Literature DB >> 28723932

The nucleoid occlusion factor Noc controls DNA replication initiation in Staphylococcus aureus.

Ting Pang¹, Xindan Wang¹, Hoong Chuin Lim¹, Thomas G Bernhardt¹, David Z Rudner¹.

Abstract

Successive division events in the spherically shaped bacterium Staphylococcus aureus are oriented in three alternating perpendicular planes. The mechanisms that underlie this relatively unique pattern of division and coordinate it with chromosome segregation remain largely unknown. Thus far, the only known spatial regulator of division in this organism is the nucleoid occlusion protein Noc that inhibits assembly of the cytokinetic ring over the chromosome. However, Noc is not essential in S. aureus, indicating that additional regulators are likely to exist. To search for these factors, we screened for mutants that are synthetic lethal with Noc inactivation. Our characterization of these mutants led to the discovery that S. aureus Noc also controls the initiation of DNA replication. We show that cells lacking Noc over-initiate and mutations in the initiator gene dnaA suppress this defect. Importantly, these dnaA mutations also partially suppress the division problems associated with Δnoc. Reciprocally, we show that over-expression of DnaA enhances the over-initiation and cell division phenotypes of the Δnoc mutant. Thus, a single factor both blocks cell division over chromosomes and helps to ensure that new rounds of DNA replication are not initiated prematurely. This degree of economy in coordinating key cell biological processes has not been observed in rod-shaped bacteria and may reflect the challenges posed by the reduced cell volume and complicated division pattern of this spherical pathogen.

Entities: Chemical Disease Gene Mutation Species

Mesh：

Substances：

Year: 2017 PMID： 28723932 PMCID： PMC5540599 DOI： 10.1371/journal.pgen.1006908

Source DB: PubMed Journal: PLoS Genet ISSN： 1553-7390 Impact factor: 5.917

Introduction

Binary fission in bacteria is carried out by a multiprotein complex called the divisome [1]. Assembly of this complex initiates with the formation of a ring-like structure at mid-cell called the Z-ring composed of the tubulin homolog FtsZ [2]. The Z-ring functions as a dynamic scaffold for the recruitment and assembly of the division machinery. In rod-shaped bacteria like E. coli and B. subtilis, midcell localization of the Z-ring is controlled by two negative regulatory systems: Min and nucleoid occlusion [1, 3]. The Min system prevents Z-ring assembly at the poles while nucleoid occlusion blocks its assembly over of the nucleoid; together they ensure that division occurs at mid-cell. In E. coli, nucleoid occlusion is mediated by SlmA, a TetR family DNA binding protein [4]. SlmA directly inhibits FtsZ polymerization and this inhibition is stimulated by binding to specific DNA sequences [5-7]. In B. subtilis, nucleoid occlusion requires a ParB homolog called Noc [8]. The mechanism by which Noc inhibits Z-ring formation is less clear. Noc forms higher order nucleoprotein complexes [9] that associate with the cell membrane via an amino-terminal amphipathic helix and these complexes have been suggested to physically occlude the assembly of the division machinery [10]. Neither the Min system nor the nucleoid occlusion proteins are essential in E. coli or B. subtilis [4, 8, 11, 12]. However, defects in both regulatory systems results in a lethal division block [4, 8]. It was this synthetic lethal relationship that initially facilitated the identification of Noc and SlmA. Importantly, the specific binding sites for SlmA and Noc are distributed throughout the origin-proximal portions of their respective chromosomes and are largely absent in the region surrounding the terminus [6, 9, 13]. During the chromosome replication-segregation cycle in both organisms, the origin regions are segregated toward the cell poles and the terminus is brought to mid-cell, where it remains for the majority of the cell cycle [14, 15]. As DNA replication nears completion, chromosome-bound nucleoid occlusion factors are depleted from mid-cell, relieving division inhibition at this site. Accordingly, SlmA and Noc are not only thought to function in division site selection, but also in coordinating cell division with chromosome replication and segregation [6, 9]. Unlike rod-shaped bacteria, where the same perpendicular plane is used for binary fission, cell division alternates between three consecutive perpendicular planes in the spherical bacterium Staphylococcus aureus [16]. The mechanisms governing division site selection in this major human pathogen are poorly understood. S. aureus does not encode the Min system, but does have a homolog of B. subtilis Noc (48% identity, 65% similarity). A previous study showed that S. aureus cells lacking Noc are impaired in division and on average are larger than wild-type [17]. Furthermore, Δnoc mutants displayed an elevated frequency of cells with multiple Z-rings and division events bisecting the chromosome. Thus, a role for Noc in the spatial regulation of division is conserved in S. aureus. Even though S. aureus cells lack a Min system, Noc is not essential for viability [17]. Additional division regulators are thus likely to operate in this bacterium. By analogy with the Min- Noc- phenotype in rod-shaped organisms, we reasoned that defects in such regulators would result in a synthetically lethal or sick phenotype in combination with a noc deletion. To identify these factors we used transposon-sequencing (Tn-Seq) [18] to screen for genes that when inactivated result in a synthetically lethal with noc (Sln) phenotype. Two sln genes were identified in this screen, comEB and rhomboid (rbd). To further characterize the nature of the synthetic lethal defect of Δnoc Δrbd and Δnoc ΔcomEB mutants, suppressors that allowed growth of the double mutants were selected. Surprisingly, in both cases, suppressor mutations that mapped to the dnaA gene encoding the initiator of DNA replication were isolated, suggesting a role for Noc in controlling origin firing. Indeed, S. aureus cells lacking Noc were found to over-initiate replication, and the dnaA suppressor mutations ameliorated the over-replication phenotype and significantly reduced the severity of the division defects displayed by Δnoc cells. Reciprocally, we found that over-expression of DnaA enhanced the over-initiation and cell division phenotypes of cells lacking Noc. Altogether, our data reveal that S. aureus Noc coordinates division with chromosome replication and segregation by controlling replication initiation as well as preventing divisome formation over the origin-proximal region of the chromosome. This degree of economy in coordinating key cell biological processes may reflect the challenges posed by the smaller size and complicated division pattern of this spherical bacterium.

