Description: The data is from a mesocosm experiment set up outside Lima, Peru to study the influence of upwelling of oxygen minimum zone (OMZ) water. The mesocosm bags were 2 m in diameter and extended from the surface down to 19 m depth, where the last 2 m was a conical sediment trap. Eight mesocosm bags were used and they were moored at 12.0555°S; 77.2348°W just north of Isla San Lorenzo where the water depth is ~30 m. The experiment was started 25 February 2017 by closing the mesocosm bags and were run for 50 days. Two treatments were used (water with different OMZ signature), each with four replicates. Water (100 m3) from the OMZ was collected from two locations and depths. The first was collected from 12.028323°S; 77.223603°W from 30 m depth, and the second one from 12.044333°S; 77.377583°W from 70 m depth. The original aim was to collect severe and moderate OMZ signature water (differing in e.g. nitrate concentrations) from the first and second site, respectively. This assumption was based on long-term monitoring data, however, the chemical properties (e.g. nitrate concentration) was more similar in these water masses than anticipated, rather reflecting low and very low OMZ signatures from site 1 and 2 respectively. To have a baseline of measured variables, the mesocosms where closed and environmental and biological variables were determined over 10 days. After this period, the OMZ water was added to the mesocosms in two steps on day 11 and 12 after the enclosure of the mesocosms. As the mesocosms contain a specific volume (~54 m3), the process of adding the OMZ water started with first removing water from the mesocosms. The water removed (~20 m3) was pumped out from 11-12 m depth. A similar volume of OMZ water, from both collection sites, was then pumped into four replicate mesocosms each. The OMZ water was pumped into the mesocosms moving the input hose between 14-17 m depth. The water collected at 30 m depth was pumped into mesocosms M1, M4, M5 and M8 having a low OMZ signature and water from 70 m depth into mesocosms M2, M3, M6 and M7 having a very low OMZ signature. Due a halocline at 12 m depth (see below), the added OMZ water was not immediately mixed throughout the mesocosm bag. Sampling took place every second day over a period of 50 days, and all variables were taken with an integrated water sampler (HydroBios, IWS) pre-programed to fill from 0 – 10 m depth and all samples consisted of this integrated samples from the upper 10 m. The samples were stored dark in cool boxes and brought back to the laboratory and processed right away. Sampling took place in the morning, and the samples were usually back in the laboratory around noon. Measured variables included inorganic nutrients, dissolved organic nutrients, extracellular enzyme activity: leucine aminopeptidase (LAP) and alkaline phosphatase activity (APA), and the phytoplankton and bacterial community composition.

Description: The data is from a mesocosm experiment set up outside Lima, Peru to study the influence of upwelling of oxygen minimum zone (OMZ) water. The mesocosm bags were 2 m in diameter and extended from the surface down to 19 m depth, where the last 2 m was a conical sediment trap. Eight mesocosm bags were used and they were moored at 12.0555°S; 77.2348°W just north of Isla San Lorenzo where the water depth is ~30 m. The experiment was started 25 February 2017 by closing the mesocosm bags and were run for 50 days. Two treatments were used (water with different OMZ signature), each with four replicates. Water (100 m3) from the OMZ was collected from two locations and depths. The first was collected from 12.028323°S; 77.223603°W from 30 m depth, and the second one from 12.044333°S; 77.377583°W from 70 m depth. The original aim was to collect severe and moderate OMZ signature water (differing in e.g. nitrate concentrations) from the first and second site, respectively. This assumption was based on long-term monitoring data, however, the chemical properties (e.g. nitrate concentration) was more similar in these water masses than anticipated, rather reflecting low and very low OMZ signatures from site 1 and 2 respectively. To have a baseline of measured variables, the mesocosms where closed and environmental and biological variables were determined over 10 days. After this period, the OMZ water was added to the mesocosms in two steps on day 11 and 12 after the enclosure of the mesocosms. As the mesocosms contain a specific volume (~54 m3), the process of adding the OMZ water started with first removing water from the mesocosms. The water removed (~20 m3) was pumped out from 11-12 m depth. A similar volume of OMZ water, from both collection sites, was then pumped into four replicate mesocosms each. The OMZ water was pumped into the mesocosms moving the input hose between 14-17 m depth. The water collected at 30 m depth was pumped into mesocosms M1, M4, M5 and M8 having a low OMZ signature and water from 70 m depth into mesocosms M2, M3, M6 and M7 having a very low OMZ signature. Due a halocline at 12 m depth (see below), the added OMZ water was not immediately mixed throughout the mesocosm bag. Sampling took place every second day over a period of 50 days, and all variables were taken with an integrated water sampler (HydroBios, IWS) pre-programed to fill from 0 – 10 m depth and all samples consisted of this integrated samples from the upper 10 m. The samples were stored dark in cool boxes and brought back to the laboratory and processed right away. Sampling took place in the morning, and the samples were usually back in the laboratory around noon. Measured variables included inorganic nutrients, dissolved organic nutrients, extracellular enzyme activity: leucine aminopeptidase (LAP) and alkaline phosphatase, and the phytoplankton and bacterial community composition.

