Abstract
Global sewage sludge production is rapidly increasing, and its safe disposal is becoming an increasingly serious issue. One of the main methods of municipal sewage sludge management is based on its agricultural use. The wastewater and sewage sludge contain numerous antibiotic resistance genes (ARGs), and its microbiome differs significantly from the soil microbial community. The aim of the study was to assess the changes occurring in the soil microbial community and resistome after the addition of sewage sludge from municipal wastewater treatment plant (WWTP) in central Poland, from which the sludge is used for fertilizing agricultural soils on a regular basis. This study used a high-throughput shotgun metagenomics approach to compare the microbial communities and ARGs present in two soils fertilized with sewage sludge. The two soils represented different land uses and different physicochemical and granulometric properties. Both soils were characterized by a similar taxonomic composition of the bacterial community, despite dissimilarities between soils properties. Five phyla predominated, viz. Planctomycetes, Actinobacteria, Proteobacteria, Chloroflexi and Firmicutes, and they were present in comparable proportions in both soils. Network analysis revealed that the application of sewage sludge resulted in substantial qualitative and quantitative changes in bacterial taxonomic profile, with most abundant phyla being considerably depleted and replaced by Proteobacteria and Spirochaetes. In addition, the ratio of oligotrophic to copiotrophic bacteria substantially decreased in both amended soils. Furthermore, fertilized soils demonstrated greater diversity and richness of ARGs compared to control soils. The increased abundance concerned mainly genes of resistance to antibiotics most commonly used in human and animal medicine. The level of heavy metals in sewage sludge was low and did not exceed the standards permitted in Poland for sludge used in agriculture, and their level in fertilized soils was still inconsiderable.
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Discover the latest articles, news and stories from top researchers in related subjects.Agricultural soils are often degraded by intensive exploitation, resulting in soil erosion and deterioration1. One possible way to reverse these negative effects is by increasing the carbon, phosphorus and nitrogen content of the soil with organic amendments such as sewage sludge2,3. Such treatment has been recommended as a method of sludge utilization by the EU Sewage Sludge Directive 86/278/EEC (SSD) and the Urban Wastewater Treatment Directive 91/271/EC. Of all the sewage sludge generated in Europe during 2019, 50% was used in agriculture, 28% was incinerated, 18% was transported to landfills, and 4% used in other areas, such as land reclamation and forestry4. Due to the global rise in wastewater production and thus, wastewater sediment, effective sludge management and the long-term risk associated with its direct use in agriculture have become important issues of environmental research5. Municipal sewage sludge is formed as a by-product of many mechanical and biological wastewater treatment processes, and is treated with quicklime to make it safe for use, from a sanitary perspective. The resulting sludge is rich in easily-assimilable phosphorus and nitrogen compounds, as well as calcium that can deacidify soil; hence, it is suitable for use as a soil amendment to reduce the cost of agricultural production. Such use is currently permissible for the cultivation of cereals, for the reclamation of degraded areas, as well as cultivation of plants not intended for human and animal consumption6. Despite the benefits, there is the main concern that sludge can contain high levels of toxic substances, heavy metals, antibiotics, personal care products, pathogens and antibiotic-resistant bacteria (ARBs) from the inflowing wastewater; these contaminants can hence be introduced into agro-ecosystems through fertilization with sewage sludge7,8,9. Although the primary concern limiting the agricultural use of sewage sludge has been its heavy metal content, research over the last decade indicates that effluents and sewage sludge from WWTPs are significant sources of antibiotics and antibiotic resistance genes (ARGs) in the environment10,11,12. Although antibiotics have traditionally been used for medical and veterinary purposes, since the 1950s they have been added as growth promoters in poultry, livestock and in fish farming10,13,14,15. The resulting massive scale and overuse of antimicrobials has accelerated the evolution of ARBs and ARGs in the environment, thus indicating potential gene exchange between the environmental and clinical resistome10,16,17. ARBs have recently become emergent environmental pollutants and represent a potentially serious global threat to human and animal health, with a rise in MDR (multidrug-resistance) bacterial strains being documented worldwide18,19,20 The dramatic increase in the number of infections caused by drug-resistant bacteria worldwide has driven interest in tracking the environmental distribution of ARBs/ARGs and identifying their associated risk to public health10. The spread of ARBs and ARGs is exacerbated by the exchange of resistance genes between humans or animals and environmental microbiota. ARBs and ARGs are known to enter the environment via a range of pathways, although most studies are focused on farms with food-producing animals, the knowledge about the transmission routes for ARGs and ARBs in soil needs to be complemented. The presence of a mixture of antibiotics and large numbers of bacteria in wastewater, and in activated sewage sludge, encourages the transfer of ARGs, and thus the number of drug-resistant bacteria. For this reason, recent reports emphasize the need to expand the list of emerging contaminants present in sediments with ARB and ARG and to eliminate them from both sediments and fertilized soils11,21,22. Furthermore, the xenobiotics and resistant microorganisms present in wastewater sediments can shape the metabolic activity and diversity of the soil microbial community, and negatively affect the quality of the soil ecosystem12. Soil is the main source of microorganisms in terrestrial ecosystems, and its microbial communities are responsible for a number of metabolic processes that maintain soil welfare and ensure its fertility and quality. They play major roles in the mineralization of organic matter, nutrient availability, soil humus formation, and in limiting the number of pathogens. The land application of sewage sludge can influence the taxonomic structure of the indigenous soil microbial community; therefore, microbiome characteristics could be used as biological indicators to assess soil changes in response to sewage sludge amendment21,23. It was reported that some soil processes, such as nitrification, might be enhanced by fertilization with sewage sludge but at the same time other studies show different trends22,24. Some studies have demonstrated changes in the diversity and functional potential of soil microbial communities after agricultural use of dairy sewage sludge, straw, vermicompost or manures25,26,27; however, there are not many reports on the influence of the taxonomic structure of soil communities after treatment with municipal sewage sludge. Generally, our knowledge of how agricultural management shapes soil microbial community is still largely limited.
The aim of this study was to determine the short-term impacts of municipal sewage sludge application to farmland soil on the (1) soil bacterial community composition and diversity, and (2) the abundance and diversity of antimicrobial resistance genes. The study examined two different types of agricultural soils, i.e. sand and loamy sand, by a metagenomic approach.
Results
Soils characteristics
The soils used in the study were characterized by different granulometric and physicochemical properties (see Table 1). S1 was classified as sandy soil due to the high sand content of up to 85%, and S2 with a different composition as loamy sand (Table 1) according to the USDA and PSSS (Polish Society of Soil Science). Both types of soil are widespread in Poland. The pH value was another property that strongly distinguished both soils, 5.4 for S1 and 8.4 for S2. Moreover, both soils differed considerably in the content of P (0.05 in S1 and 0.16 cmol( +)·kg−1 in S2), Ca2+ (1.56 in S1 and 15.3 cmol( +)·kg−1 in S2), and Na+ (0.04 in S1 and 0.33 cmol( +)·kg−1 in S2). The greater the sum of alkaline cations in the soil and the higher pH value, the more nutrients for plants. This indicates greater availability of nutrients for plants in soil S2. The detailed granulometric composition and physicochemical parameters of both soils are depicted in Table 1, while Table S1 presents properties of sewage sludge.
Characteristics of bacterial population
Relative abundances (%) of prokaryotic communities at the phylum level were described in Fig. 1 and in the supplementary Table S2. Unfertilized soils S1 and S2 have very similar qualitative and quantitative taxonomic profiles at the phylum level. The principal bacterial members in these soils were found to belong to the Planctomycetes (38–48%), Actinobacteria (14–29%), Proteobacteria (13–15%), Chloroflexi (8–11%) and Firmicutes (5–6%) phyla (Fig. 1, Table S2). In turn, these five groups are poorly represented in the sewage sludge, used as a fertilizer (SL), however, sediment is dominated by Proteobacteria (37%), Spirochaetes (11%), Halobacteriota (10.5%) and Deinococcus (8.4%) (Fig. 1, Table S2). The fertilized soils S1SL and S2SL showed more similarities to SL, where the most dominant groups observed in the control soils have been considerably replaced by Proteobacteria and Spirochaetes (Fig. 1).
