Ciliates are unicellular eukaryotes, regularly involved in symbiotic associations. Symbionts may colonize the inside of their cells as well as their surface as ectosymbionts. Here, we report on a new ciliate species, designated as Zoothamnium mariella sp. nov. (Peritrichia, Sessilida), discovered in the northern Adriatic Sea (Mediterranean Sea) in 2021. We found this ciliate species to be monospecifically associated with a new genus of ectosymbiotic bacteria, here proposed as Candidatus Fusimicrobium zoothamnicola gen. nov., sp. nov. To formally describe the new ciliate species, we investigated its morphology and sequenced its 18S rRNA gene. To demonstrate its association with a single species of bacterial ectosymbiont, we performed 16S rRNA gene sequencing, fluorescence in situ hybridization, and scanning electron microscopy. Additionally, we explored the two partners' cultivation requirements and ecology. Z. mariella sp. nov. was characterized by a colony length of up to 1 mm. A consistent number of either seven or eight long branches alternated on the stalk in close distance to each other. The colony developed three different types of zooids: microzooids ("trophic stage"), macrozooids ("telotroch stage"), and terminal zooids ("dividing stage"). Viewed from inside the cell, the microzooids' oral ciliature ran in 1 ¼ turns in a clockwise direction around the peristomial disc before entering the infundibulum, where it performed another ¾ turn. Phylogenetic analyses assigned Z. mariella sp. nov. to clade II of the family Zoothamnidae. The ectosymbiont formed a monophyletic clade within the Gammaproteobacteria along with two other ectosymbionts of peritrichous ciliates and a free-living vent bacterium. It colonized the entire surface of its ciliate host, except for the most basal stalk of large colonies, and exhibited a single, spindle-shaped morphotype. Furthermore, the two partners together appear to be generalists of temperate, oxic, marine shallow-water environments and were collectively cultivable in steady flow-through systems.
Symbiosis, the coexistence of organisms belonging to different species in physical contact over an extended period of time [[
The genus Zoothamnium Bory de St. Vincent, 1824 is assigned to the class Oligohymenophorea de Puytorac et al., 1974, the subclass Peritrichia Stein, 1859, the order Sessilida Kahl, 1933, and the family Zoothamnidae, Sommer 1951 [[
Here, we report on the discovery of a new Zoothamnium species in shallow water environments of the northern Adriatic Sea in 2021. Bacteria covered the surface of the colony, indicating a symbiotic association. We used various microscopic and molecular biological tools, to formally describe this new ciliate species and to demonstrate its monospecific association with a new genus of bacterial ectosymbiont. Additionally, we investigated habitat preferences and cultivation requirements of the two partners.
Permissions to access the subtidal mudflat Stjuža and the canal Lera were granted by the Strunjan Landscape Park and the Naturepark Sečoveljske soline, respectively. The subtidal sediment in front of the Marine Biology Station Piran is publicly accessible. We confirm that our field study did not include endangered or protected species.
We sampled colonies of the new Zoothamnium species from wooden- and plastic cubes (12 cm x 11.2 cm x 11.2 cm), that had been deployed in the context of a different project, at three distinct marine sites in the northern Adriatic Sea (Mediterranean Sea) in 2021 and 2022. Beside these experimentally deployed cubes, we sampled further specimens from rocks, macroalgae, dead bryozoans, and cable ties, collected at the same sites. The sites represented the subtidal sediment in front of the Marine Biology Station Piran, the subtidal mudflat Stjuža located in the Strunjan Landscape Park, and the canal Lera extending through the Naturepark Sečoveljske soline (Fig 1). The sampling depth ranged from 1.5 m (subtidal mudflat), over 2.5 m (canal), to 3.5 m (subtidal sediment). Whenever we sampled at one of those sites, we measured the seawater's temperature and oxygen concentration using a Fibox 4 (PreSens) as well as pH and salinity using a WTW Multi 340i (Wissenschaftlich-Technische Werkstätten).
