity of plant species and functional groups. Oikos 102, 45–56 (2003).
De Deyn, G. B., Raaijmakers, C. E., van Ruijven, J., Berendse, F. & van der Putten, W. H. Plant species identity and diversity effects on different trophic levels of nematodes in the soil food web. Oikos 106, 576–586 (2004).
Eissfeller, V., Langenbruch, C., Jacob, A., Maraun, M. & Scheu, S. Tree identity surpasses tree diversity in affecting the community structure of oribatid mites (Oribatida) of deciduous temperate forests. Soil Biol. & Biochem. 63, 154–162 (2013).
Hooper, D. U. et al. Interactions between aboveground and belowground biodiversity in terrestrial ecosystems: Patterns, mechanisms, and feedbacks. Bioscience 50, 1049–1061 (2000).
Strecker, T., Mace, O. G., Scheu, S. & Eisenhauer, N. Functional composition of plant communities determines the spatial and temporal stability of soil microbial properties in a long-term plant diversity experiment. Oikos 125, 1743–1754 (2016).
Acknowledgements
We thank the Chinese Academy of Sciences and Xishuangbanna Tropical Botanical Garden for hosting J.M.A. and D.S. for their visit, in providing important laboratory & logistical support. D.S. would like to thank Director, NEERI for providing constant laboratory support for the research and manuscript work. Plagiarism has been checked using iThenticate software at CSIR-NEERI, Nagpur and the KRC number is CSIR-NEERI/KRC/2018/MARCH/EBGD/1.
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D.S. Field sampling and design, fieldwork, extractions of DNA, bioinformatics and statistical analyses, interpretation of results in ecological terms, writing of paper; F.S. design of field sampling scheme and provision of site floristic data; Y.S.J. bioinformatics support; K.W.T. advice on field sampling scheme and choice of sites; X.Y. Advice of soil chemical and physical analysis procedures; J.W. Soil analyses and collation of data; D.K. writing of paper; D.P. Advice on bioinformatics strategies; J.M.A. Initial study concept and broad design, participation in fieldwork, interpretation of data in ecological terms and writing of paper.
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Singh, D., Slik, J.W.F., Jeon, YS. et al. Tropical forest conversion to rubber plantation affects soil micro- & mesofaunal community & diversity. Sci Rep 9, 5893 (2019). https://doi.org/10.1038/s41598-019-42333-4
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DOI: https://doi.org/10.1038/s41598-019-42333-4
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