The relationships between prokaryotic communities at different levels of treatment were investigated with co-occurrence network analysis using Spearman’s correlation (Fig. 2). Relative abundances (%) at the species level were also included in the network, however specific values were described in supplementary Table S3 and Fig. S1. Topological features for the construction of the network were described in supplementary Table S4 and Table S5. The network was constructed with a total of 365 significant correlations between taxa, from which positive relationships were more abundant than negative (222 over 143, respectively, Table S5). The network revealed two clusters composed of taxa mainly observed in the unfertilized soils (S1 S2 and S1), which were distanced from the other three clusters composed of taxa mainly observed for fertilized soils (S1SL S2SL and S2SL) and sewage sludge (SL) (Fig. 2). Such distance was supported by the highest number of negative relationships between the clusters from unfertilized soils when compared to the fertilized soils (138, Table S5), indicating that these treatments were significantly different from each other. In fact, species that were registered in large quantities for unfertilized soils, such as the Planctomycetes Fimbriiglobus ruber (21–27%), Paludisphaera borealis (9–10%), Gemmata obscuriglobus (5–7%) and Sphingulisphaera acidiphila (3–4%) and the Actinobacteria Thermoleophilum album (12–22%) and Patulibacter medicamentivorans (2–7%), were depleted in the fertilized soils (Figs. 2, S1, Table S3). Furthermore, almost no significant correlations were observed between clusters of unfertilized soils and SL (only 2 negative correlations, Table S5), suggesting that prokaryote composition between them is also different. In fact, many species that were registered with high abundance for SL, such as the β-Proteobacteria Thiobacillus denitrificans (9.1%) and Brachymonas denitrificans (7%), the α-Proteobacteria Sphingopyxis granuli (5.2%), the Deinococcus Thermus thermophilus (8.4%), and the Halobacteriota Methanosarcina mazei (10.5%), were not observed in unfertilized soils (Fig. 2, Table S3 and Fig. S1). In contrast, a higher number of positive correlations (34), when compared to negative (2), between fertilized soils (S1SL S2SL and S2SL) and sewage sludge (SL) clusters suggested a greater similarity between these treatments (Table S5). The high relative abundances of shared species between fertilized soils and SL, including the Spirochaetes Leptonema illini (11–19%) and β-Proteobacteria T. denitrificans (5–9%), corroborates the similarity between both treatments (Fig. 2, Table S3 and Fig. S1). An important element differentiating the fertilized soils was the composition of three species of ϒ-Proteobacteria belonging to the Geobacter anodirudecens (17–25%), G. soli (9–12%) and G. sulfurreducens (4–6%), which were generally depleted in any of the other treatments (Fig. 2, Table S3 and Fig. S1).
The number of shared and distinct species between the different types of soils was summarized in the form of Venn diagrams in Fig. 3. A total of twenty six shared prokaryotic taxa were present in both unfertilized S1 and S2 soils (Fig. 3a). The number of shared species increased to eighty between fertilized S1SL and S2SL, and the number of distinct species increased to forty and forty three, respectively (Fig. 3b). In addition, only five species were shared and thirty were distinct between soil S1 and fertilized S1SL, and merely two were shared, and thirty four were exclusive between S2 and S2SL (Fig. 3c,d respectively). In contrast, sixty one taxa were shared for SL and S1SL and forty six for SL and S2SL. However, no prokaryotic species were shared between the sewage sludge and any of the control soils S1 and S2 (Fig. 3c,d).
The differences in soil prokaryotic communities between all samples were described with principal coordinate analysis (PCoA) in Fig. 4. The horizontal axis (coordinate 1–72.6% of variability) indicates no differences in prokaryotic communities between the unfertilized S1 and S2 soils. These soils showed greater differences when compared to the fertilized soils (S1SL and S2SL) and to the sludge sample (Fig. 4a). The vertical axis (coordinate 2–12.9% of variability) indicates variation within replicate samples for the amended soils S1SL and S2SL (Fig. 4a). The two soils demonstrated greater differences in taxa between unfertilized controls and fertilized samples (horizontal axis), than between replicates (vertical axis) (Fig. 4a) which was also observed to be statistically significant (Fig. 4b).
The average abundance of oligotrophic and copiotrophic bacteria per gram of soil or sediment was presented in Fig. 5. The number of both, oligotrophs and copiotrophs in S2 was an order of magnitude higher compared to S1 (Fig. 5a, b), the S2 soil presented over three times more oligotrophs than copiotrophs, and in S1 the numerical ratio was 2:1 (Fig. 5a,b, Table S8). Moreover, the numbers of both group of bacteria and proportion between them in S1 and S2 did not change after seven weeks of experiment (Fig. 5a,b). The number of oligotrophs and copiotrophs in both soils increased by about one order of magnitude after fertilization in day 0, however, seven weeks later the abundance of oligotrophs decreased approximately twofold, whereas the abundance of copiotrophs remained at the same level in both, S1SL and S2SL. Thus, seven weeks after the application of sediment, the numerical ratio of oligotrophs to copiotrophs in both fertilized soils decreased considerably, i.e. approximately twice in S1SL compared to the S1 and as much as tenfold in S2SL compared to the S2 at day 0 (Table S8).
The content of heavy metals and ARGs
The metal content in soils and sludge samples were summarized in Table 2. The very low level of metals was found in all tested soil samples, in some cases at the detection limit. Sewage sludge contained the highest quantity of all analyzed metals. All four experimental soils, both controls and fertilized samples, contained considerably lower levels of metals than SL (Table 2).
The relative abundances (%) of ARGs were compared between different soil treatments and summarized in Fig. 6. Interestingly, ARGs profiles were characterized by high similitude indices between all samples (BC = 0.95–0.98) (Fig. 6). Almost all ARGs displayed the greatest similarity between samples S1SL and SL (0.98), with exception of rifamycin resistance genes (Fig. 6). Sample S2SL also showed high similarity to SL and S1SL (BC = 0.97); however, S2SL presented lower abundances of ARGs regarding fluoroquinolones and aminoglycosides compared to S1SL (Fig. 6); in addition, unfertilized S1 and S2 demonstrated lower relative abundances of ARGs than the other three samples. The two control soils differed in the quantity of ARGs conferring resistance to fluoroquinolones, bacitracin and aminoglycosides (Fig. 6).
The hit numbers of seven groups of ARGs were analyzed in Fig. 7a.The presented results include a set of ARGs for which the largest differences were recorded between samples. It is possible to observe a higher number of ARGs in the heat map profiles for SL, S1SL and S2SL when compared to the controls S1 and S2 (Fig. 7a). Fluoroquinolones, tetracyclines and macrolides resistance genes were the most abundant in the constructed metagenomes for all samples. Four genes associated with the resistance to sulfonamides were also present in large numbers. Populations of genes conferring resistance to vancomycin, aminoglycosides and trimethoprim were also found, but in smaller numbers. The least abundant genes in the tested samples were the genes responsible for resistance to β-lactams and erythromycin (Fig. 7a). The vast majority of genes were more numerous or much more numerous in fertilized soil samples S1SL and S2SL compared to unfertilized S1 and S2. Some genes were even more abundant in fertilized soils than in the sludge itself (Fig. 7a). Cluster analysis based on the content of ARGs in the samples was described in Fig. 7b. The results revealed higher similitude between the amended samples S1SL and S2SL with sludge (BC = 076), when compared to their respective controls S1 and S2 (BC = 0.60) (Fig. 7b).
The diversity, richness and evenness indices according to the relative abundance of antibiotic-resistance genes are presented in Fig. 8a–c. In general, the fertilized soils (S1SL and S2SL) demonstrated higher Shannon Wiener diversity (Fig. 8a), Pielou’s evenness (Fig. 8b) and Chao richness (Fig. 8c.) than their respective controls (S1 and S2). Furthermore, all three indices were generally similar between the fertilized soils (S1SL and S2SL) and SL (Fig. 8a–c). These results suggest that the fertilized soils (S1SL and S2SL) demonstrate greater richness and relative ARG abundance than the controls (S1 and S2), which was most likely associated to the fertilization of soils with sludge. The richness index was arguably the most valuable for describing differences between samples, since fertilized soils generally presented up to 135 (S1SL) and 93 (S2SL) exclusive ARGs which were absent from the respective control soils, S1 and S2 (Fig. 8c). In contrast, the Simpson’s dominance index was lower for the fertilized samples (S1SL, S2SL) and sewage sludge (SL) compared to the controls (Fig. 8d), suggesting that the ARGs were more evenly distributed in the fertilized samples S1SL and S2SL, and sewage sludge (SL) than in the controls (S1, S2). This observation was also supported by the fact that a higher evenness index was recorded for the fertilized samples and sludge sediment than the controls (Fig. 8b).