Graph: a) Map showing the Adriatic Sea, reprinted from GeoMapApp () under a CC BY license, with permission from William B. F. Ryan, original copyright 2009 [[
We cultivated colonies of the new Zoothamnium species by placing macroalgae, dead bryozoans, and cable ties, populated by the colonies, underneath an inverted glass container inside a tank with continuous flow of seawater for several days. Between the glass container and the flow-through tank, we left a narrow gap to promote swarmer settlement on the glass surface while allowing water exchange. The seawater that ran through the flow-through tank originated from the subtidal sediment sampling site and exhibited an oxygen concentration of 200 μmol L
We fixed and stored colonies for DNA extraction and fluorescence in situ hybridization (FISH) alongside colonies designated as type specimens in 100% ethanol. In addition, we fixed colonies for scanning electron microscopy as well as further potential type specimens in a modified Trump's fixative (2.5% glutaraldehyde, 2% paraformaldehyde in sodium cacodylate 0.1 mol L
We observed and took micrographs of colonies in vivo, using bright-field and differential interference contrast (DIC) optics on a Leica DM2000 microscope equipped with a Leica DFC295 camera. We used these micrographs to precisely measure entire colonies and individual cells as well as to generate accurate drawings. In order to unveil the kinetosomes, the nuclei and the silverline system, we applied the pyridinated silver carbonate impregnation method, following Fernández-Galiano's protocol [[
Graph: Fig 2 info:doi/10.1371/journal.pone.0300758.g002
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Table 1 Site, substrate, and date of samples used for various methods.
quantity sampling site substrate sampling date specimen state application 2 subtidal sediment wooden cube March 2021 100% EtOH 18S sequencing 1 subtidal sediment wooden cube July 2021 100% EtOH 18S sequencing 2 subtidal mudflat wooden cube July 2021 100% EtOH 18S sequencing 7 subtidal sediment wooden cube August 2021 100% EtOH 18S sequencing 4 subtidal sediment wooden cube February 2022 100% EtOH 18S sequencing 3 subtidal sediment rock February 2022 100% EtOH 18S sequencing 1 subtidal mudflat rock February 2022 100% EtOH 18S sequencing 2 canal wooden cube February 2022 100% EtOH 18S sequencing 1 canal plastic cube February 2022 100% EtOH 18S sequencing 4 subtidal sediment wooden cube July 2022 100% EtOH 18S sequencing 1 subtidal sediment plastic cube August 2022 100% EtOH 18S sequencing 1 subtidal sediment wooden cube March 2021 100% EtOH 18S- and 16S sequencing 1 subtidal sediment wooden cube July 2021 100% EtOH 18S- and 16S sequencing 1 subtidal mudflat wooden cube February 2022 100% EtOH 18S- and 16S sequencing 2 canal macroalgae August 2022 100% EtOH FISH 2 cultivation glass August 2022 100% EtOH FISH 3 canal dead bryozoans August 2022 Trump's fixative SEM 3 canal cable ties August 2022 Trump's fixative SEM 3 cultivation glass August 2022 Trump's fixative SEM 3 canal wooden cube August 2022 Trump's fixative Type specimens 10 canal wooden cube August 2022 100% EtOH Type specimens 1 cultivation glass August 2022 alive microscopy 1 cultivation glass August 2022 alive Fernández-Galiano 1 canal wooden cube August 2022 alive LIVE/DEAD
We extracted DNA from 31 colonies using the DNeasy Blood & Tissue Kit (Qiagen) according to the manufacturer's instructions, except for one minor modification of the reaction volume. Instead of 200 μl elution buffer, we added 100 μl. Subsequently, we amplified the 18S rRNA genes from all 31 DNA extracts by PCR using the universal eukaryotic primers 82 forward [[
To separately clone amplified 16S rRNA genes, we applied the TOPO-TA cloning kit (Invitrogen) according to the manufacturer's instructions. For each cloning reaction we selected 17 to 18 clones and amplified their inserted 16S rRNA gene by PCR with the M13 forward and M13 reverse primers. Following that, we had both the 18S rRNA genes and the 16S rRNA genes sequenced via Sanger sequencing. We further processed the obtained sequences using Geneious Prime 2022 (https://
We compared the processed 16S and 18S rRNA gene sequences with the National Center for Biotechnology information NCBI (https://
We designed two oligonucleotide probes, specific for the new ectosymbiont phylotype, using Geneious Prime 2022. Both probes hybridize to easily accessible regions of the 16S rRNA gene, in order to produce the brightest signals possible [[
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Table 2 Probes used for fluorescence in situ hybrization.