Results

A screen for synthetic lethal partners with noc identifies rbd and comEB

To identify potential division site regulators, we screened for genes that become essential in the absence of S. aureus Noc (Noc) using Transposon-sequencing (Tn-seq) [18]. A wild-type S. aureus RN4220 strain and a Δnoc derivative were mutagenized with a Mariner-based transposon [19]. The resulting libraries were separately pooled and the transposon-genomic DNA junctions of all insertions in the libraries were mapped by massively parallel DNA sequencing. For each library, we detected insertions in ~30% of the potential Mariner insertion sites at TA dinucleotides, and each insertion site was detected by an average of ~50 reads. Transposon insertions in several genes were statistically underrepresented in the Δnoc library compared to the wild-type library as assessed by the Mann-Whitney U test (). To validate the candidate synthetic lethal with Δnoc (sln) genes, we constructed a Noc depletion strain in which noc was expressed under the control of an anhydrotetracycline (aTc)-inducible promoter (P) in the S. aureus HG003 background. Transposon-insertion mutants in the candidate genes were obtained from the Nebraska Transposon Mutant Library [20] and transduced into the Noc-depletion strain grown in the presence of inducer and then tested for their ability to form colonies in its absence. Transposon insertions in comEB and rbd were the only mutants that resulted in a strong dependence on noc expression for viability (). We therefore focused our analysis on these two factors. Insertion-deletion mutations in comEB and rbd were generated and the synthetic lethality upon depletion of Noc was confirmed (). The rbd gene encodes a member of the Rhomboid family of membrane-embedded serine proteases [21, 22]. ComEB is homologous to deoxycytidylate deaminase, an enzyme in one of the dTTP synthesis pathways [23].

Identification of synthetic lethal partners of Δnoc in S. aureus.