Discussion
The present study used a metagenomic approach to study the effect of sewage sludge application on soil microbial communities and on the possible spread of ARGs during the seven-weeks field experiment. The two soil types were collected from a rye field (S1) and an onion field (S2), as shown in Table 1; the most significant differences between soils concerned the granulometric properties, pH and the levels of P, Ca and Na ions (Table 1). Our study revealed, that two soils from the different location and of different uses can be characterized by similar proportions of bacterial phyla despite significant differences in soil granulometric properties and pH. The sewage sludge application altered relevantly the structure of soil microbial community compared to unfertilized control soils.
Before fertilization, Planctomycetes and Actinobacteria phyla predominated in both tested soils; these microbes are known to be important components of the soil microbial community, and were the major contributors to the both soils quality before amendment. The Planctomycetes, with dominant species in the present study belonging to F. ruber, G. obscuriglobus, P. borealis and S. acidiphila (Fig. 2, Table S3 and Fig. S1), is regarded as the fifth most abundant bacterial phylum in soil that play key roles in global carbon and nitrogen cycles28,29.
The Actinobacteria, with dominant species in the present study belonging to P. medicamentivorans and T. album (Fig. 2, Table S3 and Fig. S1), is another key group of soil bacteria dominant in the rhizosphere, occupying several different ecological niches, including the ability to thrive in harsh environments, nutrient cycling, plant growth promotion, nitrogen fixation, anti-phytopathogenic and saprophytic activity (animal and plant debris decomposition), among others30,31. They have the genetic potential for the production of a wide spectrum of secondary metabolites32,33,34; indeed, about 10 000 antibiotics, i.e. 45% of all known bioactive microbial metabolites, have been isolated from Actinobacteria35. As such, this phylum has both, considerable ecological and pharmacological potential. A large proportion of Actinobacteria (30%) was found in soil S1 even though the pH was acidic. It has been previously reported that phylum proportions can be strongly influenced by soil pH, especially that Actinobacteria tend to be found in higher proportions in ecosystems, where the pH is relatively high36. However, pH is not the only factor that can influence bacterial community composition. In the present study, seven weeks after treatment with sludge, the abundance of these two bacterial phyla decreased seven- to nine-fold in the fertilized soils, which, considering their complex role played in the ecosystem, is highly undesirable (Fig. 1).
Interestingly, the proportions of the Chloroflexi, Proteobacteria and Firmicutes phyla were essentially similar in both S1 and S2 (Fig. 1). The Chloroflexi, a relatively unexplored phylum with the majority of its representatives being unculturable, has shown to be ubiquitous throughout terrestrial to aquatic environments by the use of culture-independent methods28,37. They are ecologically and physiologically diverse, and often key agents in oxygen-, nutrient‐, and light‐limited environments38,39. Metagenomic analysis has further extended their role in fundamental biogeochemical cycles40,41. In our study, the Chloroflexi was the fourth most numerous phylum in both soils (8% in S1 and 11% in S2). However, 50 days after soil fertilization, their relative abundance decreased drastically to a level comparable to that in sewage sludge (0.8% in S1SL, 1.3% in S2SL, 0.5% in SL) (Fig. 1, Table S2).
The Proteobacteria, a group with large proportions for both soils in the present study (13.5% in S1 and 15% in S2; Fig. 1), is a phylum of Gram-negative bacteria prevalent in soil ecosystems with many members associated with a wide range of functions involved in carbon, nitrogen, and sulphur cycling. However, seven weeks after fertilization, their relative abundance drastically increased in both soils (63% in SSL1 and 50% in S2SL), with the appearance of new species, especially among β-P and Δ-Proteobacteria such as T.denitrificans, Thiobacillus sp. and three species of Geobacter absent previously in unfertilized soils (Fig. 2). Interestingly, they were considerably less abundant in the sludge than in the sludge-impacted S1SL and S2SL (Table S3 and Fig. S1). This indicates that Geobacter has adapted well to the soil environment—a genus capable of dissimilatory reduction of Fe(III) oxides, which is an important process for the oxidation of organic matter in terrestrial anoxic environment42,43,44. Furthermore, four species of α-Proteobacteria that were abundant in S1 and S2 (M. superfactus, M. marginalis, D. thermohalophilum and B. lablabi) decreased considerably following soil treatment with sludge, reaching similar levels as in sewage sludge (Fig. 2, Table S3 and Fig. S1). This decline in S1SL and S2SL may be due to the presence of harmful components or competitive bacteria in the sewage sludge added to the soil.
Spirochaetes bacteria were not detected in S1 or S2 (Fig. 1), with Leptonema illini as the only species observed in fertilized S1SL and S2SL, and sewage sludge. This species found a favorable environment in soils after fertilization, where it multiplied to higher level than in sewage sludge, possibly influenced by sludge components.
Within the phylum Firmicutes, two species dominated in both soils: the spore-forming, thermophilic Hydrogenibacillus schlegelii (Fig. 2)—a facultative anaerobe that can oxidize hydrogen aerobically45, and the moderately-thermophilic facultative anaerobe Limnochorda pilosa (Fig. 2)—capable of denitrification46. Approximately 6% of the prokaryotic community of S1 and S2 comprised taxonomic units that could be considered rare taxa, i.e. whose relative abundance was less than 1%. Jiao and Lu47 and Xiong et al.48, report that the soil and crop system microbiomes comprise a few abundant taxa with a wide niche breadth, and a greater diversity of rare taxa with greater niche specificity. Furthermore, Zhang et al.49 report that within each microbial community, rare species played a more important role in driving ecosystem multifunctionality than abundant species.
The presented results could be compared and discussed on the background of other authors interesting research, who have reported that microbial communities in North American soils tend to be dominated by α-Proteobacteria, Acidobacteria and Actinobacteria, as opposed to the Planctomycetes, Bacteroidetes and Firmicutes which, have typically been found to be less abundant50.
Sewage sludge had an entirely different taxonomic composition to soils, with a much higher proportion of Proteobacteria (38% in sludge versus 13% in S1 and 15% in S2), Spirochaetes (11%), rare taxa (18%), Halobacteriota (10%) and Deinococcus (9%). The PCoA analysis found the addition of sludge composts to soils to result in significant disturbances in the soil microbial community (Fig. 4). Before fertilization, the two soils demonstrated as much as 70% similarity, with this value falling to only 16.6% when comparing S1 with S1SL and 5.8% for S2 and S2SL. The data given in Figs. 1, 2 and 4 suggest that application of sewage sludge had a stronger effect on changes in the bacterial community in S2 than S1.
A soil microbial community comprises a continuum of microorganisms with various carbon requirements. Such bacteria have evolved two distinct ecological strategies according to substrate concentration: oligotrophs favour environments with low levels of nutrients, while copiotrophs (eutrophs) are adapted to live among richer resources. A number of studies suggest that nutrient availability plays an important role in determining the structure and ecological strategy of bacterial communities in nature. Animal-associated microbiota are dominated by copiotrophic bacteria, whereas free-living and plant-associated bacterial communities are mostly dominated by oligotrophs51,52,53. In our study we have adopted the term oligotrophy to estimate bacteria with low requirements in relation to the carbon concentration in their habitat, and copiotrophy to count those with higher requirements. However, this phenomenon is more complex and described in the source literature. The culture method used in the presented study is one of many proposed and described in the literature, though all methods are based on the application of different carbon concentrations in bacteriological media used to differentiate the nutritional requirements of bacterial cells.Although oligotrophs and copiotrophs are ubiquitous in the global ecosystem, their relative abundance and importance in particular ecosystems are still somewhat unclear; therefore, the present study examined the abundance of oligotrophic and copiotrophic bacteria in the analyzed soils. It was found that in both soils, the number of oligotrophic and copiotrophic bacteria increased, and the ratio of oligotrophs to copiotrophs decreased substantially seven weeks after fertilization (Fig. 5). This may indicate that fertilization with sewage sludge may disturb the natural biological balance of the soil, as well as the processes occurring in it, and potential functions of microorganisms as a whole community.