probe specificity sequence reference EUB338 most bacteria (EUBI + II + III) 5'-GCT GCC TCC CGT AGG AGT-3' [ EUB338II most bacteria (EUBI + II + III) 5'-GCA GCC ACC CGT AGG TGT-3' [ EUB338III most bacteria (EUBI + II + III) 5'-GCT GCC ACC CGT AGG TGT-3' [ NON338 negative control 5'-ACT CCT ACG GGA GGC AGC-3' [ ZMS152 New ectosymbiont phylotype 5'-TNT GCG GTA TTA GCC AAT GTT-3' this study ZMS1239 New ectosymbiont phylotype 5'-TCC GGA CTA AGA TCA GAT TTA-3' this study
We rinsed nine colonies, retained in a modified Trump's fixative, with ultrapure water, to subsequently postfix them in a mixture of 0.1M sodium cacodylate buffer and 1% osmium tetroxide. After rinsing them again with ultrapure water, we dehydrated the colonies in a graded series of ethanol with a final 100% acetone step. Next, we transferred them into 1:1 acetone/hexamethyldisilazane (HMDS) and then into 100% HMDS, where we left them to air-dry. As a final preparation step, we mounted the air-dried colonies on stubs and sputter gold coated them utilizing a JEOL JFC-2300HR. We observed the ready prepared colonies with a JEOL IT 3000 scanning electron microscope.
The electronic edition of this article conforms to the requirements of the amended International Code of Zoological Nomenclature, and hence the new names contained herein are available under that Code from the electronic edition of this article. We registered this published work and the nomenclatural acts it contains in ZooBank, the online registration system for the ICZN. The ZooBank LSIDs (Life Science Identifiers) can be resolved and the associated information viewed through any standard web browser by appending the LSID to the prefix "
We followed the classification system proposed by Lynn, 2008 [[
Phylum: Ciliophora Doflein, 1901
Class: Oligohymenophorea de Puytorac et al., 1974
Subclass: Peritrichia Stein, 1859
Order: Sessilida Kahl, 1933
Family: Zoothamnidae Sommer, 1951
Genus: Zoothamnium Bory de St. Vincent, 1824
Star-shaped Zoothamnium species up to 1 mm in length with three different types of zooids: microzooids ("trophic stage"), macrozooids ("telotroch stage"), and terminal zooids ("dividing stage"). Colonies developed a final number of either seven or eight long branches that originated alternately on the stalk in close distance to each other. In fully developed colonies, the terminal zooids were restricted to the distal ends of the branches (terminal branch zooids). A terminal zooid on the tip of the stalk (top terminal zooid) only existed in young colonies during colony development. The microzooids were inverted bell-shaped and developed alternately on the branches. The macrozooids exhibited a roundish to ellipsoid shape and were located at the proximal ends of the branches. Undividing terminal zooids resembled the microzooids in shape and size. Dividing terminal zooids became ellipsoid. One or two macrozooids developed per colony. The macronucleus of the microzooids was S-shaped. The macronucleus of the macrozooids appeared thick, constant in diameter, with multiple coils. Viewed from inside the cell, the microzooids' oral ciliature performed two turns in a clockwise direction. The oral ciliature exhibited a conspicuous curve-shape in the very beginning before initiating its first turn. Species found in marine shallow water environments.
We collected all type specimens from experimentally deployed wooden cubes at the canal Lera in August 2022 (northern Adriatic Sea; 45° 29' 46.7" N, 13° 35' 36.7" E; water depth 2.5 m, water temperature: 26.3°C, salinity: 36.4, pH: 8.1).
We embedded the holotype (NHM-EV-5888) and two paratypes (NHM-EV-5889 and NHM-EV-5890), which we had previously fixed in a modified Trump's fixative, in glycerol, mounted them on microscopic slides, and stored them at the Naturhistorisches Museum (NHM), Wien (Austria). Additionally, we stored ten paratypes (NHM-EV-21536), fixed in 100% ethanol, at the NHM.
We deposited the 18S rRNA gene sequence of Zoothamnium mariella sp. nov. in the GenBank database under the accession number OR381572.
Taxonomy. Zoothamnium mariella Kendlbacher, Winter & Bright sp. nov. urn:lsid:zoobank.org:pub:57CC07A5-ECED-4FDF-9E3D-FACA53FBBFC3.
The Latin name 'Mariella' translates as star of the sea. We utilized it as a species epithet, treated as a noun in apposition, to emphasize the species' marine habitat as well as its star-shaped appearance.
