Sample collection

Samples of hypolithic microbial communities were collected from 77 sites as part of a systematic vegetation survey of the Vestfold Hills, East Antarctica (Fig. 1a,b) between December 2019 and February 2020 (detailed sample methodology in T. Travers et al., unpublished data 2024). Hypolithic communities of the Vestfold Hills are most common in areas with high wind exposure and flat or shallow north-east-facing slopes of salt-enriched ground, and they are found in areas far from snowmelt (T. Travers et al., unpublished data 2024). Topographical factors including wind exposure, aspect and slope create the conditions that expose and orientate quartz cobbles of an appropriate size at the surface of glacial valley beds, allowing colonization by hypolithic communities. The ice-free area was divided into 10 strata based on elevation, slope, solar radiation (as a proxy for aspect) and terrain roughness derived from the Reference Elevation Model of Antarctica (Howat et al. Reference Howat, Porter, Smith, Noh and Morin2019), with 200 random points generated within each stratum. These points were used as prospective site locations for this survey, with sampling occurring widely to maximize regional cover and locally to maximize habitat variability.

Figure 1. a. Map of hypolithic communities examined across the Vestfold Hills. The filled grey area is ice free. There are two types of water bodies: 1) marine areas including fjords and 2) lakes. Continental ice lies to the east and south. Sites are colour-coded by salinity (red = high, blue = low). There were 77 sites in total (51 with both bacteria and eukaryotic analyses, 15 with bacteria only, 9 with eukaryote only; 16 were low salinity, 61 were high salinity). The positions of two interpretations of the regional soil salinity transitional boundary termed the ‘salt line’ are shown. b. Example field site and c. hypolithic community in situ and d. showing community.

At each study site, quartz rocks were carefully lifted and turned over. If hypolithics were present (Fig. 1c,d), a small portion was scraped with the edge of a sterile tube, such that scrapings fell into the tube. Variation in colour of microbial communities across the hypolithic surface was observed. Scrapings attempted to include all colour variations. Additional material on the soil surface directly under the rock was also collected, if abundant. Each sample was taken from a single rock, such that more than one sample could be collected per site if multiple hypolithic communities were found. No equipment was reused between samples. At a small number of sites, entire rocks supporting hypolithic communities were transferred to sterile Ziplock bags; otherwise, rocks were carefully returned to their original position. Visible disturbance was kept to a minimum (e.g. footprints) and, if needed, restored before leaving the site. Samples were stored at -20°C in Antarctica and in transit and at -80°C at the Australian Antarctic Division, Tasmania, for ~3 months prior to analysis.

Edaphic factors

We refer to salt-enriched sites to the west and north of the ‘salt line’ as high salinity and sites with salt-poor ground to the east and south nearest the ice sheet as low salinity. Water availability at each site was categorized as dry, moist, wet-ephemeral or wet-permanent (sample metadata in Table S1). This schema attempted to identify site water availability over the summer despite each site being visited only once. Features such as the size and position of snowbanks and seeps relative to hypoliths informed site classification, with a smooth surface and lack of cobbles indicating the presence of local snowbanks earlier in the season. Relative rock size was estimated from site photographs. Attempts to measure soil conductivity and water content were complicated by dry soils and rocky sites, respectively, leading to sparse, incomplete datasets that were not used.

DNA extraction and sequencing

DNA was extracted from ~100 mg of hypolithic material and an extraction control (no material) using the QIAGEN DNeasy PowerSoil kit. We followed the manufacturer's instructions with the exception that samples were homogenized in the PowerBead tube using a FastPrep-24 (MP Biomedicals) at 4.5 m/s for 45 s. The extracted DNA was quantified using the Qubit 2.0 (dsDNA High Sensitivity kit), and sample DNA concentrations were normalized to 2 ng/μl.

The V4 and V5 regions of bacterial 16S ribosomal RNA (rRNA) genes were amplified with the primers 515F-Y and 926R (Quince et al. Reference Quince, Lanzen, Davenport and Turnbaugh2011, Parada et al. Reference Parada, Needham and Fuhrman2016). The V4 region of the eukaryote 18S rRNA gene was amplified using the primers V4 18S Next.Rev and V4 18S Next.For (Piredda et al. Reference Piredda, Tomasino, D'Erchia, Manzari, Pesole and Montresor2017). High-throughput sequencing libraries were prepared as per Clarke et al. (Reference Clarke, Beard, Swadling and Deagle2017). Specifically, polymerase chain reaction (PCR) amplifications were performed in two rounds: the first to amplify the target gene and add sample-specific 6 bp multiplex-identifier (MID) tags (forward and reverse primer) and Illumina sequencing primers and the second to add sequencing adapters and additional 8 bp MID tags. Using two rounds of tagging reduces the chances of contamination or sequencing artefacts such as tag-jumping leading to false positives, as reads must include two pairs of unique MID tags to be assigned to a given sample.