Some studies indicate that around 70% of non-degraded antibiotics are transferred to sewage sludge54. Studies on the long-term exposure of environmental bacterial strains to low concentrations of antibiotics indicate that the subinhibitory concentrations of antimicrobials in many environmental samples may influence bacterial ecology, and could drive the selection of antibiotic-resistant bacterial cells. Such selective pressure may also increase the proliferation of ARGs in soil; this is of particular concern, as soil contains numerous bacterial genera of clinical importance55,56. Furthermore, antimicrobials and resistant bacteria can shape the diversity and metabolic activity of the soil microbial community, thus negatively affecting the quality of the soil ecosystem57. Our findings indicate that the amended soils (S1SL and S2SL) demonstrate greater richness and relative ARG abundance than the controls (S1 and S2), which was most likely related to the fertilization of soils with sewage sludge (Fig. 6; Fig. 8). The most numerous groups of ARGs in the fertilized soils and sewage sludge were those encoding resistance to fluoroquinolones, macrolides, tetracyclines and sulfonamides; this coincides with the list of antibiotics most widely prescribed in human medicine (tetracyclines, macrolides, β-lactams) and veterinary medicine (tetracyclines, sulfonamides, β-lactams)58,59,60. Furthermore, numerous studies have reported the presence of quinolone, tetracycline macrolide, and sulfonamide antibiotics in sewage sludge61,62,63.
Synthetic and semi-synthetic antibiotic residues, such as fluoroquinolones and sulfonamides, possess high chemical stability and resistance to degradation, and are hence often detected in the environment64,65. This may explain the high abundance of resistance genes to these antibiotics in the sewage sludge and sludge-fertilized soils used in our experiment. Prolonged exposure to subinhibitory concentrations of antimicrobials may favours the horizontal transfer of drug resistance genes (HGT-horizontal gene transfer) between bacterial cells; this transfer can occur between different species and genera, and between non-pathogenic bacteria and pathogens, resulting in the selection of resistant bacterial cells10,66,67,68,69,70,71. Some vancomycin resistance genes were also found to be more prevalent in the fertilized soil samples than the control soils; higher abundance of these genes is clearly marked in amended soil, even assuming that soil-autochthonous Gram-negative bacteria are, to some extent, naturally resistant to vancomycin due to their cell wall properties. The genes conferring resistance to vancomycin are of particular environmental concern; their concentrations, as well as those of ARGs offering resistance to tetracyclines, macrolides and polymyxin, can increase in sewage sludge after anaerobic digestion in WWTP72,73. Furthermore, although β-lactams are among the most frequently prescribed in both, human and veterinary medicine, β-lactam ARGs were not found to be as abundant in our fertilized S1SL and S2SL soils (Fig. 7). The presented results include a set of ARGs for which the largest differences were recorded between samples, excluding a considerable number of those, for which no strong differences were noted. This study opens questions for more detailed analyses with a larger number of sewage sludge from several WWTPs, and the employing of more comprehensive analytical techniques to capture the full spectrum of ARGs and integrons present in the sewage sludge and soil microbial community.
A number of studies has demonstrated that the use of sewage sludge as fertilizer can increase the concentrations of heavy metals in soil74,75,76,77. As such, Polish regulations specify that sewage sludge used for agricultural purposes must meet certain standards with regard to heavy metal content. However, the level of heavy metals in the sewage sludge used in our study was only a minor percentage of the maximum loads allowed by the Polish regulations78, amounting to 6.6% for cadmium, 12.2% for copper, 4.5% for nickel, only 1.8% for lead, 6% for chromium and 25% for zinc. Such low levels did not have a significant effect on their content in the fertilized soils.
The aim of the study was to assess the impact on the soil microbial community and resistome of sewage sludge from a particular municipal WWTP in central Poland, from which sludge is used for fertilizing agricultural soils on a regular basis; the research was conducted as a preliminary, semi-quantitative analysis. The authors are aware that the presented research is limited to an experiment conducted on a single sample of sewage sludge, which may not be representative of other types of sewage sludge used in agriculture. To address these challenges, further study has been undertaken by the authors, that will aim to collect a more diverse range of sewage sludge samples from WWTPs of various sizes, which used different wastewater and sewage sludge treatment methods; the conversion of sewage sludge to a soil fertilizer can be performed by a number of methods, which greatly differ by physicochemical conditions, treatment time, and substrate/amendment composition79,80,81,82.
The complex structure of sewage sludge, which include antibiotics, microplastics, heavy metals and other composite pollutants, is an important barrier for the removal of ARGs83. Although, different treatments have been pointed out to reduce ARB and ARGs in sewage sludge, including stabilization, dewatering, anaerobic digestion, aerobic composting and sludge conditioning84, suitable treatment technologies are jet to be identified for specific sludge properties. Anaerobic digestion and aerobic composting were described to be the most effective treatments methods to remove ARGs, however, current methods cannot completely remove the ecological risk. Further solutions improving ARB and ARGs removal include sludge pretreatment, i.e.: addition of coagulants (Fe3+, Al3+ and free ammonia), thermal hydrolysis, alkaline and ultrasonic methods before anaerobic digestion, or bioleaching and chemical conditioning (Fe3+/CaO) before aerobic composting, among others83. Several different pre-treatments and modifications of sewage sludge management methods have been recently described, although it was clearly pointed out that proper methods to achieve high ARB and ARGs removal will largely depend on the local sludge composition and properties83. Therefore, it is highly recommended to track ARGs in produced sewage sludge to generate predictions for future risk assessment. Furthermore, this could help to identify the most appropriate treatment method for the local composition of sewage sludge prior its use as an agricultural fertilizer.
Conclusions
This metagenomic study extends the knowledge of soil microbial community and resistome after application of sewage sludge. The research revealed that initially both tested soils, despite differences in their granulometric and physicochemical properties, were dominated by the same bacterial phyla. However, the soils differed in abundance of oligotrophic and copiotrophic bacteria. Our study revealed, that two soils from the different location and of different uses can be characterized by similar proportions of bacterial phyla. Network analysis revealed that the changes occurring in the bacterial structure of both soils were of a similar nature and scale; fertilization tended to favor an increase in Proteobacteria, particularly in β-Proteobacteria and Δ-Proteobacteria in amended soils. Moreover, sewage sludge was a vast repository of ARGs, however it was characterized by low heavy metal content; amendment with sewage sludge negatively affect the richness and relative ARGs abundance in soil. The greatest increase in abundance of ARGs concerned resistance genes to the antibiotics most commonly used in human medicine and veterinary, this may pose a risk to the public health. Our findings provide the data that, alongside other scientific reports, highlight the need to critically revise the use of municipal sewage sludge for agricultural purposes85,86,87,88. To meet the urgent need for sustainable environmental and agricultural management, modern research techniques that enable a broader approach to soil quality should be widely used. Furthermore, to prevent the ARBs and ARGs contamination of soil, and frame a rational plan of response to this type of environmental threat, it is crucial to identify and track its sources. Studies that are conducted worldwide have regard to different types of soils, distinct climatic zones and different sampling times. Most importantly, the wastewater treatment methods used in different WWTPs vary from country to country and even from one WWTP to another. The method of pretreatment and the dose of sewage sludge applied, are also essential. All of the above factors should be taken into account in comprehensive research, which in turn should be the basis for the elaboration of appropriate, commonly used legal acts.
Materials and methods
Soil and sewage sludge characteristics
The study used two types of soil collected from two farmlands located in the Lodz region, Central Poland: S1 from a rye field (latitude—51.917321 N, longitude—19.442669 E) and S2 from an onion field (latitude—52.014598 N, longitude—19.310026 E). The soil sample collection sites were approximately 17 km apart. The sites were farmed to meet the own needs of the farms, and not for commercial purposes. S1 was classified as a sand according to the Soil Taxonomy USDA (United States Department of Agriculture) and PSSS (Polish Society of Soil Science)89, and S2 as a loamy sand. The picture of soils was attached as Supplementary Fig. S2.
Three 0–10 cm soil cores were collected from random sites on each farm using sterile polycarbonate tubes, and were composited into one sample to account for soil heterogeneity. The samples were transported on ice to the laboratory, where they were homogenized by hand and stored at 4 °C until analysis. The sewage sludge was collected from the large (class IV) municipal wastewater treatment plant (WWTP) located in central Poland, from which it is used for soil fertilization on a regular basis. The experiment was made in early autumn.