The Colony was composed of a stalk with alternately originating branches. Filter-feeding microzooids alternated on the branches. The macrozooids, zooids that leave the colony as swarmers to disperse and build a new colony after settling, occurred at the proximal ends of the branches. We observed between one and two macrozooids, with one being up to twice the size of the other. During colony development, the terminal zooid on the tip of the stalk (top terminal zooid) with every division produced a new terminal zooid (terminal branch zooid). Each terminal branch zooid secreted a branch and simultaneously produced the microzooids of that branch. After six to seven divisions, the top terminal zooid ceased to produce further terminal branch zooids, but instead spawned a final branch and the associated microzooids, thereby ending colony growth. Consequently, colonies of Z. mariella sp. nov. developed a maximum of either seven or eight branches (Figs 3 and 4).
Graph: Zoothamnium mariella sp. nov. Detailed drawing of an entire colony and a microzooid, both in expanded condition. mi: microzooid, ma: macrozooid, t: terminal zooid, br: branch, st: stalk, sp: spasmoneme, ad: adhesive disc, am1: adoral membranelle 1 (polykinety), pm: paroral membrane (haplokinety), in: infundibulum, cp: cytopharynx, fv: food vacuole, man: macronucleus, min: micronucleus, tl: telotrochal band, b: bacteria.
Graph: a) expanded colony, b) contracted colony, c) most basal part of the stalk, where the spasmoneme splits into bands, which bundle towards the basal end of the colony, d) ellipsoid terminal zooid on the verge of cell division, e) macrozooid, f) microzooid, g–m) oral ciliature of the microzooids, n) microzooid with emphasize on its telotrochal band. a–d) living specimens. e–n) silver-stained specimens. mi: microzooid, ma: macrozooid, t: terminal zooid, st: stalk, sp: spasmoneme, ad: adhesive disc, man: macronucles, oc: oral ciliature, pm: paroral membrane (haplokinety), am1–3: adoral membranelles 1–3 (polykineties), s: stomatogenic kinety, tl: telotrochal band.
A specialised organelle, the spasmoneme, ran uninterrupted inside the stalk and branches, extending into every zooid. It facilitated a simultaneous contraction of the entire colony. Additionally, it allowed the oral side of each zooid to contract individually. The basal end of the spasmoneme split into several bands which bundled towards the most basal part of the stalk (Fig 4). Hence, only the most basal part of the stalk and the adhesive disc lacked a spasmoneme. At the basal end of the stalk, the diameter was 15 μm (spasmoneme diameter 10 μm). It increased to 18 μm at the location of the most basal branch (spasmoneme diameter 7 μm) and decreased again to 15 μm (spasmoneme diameter 7 μm) where the top branch originated (S1 Table). The contraction of the colony took place rapidly, while the subsequent expansion was much slower. In the contracted state, the colony showed a typical zigzag pattern (Fig 4). We observed the cilia of the oral apparatus only to beat in the expanded state of the colony. Furthermore, older zooids, attached to further basally located branches, appeared to be less active.
The colony of Z. mariella sp. nov. grew up to 1 mm in length. Divided into the following parts ‐ stalk with branches, stalk without branches containing a spasmoneme, and stalk without branches lacking a spasmoneme, the resulting length ratios were 50%, 40% and 10%. The distances between the branches ranged from 15 to 70 μm. The branches exhibited diameters from 9 to 10 μm, with corresponding spasmoneme diameters from 3 to 5 μm. In a full-grown colony, the branches harbored 12 to 18 zooids (distances between zooids 23–30 μm) and reached lengths between 0.29 and 0.43 mm (S1 Table). The length of the branches, their close distance to each other on the stalk, and their small number gave the colony its distinctive star-shaped appearance.
In the expanded colony state with the oral ciliature of the microzooids beating, the microzooids displayed a bulgy, inverted bell-shaped form (average length 23.8 μm, SD 2.6 μm; average oral width 28.3 μm, SD 1.6 μm; average aboral width 6.5 μm, SD 1.0 μm; n = 20; S2 Table; Fig 3). In contrast, contracted microzooids withdrew the whole peristome with the round peristomial disc and the single oral lip, thus appearing more roundish. Orally, the microzooids' ciliature comprised a paroral membrane (haplokinety), three adoral membranelles (am 1–3; polykineties), and one short stomatogenic kinety (germinal kinety). The paroral membrane was located outside the innermost adoral membranelle (am 1). Viewed from inside the cell, the paroral membrane and the adoral membranelle 1 ran jointly in 1 1/4 turns in a clockwise direction around the peristomial disc. Where they began to run into the infundibulum, a short stomatogenic kinety of barren kinetosomes was present outside the paroral membrane. From there, the paroral membrane and the adoral membranelle 1 extended in another 3/4 turn to the posterior end of the infundibulum, where the adoral membranelle 1 was accompanied by two shorter adoral membranelles (am 2, am3). Furthermore, the paroral membrane and the adoral membranelle 1 exhibited a conspicuous curve-shape in the very beginning before initiating their first turn (Figs 4 and 5).