The first round of PCR for the 16S primers was 98°C for 30 s, followed by 25 cycles of 98°C for 5 s, 65°C for 20 s and 72°C for 20 s, and then a final extension at 72°C for 5 min. The first round for the 18S primers was 98°C for 30 s, followed by 10 cycles of 98°C for 10 s, 44°C for 30 s and 72°C for 15 s, and then 20 cycles with an annealing temperature of 62°C and a final extension at 72°C for 7 min (Piredda et al. Reference Piredda, Tomasino, D'Erchia, Manzari, Pesole and Montresor2017). Each reaction mix contained either 0.2 μM (16S) or 0.5 μM (18S) each of forward and reverse primer, 2 μg bovine serum albumin, 1 × Phusion Master Mix (New England BioLabs, Ipswich, MA, USA) and 2 ng DNA extract in a total reaction volume of 10 μl. The PCR products were diluted 1:10, and Illumina sequencing adapters were added in a second round of PCR (10 cycles with an annealing temperature of 55°C) using the same conditions as the first round, except primer concentrations were reduced to 0.1 μM each.

Products from each round of PCR were separated by electrophoresis and visualized on 2% agarose gels. Equal volumes of second-round 16S and 18S PCR products were pooled separately to create two amplicon libraries and then purified using Agencourt AMPure XP beads (Beckman Coulter, Brea, CA, USA), and the size distribution and concentration of the two libraries were assessed on a 2100 Bioanalyzer (Agilent Technologies, Santa Clara, CA, USA). The pools were diluted to 2 nM, and paired-end reads were generated on separate MiSeq runs (Illumina, San Diego, CA, USA) with the MiSeq Reagent Kit v3 (2 × 300 bp).

Data analysis

High-throughput DNA sequencing data for the 16S and 18S ribosomal RNA genes were processed following Suter et al. (Reference Suter, Polanowski, Clarke, Kitchener and Deagle2020). Sequences were assigned to sample-specific FASTQ files (available in the National Center for Biotechnology Information (NCBI) database with metadata under BioProject: PRJNA912313) using the 8 bp MID tags on the MiSeq. Paired reads were merged using USEARCH v11.0.667 (Edgar Reference Edgar2010). Only reads with exact matches to first-round 6 bp MID tags and the forward and reverse primer sequences (identified with the R package ‘ShortRead'; Morgan et al. Reference Morgan, Anders, Lawrence, Aboyoun, Pagés and Gentleman2009, R Core Team, 2017) were kept, as non-exact matches are more likely to contain sequencing errors in the remainder of the sequence. Processed sequences were then pooled and dereplicated using the USEARCH command ‘fastx_uniques'. The USEARCH command ‘unoise3′ was used to remove sequencing errors and chimaeras and to create a list of unique zOTU sequences with a minimum abundance of eight reads. Reads for each sample were then mapped to unique zOTUs to create separate zOTU tables for the 16S and 18S datasets using the USEARCH command ‘otutab'. Taxonomy was assigned to bacterial and eukaryote zOTUs using the Ribosomal Database Project (RDP) Bayesian classifier (Wang et al. Reference Wang, Garrity, Tiedje and Cole2007) based on the SILVA v132 database (Yilmaz et al. Reference Yilmaz, Parfrey, Yarza, Gerken, Pruesse and Quast2014) and a 60% probability cut-off.

Hypolithic microbial diversity (alpha-diversity)

To compare alpha-diversity (zOTU richness) in hypolithic communities, we explored the number of bacterial and eukaryote zOTUs detected at each site using rarefaction curves generated with the ‘iNEXT’ R package (Hsieh et al. Reference Hsieh, Ma, Chao and McInerny2016). We then tested the influence of categorical edaphic attributes (soil salinity and water availability) on alpha-diversity by modelling counts of zOTUs (based on zOTU tables rarefied to 8000 or 1200 reads per sample for bacteria and eukaryotes, respectively) for each site using a negative binomial generalized linear model in the ‘MASS’ R package (Venables & Ripley Reference Venables and Ripley2002).

Spatial variation in community composition (beta-diversity)

We computed the Aitchison distance (Euclidean distance for centred log-ratio (clr)-transformed data; Aitchison Reference Aitchison1986) using the ‘phyloseq’ (McMurdie & Holmes Reference McMurdie and Holmes2013) and ‘microbiome’ (Lahti & Shetty Reference Lahti and Shetty2017) R packages to explore the ecological distance (beta-diversity) amongst communities as recommended for compositional high-throughput sequencing data (Gloor et al. Reference Gloor, Macklaim, Pawlowsky-Glahn and Egozcue2017). We used the adonis function from the ‘vegan’ R package (Oksanen et al. Reference Oksanen, Blanchet, Friendly, Kindt, Legendre and McGlinn2020) to perform permutational analysis of variance (PERMANOVA; a non-parametric test that is robust to unbalanced sample sizes and is suitable for multivariate data), testing for effects of soil salinity and water availability on bacterial and eukaryotic community composition as well as inferred metabolic pathways (see below). We identified zOTUs and inferred metabolic pathways (see below) that showed differential relative abundance between sites with high compared with low salinity and between dry compared with permanently wet sites using a Welch t-test in ALDEx2 (Fernandes et al. Reference Fernandes, Macklaim, Linn, Reid and Gloor2013). We report the zOTUs and pathways with effect sizes > |1.0|, being the difference in clr-transformed relative abundance between groups divided by the overall standard deviation.

