Seasonal & annual patterns

Biological monitoring at a single point in time is typically inadequate to describe total biodiversity or to explore changes in diversity over time. Collecting multiple time-stamped samples reveals greater total (gamma) biodiversity and allows measurement of beta diversity as a temporal change. For each assay, OTU biodiversity analysis involved both counting of the number of discrete OTUs—a measure hereafter referred to as “Richness”—and the presence/absence composition of the OTUs—referred to as “Assemblage”. OTUs from each assay were examined independently so that comparisons were all made within the same experimental frameworks.

There are varying approaches for presenting eDNA metabarcoding data in terms of Assemblage and Richness. Some authors rarefy their data to normalise results for differing sequencing depth among libraries. We made the decision not to do this because sequence number and OTU accumulation curves had plateaued for each sample indicating that we had sampled the majority of the OTUs in each case (For example; S1 Fig), Pearson’s correlation tests showed there was no evidence to suggest a significant correlation between the number of sequences (i.e. sequencing depth) and the number of OTUs obtained for the 18S and 16S assays (S2 Fig). However, sequencing depth and number of OTUs (Richness) were moderately correlated (R²<0.522) for the COI assays (S2 Fig). Nevertheless, as sequencing depth variation is spread evenly across the samples (S2 Fig), we consider it unlikely that Richness or Assemblage estimates are compromised by this data treatment.

Our initial analyses of eDNA (Table 1) demonstrated strong seasonality in the Assemblage from those assays that predominately detect meroplankton, including fish, molluscs and cnidarians. This seasonality was not reflected in Richness, with the exception of the Fish assay. A pairwise analysis between seasons (S8 Table) indicated that the most consistent differences in Assemblage were detected between summer:winter, followed by spring:winter and spring:autumn. The least significant Assemblage changes were identified by the assays that predominantly detect holoplankton e.g. the Copepod assays. These detected no significant changes (after post-hoc correction) between winter:autumn, and summer:spring. These results provide a detailed example for multi-year marine biodiversity surveys based on eDNA.

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Table 1. Significance of changes to the Operational Taxonomic Unit (OTU) Richness (a count of the number of OTUs in each sample) & Assemblage (the OTUs making up each sample) during different time periods within the five-year eDNA data including F statistics (F)—PERMANOVA+ [42].

https://doi.org/10.1371/journal.pgen.1007943.t001

The Fish assay revealed strong seasonality in both Richness and Assemblage (Fig 2). A pairwise analysis showed significant changes between all seasons for the Assemblage as well as Richness (S8 Table), the two exceptions were for Richness between the adjacent seasons summer:spring and winter:autumn. Most fish are only present in the zooplankton community after broadcast spawning their eggs or during their pelagic larval phase, so these seasonal changes make biological sense [24]. Seasonal fluctuations have been previously observed in fish using eDNA extracted from water [43, 44]. However, these studies were limited to durations of six and twelve months respectively. The current study provides additional and enduring evidence for the ability of eDNA to detect of seasonality over an extended period (5 years) and further incorporates a much broader range of biodiversity.

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Fig 2.

Seasonality in eDNA revealed by the Fish assay: (A) Number of Operational Taxonomic Units (OTUs) at each time point (Richness; p < 0.001) and (B) Diversity of OTUs as exhibited by a non-parametric multivariate analysis (Assemblage; k = 3, stress = 0.15, p < 0.001), the coloured lines extrude from the centroids of each season towards the variation of Assemblage in each sample.

https://doi.org/10.1371/journal.pgen.1007943.g002

OTUs that characterise particular time periods were identified by indval analysis [45]. The strong seasonality in the Fish OTUs suggests that they might be driving significant differences identified in the seasonal indval analyses across all assays (S9 Table), but this was not the case. Spring was characterised by a significant indicator matched to Labridae (a speciose fish family), but Calcinus dapsiles (a hermit crab) and Evadne spinifera (a water flea) were the summer’s four top indicators. Calcinus dapsiles are only planktonic as larvae and only present seasonally, but E. spinifera is part of the plankton for its entire life.