Description: The data is from a mesocosm experiment set up outside Lima, Peru to study the influence of upwelling of oxygen minimum zone (OMZ) water. The mesocosm bags were 2 m in diameter and extended from the surface down to 19 m depth, where the last 2 m was a conical sediment trap. Eight mesocosm bags were used and they were moored at 12.0555°S; 77.2348°W just north of Isla San Lorenzo where the water depth is ~30 m. The experiment was started 25 February 2017 by closing the mesocosm bags and were run for 50 days. Two treatments were used (water with different OMZ signature), each with four replicates. Water (100 m3) from the OMZ was collected from two locations and depths. The first was collected from 12.028323°S; 77.223603°W from 30 m depth, and the second one from 12.044333°S; 77.377583°W from 70 m depth. The original aim was to collect severe and moderate OMZ signature water (differing in e.g. nitrate concentrations) from the first and second site, respectively. This assumption was based on long-term monitoring data, however, the chemical properties (e.g. nitrate concentration) was more similar in these water masses than anticipated, rather reflecting low and very low OMZ signatures from site 1 and 2 respectively. To have a baseline of measured variables, the mesocosms where closed and environmental and biological variables were determined over 10 days. After this period, the OMZ water was added to the mesocosms in two steps on day 11 and 12 after the enclosure of the mesocosms. As the mesocosms contain a specific volume (~54 m3), the process of adding the OMZ water started with first removing water from the mesocosms. The water removed (~20 m3) was pumped out from 11-12 m depth. A similar volume of OMZ water, from both collection sites, was then pumped into four replicate mesocosms each. The OMZ water was pumped into the mesocosms moving the input hose between 14-17 m depth. The water collected at 30 m depth was pumped into mesocosms M1, M4, M5 and M8 having a low OMZ signature and water from 70 m depth into mesocosms M2, M3, M6 and M7 having a very low OMZ signature. Due a halocline at 12 m depth (see below), the added OMZ water was not immediately mixed throughout the mesocosm bag. Sampling took place every second day over a period of 50 days, and all variables were taken with an integrated water sampler (HydroBios, IWS) pre-programed to fill from 0 – 10 m depth and all samples consisted of this integrated samples from the upper 10 m. The samples were stored dark in cool boxes and brought back to the laboratory and processed right away. Sampling took place in the morning, and the samples were usually back in the laboratory around noon. Measured variables included inorganic nutrients, dissolved organic nutrients, extracellular enzyme activity: leucine aminopeptidase (LAP) and alkaline phosphatase activity (APA), and the phytoplankton and bacterial community composition.

Description: The microbiota of multicellular organisms undergoes considerable changes during development but the general mechanisms that control community assembly and succession are poorly understood. Here, we use bacterial recolonization experiments in Nematostella vectensis as a model to understand general mechanisms determining bacterial establishment and succession. We compared the dynamic establishment of the microbiome on the germfree host and on inert silica. Following the dynamic reconstruction of microbial communities on both substrates, we show that the initial colonization events are strongly influenced by the host but not by the tube, while the subsequent bacteria-bacteria interactions are the main cause of bacterial succession. Interestingly, the recolonization pattern on adult hosts resembles the ontogenetic colonization succession. This process occurs independently of the bacterial composition of the inoculum and can be followed at the level of individual bacteria, suggesting that priority effects are neglectable for early colonization events in Nematostella . To identify potential metabolic traits associated with initial colonization success and potential metabolic interactions among bacteria associated with bacterial succession, we reconstructed the metabolic networks of bacterial colonizers based on their genomes. These analyses revealed that bacterial metabolic capabilities reflect the recolonization pattern, and the degradation of chitin might be a selection factor during early colonization of the animal. Concurrently, transcriptomic analyses revealed that Nematostella possesses two chitin synthase genes, one of which is upregulated during early recolonization. Our results show that early colonization events are strongly controlled by the host while subsequent colonization depends on metabolic bacteria-bacteria interactions largely independent of host development.