Graph: pm: paroral membrane (haplokinety), am1–3: adoral membranelles 1–3 (polykineties), s: stomatogenic kinety.
The microzooids' pellicula was plain with a striped silverline system (width of the striae 1.0–1.2 μm; S2 Table). Their somatic ciliature was located at about two-thirds distance from the peristomial disc, reduced to a single irregular row of barren kinetosomes, forming the telotrochal band. The macronucleus extended through the entire microzooid and was S-shaped (Figs 3 and 4). Adjacent to the macronucleus, was a single, small, spherical micronucleus.
Expanded terminal zooids showed a bulgy, inverted bell-shaped form, resembling the microzooids in shape and morphological attributes (average length 28.8 μm, SD 3.6 μm; average oral width 28.7 μm, SD 1.5 μm; average aboral width 6.8 μm, SD 1.1 μm; n = 20; S2 Table). Contracted terminal zooids appeared roundish. Furthermore, we occasionally found terminal zooids with an ellipsoid shape (average core width 34.3 μm, SD 5 μm; n = 4; S2 Table) and an enlarged macronucleus, filling up almost the entire cell body (Fig 4). We presumed these zooids to be on the verge of cell division.
The macrozooids were comparably large, roundish to ellipsoid, cells with core widths ranging from 48 to 121 μm (average core width 73.4 μm, SD 23.0 μm; n = 20; S2 Table). Their macronucleus appeared thick, constant in diameter, with multiple coils. Due to its dimensions, it filled up almost the entire cell (Fig 4). The macrozooids' pellicula had concave bands on its surface, running transverse to the oral-aboral axis of the cell. The width of these striae varied between individual cells and ranged from 0.9 to 3.3 μm (S2 Table). Aborally, a telotrochal band with multiple circular rows of kinetosomes was located at the centre of the cell, arranged like the striae. We observed this telotrochal band to be partly ciliated in attached macrozooids and fully ciliated in free-swimming macrozooids as well as macrozooids about to detach from the colony.
Lengthwise, the 31 processed 18S rRNA gene sequences ranged from 1508 to 1535 base pairs. They exhibited sequence similarities of 100%, indicating that all belonged to the same species. Zoothamnium mariella sp. nov. grouped within the monophyletic clade II of the family Zoothamnidae along with Z. alternans populations from China and the USA, Z. ignavum, Z. niveum, Z. plumula, and Z. pelagicum (Fig 6). With a sequence similarity of 94.67%, the closest relative and sister taxon of Z. mariella sp. nov. was Z. ignavum. (82% ML, 88% MP).
Graph: The numbers in parentheses are the NCBI accession numbers for each species and the numbers at the nodes represent Maximum Likelihood and Maximum Parsimony bootstrap values greater than or equal to 70%. The scale bar corresponds to 1 substitution per 200 nt positions.
Phylum: Proteobacteria Stackebrandt et al., 1988
Class: Gammaproteobacteria Garrity et al., 2005
Order: Unclassified
Family: Unclassified
Same as for the host species Zoothamnium mariella sp. nov.
We deposited the 16S rRNA gene sequence of Candidatus Fusimicrobium zoothamnicola gen. nov., sp. nov. in the GenBank database under the accession number OR387482.
The generic name Fusimicrobium is a combination of the latin word 'fusus' (spindle) and 'microbium' (microbe) and highlights the microbe's spindle-shaped appearance. The species epithet zoothamnicola translates as inhabitant of Zoothamnium and refers to the species' symbiotic association with Zoothamnium mariella sp. nov.