Wastewater treatment plants are graded by size based on population equivalent (p.e.) and wastewater outflow as specified in Polish regulations. A class IV WWTP serves 15,000–99,999 population equivalents—based on the provisions of the Regulation of the Minister of Maritime Economy and Inland Navigation, Journal of Laws, 2019, item 1311, dated 12 July 2019, which implements the provisions of Council Directive 91/271/EEC. The sampled plant is a mechanical and biological sewage treatment plant with chemical support for phosphorus precipitation and the processing of excess sludge generated by autothermal thermophilic sludge stabilization. Its task is to process social, domestic and industrial sewage from the local area, as well as sewage transported by truck from areas not covered by the sewerage system. The particular WWTP is impacted by both industrial (knitting and hosiery) and anthropogenic activity in its catchment.
Pot experiment
The soil and sludge were crushed and sieved through a 2 mm mesh, the soil was fertilized with sewage sludge at a loading rate of 9 tons per hectare, the dose recommended by Polish Law90, then 1 kg of soil, fertilized soil and sewage sludge were loaded into each 1 L pot. The experiment was conducted for seven weeks under field conditions. Samples were collected on day zero for microbiological analysis and again on day 50 for metagenomics and microbiological analysis. Irrigation was performed using distilled and filtered (0.22 µm pore size) water throughout the experiment to avoid introducing extraneous bacterial cells and ARGs into the treated samples (S1SL and S2SL) and samples of soils without sewage sludge (S1 and S2) and sewage sludge alone (SL) as controls.
Physico-chemical analysis
Organic matter was removed from the samples by combustion of at medium temperature (375–800 °C) in a temperature-regulated muffle furnace79, following which, dry ash content was determined. It is important to note that values derived from loss-on-ignition results should only be considered as approximate91. The pH was analyzed potentiometrically in H2O and 1 mol dm3 KCl based on air-dried fine earth samples using a soil/solution ratio of 1:2.5. The pH of the soil was determined potentiometrically in accordance with standards92. The available forms of phosphorus (P) and potassium (K) were determined using the Egner-Riehm method93. The exchangeable forms of magnesium (Mg) were determined using a buffered barium chloride solution (pH 8.1)82. Soil carbon (C), hydrogen (H) and nitrogen (N) contents were determined by dry combustion using a CHN elemental analyzer (CHNS, Perkin Elmer, Series II). Exchangeable bases (EB) (i.e., Ca, Mg, K, and Na) were extracted from the soils using 1 mol dm3 ammonium chloride at pH 8.2. The samples were washed once using deionized water and water-soluble salts were removed by exchangeable base extractions. Base contents in extracts were measured using flame atomic absorption spectrometry (Ca and Mg) and flame emission spectroscopy (K and Na). Trace element (Cd, Cr, Ni, Zn, Pb, Cu, Cr, Mn, Fe) concentrations were determined after hot digestion in a mixture of HNO3 and HClO4 (3:2 v/v). The analysis was performed using an inductively-coupled plasma optical emission spectrophotometer (Perkin Elmer ICP-OES Optima 7300 DV) according to US EPA Method 200.794. The quality of the analysis was verified by comparison with a certified reference material (CRM023–050). The recoveries for metals ranged from 89 to 102%. Samples were analyzed in three replicates, for which the relative standard deviations (%RSDs) were less than 10%.
Microbiological analyses
Briefly, 10 g samples were suspended in 90 ml of autoclaved water and shaken on a rotary shaker at 120 rpm for half an hour at room temperature. A series of dilutions from 10−1 to 10−7 was prepared in sterile 0.85% NaCl, and 100 µl of each dilution was plated on to media. Microbiological media according to Hattori and Hattori95 was used to estimate the number of copiotrophs (NA- nutrient agar) and oligotrophs (NA diluted 100 times in sterile water). The media were supplemented with 50 µg∙ml−1 of cycloheximide (Sigma-Aldrich) to avoid fungal growth. The plates were incubated at 25 °C for seven days for copiotrophs and 21 days for oligotrophs before counting. All experiments were performed in triplicate, and all bacterial counts were expressed as colony-forming units (CFU) per 1 g of dry soil or sewage sludge.
Metagenomic DNA isolation and Shotgun sequencing
Total genomic DNA was extracted from 500 mg (wet mass) of soil and sewage sludge using the FastDNA™ SPIN Kit for Soil (MP Biomedicals, Santa Ana, CA), procedure was conducted according to the manufacturer. The concentration and purity of DNA were estimated by agarose gel electrophoresis and ultraviolet absorbance (Multiscan Sky, Thermo Scientific Inc.). DNA was stored at -200C for further analysis. DNA libraries were processed using the NexteraXT DNA library preparation kit (Illumina) according to the manufacturer’s instructions. The quality of the libraries was assessed on the Agilent Bioanalyzer 2100 system with the Agilent High Sensitivity DNA kit. The libraries were normalized with qPCR using the NEBNext Library Quant Kit for Illumina (New England Biolabs). Metagenomics were performed by shotgun sequencing with the use of the Illumina NovaSeq 6000 platform; the procedure was based on paired-end reads of 2 × 150 bp and a maximum assumption of 40 million paired reads per sample. Original datasets as FASTQ files were uploaded to the NCBI Sequence Read Archive under the project PRJNA1067294, with bio samples for S1 (SAMN39522689—SAMN39522691), S2 (SAMN39522692—SAMN39522694), S1SL (SAMN39522697—SAMN39522699), S2SL (SAMN39522700—SAMN39522702), and SL (SAMN39522695—SAMN39522696).
Bioinformatic analysis
Sequences were edited before formal analysis. First, they were pre-trimmed to reduce sample contamination, a palindromic algorithm was used for sequence alignment with appropriate adaptors. The trimmed sequences were mined for the presence of antibiotic-resistance genes using the DeepARG tool in the conda environment for Python 2. Short sequences (Shotgun) were analyzed as reads according to Arango-Argoty et al.,96. The database hosted by Zenodo (https://zenodo.org/records/8280582) was used to identify ARG-like ORFs with a default condition of probability ≥ 80%. Hit numbers of filtered ARGs were normalized with the 16S rRNA gene using the Kraken2 tool and the results were scaled in a 1:100,000 ratio to optimize their interpretation. Taxonomic units were also classified with Kaiju software to phylum, genus and species level, according to Menzel et al.97. Sequences were filtered according to recommended default parameters (length ≥ 11 aa, match score ≥ 65, and e-value ≥ 1 × 10–2). The reference database of kaiju proGenomes v3 was chosen for taxonomical characterization (https://progenomes.embl.de). For the purpose of the present study, only sequences belonging to bacteria and archaea were considered for analysis.
Analysis of data
Bacterial and archaeal taxonomic data was visualized with the phyloseq package. The taxa that were exclusive to each sample, and those that were shared, were plotted in venn diagrams with the ggvenn package, both in R environment. Furthermore, distance between sample replicates was visualized with principal coordinate analysis (PCoA) according to the taxonomical composition. Significant differences between samples were tested with the Kruskal–Wallis and Mann–Whitney test pairwise. Alpha diversity indices, including Shannon–Wiener (H), Richness (Chao), Pielou’s eveness (J) and Simpson’s dominance (D), were used to describe the composition of ARGs in the samples. Finally, cluster analysis based on the Bray Curtis similarity index was used to visualize the differences in ARG composition and metal concentration between samples. The PCoA, statistical differences, diversity and cluster analyses were performed with PAST 4.12 software98.
Co-occurrence network analysis was performed to investigate the relationship between microbial communities at different levels of treatment. The network was constructed and visualized with the software Cytoscape 3.10.2 (https://cytoscape.org/), focusing on prokaryote interactions with high and significant Spearman’s correlations (rs > 0.56 and p < 0.05). The significance (p values) was adjusted for multiple testing with Bonferroni correction. Topological features were used to construct the network, including nodes as an estimable species marker (prokaryote) and edges as the correlation weight between two defined nodes. Positive and negative correlations between nodes were used to identify key taxa that were replaced or enriched in amended soils (S1SL and S2SL), when compared to sewage sludge (SL) and the control soils (S1 and S2).