Correlations between geographical distance and hypolithic community dissimilarity

We used a Mantel test to investigate correlations between geographical distance separating individual hypoliths and community dissimilarity (Aitchison distance) amongst bacterial and eukaryotic hypolithic communities, and we report the Pearson correlation coefficient to detect a positive or negative relationship.

Inferring bacterial metabolic pathways

In the absence of metagenomic data, we used PICRUSt2 (version 2.4.1; Phylogenetic Investigation of Communities by Reconstruction of Unobserved States; Langille et al. Reference Langille, Zaneveld, Caporaso, McDonald, Knights and Reyes2013, Douglas et al. Reference Douglas, Maffei, Zaneveld, Yurgel, Brown and Taylor2020), which wraps several tools (EPA-ng, Barbera et al. Reference Barbera, Kozlov, Czech, Morel, Darriba, Flouri and Stamatakis2019; Gappa, Czech et al. Reference Czech, Barbera and Stamatakis2020; castor, Louca & Doebeli Reference Louca and Doebeli2018; SEPP, Mirarab et al. Reference Mirarab, Nguyen, Warnow, Altman, Dunker, Hunter, Murray and Klein2011; MinPath, Ye & Doak Reference Ye and Doak2009) to predict functional gene content and metabolic pathway abundances for hypolithic bacterial communities based on our 16S data. PICRUSt2 infers the genomic content for a given 16S rRNA sequence based on averaging over bacterial genomes with the most similar 16S rRNA sequences available in the Integrated Microbial Genomes database (Markowitz et al. Reference Markowitz, Chen, Palaniappan, Chu, Szeto and Grechkin2012). The Nearest Sequenced Taxon Index (NSTI) was calculated for each zOTU to estimate the similarity of zOTUs to available genome data; only zOTUs with NSTI < 2 were used for the analysis (98.7% of zOTUs, 99.8% of reads). The accuracy of predicted metagenomes for each sample was estimated based on the NSTI weighted by the abundance of each zOTU. Pathways were categorized into superclasses based on their classification in the curated MetaCyc database of experimentally deduced metabolic pathways from all domains of life (Caspi et al. Reference Caspi, Billington, Fulcher, Keseler, Kothari and Krummenacker2018).

Contribution of selection and dispersal processes to community turnover

We explored the contribution of selection and dispersal processes to ecological turnover between hypolithic communities using a series of null models as per Stegen et al. (Reference Stegen, Lin, Fredrickson, Chen, Kennedy and Murray2013, Reference Stegen, Lin, Fredrickson and Konopka2015). The first null model estimates the contribution of selection (both homogeneous and variable) using phylogenetic turnover between communities. Where phylogenetic turnover was consistent with the first null model (see below), a second null model using the Raup-Crick metric incorporating Bray-Curtis dissimilarities (RC_Bray) compares observed and expected levels of community turnover without using phylogenetic information to infer the influence of homogenizing dispersal and dispersal limitation. The same approach was applied to both bacterial communities and microbial eukaryotic communities (excluding metazoans) so that the results could be compared with those for lake microbial communities in the Vestfold Hills (Logares et al. Reference Logares, Tesson, Canback, Pontarp, Hedlund and Rengefors2018).

To explore phylogenetic turnover between communities, bacterial and eukaryote phylogenetic trees were generated in QIIME 1.8 (Caporaso et al. Reference Caporaso, Kuczynski, Stombaugh, Bittinger, Bushman and Costello2010) by aligning 16S and 18S sequences using MUSCLE (Edgar Reference Edgar2004) or PyNAST (Caporaso et al. Reference Caporaso, Bittinger, Bushman, DeSantis, Andersen and Knight2009), filtering the alignment (removing 0.0005% most variable positions and those that were > 80% gaps) and building the tree using FastTree 2.1.3 (Price et al. Reference Price, Dehal and Arkin2010). The mean phylogenetic distance between each zOTU in one community and its closest relative in a second community was calculated as the between-community mean nearest taxon distance (βMNTD). A null-model distribution of βMNTD was generated by randomly shuffling zOTUs across the tips of the phylogeny (999 permutations). β-nearest taxon indices (βNTIs) were calculated as the difference between the observed βMNTD and the mean of the null distribution, expressed in units of standard deviations; significant deviations (βNTI values < -2 or > +2) represent variable selection (βNTI > 2) or homogeneous selection (βNTI < -2).

Where phylogenetic turnover was consistent with the null model (|βNTI| < 2), we used the RC_Bray to compare observed and expected levels of community turnover without using phylogenetic information. Significant deviations from the null distribution represented homogenizing dispersal (RC_Bray < -0.95) or dispersal limitation (RC_Bray > +0.95), whereas comparisons consistent with the null distributions for both βNTI and RC_Bray suggested no single ecological process dominated compositional turnover (referred to as ‘drift’ in Stegen et al. Reference Stegen, Lin, Fredrickson, Chen, Kennedy and Murray2013).