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Received 12 Jun 2014 | Accepted 24 Jul 2014 | Published 15 Sep 2014

Nika Pende1,*, Nikolaus Leisch1,*, Harald R. Gruber-Vodicka2, Niels R. Heindl1, Jrg Ott3, Tanneke den Blaauwen4 & Silvia Bulgheresi1,5

Two long-standing paradigms in biology are that cells belonging to the same population exhibit little deviation from their average size and that symmetric cell division is size limited. Here, ultrastructural, morphometric and immunocytochemical analyses reveal that two Gammaproteobacteria attached to the cuticle of the marine nematodes Eubostrichus fertilis andE. dianeae reproduce by constricting a single FtsZ ring at midcell despite being 45 mm and 120 mm long, respectively. In the crescent-shaped bacteria coating E. fertilis, symmetric

FtsZ-based ssion occurs in cells with lengths spanning one order of magnitude. In theE. dianeae symbiont, formation of a single functional FtsZ ring makes this the longest unicellular organism in which symmetric division has ever been observed. In conclusion, the reproduction modes of two extraordinarily long bacterial cells indicate that size is not the primary trigger of division and that yet unknown mechanisms time the localization of both DNA and the septum.

DOI: 10.1038/ncomms5803 OPEN

Size-independent symmetric division in extraordinarily long cells

1 Department of Ecogenomics and Systems Biology, University of Vienna, Althanstrasse 14, 1090 Vienna, Austria. 2 Department of Symbiosis, Max Planck Institute for Marine Microbiology, Celsiusstrasse 1, D-28359 Bremen, Germany. 3 Department of Limnology and Biooceanography, University of Vienna, Althanstrasse 14, 1090 Vienna, Austria. 4 Department of Bacterial Cell Biology, Swammerdam Institute of Life Sciences, Faculty of Science, University of Amsterdam, Science Park 904, 1098 XH Amsterdam, the Netherlands. 5 Center for Anatomy and Cell Biology, Medical University of Vienna, Wahringerstrasse 10, 1090 Vienna, Austria. * These authors contributed equally to this work. Correspondence and requests for materials should be addressed to S.B.(email: mailto:[email protected]

Web End [email protected] ).

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The spatial control of bacterial growth, division and morphologyas well as the mechanisms of DNA organization and segregationhas been investigated only in a

handful of cultivable organisms so far1. Given the overwhelming phylogenetic and morphological diversity of microbes, our current knowledge on their cell biology likely represents only a tiny piece of the overall picture. This is regrettable given that the void in antibiotics discovery2, coupled with an increasing awareness about the role of uncultivable, non-pathogenic microbes in animal health, implies major applied benets from studying how environmental bacteria reproduce.

Most known bacteria are between 0.4 and 2 mm in diameter, and 0.5 and 5 mm in length. Model rod-shaped bacteria control their overall size by varying their cell length, which, in turn, is under control of the division apparatus3,4. Escherichia coli, for example, can grow into long, aseptate laments with regularly spaced nucleoids following mutations in lamentous temperature sensitive (fts) genes, which direct the assembly of the division apparatus5. Although these E. coli mutants cannot build a functional constricting ring and nally lyse, DNA replication and chromosome segregation continue unaffected for several generations.

The metabolic status of the cell may also affect bacterial length: Bacillus subtilis is longer when incubated in a nutrient-rich medium and shorter when nutrients are limited6,7. In the former case, B. subtilis accumulates a metabolite that induces a glucosyltransferase. This, in turn, inhibits FtsZ polymerization so that cell division is delayed and the cells grow longer8. In a striking example of convergent evolution, the size of E. coli is similarly linked to nutrient availability by a different but functionally analogous glucosyltransferase912.

With the sole exception of the giant surgeonsh gut symbiont13, the molecular basis of the reproduction of naturally occurring long to giant bacteria (longest length between 10 and 750 mm) is unexplored. Many of them are marine sulphur-oxidizing bacteria (SOBs) and contain large nitrate and sulphur inclusions that reduce the volume of their active cytoplasm14. Here we investigated the molecular mechanisms underlying the reproduction mode of two extraordinarily long bacteria coating the newly described nematode species Eubostrichus fertilis (Fig. 1ad and Supplementary Fig. 1a)15 and E. dianeae16,17 (Supplementary Fig. 1b; hereafter we refer to these lamentous bacteria as Efs and Eds, respectively). Eds contains strongly refracting spherical cytoplasmic inclusions17 and Raman

microspectrometry proved that at least some of these contain elemental sulphur18,19. Although these data suggest that Eds may store and oxidize sulphur, previous 16S ribosomal RNA (rRNA) gene-based analyses of the E. dianeae-associated bacterial community did not yield any SOB 16S rRNA gene sequence20. As for E. fertilis, crescent-shaped bacteria are attached with both poles to their nematode host so that their long axis is always parallel to the hosts anteriorposterior axis. This, combined with their shifted alignment to one another around the worm circumference, confers a rope-like appearance (Fig. 1a), similar to that observed for E. cf. parasitiferus16,17,E. topiarius21 and Adelphus rolandi22. Although DNA staining of E. cf. parasitiferus-associated bacteria revealed several nucleoids in each cell17, binary ssion was detected neither in these, nor in Eds cells. It was therefore hypothesized that both ectosymbionts elongate without dividing, possibly due to nematode-secreted inhibitors17.

This study was designed to determine how supersized bacteria associated with two Eubostrichus nematodes reproduce on their respective hosts.