From a total of 52 screened clones, 36 carried the 16S rRNA gene sequence belonging to Candidatus Fusimicrobium zoothamnicola gen. nov., sp. nov. These 36 sequences exhibited a length of 1457 base pairs and sequence similarities between 99.36 and 100%. The remaining 16 clones contained 16S rRNA gene sequences from different random marine bacteria. Phylogenetic analyses revealed that Ca. Fusimicrobium zoothamnicola gen. nov., sp. nov. belongs to the class of Gammaproteobacteria. Within this class, it formed a monophyletic clade with the thiotrophic ectosymbiont of Pseudovorticella sp. (Peritrichia, Sessilida, Vorticellidae), the ectosymbiont of Zoothamnium ignavum Candidatus Navis piranensis, and a free-living bacterium associated with intertidal hydrothermal vents from southern California (Fig 7). With a 16S rRNA gene similarity of 91.36%, the closest relative and sister taxon of Ca. Fusimicrobium zoothamnicola gen. nov., sp. nov. turned out to be the free-living vent bacterium. Moreover, Z. niveum's ectosymbiont Ca. Thiobius zoothamnicola proved to be only distantly related.
Graph: The numbers in parentheses are the NCBI accession numbers for each species and the numbers at the nodes represent Maximum Likelihood and Maximum Parsimony bootstrap values greater than or equal to 70%. The scale bar corresponds to 5 substitutions per 100 nt positions.
The two newly designed FISH probes, ZMS152 and ZMS1239, both showed at least one mismatch to all other 16S rRNA gene sequences available in the public databases. Performing FISH with the two probes resulted in bright signals which confirmed that Ca. Fusimicrobium zoothamnicola gen. nov., sp. nov., indeed, is the ectosymbiont of Zoothamnium mariella sp. nov. Optimal formamide concentrations in the hybridization buffer proved to be 20% for ZMS152 and 10% for ZMS1239, precisely matching the formamide curve generated by mathFISH. Generally, all bacteria inhabiting the surface of Z. mariella sp. nov. hybridized with the symbiont-specific probes as well as the EUB mix probe set, demonstrating that no additional bacteria contributed to the bacterial coat. The ectosymbionts colonized the surfaces of microzooids, terminal zooids, macrozooids, branches, and stalk (Fig 8). In large colonies, we occasionally found the basal part of the stalk to be overgrown by various unspecific bacteria (S1 Fig) which hybridized solely with the EUB mix probe set. Performing FISH with the nonsense probe NON338 did not yield a detectable fluorescence signal, indicating that all signals originated from specific binding of the probes rather than unspecific staining or autofluorescence.
Graph: a, b, c) LIVE/DEAD staining, d,h) DAPI (blue), e, i) EUB mix in Cy5 (green), f, j) probe ZMS152 and ZMS1239 in Cy3 (red), g, k) overlay of the three colours, mi: microzooid, ma: macrozooid, t: terminal zooid, st: stalk, br: branch.
During the fixation process for SEM, apparently the colonies have partly lost their ectosymbionts. Living specimens, either viewed with DIC optics (S2 Fig) or treated with the LIVE/DEAD staining kit (Fig 8), or ethanol-fixed specimens used for FISH (Fig 8), showed a consistent bacterial coat throughout. In contrast, colonies prepared for and observed by SEM were only fragmentarily covered by bacteria (Fig 9). This fragmented bacterial coat consisted exclusively of spindle-shaped cells (average length 2.4 μm, SD 0.6 μm; average width 0.4 μm, SD 0.1 μm; n = 20; S3 Table) and extended from the basal part to the top end of the stalk, over the branches, and onto all three types of zooids. On the stalk, the branches, the microzooids, and the terminal zooids, we found the symbionts arranged in a monolayer. On the macrozooids they appeared to overlap in a multilayered fashion, with not every symbiont cell in direct contact with the host (Fig 9). We could not determine, however, whether this was a further artifact caused by the fixation. At an average length of 2.6 μm (SD 0.2 μm; n = 14; S3 Table) the symbionts initiated binary fission, forming two equally long daughter cells.
Graph: a) entire colony in contracted state, b) stalk with bacterial coat, c) branch with microzooids and a terminal zooid, d) microzooid, e) macrozooid, f) bacteria colonizing macrozooid, g) barely colonized macrozooid, h) barely colonized microzooid. mi: microzooid, t: terminal zooid, st: stalk, br: branch, sc: somatic ciliature.