(A) Transposon insertion profiles for selected regions of the chromosome for both wild-type and Δnoc strains. The height of each line in the profile represents the number of sequencing reads corresponding to a transposon insertion at the indicated genome position. Transposon insertions in the comEB and rbd genes were significantly under-represented in the Δnoc mutant relative to wild-type. (B) Spot dilutions of wild-type HG003 (wt) and the indicated derivatives. Cells were grown overnight in the presence of aTc (100 ng/ml). The resulting cultures were normalized to an OD600 of 0.2, 10-fold serially diluted, and spotted (5 μl) onto agar medium with and without inducer as indicated. Plates were incubated overnight at 37°C and photographed.

Inactivation of ComEB or Rbd enhances the division defects of Δnoc mutants

Next, we investigated the cytological phenotypes of the Noc- ComEB- and Noc- Rbd- mutants. Cells lacking Rbd or ComEB but with functional Noc grew at rates similar to wild-type () and appeared similar in size and morphology by fluorescence microscopy (). By contrast and as expected, depletion of Noc in the mutant backgrounds resulted in severe growth defects (). Examination of these Noc-depleted cells by fluorescence microscopy after 6 hours of growth in the absence of inducer revealed an increase in cell size, indicative of a defect in cell division. Specifically, the average volume of cells lacking Noc was ~69% greater than wild-type, while cells depleted of Noc in the absence of Rbd or ComEB were even larger (~86% and ~107% greater than wild-type) (). To investigate the defects in cell division at higher resolution, we visualized stained thin-sections by transmission electron microscopy. Cells lacking Noc or Rbd alone displayed a low frequency (4–6%) of abnormal and incomplete septa that were not oriented orthogonal to each other (). Such aberrant divisions were even more prevalent (~27%) in cells lacking both proteins, and the frequency of lysed cells also increased (~24%) (). Collectively, these results indicate that the loss of ComEB or Rbd exacerbates the division defects of Δnoc cells, ultimately resulting in lysis.

Characterization of the synthetic lethal with Δnoc phenotypes.

(A) Growth curves of the indicated strains from Fig 1B. Overnight cultures grown in the presence of aTc (100 ng/ml) were washed to remove inducer and used to inoculate fresh medium without inducer to an OD600 of 0.01. The resulting cultures were grown at 37°C to an OD600 of 1, followed by a second round of dilution to an OD600 of 0.01 (or 0.04 for Noc depletion in the ΔcomEB background). Growth during Noc depletion was then monitored by standard OD600 measurements. (B) Representative images of cells grown as described in A (for 5 mass doublings), except for the Noc depletion strains, which were examined after 13 mass doublings. Cultures were collected at OD600 ~ 0.4, washed and resuspended in phosphate buffered saline (1XPBS) prior to labeling with fluorescent vancomycin (Van-FL). Cells were visualized by phase contrast (Phase) and fluorescence (Van-FL) microscopy. Average cell size (μm3) ± standard deviation of each strain is indicated below each image (n>100). Scale bar indicates 1 μm. (C) Electron micrographs of the indicated strains. Overnight cultures of HG003 (wt) and mutant derivatives (Δnoc, Δrbd, and Δnoc Δrbd) were grown under permissive conditions (half-strength LB without NaCl (0.5XLB no NaCl) at 30°C) to an OD600 of 0.5. Cells were then washed, and diluted to an OD600 of 0.02 and grown under non-permissive conditions (LB with 0.5% NaCl medium at 37°C) for ~4 mass doublings. Cells were then harvested, processed, and visualized by electron microscopy as described in Methods. Scale bar indicates 500 nm. Larger fields of cells can be found in S1 Fig.

Fig 1

Identification of synthetic lethal partners of Δnoc in S. aureus.