ResultsOne bacterial phylotype coats each nematode species. To molecularly identify the lamentous bacteria coating E. fertilis and E. dianeae, we extracted genomic DNA (gDNA) from single symbiotic worms and constructed bacterial 16S rRNA gene libraries. Based on BLASTN search, we identied three and seven SOB 16S rRNA sequences in the E. fertilis and E. dianeae libraries, respectively. We compared these SOB sequences to those of other stilbonematid and oligochaete symbionts, as well as to those of bacteria belonging to the Chromatiaceae and other uncultured Gammaproteobacteria that are 495% similar to the symbionts. The resulting 16S rRNA gene-based phylogenetic tree (Fig. 2) shows that the representative SOB sequences, each obtained either from the E. fertilis or the E. dianeae 16S rRNA gene library (GenBank accession numbers KF278590 and KF278587, respectively) belong to the Marine Oligochaete and Nematode Thiotrophic Symbionts (MONTS) cluster of Gammaproteobacteria23 and are most closely related toE. topiarius-associated bacteria. To conrm that the MONTS 16S rRNA sequences obtained in our libraries originated from Efs and Eds, we applied uorescence in situ hybridization (FISH) probes specically targeting those sequences (probe Efs1057 and

Figure 1 | Scanning electron microscope (SEM) micrographs of the E. fertilis ectosymbiont. (a) Central portion of the bacterial coat and (bd) single constricted Efs cells of different lengths. Scale bar, 20 mm in a, 1 mm in b and 5 mm in c,d.

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Eubostrichus topiarius associated bacterium 1 FM955324 Eubostrichus topiarius associated bacterium 2 FM955325

Eubostrichus dianeae ectosymbiont KF278587

Eubostrichus topiarius associated bacterium 3 FM955326 Eubostrichus fertilis ectosymbiont KF278590

Acropora palmata associated bacterium C20 GU118064

Acropora palmata associated bacterium P04 GU118120 Laxus oneistus ectosymbiont KF278591

Olavius crassitunicatus Gamma1 endosymbiont clone g1-P14-I-18AJ620507 Astomonema sp. endosymbiont clone LSI-A2 DQ408758

Astomonema sp. endosymbiont clone LSI-A1 DQ408757 Olavius loisae Gamma1 endosymbiont AF104472 Olavius ilvae Gamma 1 endosymbiont clone OilvEIV1-1 AJ620498

Laxus cosmopolitus associated bacterium clone 3 AJ319039 Robbea sp. 1 ectosymbiont SB-2008 EU711427Laxus cosmopolitus associated bacterium FM955323

Stilbonema majum ectosymbiont clone 5 HM776017 Stilbonema sp. associated bacterium 5 I 11 FM955330

Stilbonema sp. associated bacterium 5 I 2 FM955329 Stilbonema sp. associated bacterium 8 II 6 FM955331 Robbea sp. associated bacterium 252 II 14 FM955327 Robbea sp. 3 ectosymbiont SB-2008 EEU711428 Olavius algarvensis Gamma1 endosymbiont AAF328856 Robbea sp. associated bacterium 253 I 14 FM955328 Catanema sp. associated bacterium 3 VII 7 FM955322Robbea sp. 2 ectosymbiont SB-2008 EEU711426

Inanidrilus makropetalos Gamma1 endosymbiont clone SpecB-g1-3-16AJ890094 Inanidrilus leukodermatus Gamma1 endosymbiont SSOU24110Inanidrilus leukodermatus Gamma1 endosymbiont clone Ileu2 AJ890100 Uncultured gamma proteobacterium clone ANOX-045 J JF344607Uncultured gamma proteobacterium clone OXIC-054 J JF344324Uncultured gamma proteobacterium clone RODAS-122 J JF344100Marichromatium purpuratum 984 AFWU01000015

Thiocapsa marina 5811 AFWV01000002

Allochromatium vinosum DSM 180 NC_013851 Thiorhodococcus drewsii AZ1 AFWT01000001

MONTSChromatiaceae

98 | 0.96 66 | 0.99

100 | 1.00

31 | -

100 | 1.00

Eubostrichus

symbionts and

associated

bacteria

52 | 0.94

21 | 0.69

37|0.67

98 | 0.99

31 | 0.54

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64 | 0.97

96 | 1.00

56 | 0.85

70 | 0.77

100 | 1.00

100 | 1.00

100 | 1.00

80 | 0.70

89 | 1.00

100 | 1.00 50 | 0.9547 | 0.91

60 | 0.98

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55 | 0.98

100 | 1.00

94 | 0.99

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100 | 1.00

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42 | 0.68

0.05

Figure 2 | Gammaproteobacterial 16S rRNA gene tree based on the most likely RAxML tree (GTR I G model of substitution). Rapid bootstrapping

(RAxML) and posterior probability (MrBayes) node support is given for all nodes. The minus symbol ( ) instead of a posterior probability in the

Eubostrichus-associated bacteria cluster indicates that this node was not resolved in the MrBayes consensus. The Chromatiaceae outgroup is indicated with grey font colour. Scale bar represents the mean number of nucleotide substitutions per site. GenBank accession numbers are indicated after the names of the sequences.