Flaccisagitta enflata (a chaetognath or predatory arrow worm) and the copepods Farranula gibbula and Centropages orsinii were the most significant indicators for autumn. The copepods, Canthocalanus pauper and Centropages furcatus were found in winter. The genetic assignment of C. orsinii and C. furcatus are of interest as they are typically tropical species found in the Indian Ocean [46] indicating that they are likely to have been swept south by the warm water Leeuwin current (Fig 1A) in each year [47]. These indicator species analyses generate lists of target taxa that provide a more refined picture of seasonal changes in biodiversity—S9 Table lists all significant seasonally variable OTUs.

The years 2010 to 2014 showed changes in the Assemblage identified by several of the assays (Table 1); the pairwise analysis (S10 Table) identified when these changes occurred. The OTUs that most strongly characterise each year are presented in S11 Table. Six assays showed significant changes in Assemblage between 2010 and 2011 and each of the three subsequent years (S10 Table). In particular, the Assemblage from Copepod 1, Mollusca and Cnidaria assays responded strongly. This pattern suggests a biotic regime shift in response to an environmental anomaly. S11 Table lists all significant yearly variable OTUs.

Biotic heatwave effects

The Rottnest Island area has global significance as it is situated within a site of high biodiversity that is largely endemic [36]. This sample set was particularly significant because it encompasses two uncharacteristic summer temperature extremes in 2011 and 2012. The WA marine heatwave was originally defined as occurring between November 2010 and April 2011 [38]. However, similarly high sea surface temperatures (SST) were recorded during the following year [48–50] (Fig 2B & S3 Fig). In this study, periods for the heatwaves were: “Heatwave 1”, a five-month heatwave, as described in Pearce and Feng (2013); and “Heatwave 2”, which encompasses Heatwave 1 and extends across a 17-month period from November 2010 –May 2012 (Fig 1B). The Assemblage from most assays (except Crustacea, Fish) responded significantly to the designated heatwave periods (Table 1).

The most significant changes in the Assemblage were between the periods pre- and post-Heatwave 1 (S12 Table). For Heatwave 2, significant differences were seen before, after, as well as during the thermal event (S12 Table). Analyses of both heatwave periods suggest that there were significant, and potentially persistent, changes that occurred within the zooplankton communities as a result of these collective temperature anomalies. Only ongoing research will determine whether these changes are permanent, however, climate-mediated change has already been reported in the same study area where Wernberg (et al.) [39] reported that a kelp dominated nearshore ecosystem shifted to a more tropicalised system containing seaweed turf.

The value of employing assays with different taxonomic specificities is shown by the lack of significant heatwave-induced Assemblage changes observed for some assays. No change was detected using the Crustacea and Fish assays. The taxa detected by these assays are generally long-lived with pelagic larval phases, so any significant change in these groups is likely to occur gradually and would only be detected with an even longer-term study. The Heatwaves had less significant effects on Richness, however the Copepod 1 and 3 assays demonstrated changes in Richness, particularly between before and after the thermal anomaly periods (S12 Table).

The Copepod 1 assay illustrates the effects of Heatwaves 1 and 2 on the Assemblage and Richness (Fig 3). The Copepod 1 assay was designed in silico to focus on the genus Triconia, but, as is common in metabarcoding approaches, in vitro, the assay detects a much wider range of copepods as well as other arthropods.

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Fig 3. Heatwave effects revealed by Copepod 1 eDNA assay “Heatwave 1” and “Heatwave 2” are indicated.