Description: The associated microbiota of marine invertebrates plays an important role to the host in relation to fitness, health, and homeostasis. Cooperative and competitive interactions between bacteria, due to release of, for example, antibacterial substances and quorum sensing (QS)/quorum quenching (QQ) molecules, ultimately affect the establishment and dynamics of the associated microbial community. Aiming to address interspecies competition of cultivable microbes associated with emerging model species of the basal animal phyla Cnidaria (Aurelia aurita) and Ctenophora (Mnemiopsis leidyi), we performed a classical isolation approach. Overall, 84 bacteria were isolated from A. aurita medusae and polyps, 64 bacteria from M. leidyi, and 83 bacteria from ambient seawater, followed by taxonomically classification by 16S rRNA gene analysis. The results show that A. aurita and M. leidyi harbor a cultivable core microbiome consisting of typical marine ubiquitous bacteria also found in the ambient seawater. However, several bacteria were restricted to one host suggesting host-specific microbial community patterns. Interbacterial interactions were assessed by (a) a growth inhibition assay and (b) QS interference screening assay. Out of 231 isolates, 4 bacterial isolates inhibited growth of 17 isolates on agar plates. Moreover, 121 of the 231 isolates showed QS-interfering activities. They interfered with the acyl-homoserine lactone (AHL)-based communication, of which 21 showed simultaneous interference with autoinducer 2. Overall, this study provides insights into the cultivable part of the microbiota associated with two environmentally important marine non-model organisms and into interbacterial interactions, which are most likely considerably involved in shaping a healthy and resilient microbiota.

Description: Due to ocean acidification and global warming, surface seawater of the western Baltic Sea is expected to reach an average of ∼1100 μatm pCO2 and an increase of ∼5°C by the year 2100. In four consecutive experiments (spanning 10–11 weeks each) in all seasons within 1 year, the abiotic factors temperature (+5°C above in situ) and pCO2 (adjusted to ∼1100 μatm) were tested for their single and combined effects on epibacterial communities of the brown macroalga Fucus vesiculosus and on bacteria present in the surrounding seawater. The experiments were set up in three biological replicates using the Kiel Outdoor Benthocosm facility (Kiel, Germany). Phylogenetic analyses of the respective microbiota were performed by bacterial 16S (V1-V2) rDNA Illumina MiSeq amplicon sequencing after 0, 4, 8, and 10/11 weeks per season. The results demonstrate (I) that the bacterial community composition varied in time and (II) that relationships between operational taxonomic units (OTUs) within an OTU association network were mainly governed by the habitat. (III) Neither single pCO2 nor pCO2:Temperature interaction effects were statistically significant. However, significant impact of ocean warming was detected varying among seasons. (IV) An indicator OTU (iOTU) analysis identified several iOTUs that were strongly influenced by temperature in spring, summer, and winter. In the warming treatments of these three seasons, we observed decreasing numbers of bacteria that are commonly associated with a healthy marine microbial community and—particularly during spring and summer—an increase in potentially pathogenic and bacteria related to intensified microfouling. This might lead to severe consequences for the F. vesiculosus holobiont finally affecting the marine ecosystem.

Description: Heme b is an iron-containing cofactor in hemoproteins that participates in the fundamental processes of photosynthesis and respiration in phytoplankton. Heme b concentrations typically decline in waters with low iron concentrations but due to lack of field data, the distribution of heme b in particulate material in the ocean is poorly constrained. Here we report particulate heme b distributions across the Atlantic Ocean (59.9°N to 34.6°S). Heme b concentrations in surface waters ranged from 0.10 to 33.7 pmol L−1 (median = 1.47 pmol L−1, n = 974) and were highest in regions with a high biomass. The ratio of heme b to particulate organic carbon (POC) exhibited a mean value of 0.44 μmol heme b mol−1 POC. We identified the ratio of 0.10 µmol heme b mol−1 POC as the cut-off between heme b replete and heme b deficient (anemic) phytoplankton. By this definition, we observed anemic phytoplankton populations in the Subtropical South Atlantic and Irminger Basin. Comparison of observed and modelled heme b suggested that heme b could account for between 0.17–9.1% of biogenic iron. Our large scale observations of heme b relative to organic matter provide further evidence of the impact of changes in iron supply on phytoplankton iron status across the Atlantic Ocean.