Eds214, respectively) to whole mount Eubostrichus nematodes. All bacteria attached to the host surface were triple stained by the bacterial probe EUB338, by the Gammaproteobacteriaspecic probe GAM42a and by the respective MONTS-specic probes (Fig. 3 and Supplementary Fig. 2). This conrms that the MONTS 16S rRNA gene sequences obtained in our libraries originated from the lamentous bacteria coating E. fertilis and E. dianeae. Moreover, given that all bacteria detected by the Eubacteria-specic probe were also detected by the Gammaproteobacteria- and MONTS-specic probe, the non-MONTS 16S rRNA gene sequences identied in our libraries, including those attributable to Deltaproteobacteria (Supplementary Fig. 2) did not originate from cuticle-associated bacteria. In conclusion, Efs and Eds are two novel distinct MONTS phylotypes, each one associated with the respective host species. The phylogenetic placement of Eds and Efs is consistent with that observed for all marine nematode

ectosymbionts characterized by full 16S rRNA-gene cycle so far2426. Moreover, given that Efs and Eds were the only bacteria detected on the surface of their respective hosts, these newly characterized stilbonematid ectosymbioses also appear to be monospecic.

The nematode symbionts express the tubulin homologue FtsZ. In the model gammaproteobacterium E. coli, cell division is initiated by polymerization of the tubulin homologue FtsZ into a ring (the Z-ring) and its subsequent constriction2729. In E. coli cells, the ring is usually positioned at midcell, perpendicular to the longitudinal axis30. After the self-assembly the Z-ring starts to constrict, thereby directing the division of the cell, which results in two equal daughter cells. Given that FtsZ mediates binary ssion in all known Gammaproteobacteria, including the longitudinally dividing MONTS associated with Laxus

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Figure 3 | FISH/laser-scanning confocal microscopy (LSCM) of ectosymbionts attached to the worm surface. Images of the Efs coat are shownin ae and images of the Eds coat in fj. a and f are the corresponding bright eld images of be and gj, respectively. Each single symbiont is triple stained with specic probes targeting Eubacteria (b and g), Gammaproteobacteria (c and h), and the symbiont (Efs1027 and Eds214, respectively; d and i).(e) and (j) are overlay pictures of (bd) and (gi), respectively. A single Efs cell is shown in the insets in (ae). Scale bar, 25 mm for all images and 5 mm for the insert.

Table 1 | Size measurements of the Eubostrichus fertilis and the Eubostrichus dianeae symbionts.

Eubostrichus fertilis symbiont (n 2,731)

oneistus31, and it is part of the genetic repertoire of three additional MONTS (genome drafts available upon request at http://rast.nmpdr.org/rast.cgi

Web End =http://rast.nmpdr.org/rast.cgi ), we hypothesized that Efs and Eds also express the ftsZ gene. By using degenerate PCR primers on gDNA extracted from single symbiotic nematodes, we homology cloned Efs and Eds ftsZ-gene fragments. The predicted Efs FtsZ protein fragment (322 amino acids) had 83% sequence identity with that of the L. oneistus ectosymbiont, and 67% with that of E. coli K12, whereas the corresponding sequence identities for the predicted Eds FtsZ protein fragment (336 amino acids) were 84% and 66%, respectively. The Eubostrichus symbiont FtsZ proteins cluster with other MONTS FtsZ proteins in our phylogenetic reconstruction (Supplementary Fig. 3). To assess if the Eubostrichus ectosymbionts express FtsZ, a commercially available anti-E. coli FtsZ antibody was tested on Western blots of protein extracted from host-dissociated ectosymbionts. This resulted in the specic detection of protein bands of B40 kDa, the predicted molecular weight of E. coli FtsZ (Supplementary Fig. 4). In conclusion, both Efs and Eds express the cell division protein FtsZ and their genes are phylogenetically related to theL. oneistus ectosymbiont FtsZ and form a 16S rRNA gene-concordant cluster.

Symmetric FtsZ-based ssion in 4 to 45 lm-long Efs cells. Morphometric analysis of 2,731 Efs cells showed a length range of3.5444.55 mm and a width range of 0.381.21 mm (Table 1; Supplementary Fig. 5) and scanning electron microscopy (SEM) analysis revealed constricted cells of lengths ranging from 6.1 to23.2 mm (Fig. 1bd). Consistently, Efs cell length distribution indicated that most length values are similarly represented in the population (Supplementary Fig. 5). To test the hypothesis that Efs cells can divide at any length, we immunostained them with an anti-FtsZ antibody and analyzed its localization pattern. FtsZ rings appeared in 77/662 cells (11.6%) between 3.5 and 45 mm long (Fig. 4a,b,d,f and Supplementary Fig. 6). Unsegregated DNA localized at midcell in cells with homogeneous FtsZ staining (Fig. 4e left plot and representative image in Fig. 4c), whereas DNA was already segregated in cells with mid-cell (non-ring) FtsZ accumulation (Fig. 4e, middle plot). In cells showing a

Z-ring (e.g. insert Fig 4d insert), we observed symmetric DNA segregation both in terms of localization and of uorescence signal intensity (Fig. 4e, rightmost plot). Of note, in these cells, the DNA signal was often highly fragmented as if originating from several nucleoids (see for example Fig. 4b or Supplementary Fig. 6b,n). Mid-cell membrane constriction in correspondence with mid-cell FtsZ signal indicates that FtsZ polymerized into a functional constricting ring (Fig. 4f). FtsZ uorescence proles of 662 cells aligned from the shortest to longest (left to right in Supplementary Fig. 7ad) did neither indicate a continuous FtsZ uorescence accumulation at midcell, nor a continuous DNA partitioning pattern as Efs lengthens. However, most of the cells displaying mid-cell FtsZ signal (62.3%; Supplementary Table 1) were 1530-mm long. We conclude that Efs cells divide by

FtsZ-based ssion and may symmetrically segregate the DNA at virtually every length leading to a 10-fold variation in cell length.