(A) Changes in the number of Operational Taxonomic Units (OTUs) over time (Richness: Heatwave 1; p < 0.01 & Heatwave 2; p < 0.05) and (B) changes in the diversity of the OTUs revealed by non-parametric multivariate analysis (Assemblage; k = 3, stress = 0.15, both p < 0.001), the coloured lines extrude from the centroids of each time period towards the variation in Assemblage from each sample.

https://doi.org/10.1371/journal.pgen.1007943.g003

OTUs characterising the periods defined by the heatwaves were identified by indval analysis. The OTUs corresponding to Paracalanus indicus (a copepod) and Pythiales (an order of water mould) are strong indicators for the ‘before’ periods (S13 & S14 Tables). The Copepod 1 OTUs characterising the heatwave ‘during’ periods were significantly different; only ten OTUs (11%) overlap. The best indicator for Heatwave 1 was Hexanauplia (the class which contains all copepods); this OTU is also an indicator for Heatwave 2 (S13 & S14 Tables). For the ‘after’ periods, nine OTUs are shared between them (15%). Nine anonymous copepod OTUs (15%) were strongly associated with the ‘after’ of both heatwave periods. This demonstrates the advantage of the OTU approach and provides an opportunity for taxonomists to link these sequences to the species that they provisionally represent.

These time-stamped metabarcoding data show, for the first time, that eDNA metabarcoding is able to track biotic shifts in response to seasonal and annual changes, as well as identify a known temperature anomaly that threatened global biodiversity hotspots on the west coast of Australia. This result has obvious implications for biomonitoring of oceans in the face of anthropogenic pressures including climate change, acidification, pollution, fishing and aquaculture impacts. The Assemblage and Richness data provided by eDNA metabarcoding can be integrated with other abiotic factors to develop a more holistic picture of how biomes respond to a variety of environmental factors.

Biological response to abiotic change

Biological samples analysed in this study were collected alongside complementary measurements of physical and chemical characteristics of the sampling site. Sea surface temperature (SST) and the concentrations of salinity and silicate (an important nutrient in oceans), were all important explanatory abiotic variables for both Richness and Assemblage across the majority of metabarcoding assays (Table 2). These variables feature in either the ‘best’ or the most parsimonious alternative models for all of the assays used (Tables 2 and S15).

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Table 2. Relationship between sea surface temperature (SST) and abiotic factors, and OTU richness (the number of OTUs in each sample)—nbGLM (negative binominal Generalised Linear Model; [52])—and assemblage (what OTUs are in each sample)—DistLM (Distance based Linear Model; [42])—as indicated by each assay.

https://doi.org/10.1371/journal.pgen.1007943.t002

SST and salinity explained a large portion of the biological variation we observed. The assay most sensitive to the abiotic factors was Copepod 3; where SST, and concentrations of salinity, and silicate explained 22.7% of the variation in Assemblage, and SST and salinity concentration explained 39.2% of the variation in Richness (Table 2).

Richness increased significantly with warmer SST for most assays, with the exception of Copepod 1 and Copepod 2, which showed an insignificant negative relationship to SST (Table 2). Richness conversely decreased with increasing salinity for the Copepod, Crustacean, and Universal assays, but reacted positively in the Cnidaria, Fish, and Mollusca results. Silicate correlations had the opposite pattern, being positively correlated with Richness in the Copepod, Crustacean, and Universal results, but negatively correlated to Richness when measured against the Cnidaria, Fish, and Mollusca assays (Table 2). These results are likely due to an indirect link between the environmental variables to the zooplankton composition via direct links upon the phytoplankton [51]. These results illustrate the different niches that zooplankton can exploit within an ecosystem. As one group of zooplankton find conditions uninhabitable and diminishes locally, another group will thrive within the niche.

Conclusion

A recent editorial on marine monitoring [53] argued for a pressing need to make the shift from site-specific approaches to a functional, whole-sea system of monitoring. Here we show that eDNA metabarcoding is capable of responding to this challenge. Multi-year sample sets appropriate for eDNA analysis have not been previously available. Had this study been limited to a single point in time or even over the course of a year, where the longer-term patterns of change would be missed. Our study included two ‘marine heatwave’ periods and these data demonstrated that, using an effective eDNA metabarcoding toolkit, ecologically significant trends can be identified in response to a known environmental perturbation.