We encountered the symbiosis on various substrates (sunken wood, plastics, dead bryozoans, macroalgae, shells, and rocks) at all three sampling sites during summer and winter seasons. Consequently, both partners were exposed to changing biotic factors as well as physicochemical conditions of the surrounding seawater. We measured oxygen concentrations ranging from 168 to 267 μmol L
The cultivation experiment under oxic, flow-through conditions, resulted in dense populations of symbiotic Zoothamnium mariella sp. nov. populating the surface of the glass container. In addition, we found two other Zoothamnium species colonizing the glass surface, Z. ignavum and a so far undescribed species. However, both species appeared in low numbers, compared to Z. mariella sp. nov.
We identified Zoothamnium mariella sp. nov. as a member of the genus Zoothamnium due to its sessile, colonial appearance, with individual zooids connected by a common stalk and branches. Furthermore, stalk and branches were internally traversed by a continuous spasmoneme which extended into every zooid and enabled the entire colony to contract in a typical zig-zag pattern. The conspicuous morphology of the colony resulted from the peculiar behaviour displayed by the terminal zooid on the tip of the stalk (top terminal zooid) during colony development. As in any other species of the genus [[
A similar growth pattern does not exist in any other clade II Zoothamnium species [[
Besides this difference, the colony of Z. mariella sp. nov. showed morphological similarities to Z. ignavum and Z. alternans that could potentially lead to confusion between the species. When dividing a Z. mariella sp. nov. colony in two parts, stalk with branches, and stalk without branches, the resulting relative lengths were 50% and 50%. This ratio resembled a lot the one displayed by Z. ignavum colonies, which was 40% and 60%. However, in Z. mariella sp. nov. 80% of the stalk without branches was traversed by a spasmoneme, compared to only 50% in Z. ignavum. With a maximum colony length of 1 mm, Z. mariella sp. nov. was slightly shorter than the 1.8 mm long Z. ignavum. Nevertheless, it grew longer branches. The longest branches in Z. ignavum colonies harbored about 14 zooids. In Z. mariella sp. nov. we counted up to 18 zooids attached to a single branch, with distances between the zooids corresponding to those of Z. ignavum [[
Z. mariella sp. nov, Z. ignavum, and Z. alternans can further be differentiated by investigating their oral ciliature. The paroral membrane and the adoral membranelle 1 of Z. mariella sp. nov. and Z. ignavum began with 1 1/4 turns around the peristomial disc. From there, they extended into the infundibulum performing another 3/4 turn in Z. mariella sp. nov. and 1/4 turn in Z. ignavum. In Z. alternans, the paroral membrane and the adoral membranelle 1 made 1 1/3 turns around the peristomial disc before entering the infundibulum, where they performed another full turn (Table 3). Furthermore, the paroral membrane and the adoral membranelle 1 of Z. mariella sp. nov. exhibited a conspicuous curve-shape in the very beginning, neither present in Z. ignavum nor in Z. alternans [[
Graph
Table 3 Comparison between Zoothamnium mariella sp. nov, Z. ignavum, and Z. alternans.
colony (S1 Table) max. size [mm] 1 1.8 1.2 st + br + sp [%] 50 40 80 st ‐ br + sp [%] 40 30 10 st ‐ br–sp [%] 10 30 10 branches 7–8 at least 22; variable at least 19; variable microzooids (S2 Table) length [μm] 23.8 ± 2.6 39.4 ± 3 48.4 ± 4.9 oral width [μm] 28.3 ± 1.6 28.8 ± 3.1 29.3 ± 1.7 aboral width [μm] 6.5 ± 1 8.2 ± 1.9 - oral ciliature 1 ¼ turns around the peristomial disc, infundibular kineties perform another ¾ turn 1 ¼ turns around the peristomial disc, infundibular kineties perform another ¼ turn 1 1/3 turns around the peristomial disc, infundibular kineties perform another full turn macronucleus S-shaped S-shaped J-shaped habitat marine marine marine reference this study [ [
1 st + br + sp: stalk with branches and spasmoneme; st ‐ br + sp: stalk without branches but with spasmoneme; st ‐ br ‐ sp: stalk without branches and spasmoneme
Molecular phylogenetic analyses based on the 18S rRNA gene sequence revealed that Z. mariella sp. nov. belongs to clade II of the family Zoothamnidae [[
Microscopic investigations and molecular biological analyses demonstrated that a single species of bacteria, Candidatus Fusimicrobium zoothamnicola gen. nov., sp. nov., forms an ectosymbiotic association with Zoothamnium mariella sp. nov. These bacteria densely populated the stalk, the branches, the macrozooids, the microzooids, and the terminal zooids.