Symmetric FtsZ-based ssion in up to 120-lm-long Eds cells. Each Eds lament is attached to the nematode host by one of its poles (Supplementary Fig. 1b,d). Morphometric analysis of 2,743 Eds cells showed a length range 16.5120.2 mm and a width range of 0.41.4 mm (Table 1), albeit most cells are B50-mm long (Supplementary Fig. 5). To assess if Eds divides via FtsZ-based ssion, we immunostained it with an anti-FtsZ antibody and

Eubostrichus dianeae symbiont (n 2,743)

length (lm) width (lm) length (lm) width (lm) Minimum 3.54 0.38 16.46 0.41

Maximum 44.55 1.21 120.22 1.40 Mean 16.23 0.60 49.70 0.75 s.d. 7.06 0.08 14.70 0.12

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FtsZ DNA

30

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Figure 4 | FtsZ and DNA localization pattern in Efs cells. (ad) From left to right, phase contrast, FtsZ uorescence, DNA uorescence and FtsZ (green)/DNA (red) overlay images of immunostained Efs cells of different lengths (a,b and d have FtsZ rings and segregated DNA, c has neither mid-cell FtsZ accumulation nor segregated DNA). Insets in d show an LSCM image of an FtsZ ring from a different cell. e shows average uorescenceproles of 549 cells displaying neither FtsZ mid-cell accumulation nor DNA segregation (left), 36 cells with both non-ring FtsZ accumulation at mid-cell (middle) and segregated DNA, and 77 cells with FtsZ rings and segregated DNA (right). FtsZ uorescence (green) and DNA uorescence (red) expressed in arbitrary units (a.u.) are plotted along the cell length expressed in percentage. LSCM images of an immunostained Efs constricted cellare shown in f, from left to right bright eld, FtsZ uorescence and overlay. Scale bars. 2 mm in a, 5 mm in b,c and f and 10 mm in d.

analyzed its localization pattern. In the shortest cells, FtsZ was homogenously distributed throughout the cell, whereas unsegregated DNA localized at midcell (Fig. 5ad, the shortest cells correspond to the bars occupyingapproximatelythe leftmost third of the prole; representative single cell in Fig. 5e and leftmost plot in h). In the medium length cells, FtsZ uorescence accumulated in a central portion of the cell between the segregated DNA (central third of each prole in Fig. 5ad, representative image in f and central plot in h). In the longest cells, FtsZ appeared as a sharp, mid-cell band and DNA was further segregated into the two prospective daughter cells (rightmost third of each prole in Fig. 5ad, representative image in g and rightmost plot in h). Notably, and as observed for Efs, only a small fraction of the Eds cells displayed FtsZ rings (87/772,11.27%). However, all of them were longer than 30 mm, indicating that the propensity of Eds to divide increases as it lengthens (Supplementary Table 1). Plotting the DNA uorescence emitted by 301 cells with non-segregated DNA (representative image in Supplementary Fig. 8b) and by 237 cells with segregated DNA (representative image in Supplementary Fig. 8c) against the cell length conrmed symmetric partitioning of the DNA into the two prospective daughter cells (Supplementary Fig. 8a). As observed

in Efs cells displaying FtsZ rings, the DNA signal was often highly fragmented as if originating from several nucleoids (Supplementary Fig. 8c). Further, confocal microscopy revealed that mid-cell FtsZ polymerizes into a circular ring in Eds and that this is functional as it can drive cell membrane constriction (Fig. 5i). We conclude that the gammaproteobacterium Eds, despite its extraordinary length, divides transversally and symmetrically by means of a single, constricting FtsZ ring placed at midcell.

DiscussionIn this study we investigated the reproduction modes of two naturally occurring supersized bacteria at the molecular level. This is the only such study besides that on the rmicute symbiont inhabiting the surgeonsh gut13, and the rst one involving environmental sulphur-oxidizing Gammaproteobacteria (as shown by our 16S rRNA gene-based phylogeny). Although previous morphological studies suggested that Eubostrichus-associated lamentous bacteria do not divide17, we provided morphometric and immunocytochemical evidence that both Efs and Eds undergo binary ssion. As shown by FISH with specic probes targeting their rRNA genes, only Efs and Eds are

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12,000

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Figure 5 | FtsZ and DNA localization pattern in Eds cells. Cell length, FtsZ uorescence, DNA uorescence and overlay of FtsZ (green) and DNA (red) uorescence of 562 Eds cells are represented in ad, respectively. Cells are sorted by increasing cell length from left to right that is, the leftmostbar represents the shortest and the rightmost bar the longest cell. Cell length ranges from 16.46 to 82.54 mm (mean 43.1612.30). Dotted white line in bd indicates the cell outline. (eg) Phase contrast, FtsZ uorescence, DNA uorescence and FtsZ (green)/DNA (red) overlay images of immunostained