Data availability
Original datasets as FASTQ files were uploaded to the NCBI Sequence Read Archive under the project PRJNA1067294, with bio samples for S1 (SAMN39522689—SAMN39522691), S2 (SAMN39522692—SAMN39522694), S1SL (SAMN39522697—SAMN39522699), S2SL (SAMN39522700—SAMN39522702), and SL (SAMN39522695—SAMN39522696).
References
Bastida, F., Selevsek, N., Torres, I., Hernandez, T. & Garcia, C. Soil restoration with organic amendments: Linking cellular functionality and ecosystem processes. Sci. Rep. 5, 15550. https://doi.org/10.1038/srep15550 (2015).
WWAP (2017) The United Nations world water development report. Wastewater: The Untapped Resource (Cambridge University Press, Paris, 2017).
Tyrrell, C., Burgess, C. M., Brennan, F. P. & Walsh, F. Antibiotic resistance in grass and soil. Biochem. Soc. Trans. 47, 477–486. https://doi.org/10.1042/BST20180552 (2019).
Collivignarelli, M. C. et al. Legislation for the reuse of biosolids on agricultural land in Europe: Overview. Sustainability. 11(21), 6015. https://doi.org/10.3390/su11216015 (2019).
Shaddel, S., Bakhtiary-Davijany, H., Kabbe, C., Dadgar, F. & Østerhus, S. W. Sustainable sewage sludge management: From current practices to emerging nutrient recovery technologies. Sustainability 11(12), 3435. https://doi.org/10.3390/su11123435 (2019).
Boudjabi, S. & Chenchouni, H. On the sustainability of land applications of sewage sludge: How to apply the sewage biosolid in order to improve soil fertility and increase crop yield. Chemosphere 282, 131122. https://doi.org/10.1016/j.chemosphere.2021.131122 (2021).
Fijałkowski, K., Rorat, A., Grobelak, A. & Kacprzak, M. J. The presence of contaminations in sewage sludge: The current situation. J. Environ. Manag. 203, 1126–1136. https://doi.org/10.1016/j.jenvman (2017).
Östman, M., Lindberg, R. H., Fick, J., Björn, E. & Tysklind, M. Screening of biocides, metals and antibiotics in Swedish sewage sludge and wastewater. Water Res. 15(115), 318–328. https://doi.org/10.1016/j.watres.2017.03.011 (2017).
Liew, C. S. et al. A review on recent disposal of hazardous sewage sludge via anaerobic digestion and novel composting. J. Hazard. Mater. Part A https://doi.org/10.1016/j.jhazmat.2021.126995 (2022).
Serwecinska, L. Antimicrobials and antibiotic-resistant bacteria: A risk to the environment and to public health. Water 12, 3313. https://doi.org/10.3390/w12123313 (2020).
Buta, M., Hubeny, J., Zieliński, W., Harnisz, M. & Korzeniewska, E. Sewage sludge in agriculture: The effects of selected chemical pollutants and emerging genetic resistance determinants on the quality of soil and crops: A review. Ecotoxicol. Environ. Saf. 214, 112070. https://doi.org/10.1016/j.ecoenv.2021.112070 (2021).
Markowicz, A., Bondarczuk, K., Cycoń, M. & Sułowicz, S. Land application of sewage sludge: Response of soil microbial communities and potential spread of antibiotic resistance. Environ. Pollut. 271, 116317 (2021).
FAO. The State of World Fisheries and Aquaculture,in: Contributing to Food Security and Nutrition for All (FAO Press, Rome, https://www.fao.org/3/a-i5555e.pdf 2016).
WHO, Food and Agricultural Organization of the United Nations, World Organisation for Animal Health, in: Monitoring Global Progress on Addressing Antimicrobial Resistance: Analysis Report of the Second Round of Results of AMR Country Self-Assessment Survey (WHO Press, 2018).
ECDC, Antimicrobial Consumption Report https://www.ecdc.europa.eu/en/antimicrobial-consumption/database/rates-country? (2020).
Denissen, J. et al. Prevalence of ESKAPE pathogens in the environment: Antibiotic resistance status, community-acquired infection and risk to human health. Int. J. Hyg. Environ. Health 244, 114006 (2022).
Kasanga, M. et al. Antimicrobial resistance patterns and risk factors associated with ESBL-producing and MDR Escherichia coli in hospital and environmental settings in Lusaka, Zambia: Implications for one health. Microorganisms 11, 1951. https://doi.org/10.3390/microorganisms11081951 (2023).
Serwecińska, L., Kiedrzyńska, E. & Kiedrzyński, M. A cachment-scale assessment of the sanitary conditions of treated wastewater and river water based on fecal indicator bacteria and carbapenem-resistant Acinetobacter spp.. Sci. Total Environ. 750, 142266. https://doi.org/10.1016/j.scitotenv.2020.142266 (2021).
Bumbangi, F. N. et al. Evidence of community-wide spread of multi-drug resistant Escherichia coli in young children in Lusaka and Ndola Districts, Zambia. Microorganisms 10, 1684 (2022).
Ito, H. et al. Social dilemma in the excess use of antimicrobials incurring antimicrobial resistance. Sci. Rep. 12, 21084. https://doi.org/10.1038/s41598-022-25632-1 (2022).
Wang, M. et al. Long-term biosolids application alters the composition of soil microbial groups and nutrient status in a pine plantation. Biol. Fert. Soils 53, 799–809 (2017).
Markowicz, A., Bondarczuk, K., Wiekiera, A. & Sułowicz, S. Is sewage sludge a valuable fertilizer? A soil microbiome and resistome study under field conditions. J Soils Sedim. 21, 2882–2895. https://doi.org/10.1007/s11368-021-02984-1 (2021).
Pardo, T., Clemente, R., Epelde, L., Garbisu, C. & Bernal, M. P. Evaluation of the phytostabilisation efficiency in a trace elements contaminated soil using soil health indicators. J. Hazard Mater. 268, 68–76 (2014).
Kelly, J. J., Policht, K., Grancharova, T. & Hundal, L. S. Distinct responses in ammonia-oxidizing archaea and bacteria after addition of biosolids to an agricultural soil. Appl. Environ. Microbiol. 77, 6551–6558 (2011).
Ros, M., Klammer, S., Knapp, B., Aichberger, K. & Insam, H. Long term effects of soil compost amendment on functional and structural diversity and microbial activity. Soil Use Manag. 22, 209–218 (2006).
Frąc, M., Oszust, K. & Lipiec, J. Community Level Physiological Profiles (CLPP), characterization and microbial activity of soil amended with dairy sewage sludge. Sensors 12, 3253 (2012).
Tian, X. et al. Responses of soil microbial community structure and activity to incorporation of straws and straw biochar and their effects on soil respiration and soil organic carbon thurnover. Pedosfere 29, 492–503 (2019).
Delgado-Baquerizo, M. A global atlas of the dominant bacteria found in soil. Science 359(6373), 320–325. https://doi.org/10.1126/science.aap9516 (2018).
Wiegand, S., Jogler, M. & Jogler, Ch. On the maverick Planctomycetes. FEMS Microbiol. Rev. 42, 739–760. https://doi.org/10.1093/femsre/fuy029 (2018).
van der Meij, A. et al. Inter- and intracellular colonization of Arabidopsis roots by endophytic actinobacteria and the impact of plant hormones on their antimicrobial activity. Antonie Van Leeuwenhoek 111, 679–690. https://doi.org/10.1007/s10482-018-1014-z (2018).
Narsing Rao, M. P., Lohmaneeratana, K., Bunyoo, C. & Thamchaipenet, A. Actinobacteria-plant interactions in alleviating abiotic stress. Plants 11, 21. https://doi.org/10.3390/plants11212976 (2022).
Lam, K. S. Discovery of novel metabolites from marine actinomycetes. Curr. Opin. Microbiol. 9, 245–251. https://doi.org/10.1016/j.mib.2006.03.004 (2006).
Lewin, G. R. et al. Evolution and ecology of Actinobacteria and their bioenergy applications. Annu. Rev. Microbiol. 70, 235–254. https://doi.org/10.1146/annurev-micro-102215-095748 (2016).
Sivakala, K. K. et al. Desert environments facilitate unique evolution of biosynthetic potential in Streptomyces. Molecules 26(3), 588 (2021).