Mutations in dnaA suppress the synthetic lethal with Δnoc phenotypes

In an attempt to elucidate the potential roles of ComEB and Rbd in cell division we sought to identify suppressors of the observed synthetic lethal phenotypes. To do so, we first identified conditions that support growth of the ΔcomEB or Δrbd mutant upon depletion of Noc () (see Materials and Methods). The permissive plating conditions were then used to generate Δnoc ΔcomEB and Δnoc Δrbd double deletion mutants. To isolate suppressors, the double mutants were grown in liquid medium under permissive conditions and then plated on solid agar under restrictive conditions. Nine suppressors of each double mutant pair were mapped using whole genome sequencing and confirmed by Sanger sequencing (). Two of the Δnoc Δrbd suppressors and one of the Δnoc ΔcomEB suppressors mapped to the dnaA gene encoding the replication initiator protein () [24, 25]. One of the suppressors of Δnoc Δrbd had a 56 bp deletion in the 5’ UTR of dnaA (sup 1), while another encoded a DnaA variant with a V141L substitution within the ATPase domain (Domain III) (sup 2). Similarly, a variant with an R254Q substitution in Domain III (sup 3) suppressed the Δnoc ΔcomEB phenotype. Although we had hoped that the suppressors would shed light on a potential role for ComEB and Rbd in cell division regulation, the fact that mutations in dnaA suppressed both the Δnoc ΔcomEB and Δnoc Δrbd growth defects suggested that it was some aspect of the Noc- phenotype that was most likely being corrected by the suppressors. These findings raised the intriguing possibility that Noc function is linked to DNA replication. Accordingly, we decided to focus the remainder of this study on this potential connection. The possible roles of ComEB and Rbd in cell division and the cause of the synthetic lethal with Δnoc phenotype will be the subject of a separate report (see Discussion).

Suppressors of the Δnoc Δrbd and Δnoc ΔcomEB mutants map to the dnaA locus.

(A) Spot dilutions of Δnoc Δrbd, Δnoc ΔcomEB and derivatives harboring the indicated suppressor mutation were grown under their respective permissive conditions overnight. They were then washed, serially diluted, and plated as described in Fig 1. (B). Schematic diagram of the dnaA locus indicating the location of each of the three suppressors isolated. Genome position 1 indicates the origin.

Cells lacking Noc over-replicate

DnaA is the replication initiation protein in most bacteria [24, 25]. It is an AAA+ ATPase that exists in both ATP- and ADP-bound forms. ATP-bound DnaA binds cooperatively to sequence elements (called DnaA boxes) in the replication origin, and catalyzes the unwinding of double stranded DNA. DNA unwinding leads to the ordered loading of helicase and the rest of the replication machinery followed by the initiation of bi-directional replication. To investigate whether cells lacking Noc have defects in the initiation of DNA replication we performed marker-frequency analysis using quantitative PCR (qPCR) and whole genome sequencing. This analysis revealed that the Δnoc mutant had a higher origin to terminus (ori:ter) ratio than wild-type cells and this increase could be suppressed by the dnaA suppressor mutations (), raising the possibility that the absence of Noc causes over-initiation of DNA replication.

Over-replication phenotype of Δnoc mutants.