Eds cells of different lengths displayed from left to right in e and f and top to bottom in g. h shows average uorescence proles of 301 cells with homogeneous FtsZ staining and non-segregated DNA (left), 189 cells with FtsZ accumulation at mid-cell and segregated DNA (middle), and 54 cells with FtsZ rings and segregated DNA (right). FtsZ uorescence (green) and DNA uorescence (red) expressed in arbitrary units (a.u.) are plotted alongthe cell length in percentage. LSCM images of a constricted immunostained Eds cell is shown in i, bright eld and corresponding FtsZ uorescence below. Inset shows an LSCM image of a FtsZ ring from a different cell. Scale bars, 10 mm in e and f, 20 mm in g and 2 mm in i.

detectable on the surface of their respective hosts. Therefore, each nematode is carrying a virtually pure bacterial cell culture. This enabled us to analyze the localization pattern of the key division protein FtsZ and of the DNA in hundreds of symbiont cells. The fact that Eds appears to be the only bacterium coating its host seems to contradict a former study20, which suggested a high level of bacterial diversity associated with the nematode. However, all 16S rRNA gene sequences obtained in that rst study originated from bacteria commonly found in marine environments; given

the lack of whole nematode FISH-based evidence, these sequences likely originated from bacteria localized on nematode regions other than the cuticle (for example, the gut). Alternatively (or in addition), environmental bacteria non-stably associated with E. dianeae may also have been represented in the previously reported 16S rRNA gene library. Although our libraries were not extensively sequenced, they also contained non-MONTS 16S rRNA gene sequences (see Methods). Despite their heterogeneity, we could identify only a single MONTS phylotype (GenBank

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KF278587) and this appeared to be the only one present on the nematode cuticle by FISH. The lack of SOB sequences in the library constructed by Polz et al.20 could be due to a PCR bias, which we might have circumvented by using a shorter and more degenerate universal forward primer (616F instead of 27F). In conclusion, although we cannot exclude that bacteria other than Eds may occasionally be found on the E. dianeae surface, all nematode-coating bacteria visualized in our FISH analysis belong to a single MONTS phylotype. We observed the same for E. fertilis, suggesting high host-symbiont specicity for this newly described association as well.

The fact that there are no FtsZ rings overlapping with strong DNA signal is consistent with what is observed in E. coli and probably due to the phenomenon of nucleoid occlusion32; however, Efs and Eds DNA did not occupy the rst and the last 20% of the cell length at any cell stage (Figs 4e and 5h and Supplementary Fig. 8), suggesting yet unknown mechanisms excluding DNA from the poles and preventing FtsZ polymerization in the rst and the last 20% of the Eubostrichus ectosymbiont cells. Besides nucleoid occlusion, a second negatively acting mechanism, the Min system, dictates the selection of division sites in model bacteria5. In E. coli, the FtsZ inhibitor MinC, driven by the MinD and MinE proteins, oscillates back and forth between the two cell poles. As a consequence, MinC concentration is highest at the poles and lowest near midcell. As the cell elongates, the concentration near the cells centre is reduced until it becomes so low that FtsZ can polymerize and constrict the cell. Therefore, cell length is determined by the amount of MinC so that larger amounts produce longer cells33. The complete min operon is present in all the MONTS genomes sequenced so far (ref. 31 and genomic data available upon request for three additional MONTS at http://rast.nmpdr.org/rast.cgi

Web End =http://rast.nmpdr.org/ http://rast.nmpdr.org/rast.cgi

Web End =rast.cgi ), whereas there is no genomic evidence of another well-described FtsZ-positioning system, the DivIVA system. However, the analysis of symbiont MinC localization pattern is needed to draw conclusions about the involvement of the Min system in Eubostrichus ectosymbionts FtsZ-ring positioning.

Besides marine nematode ectosymbionts, several oversize endosymbionts have been described, such as legume-nodulating Alphaproteobacteria34, the gammaproteobacterium associated with Sitophilus weevils35, the bacteroidete Sulcia inhabiting sharpshooters36 and the rmicute Epulopiscium spp. thriving in the surgeonsh gut37. In the rst two systems, host-secreted antimicrobial peptides (nodule-specic cysteine-rich peptides38 and Coleopterycin-A39, respectively) inhibit bacterial ssion but not genome replication, which results in polyploidy. By blocking bacterial reproduction, hosts may better control the number and location of their endosymbionts34,39. The factors that trigger Epulopiscium sp. morphotype B extreme growth are still elusive, but polymerization of two polar FtsZ rings results in two intracellular daughter cells. These grow within the mother cell cytoplasm and are eventually released by perforating the mother cell envelope. Surprisingly, only a small portion of the mother DNA is passed on to the offspring13,40, as reviewed in ref. 41. The fragmentation of the DNA staining frequently observed in Eubostrichus-associated laments suggests that they are polyploid (as is the case for all aforementioned oversize endosymbionts) and that chromosomes are segregated prior to and independently from septation. This is consistent with the hypothesis that condensation resolution should be sufcient to segregate replicated sister chromosomes before cytokinesis42. However, more sensitive techniques such as FISH with oriC-specic probes are needed to determine the maximum genome copy numbers and the segregation dynamics in dividing Efs and Eds.

FtsZ immunostaining of Eubostrichus-coating bacteria revealed that, despite their large size and the likely presence of multiple

genomes, they divide by symmetric transverse ssion. Therefore, in contrast to all aforementioned endosymbionts that grow to extraordinary sizes because they either do not divide or they do so atypically, Eubostrichus-coating bacteria may become outstandingly long due to a delay in canonical binary ssion. Given that Eds and Efs have not been isolated yet, we do not know whether nematode-secreted molecules mediate this delay or whether this delay is intrinsic to the bacteria. In the rst case, Eds and Efs would represent the rst bacteria whose growth is under host control in an ectosymbiosis, a form of association commonly considered less intimate than endosymbiosis. Besides cultivation, morphometric analysis of ectosymbionts associated with juvenile nematodes might reveal a correlation between bacterial length and host developmental stage.