The 16S rRNA gene sequence assigned the ectosymbiont Ca. Fusimicrobium zoothamnicola gen. nov., sp. nov to a monophyletic clade within the Gammaprotoebacteria. Also, the ectosymbiont of Z. ignavum Ca. Navis piranensis, the thiotrophic ectosymbiont of Pseudovorticella sp. (Peritrichia, Sessilida, Vorticellidae), and a free-living bacterium associated with intertidal hydrothermal vents from southern California belonged to this clade. The ectosymbionts of the two host sister taxa, Z. mariella sp. nov and Z. ignavum, both from the northern Adriatic Sea, however, were not found to be sister taxa themselves. Instead, the sister taxon of Ca. Fusimicrobium zoothamnicola gen. nov., sp. nov. turned out to be the free-living vent bacterium [[
At the basal part of the stalk of large Z. mariella sp. nov. colonies, we, occasionally, found the monospecific bacterial coat to be replaced by various, unspecific bacteria. Similar nonspecific epigrowth occurred in Z. ignavum [[
In the Z. mariella sp. nov. symbiosis, the bacterial coat comprised only a single, spindle-shaped morphotype of Ca. Fusimicrobium zoothamnicola gen. nov., sp. nov. This morphological uniformity suggests that the nutritional supply for the ectosymbionts is similar regardless of location on the host, because cell form modulations in bacteria are considered to be exclusively related to nutrition [[
We found this new symbiosis between Zoothamnium mariella sp. nov. and Candidatus Fusimicrobium zoothamnicola gen. nov., sp. nov. in three different shallow water habitats in the northern Adriatic Sea, a subtidal sediment, a subtidal mudflat, and a canal, on various substrates (sunken wood, plastics, dead bryozoans, macroalgae, shells, and rocks), in summer and in winter. It tolerates at least temperatures ranging from 8°C to 27°C as well as oxygen concentrations between 168 and 267 μmol L
The cultivation experiment, in which countless symbiotic Z. mariella sp. nov. colonies grew on a glass surface in untreated seawater, ultimately demonstrated that this symbiosis prospers under oxic conditions without a source of sulfide. A further Zoothamnium-bacteria symbiosis cultivable in steady flow–through systems is the thiotrophic ectosymbioses between Z. niveum and Ca. Thiobius zoothamnicola. In their 1996 redescription of Z. niveum, Bauer-Nebelsick et al. have already mentioned that the ectosymbiotic bacteria are probably sulfide oxidizers. They based their conclusion on the ectosymbionts' conspicuous white colour, indicative of inclusions of elemental sulfur, and the presence of ribulose-l,5-bisphosphate carboxylase oxydase, a key enzyme in the Calvin-Benson cycle [[
S1 Fig
Epifluorescent micrographs showing unspecific bacterial epigrowth on the basal part of the stalk of large Zoothamnium mariella sp. nov. colonies.
a, d) DAPI (blue), b, e) EUB mix in Cy5 (green), c, f) probe ZMS152 and ZMS1239 in Cy3 (red) did not hybridize.(TIF)
S2 Fig
Differential interference contrast (DIC) micrographs of living Zoothamnium mariella sp. nov. colonies with bacterial coat.
a) branch with microzooids and a terminal zooid, b) microzooid, c) branch. mi: microzooid, t: terminal zooid, br: branch.(TIF)
S1 Table
Measurements taken from micrographs of living Zoothamnium mariella sp. nov. colonies.
(XLSX)
S2 Table
Morphometric characterization of Zoothamnium mariella sp. nov. zooids based on micrographs of living specimens.
(XLSX)
S3 Table
Morphometric characterization of Ca. Fusimicrobium zoothamnicola based on SEM-micrographs.
(XLSX)
We thank Florian Scharhauser for valuable advice on cloning and probe design as well as Salvador Espada–Hinojosa for help with the phylogenetic analyses. Furthermore, we are grateful to Aharon Oren and Alessandro Minelli for sharing their extensive knowledge about bacterial and zoological nomenclature, respectively. Finally, we would like to acknowledge the Marine Biology Station Piran for their warm hospitality and the Core Facility of Cell Imaging and Ultrastructure Research at the University of Vienna for support on the scanning electron microscope.
By Vincent Kendlbacher; Teresa Maria Rosa Winter and Monika Bright
Reported by Author; Author; Author