Marker-frequency analysis of the indicated S. aureus and B. subtilis strains. (A) Cells of HG003 (wt) and its indicated derivatives were grown in LB with 0.5% NaCl medium at 37°C to OD600 ~ 0.4. Cells were then harvested and genomic DNA isolated. The oriC-to-terminus (ori:ter) ratio of each strain was then determined by quantitative PCR (qPCR) using primers specific for the relevant chromosomal regions. The results are shown as the average ± standard deviation (n = 3). The p-values of relevant pairs of samples were calculated and indicated on the bar graph. p > 0.05 (ns), p ≤ 0.05 (*), p ≤ 0.01 (**), p ≤ 0.001 (***). (B) Genome-wide DNA content of the indicated strains. Overnight cultures of S. aureus strain RN4220 (wt), Δnoc, Δnoc sup1, and Δnoc cells expressing noc under the control of the P promoter were diluted to OD600 = 0.01 and grown in TSB medium without or with inducer (aTc) at 37°C. Genomic DNA was isolated after 5 mass doublings and analyzed by whole-genome sequencing. The total sequencing reads from each strain were normalized to 51 million and the data plotted in 30 kb bins (circles). Blue lines and grey area represent the smoothed conditional mean and 95% confidence band for the regression curve, respectively (spanS = 0.08). The data from one of two biological replicates are shown. The ori:ter ratios indicated below the plots were determined using the 30kb bins spanning the origin and terminus. The partial suppression of Δnoc, P-noc in the absence of aTc is likely due to leaky expression. (C) Ratio of genomic profiles. The genomic profiles in (B) were re-plotted as ratios relative to wild-type. (D) The ori:ter ratios of S. aureus HG003 (wt) and its indicated derivatives were determined by qPCR as described above. The Δnoc Δrbd strain was first grown under permissive conditions (0.5X LB no NaCl, 30°C) to OD600 ~0.4, then back diluted into nonpermissive conditions (LB 0.5% NaCl medium, 37°C) at an OD600 ~0.04 and harvested at OD600 ~0.4. (E) Cells of S. aureus HG003 (wt) and its indicated derivatives were grown and the ori:ter ratios determined as described above. Similarly, B. subtilis strain PY79 (wt) and its indicated derivatives were grown in CH medium at 30°C. The ori:ter ratios were determined using similar primer sets and qPCR conditions as used for S. aureus (n = 3). The ori:ter ratios of S. aureus HG003 (wt) and Δnoc cells are replotted from (D) for direct comparison. (F). Immunoblot analysis of Noc protein levels in the indicated strains. Cell extracts were prepared from the same cultures used in (B). The relative Noc protein levels were determined by normalizing to the cross-reacting protein band (asterisk) and then to wt (n = 3, SD = 0.40). An increase in the ori:ter ratio can be caused by over-initiation of DNA replication or a reduction in replication elongation rates or fork stalling and/or collapse. The latter situation could be relevant in this case because cells lacking Noc have an increased frequency of chromosome guillotining [17], which would lead to fork stalling. To investigate the nature of the defect in the Δnoc mutant, we quantitatively assessed DNA content relative to cell volume as a proxy for cell mass in single cells [26, 27]. Fixed permeabilized cells were stained with propidium iodide and analyzed by phase contrast and fluorescence microscopy. Consistent with the idea that cells lacking Noc over-initiate, the Δnoc mutant had a higher DNA content relative to cell volume compared to wild-type and the dnaA (sup1) mutation restored this ratio to wild-type levels (). Further support for a role for Noc in controlling replication initiation comes from an experiment in which we attempted to correct the increase in the ori:ter ratio by expressing noc in trans from an aTc-inducible promoter. As anticipated, modest (~2.3-fold) over-production of Noc in the Δnoc mutant () led to a reduction in the ori:ter ratio (). However, comparison of the genomic profile relative to wild-type () revealed that the ori:ter ratio was even lower than wild-type, consistent with the idea that Noc acts as a negative regulator of replication initiation. Finally, to address whether the increase in the ori:ter ratio in the Δnoc mutant resulted from fork stalling due to division on top of the chromosomes, we performed genome-wide marker frequency analysis on wild-type and Δnoc strains before and after inhibition of cell division using the FtsZ inhibitor PC190723 [28]. We carried out whole genome sequencing of wild-type and the Δnoc mutant prior to the addition of the drug and approximately 2 and 4 mass doublings after its addition. Despite the strong block to cell division, the increase in the ori:ter ratio in the Δnoc mutant persisted (). Importantly, we found that DNA content increased after drug addition (), indicating that the division-inhibited cells continued DNA replication. Thus, chromosome guillotining cannot account for the increase in the ori:ter ratio in the Δnoc mutant. Altogether, these experiments are most consistent with a model in which Noc functions to limit replication initiation and in its absence cells over-initiate. Marker-frequency analysis in cells lacking Rbd or ComEB revealed that these mutants were not impaired in replication initiation (). Furthermore, the ori:ter ratio in the Δnoc Δrbd double mutant was similar to the Δnoc single mutant (), indicating that the Rbd- defect did not exacerbate the over replication phenotype of Noc- cells. Because Noc shares 48% identity with its B. subtilis counterpart (Noc), we wondered whether B. subtilis cells lacking Noc also over-initiate. Marker-frequency analysis revealed that the B. subtilis Δnoc mutant had an ori:ter ratio similar to wild-type (). As a control, we examined the ori:ter ratios of B. subtilis cells lacking the ParB homolog Spo0J and the ParA homolog Soj. Previous studies indicate that Soj (ParA) functions as both an activator and inhibitor of DnaA, while Spo0J (ParB) promotes the inhibitory activity of Soj [29, 30]. As reported previously, both mutants had over-initiation phenotypes (), but neither was as pronounced as in S. aureus Δnoc cells. In addition to Noc, S. aureus cells encode a second ParB-like protein (ParB) that is 47% identical to Spo0J (ParB), although they lack a ParA counterpart. A mutant lacking ParB had an ori:ter ratio similar to wild-type cells (), indicating that among the ParB related proteins in S. aureus, a role in replication control is restricted to Noc.