Description: Highlights: • Non-indigenous species (NIS) are increasingly recognized as a matter of concern. • The microbiome of native and NIS gelatinous zooplankton organisms are compared. • Next generation sequencing confirms sign. Species specific microbiome differences. • Indicator OTUs include bacteria which contain known pathogenic strains. • Microbiome monitoring of NIS should be considered for aquaculture risk assessments. Abstract: The translocation of non-indigenous species (NIS) around the world, especially in marine systems, is increasingly being recognized as a matter of concern. Species translocations have been shown to lead to wide ranging changes in food web structure and functioning. In addition to the direct effects of NIS, they could facilitate the accumulation or translocation of bacteria as part of their microbiomes. The Baltic Sea harbours many non-indigenous species, with most recent detection of the jellyfish Blackfordia virginica and the comb jelly Mnemiopsis leidyi in the low saline southwestern Baltic Sea. In this study, we used a multidisciplinary approach and investigated three gelatinous zooplankton species that co-occur in the same environment and feed on similar zooplankton food sources but show different histories of origin. The aim was to conduct a comparative microbiome analysis of indigenous and non-indigenous gelatinous zooplankton species in the low-saline southwestern Baltic Sea. Next-generation 16S rRNA marker gene sequencing of the V1/V2 region was employed to study the bacterial microbiome compositions. All tested species showed significant differences in their microbiome compositions (one way ANOSIM, R = 1, P 〈 0.008) with dissimilarities ranging from 85 to 92%. The indigenous jellyfish Aurelia aurita showed the highest bacterial operational taxonomic unit (OTU) richness. The overall differentiation between microbiomes was driven by eight indicator OTUs, which included Mycoplasma and Vibrio species. These bacteria can be problematic, as they include known pathogenic strains that are relevant to human health and aquaculture activities. Our results suggest that the impact assessment of NIS should consider potential pathogenic bacteria, enriched in the environment due to invasion, as potential risks to aquaculture activities.

Description: All multicellular organisms are associated with microbial communities, ultimately forming a metaorganism. Several studies conducted on well-established model organisms point to immunological, metabolic, and behavioral benefits of the associated microbiota for the host. Consequently, a microbiome can influence the physiology of a host; moreover, microbial community shifts can affect host health and fitness. The present study aimed to evaluate the significance and functional role of the native microbiota for life cycle transitions and fitness of the cnidarian moon jellyfish Aurelia aurita. A comprehensive host fitness experiment was conducted studying the polyp life stage and integrating 12 combinations of treatments with microbiota modification (sterile conditions, foreign food bacteria, and potential pathogens). Asexual reproduction, e.g., generation of daughter polyps, and the formation and release of ephyrae were highly affected in the absence of the native microbiota, ultimately resulting in a halt of strobilation and ephyra release. Assessment of further fitness traits showed that health, growth, and feeding rate were decreased in the absence and upon community changes of the native microbiota, e.g., when challenged with selected bacteria. Moreover, changes in microbial community patterns were detected by 16S rRNA amplicon sequencing during the course of the experiment. This demonstrated that six operational taxonomic units (OTUs) significantly correlated and explained up to 97% of fitness data variability, strongly supporting the association of impaired fitness with the absence/presence of specific bacteria. Conclusively, our study provides new insights into the importance and function of the microbiome for asexual reproduction, health, and fitness of the basal metazoan A. aurita.

Description: The Peruvian upwelling system is a highly productive ecosystem with a large oxygen minimum zone (OMZ) close to the surface. In this work, we carried out a mesocosm experiment off Callao, Peru, with the addition of water masses from the regional OMZ collected at two different sites simulating two different upwelling scenarios. Here, we focus on the pelagic remineralization of organic matter by the extracellular enzyme activity of leucine aminopeptidase (LAP) and alkaline phosphatase activity (APA). After the addition of the OMZ water, dissolved inorganic nitrogen (N) was depleted, but the standing stock of phytoplankton was relatively high, even after N depletion (mostly 〉 4 µg chlorophyll a L−1). During the initial phase of the experiment, APA was 0.6 nmol L−1 h−1 even though the PO concentration was 〉 0.5 µmol L−1. Initially, the dissolved organic phosphorus (DOP) decreased, coinciding with an increase in the PO concentration that was probably linked to the APA. The LAP activity was very high, with most of the measurements in the range of 200–800 nmol L−1 h−1. This enzyme hydrolyzes terminal amino acids from larger molecules (e.g., peptides or proteins), and these high values are probably linked to the highly productive but N-limited coastal ecosystem. Moreover, the experiment took place during a rare coastal El Niño event with higher than normal surface temperatures, which could have affected enzyme activity. Using a nonparametric multidimensional scaling analysis (NMDS) with a generalized additive model (GAM), we found that biogeochemical variables (e.g., nutrient and chlorophyll-a concentrations) and phytoplankton and bacterial communities explained up to 64 % of the variability in APA. The bacterial community best explained the variability (34 %) in LAP. The high hydrolysis rates for this enzyme suggest that pelagic N remineralization, likely driven by the bacterial community, supported the high standing stock of primary producers in the mesocosms after N depletion.