INTRODUCTION

Treatment failure due to antimicrobial resistance (AMR) is considered one of the largest threats to human and animal health (1–6). Multiple studies have shown that AMR bacteria and, in some cases, antimicrobial resistance genes (ARGs) can be transferred between livestock and humans (7, 8). However, despite decades of research, it remains difficult to determine the size and importance of individual transmission pathways, partly due to the complex epidemiology of AMR. ARGs are in many cases not confined to a single bacterial species but may transmit between different gut commensal species prior to emerging in human pathogenic bacteria. Most studies conducted to date have focused on single indicator species or specific human pathogens and largely missed the emergence and dispersal of AMR in the normal gut microbiota.

With the developments in genomic sequencing, it has become technically and economically feasible to characterize any animal microbiome and their associated ARG reservoirs, the resistomes. It has also been documented that metagenomic methods offer improvements over traditional phenotypic AMR surveillance of indicator species by more closely capturing increases in AMR due to antimicrobial usage (AMU) than indicator species can (9–11).

In the Ecology from Farm to Fork Of microbial drug Resistance and Transmission (EFFORT) project, we previously analyzed pooled fecal samples from 181 pig herds and 178 broiler flocks in nine European countries using shotgun metagenomic sequencing (12). We found higher AMR loads in pigs, whereas broiler resistomes were more diverse. In addition, we identified a number of core ARGs strongly associated with the two livestock populations. This is highly important for studies trying to perform source attribution and elucidate the relative transmission of AMR between reservoirs (13). We have also shown that the farm-specific use of antimicrobial agents was significantly associated with AMR but only explains a limited amount of variation in AMR load (14, 15).

In the current study, we further expanded on the integrated analysis of European livestock resistomes (12) by including samples from veal calves, turkeys, and rainbow trout, using updated bioinformatic and downstream analyses of the combined results of all five animal categories, providing a comprehensive overview of potential human occupational and food-related exposure to livestock-related AMR within Europe. Moreover, we investigated the importance of AMU and the associations between bacterial and resistome diversity and abundance. Finally, we analyzed the association of overlap and dissimilarity in resistomes to answer whether the ARG patterns are best explained by differential selection or dispersal limitations.

MATERIALS AND METHODS

Here, we present a combined analysis of the resistomes from pigs, broilers, veal calves, turkeys, and fish from different European countries (Data S1 and S2). Comparative analyses of the resistomes of broilers and pigs have previously been published (12), as have source attribution analyses of resistomes from pigs, broilers, veal calves, and turkeys (13) and risk factor analyses for resistomes in pigs (14), broilers (15), and turkeys (16), individually. A combined analyses have, however, never been performed. Also, compared to previous studies, we updated the workflow to incorporate faster DNA alignment methods (17), filtered lower-coverage ARGs to minimize spurious signal, and analyzed the data sets using compositionally correct methods as detailed below (18). Because each data set has a fixed number of reads determined by the sequencing instrument, the number of reads assigned to each feature is not independent of each other and should be treated as part of a composition (18).

The centered log ratio (CLR), additive log ratio (ALR), and interquartile log ratio (IQLR) are examples of methods originally proposed by John Aitchison to analyze compositions and are recommended for analyzing microbiomes, which are compositional (18, 19).

Sampling procedure

Livestock from conventional pig, broiler, and turkey farms in nine European countries was sampled as previously described (12, 16). In addition, for this study, we included industrial veal calf (white/rosé), turkey, and rainbow trout productions from three countries each. A breakdown of the 538 sampled herds by livestock species and country is presented in Data S1. The protocols for farm selection and sample collection are more thoroughly described in the supplement. It is important to note that convenience and accessibility were allowed to influence herd inclusion choice, so the sampled herds could differ from average national conditions.

After 25 randomly distributed fecal samples (pigs, broilers, veal calves, and turkeys) or intestine contents (rainbow trout) were collected at each farm close to the date of slaughter (date of sale for freshly caught trout), pooled samples representing each herd were established: the 25 individual samples from each herd were pooled, with individual samples all contributing equal mass. The pooled samples were stored at −80°C locally and sent in batches on dry ice to the Technical University of Denmark (DTU).

DNA extraction and sequencing

Procedures for DNA extraction and sequencing of samples from veal calves, turkeys, and trout were designed to be as similar as possible to the ones used by Munk et al. (12) to evaluate the pig and broiler resistomes.

The trout sampling strategy deviated slightly in the following manner. At each farm, 25 live rainbow trout were collected close to their sale date. After euthanasia, the gastro-intestinal tracts were removed and frozen at −80°C and shipped for processing at DTU on dry ice. The freezing procedure made it difficult to separate fish intestines and fecal contents. Therefore, for each fish farm, 0.2 g of the intestines for each of the 25 trout was pooled, similar to the procedure of the other animal species.

After pooled veal calf and turkey samples were obtained, DNA extraction was performed as for the previous pig and broiler samples. Briefly, we extracted DNA from herd-level fecal pools using a previously published bead-beating-optimized standard operating protocol based on the QIAamp Fast DNA Stool Mini Kit (51604, Qiagen) (20).