The biodiversity detected by our multi-assay eDNA metabarcoding ‘tool kit’ was vast, and while many barcodes could be assigned within the existing taxonomic framework, almost as many could not. While it could be argued that indicator species/OTUs should perhaps be the primary focus for taxonomic scrutiny employing both morphology and genetics, it is clear that as databases and assays improve, so too will the power of eDNA to identify the taxa present in complex ecosystems like this one. The results highlighted both the importance of collecting time-stamped samples (i.e. environmental biobanks [54]) and the significance of multi-gene metabarcoding for the long-term monitoring of marine ecosystems. For example, had only the universal 18S marker been used, much of the genetic depth of information would have been lost. While the 18S markers are typically longer and produce results across a broad range of taxa, it is more conserved than other barcodes and often results must be confined to a family level of identification. The study illustrates the need to balance the cost of the multi-marker approach with the amount of data that can be generated. The future implications of this data are that eDNA will generate much-needed baseline biotic data, and identify disturbance gradients, recovery profiles and potential ‘biotic tipping points’.

Sampling

All sampling took place at the Rottnest Island National Reference Station (NRS), an Integrated Marine Observing System (IMOS [6]) site, Western Australia (Fig 1A). The site is situated at the midpoint of the sub-tropical zone of the Leeuwin current, approximately 20 km off the southwest coast of Western Australia. Abiotic sampling has occurred regularly at this site since 1951 and biological sampling by the IMOS program since 2008 [6]. The plankton sampling regime was instigated at this time and historically three separate monthly samples were taken; one for morphological analysis; one for biomass measurements and a third tow for later DNA analysis. We were provided access to these final samples.

Vertical plankton tows were taken on 55 occasions from October 2009 to January 2015, from the same site, in an almost regular monthly regime (Fig 1B). A 0.6 m wide, 3 m long drop net [55] with a100 μm mesh, which free falls at 1 ms^-1, was dropped for 45 s. The seabed depth at the Rottnest Island sampling site is 50 m, so this sampling covered 90% of the water column. Plankton was collected on the downward fall; the motion of retrieval closes the net for the upward haul. The nets are washed in fresh water (with detergent if clogged), hung out to dry and stored dry between monthly sampling.

Samples were washed down and concentrated at the codend of the drop net and transferred into a sample jar using seawater. Samples were packed on ice until placed in long-term storage at -80°C immediately after return to the laboratory. Samples were later subsampled for this study and the sub-samples preserved at -20°C prior to DNA extraction.

DNA extraction

Each plankton sample was homogenised, using a hand-held blender (OMNI Tip Homogenizer) and a hard tissue probe. About 20 μL of the resulting slurry was digested and extracted using DNAeasy Blood and Tissue kit (Qiagen) following the tissue protocol and a 2 x 100 μL elution in AE buffer. An extraction control was created during this phase. Extracts were stored at -20°C.

Metabarcoding assay design

Over 20 group-specific PCR amplicon metabarcode assays were tested for use in this study. Sequences used for in silico assay design were downloaded from the National Center for Biotechnology Information (NCBI) GenBank database [56]. Database coverage was limited across all genes, so in most instances the cytochrome oxidase I (COI) gene provided the best option for metabarcoding.

Sequences were aligned in Geneious Version R8 and consensus sequences were derived from these alignments [57]. Sequences were examined for relatively conserved regions flanking 100-200bp hyper-variable targets (S4 Fig). This examination resulted in the creation of several new metabarcoding assays. These assays, along with some that were previously described, were then tested against 20 pilot plankton samples to determine which assays, when combined, produced the broadest coverage of taxa found within zooplankton (S16 Table). From these, eight assays, including five targeting COI (predominately, three for different copepods and one each for molluscs and cnidarians), one targeting 18S rRNA (“universal”) and two targeting16S rRNA (one each for actinopterygii and malacostraca), were selected for use in this study (S1 Table).