It is intriguing to speculate that a similar mechanism coordinating B. subtilis or E. coli size with metabolic state (see Introduction) is at work in Eubostrichus symbionts. The FtsZ and DNA proles of the crescent-shaped Efs, which are attached to its host with both poles, showed that it may divide at virtually any cell length between 3 and 45 mm. The bacterial coat is highly ordered (Fig. 1a) with the short crescent-shaped cells being proximal (that is, close to the host surface) and the long crescents being distal (Supplementary Fig. 1a,c). Their chemosynthetic metabolism relies on the diffusion of reduced sulphur compounds (for example, H2S) and oxygen. If we assume that the distal Efs cells have better access to them and grow faster, less nutrients will be available for the proximal ones, which will therefore grow slower. Given that Eds laments are monopolarly attached to their host (Supplementary Fig. 1b,d), the accessibility to sulphide and oxygen does not differ among them so that they may all experience the same growth rate. The ecological advantage of the two different bacterial coat architectures remains to be determined and might be due to differences in the physiology and/or behaviour of the two Eubostrichus hosts.

Taken together, this rst molecular study of the reproduction of two environmental Gammaproteobacteria showed that they may vary over 12 times in cell length, largely exceeding the size variation observed in model bacteria, and that they can divide by FtsZ-based symmetric binary ssion up to a length of 120 mm. This implies that novel molecular machineries may time cell division and position the genome and division plane in Gammaproteobacteria, a class of several ecologically and medically important bacteria.

Methods

Nematode collection. Specimens of E. fertilis and E. dianeae were collected in December 2011/January 2012 and in March/April 2014 in B1 m depth from a sand bar off Twin Cays, Belize (16 490 25.7400 N, 88 60 21.1800 W). The nematodes were extracted from the sand by stirring the sand in seawater and pouring the supernatant through a 63-mm-pore-size mesh sieve. The content of the net was transferred into a Petri dish and single individuals were then picked by hand using ne tweezers under a dissecting microscope. E. dianeae identity was assessed morphologically according to the study by Hopper et al.16 and molecularly according to the study by Kampfer et al.43 This nematode has also been referred to as E. dianae in the literature. To establish E. fertilis identity, eukaryotic 18S rRNA gene libraries were constructed using the same two gDNA extractions employed for constructing bacterial 16S rRNA gene libraries (see below). E. fertilis 18S rRNA gene-based phylogenetic placement is published elsewhere15. For gDNA extraction, Western blotting, FISH and immunostaining, nematodes were xed in methanol and stored at 20C for transportation and storage. For SEM, nematodes were

xed with 2.5% glutaraldehyde and stored at 4 C.

Scanning electron microscopy. Worms were either directly post-xed with 1% osmium tetroxide for 2 h at room temperature, or the bacteria were rst dissociated from the nematodes by mild sonication, allowed to settle on poly-L-lysine treated coverslips and then post-xed. The samples were dehydrated in a graded ethanol series, transferred into pure acetone and critical point dried with a CPD 300 unit (Leica). After mounting, either whole worms or the bacteria-coated coverslips on stubs were gold-sputtercoated with an AGAR B7340 sputtercoater unit. Images were taken with a XL20 (Philips) using the Microscope control programme (version 7.00, FEI).

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gDNA extraction, PCR and cloning of 16S rRNA genes. For the construction of the E. dianeae and E. fertilis 16S rRNA gene libraries gDNA was extracted from two single E. dianeae and two single E. fertilis nematodes as previously described44. gDNA (2 ml) were used as template in each 50 ml PCR reaction. Fragments (1,499-nucleotide (nt)-long) of bacterial 16S rRNA genes were amplied by PCR with primers 616V (50-AGAGTTTGATYMTGGCTC-30)45 and 1492R (50-GGYT

ACCTTGTTACGACTT-30)46. Cycling conditions for the 16S rRNA gene amplication were as follows: 94 C for 4 min followed by 35 cycles of 94 C for 45 s, 49 C for 30 s, 72 C for 90 s and a nal elongation of 72 C for 10 min. We randomly picked and fully sequenced eight clones from the two E. fertilis 16S rRNA gene libraries. Three belonged to members of the MONTS23 cluster, two were from Desulfobulbaceae, one from Oceanospirillales, one from Staphylococcus and one from an unclassied bacterium. We randomly picked and fully sequenced 31 clones from the two E. dianeae 16S rRNA gene libraries. Thirteen clones were from sulphur-reducing Deltaproteobacteria, seven belonged to members of the MONTS cluster, three were from Cytophaga, ve from Rhodospirillales and three from unclassied bacteria. Sequences were assembled with CodonCode Aligner 3.7.1 software (CodonCode Corporation, Dedham, MA, USA).