Barka, E. A. et al. Taxonomy, physiology, and natural products of Actinobacteria. Microbiol. Mol. Biol. Rev. 80, 1–43. https://doi.org/10.1128/MMBR.00019-15 (2016).
Lauber, C. L., Hamady, M., Knight, R. & Fierer, N. Pyrosequencing-based assessment of soil pH as a predictor of soil bacterial community structure at the continental scale. Appl Environ Micobial 75, 5111–20 (2009).
Mehrshad, M. et al. Hidden in plain sight-highly abundant and diverse planktonic freshwater Chloroflexi. Microbiome 6(1), 176. https://doi.org/10.1186/s40168-018-0563-8 (2018).
Hug, L. A. et al. Community genomic analyses constrain the distribution of metabolic traits across the Chloroflexi phylum and indicate roles in sediment carbon cycling. Microbiome 1, 22. https://doi.org/10.1186/2049-2618-1-22 (2013).
Ward, L. M., Hemp, J., Shih, P. M., McGlynn, S. E. & Fischer, W. W. Evolution of phototrophy in the Chloroflexi phylum driven by horizontal gene transfer. Front. Microbiol. 9, 260. https://doi.org/10.3389/fmicb.2018.00260 (2018).
Gaisin, V. A. et al. Chloroflexus islandicus sp. nov., a thermophilic filamentous anoxygenic phototrophic bacterium from a geyser. Int. J. Syst. Evol. Microbiol. 67, 1381–1386. https://doi.org/10.1099/ijsem.0.001820 (2017).
Tang, K. H. et al. Complete genome sequence of the filamentous anoxygenic phototrophic bacterium Chloroflexus aurantiacus. BMC Genomics 12, 334. https://doi.org/10.1186/1471-2164-12-334 (2011).
Thamdrup, B. Bacterial manganese and iron reduction in aquatic sediments in: Advances in microbial ecology 16, 41–84 (Schink, B., Kluwer/Plenum, New York, 2000)
Straub, K. L. & Schink, B. Ferrihydrite reduction by Geobacter species is stimulated by secondary bacteria. Arch. Microbiol. 182, 175–181 (2004).
Lovley, D. R. et al. Geobacter: The microbe electric’s physiology, ecology, and practical applications. Adv Microb Physiol. 59, 1–100. https://doi.org/10.1016/B978-0-12-387661-4.00004-5 (2011).
Maker, A., Hemp, J., Pace, L. A., Ward, L. M. & Fischer, W. W. Draft genome sequence of Hydrogenibacillus schlegelii MA48, a deep-branching member of the Bacilli class of firmicutes. Genome Announc. 5(3), e00380-e416. https://doi.org/10.1128/genomeA.00380-16 (2017).
Watanabe, M., Kojima, H. & Fukui, M. Limnochorda pilosa gen. nov., sp. nov., a moderately thermophilic, facultatively anaerobic, pleomorphic bacterium and proposal of Limnochordaceae fam nov., Limnochordales ord. nov. and Limnochordia classis nov. in the phylum Firmicutes. Int. J. Syst. Evol. Microbiol. 65, 2378–2384. https://doi.org/10.1099/ijs.0.000267 (2015).
Jiao, S. & Lu, Y. Soil pH and temperature regulate assembly processes of abundant and rare bacterial communities in agricultural ecosystems. Environ. Microbiol. 22, 1052–1065. https://doi.org/10.1111/1462-2920.14815 (2020).
Xiong, C. et al. Rare taxa maintain the stability of crop mycobiomes and ecosystem functions. Environ. Microbiol. 23, 1907–1924 (2021).
Zhang, H. et al. Interaction and assembly processes of abundant and rare microbial communities during a diatom bloom process. Environ. Microbiol. 22, 1707–1719. https://doi.org/10.1111/1462-2929.14820 (2020).
Fierer, N. & Jackson, R. B. The diversity and biogeography of soil bacterial communities. Proc Natl Acad Sci U S A 103, 626–631. https://doi.org/10.1073/pnas.0507535103 (2006).
Koch, A. L. Oligotrophs versus copiotrophs. In BioEssays 23 657–661 (John Wiley & Sons, 2001).
Nemergut, D. R. et al. Decreases in average bacterial community rRNA operon copy number during succession. ISME J. 10, 1147–1156. https://doi.org/10.1038/ismej.2015.191 (2016).
Gao, Y. & Wu, M. Free-living bacterial communities are mostly dominated by oligotrophs. bioRxiv. CSH, https://doi.org/10.1101/350348 (2018).
Sun, C., Li, W., Chen, Z., Qin, W. & Wen, X. Responses of antibiotics, antibiotic resistance genes, and mobile genetic elements in sewage sludge to thermal hydrolysis pre-treatment and various anaerobic digestion conditions. Environ. Int. 133, 105156. https://doi.org/10.1016/j.envint.2019.105156 (2019).
Tello, A., Austin, B. & Telfer, T. C. Selective pressure of antibiotic pollution on bacteria of importance to public health. Environ. Health Perspect. 120, 1100–1106 (2012).
Potron, A., Poiller, L. & Nordmann, P. Emerging Broad-spectrum resistance in Pseudomonas aeruginosa and Acinetobacter baumannii: Mechanisms and epidemiology. Int. J. Antimicrob. Agents 45, 568–585 (2015).
Knapp, C. W., Dolfing, J., Ehlert, P. A. I. & Graham, D. W. Evidence of increasing antibiotic resistance gene abundances in archived soils since 1940. Environ. Sci. Technol. 44, 580–587 (2010).
Tasho, R. P. & Cho, J. Y. Veterinary antibiotics in animal waste, its distribution in soil and uptake by plants: A review. Sci. Total Environ. 563–564, 366–376. https://doi.org/10.1016/j.scitotenv.2016.04.140 (2016).
Spielmeyer, A. Occurrence and fate of antibiotics in manure during manure treatments: A short review. Sustain. Chem. Pharm. 9, 76–86. https://doi.org/10.1016/j.scp.2018.06.004 (2018).
ECDC, 2020. Distribution of Antibacterials for Systemic Use in the Community and Hospital Sector https://www.ecdc.europa.eu/en/antimicrobial-consumption/database/distribution-by-antimicrobial-group (2020).
Li, M. et al. Simultaneous analysis of 45 pharmaceuticals and personal care products in sludge by matrix solid-phase dispersion and liquid chromatography tandem mass spectrometry. Anal. Bioanal. Chem. 408, 4953–4964. https://doi.org/10.1007/s00216-016-9590-0 (2016).
Cheng, M., Wu, L., Huang, Y., Luo, Y. & Christie, P. Total concentrations of heavy metals and occurrence of antibiotics in sewage sludges from cities throughout China. J. Soils Sedim. 14, 1123–1135. https://doi.org/10.1007/s11368-014-0850-3 (2014).
Ashfaq, M. et al. Occurrence and ecological risk assessment of fluoroquinolone antibiotics in hospital waste of Lahore, Pakistan. Environ. Toxicol. Pharmacol. 42, 16–22. https://doi.org/10.1016/j.etap.2015.12.015 (2016).
Sittig, S. et al. Dynamics of transformation of the veterinary antibiotic sulfadiazine in two soils. Chemosphere 95, 470–477. https://doi.org/10.1016/j.chemosphere.2013.09.100 (2014).
Rusch, M., Spielmeyer, A., Zom, H. & Hamscher, G. Degradation and transformation of fluoroquinolones by microorganisms with special emphasis on ciprofloxacin. Appl. Microbiol. Biotechnol. 103, 6933–6948 (2019).
Chow, L. K. M., Ghaly, T. M. & Gillings, M. R. A survey of sub-inhibitory concentrations of antibiotics in the environment. J. Environ. Sci. 99, 21–27 (2021).
Blázquez, J., Couce, A., Rodríguez-Beltrán, J. & Rodríguez-Rojas, A. Antimicrobials as promoters of genetic variation. Curr. Opin. Microbiol. 15, 561–569 (2012).
Ding, M. et al. Subinhibitory antibiotic concentrations promote the horizontal transfer of plasmid-borne resistance genes from Klebsiellae pneumoniae to Escherichia coli. Front Microbiol. https://doi.org/10.3389/fmicb.2022.1017092 (2022) (PMID:36419429;PMCID:PMC9678054).