The 55 DNA extracts were assessed using qPCR for their response to each of the eight assays, which were applied to each sample’s neat extract and two dilutions (1/10 and 1/100). Extraction, non-template and positive controls (where available) were included for each assay. Each reaction comprised: 1 x Taq Gold buffer (Applied Biosystems [ABI], USA), 2 nM MgCl2 (ABI, USA), 0.4 mg/mL BSA (Fisher Biotec, Australia), 0.25 mM dNTPs (Astral Scientific, Australia), 0.4 μM each of forward and reverse primers (Integrated DNA Technologies, Australia), 0.6 μL of 1/10,000 SYBR Green dye (Life Technologies, USA), 1 U of Taq polymerase Gold (ABI, USA), 2 μL of DNA, and made up to 25 μL with PCR grade water. PCR conditions for all reactions included 95°C for 10 min followed by 50 cycles of 95°C for 30 sec, T_a (S1 Table) for 30 sec and 72°C for 45 sec, with a final extension of 72°C for 10 min. All reactions were set up in an ultra-clean laboratory used for trace and environmental DNA.

Library builds & sequencing

Fusion tagged primers incorporating specific unique combinations of six to eight base pair MID (Multiplex IDentifier) tags, assay specific primers and Illumina adaptor sequences were assigned, in duplicate, to each DNA extract (and any negative control that produced a positive result during qPCR) in a single PCR step (giving a total of over 400 unique MID tagged combinations). Many samples are multiplexed within a single library and the MID tags allow for later separation and assignment of the individual sequences to their specific assays and samples. To prevent cross contamination within the NGS workflow, the MID tag primer combinations had not been used previously for marine samples and were not reused. Conditions for the fusion tagged PCR reactions were identical to the qPCR (above) and were carried out in duplicate, using the appropriate dilution determined by the qPCR. Reactions were monitored for efficient amplification by scrutinising qPCR dynamics. Tagged amplicons were combined in roughly equimolar concentrations to produce multiplexed sequencing libraries. On each library the fusion tags were not ‘saturated’, meaning that, while there are ten reverse tags to every forward tag, each run allowed for several unused forward and reverse combinations. If unused tag combinations are subsequently detected after sequencing, the tagging process is repeated to ensure there is no tag cross over. The libraries were then size-selected using a Pippin Prep (Sage Sciences, USA) instrument and quantified using a Lab Chip (PerkinElmer, USA). All sequencing was performed using Illumina’s MiSeq following the manufacturer’s protocol with the exception of the use of custom sequencing primers and with 20 pM PhiX, on either a Standard or Nano flow cell and 300–500 cycle kits.

Taxonomic assignment

Sequences were assigned to the appropriate samples by their MID tags using Geneious R8 [57]. Initial filtering steps included ensuring the MID tags, gene specific primers and sequencing adapters, were all present in each sequence without error. Those sequences not matched were discarded from future analyses. The primers, adaptors and MID tags were removed from each of the sequences that passed these criteria, which were then filtered using a fastq filter (E_max > 0.5—USEARCH v8 [58]).

To increase the robustness of the data set, sequences were then separated into groups of unique sequences using USEARCH v8 [58]. Of these sequences, any group which contained < 1% of the total number of unique sequences was discarded—the filtered data are available for download on Data Dryad: doi:10.5061/dryad.sc673ds. This process, which may eliminate low abundance taxa, is conservative in that it ensures the removal of possible erroneous amplicons. Amplicons that passed the second filtering processes were queried against the National Center for Biotechnology Information (NCBI) GenBank nucleotide database [59] using BLASTn (Basic Local Alignment Search Tool [60]) with the default parameters and a reward of value of 1.