Homology cloning of Eubostrichus ectosymbiont ftsZ genes. gDNA was extracted from a single E. fertilis and a single E. dianeae as described above for the amplication of rRNA genes. For homology cloning of the Eds ftsZ gene, a 1,106 nt-long fragment was amplied using degenerate primers ftsz1F (50-GCVGTVA

TYAARGTBATCGG-30) and ftsZ2.1R (50-GCYGGRATRTCSAGRTAATC-30). For homology cloning of the Efs ftsZ gene, an additional amplication step was performed on the 1,106 nt-long ftsz1F-ftsZ2.1R fragment with the nested primer ftsZ1Fnes1 (50-ATCAAGGTTATCGGGGT-30). Touchdown PCR conditions for both degenerate and nested PCRs were as follows: 94 C for 3 min, followed by8 cycles at 94 C for 45 s, 5850 C for 45 s, 72 C for 75 s, followed by 27 cycles 94 C for 45 s, 50 C for 45 s, 72 C for 75 s, and a nal elongation step at 72 C for 10 min. The Efs ftsZ-gene fragment was directly sequenced in both directions. The Eds ftsZ-gene fragment was cloned as described above for the rRNA genes and four clones containing the Eds ftsZ-gene fragment were fully sequenced in both directions. All the sequences were aligned and compared with CodonCode Aligner3.7.1 software. We obtained a 967 nt-long sequence for Efs (GenBank accession number KF453620) and a 1.007 nt-long sequence for Eds (KF453619).

16S rRNA gene-based phylogenetic analysis. A bacterial 16S rRNA gene dataset was constructed by adding sequences from GenBank with 495% identity to Efs and Eds using BLASTN47 and selected Chromatiaceae as an outgroup. The sequences were aligned with MAFFT Q-INSi48. To reconstruct the phylogenetic relationsof the symbionts we used the GTR G I model with maximum likelihood

(RAxML49) and Bayesian inference (MrBayes50) based algorithms. To evaluate node stability we performed a rapid bootstrapping analysis (RAxML, 200 runs; ref. 51) and used posterior probabilities (MrBayes, two million generations, burnin of 25%).

Fluorescence in situ hybridization (FISH). By using the arb PROBE_DESIGN tool (the arb software package52; Table 2), we designed two FISH probes (Eds214 and Efs1057) specic to the SOBs identied in the E. fertilis and E. dianeae 16S rRNA gene libraries (GenBank accession numbers KF278590 and KF278587,

respectively). In addition, we designed a probe (SRB64) targeting the Deltaproteobacteria identied in the E. dianeae 16S rRNA gene library (GenBank accession number KJ877189). We conrmed their specicity by comparing them with all available sequences in GenBank, the arb-silva 114 database53 and RDP (Ribosomal Database Project) rel.10.32 (ref. 54). The Eds214 probe has 0/3/1357 non-target hits in RDP allowing for 0/1/2 mismatches, the Efs1057 0/12/3725 and the SRB64 probe 2/493/677. All probes were uorescently labelled on their 50 end (Thermo Fisher Scientic, Ulm, Germany). FISH was performed on

Eubostrichus nematodes according to the study by Manz et al.55 and as applied in the study by Bulgheresi et al.25,26. A detailed overview of all probes and formamide concentrations used in the different experiments is given in Table 2. To determine stringent hybridization conditions, a formamide series was conducted for all the probes (10, 15, 20, 25, 30, 35, 40 and 50%; refer to Table 2 for optimal incubation time, formamide percentage and probe concentrations). Nematodes were mounted in Vectashield (Vector Labs, Burlingame, CA, USA). When performing FISH with SRB64, bacteria were dissociated from E. dianeae cuticle prior to mounting. Dissociation was performed to ensure that all the bacteria attached to the cuticle would be equally prone to visual inspection, that is, to ensure that the signal emanating from putative normal-sized Deltaproteobacteria would not be masked by the numerically dominant, giant Eds cells. Symbiotic nematodes or dissociated symbionts were examined using a Leica TCS-SP2 confocal laser-scanning microscope combined with an inverted DM-IRE2 microscope (Leica Microsystems, Heidelberg, Germany). The EUB338 probe is from the study by Amann et al.56, Gam42a and Beta42a from the study by Manz et al.55 FISH probe names refer to their target on the E. coli 16S rRNA, numbering according to 57.

Bacterial cell size and uorescence measurements. Cells were immobilized on 1% agarose and photographed using a Leica TCS-SP2 confocal laser-scanning microscope combined with an inverted DM-IRE2 microscope (Leica Microsystems) or a Nikon Eclipse 50i microscope equipped with either a DS-Fi1 camera (Nikon) or a MFCool camera (Jenoptik). Epiuorescence images were acquired using the NIS Elements F 3.22 software (Nikon) or the ProgRes Capture Pro 2.8.8 software (Jenoptik) and processed using the public domain programme ImageJ58 in combination with the analysis tool Coli-Inspector59. Cell outlines were traced and cell length and width were measured automatically. Automatic tracing was manually double-checked and errors removed (for example, multiple cells counted as one). In the uorescence proles each bar represents a single bacterial cell, and the intensity of uorescence is displayed as intensity of the respective colour (Ftsz in green and DNA in red in the overlay). The cells were sorted by increasing length from left to right. For the average uorescence proles, each cell was resampled to the same length and the intensities then averaged. For the uorescence proles, data were acquired from a single immunostaining. For the morphometric analysis and the length histograms, data from multiple experiments were pooled.

Western Blotting, immunostaining and DNA staining. For Western blots, Efs and Eds protein extractsobtained from dissociated ectosymbiontswere separated by reduced SDSpolyacrylamide gel electrophoresis (PAGE) on NuPAGE 412% Bis-Tris pre-cast gels (Invitrogen). They were then transferred to Hybond ECL nitrocellulose membranes (Amersham Biosciences). Membranes were blocked for 45 min in phosphate-buffered saline (PBS) containing 5% (wt/vol) nonfat milk

Table 2 | Probes used for FISH.