Two batches of DNA extracted from calf and turkey pooled fecal samples were shipped on dry ice to Admera Health (South Plainfield, NJ, USA) where library preparation and shotgun metagenomic sequencing were performed. Briefly, after DNA fragmentation (Covaris LE220), sequencing libraries were prepared and multiplexed using the KAPA HyperPrep kit (Kapa Biosystems). While libraries corresponding to veal calf samples were prepared without PCR (same as for pigs), the library preparation for turkey samples involved limited PCR amplification (same as for broilers). The generated libraries were sequenced on the NovaSeq 6000 platform (Illumina), using a 2 × 150-bp paired-end (PE) read approach.

DNA obtained from rainbow trout samples was prepared for sequencing using the Nextera XT library preparation kit (Illumina, FC-131-1024) and sequenced in batches of six samples on the NextSeq 550 platform (Illumina) internally at DTU.

Processing and alignment of reads

Biological replicate samples were collected at eight farms: two pig farms were sampled three times each, whereas five turkey farms and one fish farm each were sampled twice. For each of these eight farms, the sample yielding the highest number of sequenced read pairs was chosen to represent the farm.

In order to remove low-quality nucleotides as well as adaptor sequences, DNA sequence read pairs were quality- and adapter-trimmed with the BBMap (v36.49) tool BBduk2 with the following arguments: qin=auto k=19 mink=11 qtrim=r trimq=20 minlength=50 (21).

Samples originating from 69 samples were sequenced more than once, usually due to low read throughput during the initial sequencing. In these cases, trimmed read pairs from all sequencing runs associated with the same sample were concatenated into combined files representing the individual farms.

Trimmed reads from each sample were aligned to the 3,081 ARGs in the ResFinder database (Bitbucket commit d3d7a6c) (22) and, separately, to a merged database of genomic sequences, as outlined below using the k-mer alignment software KMA (17) (v1.2.8). KMA was specifically designed to perform well when mapping against redundant databases such as the ones we used in this study, which contain high levels of sequence redundancy.

ResFinder offers a manually curated database of acquired ARGs, i.e., non-intrinsic genes discovered to provide bacterial AMR, with each ARG belonging to a specific AMR group and class (Data S3). Sequence reads were aligned to the ResFinder database using the KMA parameters “-mem_mode -ef −1t1 –cge -nf -nc.”

The database of genomic sequences was created by merging the following genome collections from NCBI and other sources into an indexed KMA database as previously described (23). Briefly, the latest versions of plasmids and bacterial, archaeal, human, fungal, parasite, and protozoan genomes were downloaded from NCBI (24) and supplemented with the genome collections from MetaHitAssembly (25), the Human Microbiome project (26), KVIT (27), and IMG-VR (28) as well as a previously described curated parasite database (29). This genome collection was indexed with KMA, and the trimmed reads were subsequently aligned using KMA parameters “-mem_mode -ef −1t1 -apm f -nf -nc.”

Abundance data transformations

Both bacterial taxonomy and ResFinder matrices (Data S4 to S6) were subjected to zero replacement using the “SQ” method as implemented in the cmultRpl function in the zCompositions R package (version 1.3.4) (30).

The CLRs were calculated based on those and used for, e.g., principal component analysis (PCA) and differential abundance analysis with ALDEx2. Each sample ALR for ResFinder abundances was calculated as the log ratio between the length-corrected gene abundances (nominator) and the number of bacterial fragments (denominator). Such ratios were calculated at both the level of drug classes and the individual gene clusters.

Quality control of ARG-assigned reads

To filter out low-coverage alignments before the downstream analysis of ARGs, we required that the ResFinder reference genes were at least 20% covered. Alignments with lower proportions covered had their mapped fragment count for such references set to zero.

Quality of samples from fish farms

For many of the data sets originating from fish farms, only a low number of sequence fragments could be assigned to bacterial genomes or the ResFinder database of ARGs.

We opted, however, to not completely exclude them from all analyses. Fish samples were included in PCA ordination, hierarchical clustering, and core resistome analysis if they scored higher than the least informative (i.e., lowest-scoring) sample from pig and broiler herds in at least one of the three measurement criteria: (i) absolute number of fragments mapping to the ResFinder database, (ii) proportion of all fragments mapping to the ResFinder database, and (iii) estimated Chao1 richness of ARGs.

Data analysis and visualization

All analyses of read mapping results were conducted using the open-source statistical environment R (31) version 4.0.1 (2020-06-06). Most figures were created with the R package ggplot2 (v2.3.3.2) (32). Exceptions are the heatmap in Fig. S3, which was created using the R package pheatmap (v1.0.12) (33), the network layouts in Fig. 5 created with gephi (v.0.9.2) (34), and the universality result panels in Fig. 6 made with R (v3.6).