The search output files were imported into MEGAN v5 (METaGenome ANalyzer [61]) and visualised using the LCA (lowest common ancestor) parameters: min bitscore 100.0, and reports restricted to the best 5% of matches. Taxonomic assignment was considered only when the entire length of the query sequence matched the reference database. Taxonomic hierarchy was determined using the World Register of Marine Species [62]. Negative controls were all found to be clear with the exception of the 18S Universal assay, which showed some fungal contamination.

Production of Operational Taxonomic Units (OTUs)

Clustering of similar sequences to produce OTUs was performed with USEARCH v8 [58]. The OTUs were formed from all filtered sequences from each assay using a 97% similarity threshold across all samples. The procedure also removed any potential chimeric sequences and any groups of unique sequences with an abundance of < 0.1% of the total number of unique sequences across all samples. Sequences discarded during this process were then mapped back on to existing OTUs to ensure the inclusion of all relevant data and those amplicons, which could not be mapped, were discarded. The OTUs were then assigned to the samples that they originated from and were converted to a presence/absence matrix. This approach also minimises any data misrepresentations as a result of potential unequal sequence amplification from marker choice or tag bias. The OTUs were statistically analysed in response to both temporal and abiotic factors.

Statistical analysis

Statistical analyses, were performed using PERMANOVA+ [42] add on for Primer 7 [63] and R [64] with labdsv [45], and vegan [65]. The analyses were performed on the presence/absence OTU data matrix for the sequences obtained for each assay, thus allowing for all available genetic information to be taken into consideration. A total of 55 samples were used for analysis. The initial Pearson’s correlation test of the number of sequences produced by each assay, at each time point, and the number of OTUs was performed in R [64].

To prevent the inclusion of ‘outliers’ that might skew the results, the sequences for each assay were filtered to remove any OTUs that occurred only once in the study and also any samples that contained only one OTU. The richness and assemblage (genetic diversity) data for each sample were then examined using multivariate methods (PERMANOVA [66]) to test time-based relationships such as heatwave, seasonality and inter-annual effects). Annual and seasonal effects were tested using a nested design with three factors: Year (fixed, 5 levels), Season (nested in Year, random), and Month (Nested in Season, random). Tests for heatwave effects were conducted using a single factor (fixed, either 5 month or 17 month heatwave window) with three levels (before, during, after). To illustrate these patterns, two-dimensional nonmetric multidimensional scaling (nMDS) plots were formed in R (package vegan).

The indicator species that were characteristic of years, seasons, and heatwave events were identified using indval analyses in R (package labdsv). The indval indicator value is calculated using a combination of the fidelity of an OTU to a time period and the frequency at which it occurs during that same time period. All pairwise comparisons were performed using PERMANOVA.

The role of abiotic variables in explaining variation in both the multivariate OTU assemblage, and the univariate OTU richness was analysed with linear models for each assay. Multivariate analysis was done using distance based linear models (DistLM) in PERMANOVA+. Bray-Curtis similarity matrices were constructed from the presence/absence OTU data. The abiotic variables sea surface temperature (SST) and concentrations of salinity, silicate, nitrate, phosphate, and ammonium were available for selection by the model. The ‘best’ selection procedure and the AIC selection criteria were used to select the model that best explained the variation in the OTU assemblage that was recorded for each assay. The best alternative models for each number of variables that were within 2 AIC of the selected model were also reported (S15 Table).

Univariate OTU richness was analysed for each assay with generalised linear models (GLMs) fitted in R using the functions glm [64] and glm.nb [52]. The abiotic explanatory variables available were the same as those above. During analysis the distribution of the residuals of each model were plotted and examined to select the appropriate distribution. In all cases the negative binomial distribution with a log link was used [67]. The model with the lowest AIC was selected using the best of both forward and backward selection procedures. Models within 2AIC of the selected model were also reported. To aid in the interpretation of the relationship between each abiotic variable and the OTU assemblage composition and richness were also calculated and reported for each abiotic variable.