Probe Specicity Sequence/50 modication Target RNA

Position* Formamide percentage/ incubation time (h)/ probe concentration (ng ll 1)

Reference

EUB338 Most bacteria 50-GCTGCCTCCCGTAGGAGT-30Fluorescein

16S 338355 40%/12/3.8 Amann et al.56

GAM42a Gammaproteobacteria 50-GCCTTCCCACATCGTTT-30Cy5

23S 1,0271,043 40%/12/2.4 Manz et al.55

BETA42a Betaproteobacteria 50-GCCTTCCCACTTCGTTT-30Cy3

23S 1,0271,043 40%/12/2.4 Manz et al.55

Eds214 E. dianeae ectosymbiont 50-GCTCATCATCATAGCGGAA-30

Cy3

16S 214235 40%/12/2.4 This study

Eds214mis One mismatch to theE. dianeae ectosymbiont

50-GGCTCATCATCTTAGCGGAAG-30 Cy3

16S 214235 40%/12/2.4 This study

SRB64 Sulphate-reducing

Deltaproteobacteria identied in the 16S rRNA gene library

50-TGCAAGCAACCCCTTTCTCGTT-30 Fluorescein

16S 6486 40%/12/3.8 This study

Efs1027 E. fertilis ectosymbiont 50-TCACCGCGCTCCCAAGG-30

Cy3

16S 1,0271,044 30%12/2.4 This study

Efs1027mis One mismatch to theE. fertilis ectosymbiont

50-TCACCGCGCACCCAAGG-30 Cy3

16S 1,0271,044 30%12/2.4 This study

FISH, uorescence in situ hybridization. *16S rRNA position, E. coli numbering57.

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(PBS Milk (PBSM)) at room temperature and probed overnight at 4 C with a commercially available rabbit polyclonal anti-E. coli FtsZ antibody (Agrisera, Sweden; 1:400) in PBSM (and without, as a negative control). Unbound primary antibody was removed by three washing steps in PBSM and blots were subsequently incubated for 1 h at room temperature with a horseradish peroxidase-conjugated anti-rabbit secondary antibody (1:5,000; Amersham Biosciences) in PBSM. Proteinantibody complexes were visualized using ECL Plus detection reagents and lms (Amersham Biosciences).

Immunostaining was performed as described31. Briey, xed nematodes were rehydrated and washed in PBS containing 0.1% Tween 20 (PBT, washing solution). Bacterial peptidoglycan was permeabilized by incubation for 20 min with 0.1% (wt/ vol) lysozyme at 37 C. Blocking was carried out for 1 h in PBT containing 2% (wt/ vol) bovine serum albumin (blocking solution) at room temperature. Efs and Eds were both immunostained with a 1:200 dilution of commercially available rabbit polyclonal anti-E. coli FtsZ antibody (Agrisera) in blocking solution overnight under gentle agitation at 4 C or in blocking solution alone. Unbound primary antibody was subsequently removed by three washing steps in PBT and secondary Alexa555 conjugated anti-rabbit antibody (Molecular Probes, USA) applied at a 1:500 dilution in blocking solution for 1 h at room temperature. Unbound secondary antibody was removed by three washing steps in PBT and DNA was stained with YOYO-1 Iodide (Molecular Probes) dissolved in a Tris-EDTA buffer supplemented with 50 mM potassium citrate, 0.1% Triton-X100 and 0.1 g l 1 of

RNAseA according to the study by Marie et al.60 To dissociate Efs and Eds, worms were sonicated for 40 s in the tubes prior to mounting. Bacterial solution (1 ml) was mixed with 0.5 ml of mounting medium Vectashield (Vector Labs).

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Acknowledgements

This work was supported by the Austrian Science Fund (FWF) project P22470-B17 (N.L.,

N.P., N.R.H. and S.B.), an uni:docs fellowship from the University of Vienna (N.P.),

Marie-Curie Intra-European Fellowship PIEF-GA-2011-301027 CARISYM (H.R.G.-V.)

as well as by the National Science Foundation Nemasym Research Network grant to

S. Patricia Stock (NSF-IOS 0840932). We are very grateful to the Core Facility Cell

Imaging and Ultrastructure Research of the University of Vienna for technical support.

We thank the Schleper Group of the Department of Ecogenomics and Systems Biology

and the Laboratory of Genome Dynamics, the Medical University of Vienna (particularly

Wolfgang Miller) for inspiring discussions. This work is contribution 966 from the Carrie

Bow Cay Laboratory, Caribbean Coral Reef Ecosystem Programme, the National

Museum of Natural History, Washington, DC.

Author contributions

The study was designed by S.B. Samples were collected by N.P, N.L., N.R.H., J.O. and

S.B. DNA extraction and PCR were performed by N.P., N.L. and N.R.H. Phylogenetic

analysis was performed by H.R.G.-V. Immunostaining was performed by N.P. and

N.L. Image analysis was performed by N.L., T.dB. and N.P. FISH and Western blots

were performed by N.P. Statistical analysis was done by N.L. Confocal microscopy was

performed by S.B. The manuscript was written by S.B. and corrected by N.L, N.P,

H.R.G-V., J.O. and T.dB.

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