ARG alpha diversity and richness estimation

We estimated the richness (number of different ARGs) in each sample using the bias-corrected form of the Chao1 index:

Alpha diversity was calculated as Shannon’s diversity index on the proportion of features with non-zero fragments sum-scaled to 1 (p):

Core resistomes

We established core resistomes for each category, i.e., sets of ARGs that appear in the large majority of herds sampled for each host species (90% of sampled herds). For broilers and pigs, core ARGs are genes that appeared in at least 162 sampled herds (out of 178 broiler herds or 181 pig herds). Because fewer turkey and veal calf herds were sampled, the minimum number required was only 54 herds (out of 60 turkey flocks or 61 veal calf herds). Only a few fish data sets passed the quality threshold; therefore, core fish ARGs needed to appear in at least 13 out of 14 sampled fish herds.

Core resistomes were also determined for each country cohort within all host species except fish. Here, core ARGs are genes that were detected in at least 18 herds of the same host species and from the same country.

Co-occurrence analysis of bacterial taxa and ARGs

To enable co-occurrence visualization in a network interface, we constructed a correlation matrix by calculating all pairwise Spearman’s rank correlations between bacterial genera and ARGs as well as between ARGs themselves. Zero correlations and bacteria–bacteria correlations were excluded to focus on bacteria–ARG and ARG–ARG correlations. Significant Benjamini–Hochberg correlations, corrected for multiple testiing (P < 0.01 and |ρ| > 0.8) were retained for constructing an undirected network where node sizes represent the calculated betweenness centrality and nodes were laid out using the Fruchterman–Reingold algorithm using gephi (v0.9.2) (34).

Questionnaire data

General farm characteristics, antimicrobial use (AMU group treatments), and information about biosecurity were retrieved from a standardized questionnaire completed by the farmer as published previously (14, 15, 36). The usage of antimicrobials on farms of pigs, broilers, turkeys, and veal calves has been elaborately described elsewhere (37–39).

Aggregated biosecurity scores per farm were retrieved from previous studies (for pigs [14] and broilers [15]) or newly calculated from the questionnaire based on the algorithm of the Biocheck.UGent scoring system (for veal calves [40]).

Log ratio transformation and PCA

Respecting the compositional nature of quantified ARGs (18), we transformed the filtered ARG count matrices from simplex space into real space using a log ratio transformation. In that way, true Euclidean distances between resistome compositions can be calculated as required by PCA. Because we are dealing with complex samples from different environments, we chose the IQLR transformation in order to try and correct for the asymmetric presence and absence of ARGs in the different host species cohorts (41). We used the R package ALDEx2 (v2.1.20.0) (42) to identify a set of ARGs with the medium variance within each of the four non-fish host species (i.e., variance between the first and third quartiles of variance). The geometric mean abundance of these ARGs was used as a denominator in subsequent log ratio transformations.

During such transformations, ALDEx2 estimates the technical variation of gene abundances by drawing 128 Monte Carlo samples from a Dirichlet distribution whose parameters are based on the provided fragment count matrix. While this inferred technical variation is crucial for robust differential abundance testing, it cannot be reasonably visualized in the ordination plots, heatmap, or box plots we created. Therefore, we calculated the mean of the 128 resulting log ratio matrices for use in visualizations of log ratio values.

These mean log ratio values were used to visualize the samples’ beta diversity: (i) in an ordination plot using PCA with Euclidean distances and (ii) in a heatmap displaying Ward linkage clustering of Euclidean distances.

The mean ALR ARG abundances were visualized per country and species in box plots. Overall, per species, country resistome differences were compared by performing a classic or Welch’s analysis of variance (ANOVA) (43, 44). In case of a significant difference, post hoc tests were carried out (i.e., respectively, Tukey’s honest significant difference test [Tukey HSD] [45] or a Games–Howell post hoc test [46]).

Risk factor random-effects meta-analyses in pigs, broilers, and veal calves

For pigs, broilers, and veal calves, respectively, 176, 176, and 59 farm data sets with matching questionnaires (e.g., AMU and biosecurity) and ARG data were available for analysis (14, 15, 36). We used R v3.6.3 for all risk factor analyses (47). A random-effects meta-analysis by country was run for veal calves using the R package metafor (48) (v2.4.0) as described and calculated previously in pigs and broilers (14, 15).

Dispersal limitations of livestock ARGs

If ARGs that co-occur in different farms tend to exist in similar ratios to each other, it suggests that they are similarly selected across the farms (49). Such a pattern, therefore, implies that interfarm variability is created via colonizing ARGs or dispersal limitations. Overlap, a measure for ARGs shared between samples, and dissimilarity, as a measure of variation in abundances of the shared ARGs, were calculated for all sample resistome combinations and grouped in combinations of inter- and intra-livestock species and country comparisons. Subsets of samples can vary in the degree that pairings sharing ARGs predict the relative abundances of these ARGs or the strength of the universality signature; this is named “group dynamics.” If each of these subsets of samples is still universal, the data set as a whole is universal.

Each pair of sample resistomes was compared in order to determine the relationship between their overlap and dissimilarity. Overlap was calculated as