Chow, L. K. M., Ghaly, T. M. & Gillings, M. R. A survey of sub-inhibitory concentrations of antibiotics in the environment. J. Environ. Sci. 99, 21–27. https://doi.org/10.1016/j.jes.2020.05.030 (2021).
Sanchez-Cid, C. et al. Gentamicin at sub-inhibitory concentrations selects for antibiotic resistance in the environment. ISME Commun. 2, 29. https://doi.org/10.1038/s43705-022-00101-y (2022).
Jutkina, J., Marathe, N. P., Flach, C. F. & Larsson, D. G. J. Antibiotics and common antibacterial biocides stimulate horizontal transfer of resistance at low concentrations. Sci. Total Environ. 616–617, 172–178. https://doi.org/10.1016/j.scitotenv.2017.10.312 (2018).
Yang, Y., Li, B., Zou, S., Fang, H. H. P. & Zhang, T. Fate of antibiotic resistance genes in sewage treatment plant revealed by metagenomic approach. Water Res. 62, 97–106. https://doi.org/10.1016/j.watres.2014.05.019 (2014).
Karkman, A. et al. High-throughput quantification of antibiotic resistance genes from an urban wastewater treatment plant. FEMS Microbiol. Ecol. 92, 1–7. https://doi.org/10.1093/femsec/fiw014 (2016).
Marguí, E., Iglesias, M., Camps, F., Sala, L. & Hidalgo, M. Long-term use of biosolids as organic fertilizers in agricultural soils: Potentially toxic elements occurrence and mobility. Environ. Sci. Pollut. Res. Int. 23, 4454–4464. https://doi.org/10.1007/s11356-015-5618-9 (2016).
Sohail S., Fraz Ali M., Zulfiqar U., Hussain S., Khosa S. Influence of sewage sludge and heavy fertilization on nitrate leaching in soils: An overview. In A. Mustafa & M. Naveed (Eds.), Soil Contamination – Recent Advances and Future Perspectives. IntechOpen, https://doi.org/10.5772/intechopen.107056 (2022).
Marin, E. & Rusanescu, C. O. Agricultural use of urban sewage sludge from the wastewater station in the municipality of Alexandria in Romania. Water 15(3), 458. https://doi.org/10.3390/w15030458 (2023).
Balkrishna, A. et al. Reuse of sewage sludge as organic agricultural products: An efficient technology-based initiative. Appl. Environ. Soil Sci. https://doi.org/10.1155/2024/1433973 (2024).
Dz0.U. z 2013 r. poz 21. https://isap.sejm.gov.pl/isap.nsf/download.xsp/WDU20130000021/T/D20130021L.pdf (2013).
Rahube, T. O. et al. Impact of fertilizing with raw or anaerobically digested sewage sludge on the abundance of antibiotic-resistant coliforms antibiotic resistance genes, and pathogenic bacteria in soil and on vegetables at harvest. Appl. Environ. Microbiol. 80(22), 6898. https://doi.org/10.1128/AEM.02389-14 (2014).
Nascimento, A. L. et al. Sewage sludge microbial structures and relations to their sources, treatments, and chemical attributes. Front Microbiol. 3(9), 1462. https://doi.org/10.3389/fmicb.2018.01462 (2018) (PMID:30018612;PMCID:PMC6037839).
Murray, R., Tien, Y.-C., Scott, A. & Topp, E. The impact of municipal sewage sludge stabilization processes on the abundance, field persistence, and transmission of antibiotic resistant bacteria and antibiotic resistance genes to vegetables at harvest. Sci. Total Environ. 651, 1680–1687 (2019).
Wolters, B. et al. Biosolids for safe land application: Does wastewater treatment plant size matters when considering antibiotics, pollutants, microbiome, mobile genetic elements and associated resistance genes?. Environ. Microbiol. 24(3), 1573–1589. https://doi.org/10.1111/1462-2920.15938 (2022).
Yin, S. et al. Performance of sewage sludge treatment for the removal of antibiotic resistance genes: Status and prospects. Sci. Total Environ. 907, 167862. https://doi.org/10.1016/j.scitoenv.2023.167862 (2024).
Munir, M., Wong, K. & Xagoraraki, I. Release of antibiotic resistance bacteria and genes in the effluent and biosolids of five wastewater utilities in Michingan. Water Res. 45, 681–693. https://doi.org/10.1016/j.watres.2010.08.033 (2011).
Chen, Q. et al. Long-term field application of sewage sludge increases the abundance of antibiotic resistance genes in soil. Environ. Inter. 92–93, 1–10 (2016).
Lau, C.H.-F. et al. Impact of pre-application treatment on municipal sludge composition, soil dynamics of antibiotic resistance genes, and abundance of antibiotic-resistance genes on vegetables at harvest. Sci. Tot. Environ. 587–588, 214–222 (2017).
Magid, J., Pedersen, K. E., Hansen, M., Cedergreen, N. & Brandt, K. K. Comparative assessment of the risks associated with use of manure and sewage sludge in Danish agriculture. Adv. Agron. 164, 289–334 (2020).
Xie, W. Y. et al. Long-term impact of field applications of sewage sludge on soil antibiotic resistome. Environ. Sci. Technol. 50(23), 12602–12611 (2016).
Polish Society of Soil Science in: Polskie Towarzystwo Gleboznawcze Klasyfikacja uziarnienia gleb i utworów mineralnych https://web.archive.org/web/20180204124028/http://www.ptg.sggw.pl/images/Uziarnienie_PTG_2008.pdf.pdf (2008).
Dz.U. z 2023 r poz.23 https://isap.sejm.gov.pl/isap.nsf/download.xsp/WDU20230000023/O/D20230023.pdf (2023).
Allen, S., Grimshaw, H.M., Parkinson, J.A. & Quarmby, C. Chemical analysis of ecological materials. (Oxford: Blackwell Scientific Publications. https://www.cabdirect.org/cabdirect/abstract/19751431633 1989).
International Organization for Standardization. ISO 13536:1995 Soil quality — determination of the potential cation exchange capacity and exchangeable cations using barium chloride solution buffered at pH ¼ 8,1. https://www.iso.org/standard/22180.html (1995).
Egnėr, H., Riehm, H. & Domingo, W. R. Untersuchungen uber die chemische Bodenanalyse als Grundlage fur die Beurteilung des Nährstoffzustandes der Böden. II. Chemische Extraktionsmethoden zur Phosphor- und Kaliumbestimmung. Kungliga Lantbrukshögskolans Annaler. 26, 199–215 (1960).
U.S. EPA, Method 200.7: Determination of Metals and Trace Elements in Water and Wastes by Inductively Coupled Plasma-Atomic Emission Spectrometry. Revision 4.4. Cincinnati, OH. (1994).
Hattori, R. & Hattori, T. Sensitivity to salts and organic compounds of soil bacteria isolated on diluted media. J. Gen. Appl. Microbial. 26, 1–14 (1980).
Arango-Argoty, G. et al. Deep ARG: A deep learning approach for predicting antibiotic resistance genes from metagenomic data. Microbiome 6, 1–15 (2018).
Menzel, P., Ng, K. & Krogh, A. Fast and sensitive taxonomic classification for metagenomics with Kaiju. Nat. Commun. 7, 11257. https://doi.org/10.1038/ncomms11257 (2016).
Hammer, O., Harper, D.A.T. & Ryan, P.D. Past: Paleontological statistics software package for education and data analysis. Paleontologia Electronica, 4:1–9. https://palaeo- electronica.org/2001_1/past/issue1_01.htm (2001).
Acknowledgements
The research was funded by the National Science Centre, Poland, project No. 2020/39/B/NZ9/01772
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L.S.: Conceptualization, funding acquisition, methodology, investigation, resources, validation, formal analysis, writing—original draft, writing—review and editing. A.F.N.: Methodology, formal analysis, visualization, writing—original draft, writing—review and editing. D.S.: Methodology, formal analysis. J.L.: Methodology, formal analysis. W.T.: Resources, methodology, formal analysis. M.B.: Methodology, formal analysis. M.U.: Conceptualization, funding acquisition.
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Serwecińska, L., Font-Nájera, A., Strapagiel, D. et al. Sewage sludge fertilization affects microbial community structure and its resistome in agricultural soils. Sci Rep 14, 21034 (2024). https://doi.org/10.1038/s41598-024-71656-0
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DOI: https://doi.org/10.1038/s41598-024-71656-0
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