Chromosomal distribution of Noc binding sites

In B. subtilis, Noc binds multiple sites throughout the chromosome that are enriched around the origin-proximal two-thirds of the chromosome and largely absent from the replication terminus region [9]. This distribution of binding sites is thought to ensure that Z-ring formation is coordinated with chromosome segregation [9]. Because our data suggest that in S. aureus Noc regulates replication initiation, we wondered whether it might have a distribution of DNA binding sites distinct from Noc and different from that predicted based on mapping the sequence of the Noc binding sites on the S. aureus chromosome [31]. To investigate this we determined the S. aureus Noc binding sites (NBS) by chromatin-immunoprecipitation coupled to Illumina sequencing (ChIP-seq). We used antibodies raised against Noc, which cross-reacted with the S. aureus homolog. A total of 41 chromosomal loci were identified that co-precipitated with Noc from wild-type cells compared to the Δnoc mutant (). Importantly, all but one of these loci were located in the origin-proximal half of the chromosome (between -700kb and +700kb), resulting in a distribution of binding sites that resembles the B. subtilis pattern [31]. Furthermore, as is the case in B. subtilis [9], Noc binding spanned a region of 8–10 kb surrounding the peak of enrichment (), suggesting that S. aureus Noc forms large nucleoprotein complexes at its binding sites. Finally, using motif discovery algorithms from the MEME suite [32], the consensus Noc binding site was determined, the core of which was found to be identical to the B. subtilis NBS consensus sequence [31] (). The similar distribution of Noc binding sites, the identical consensus binding sequence, and the shared ability of the Noc homologs to spread from these sites are all consistent with Noc functioning as a nucleoid occlusion factor in addition to its role in replication control identified here.

Identification of Noc binding sites.

(A) Shown are the ChIP-Seq profiles for HG003 (wt) (black) and a Δnoc derivative (magenta). The profiles were generated by normalizing the reads from ChIP-Seq samples (using anti-Noc antibodies) to those from input genomic DNA. The origin (ori) is at position 1 with positions on the left and right chromosome arms indicated as negative and positive numbers, respectively. (B) Close-up view of a region bound by Noc with the peak indicated by a dotted blue line. Note the extended spread of the peak base compared to the background signal from the Δnoc sample. (C) Close-up view of the origin region including a minor Noc binding site adjacent to the dnaA gene (green bar). The location and direction of the dnaA transcription start site are indicated by the black arrow in the inset. (D) Sequence logo of the Noc consensus binding site generated using the 41 major enrichment peaks (S7 Table) identified in the ChIP-Seq analysis.

B. subtilis noc and S. aureus noc do not cross-complement

Since the Noc proteins from B. subtilis and S. aureus are 48% identical and they have the same consensus binding site, we investigated whether they could substitute for each other in vivo. B. subtilis cells lacking the Min system and Noc are viable at 30°C but fail to grow at 42°C [8]. Accordingly, we generated his6 fusions to both B. subtilis and S. aureus noc under the control of an IPTG-inducible promoter (P) and introduced these into a ΔminD Δnoc double mutant under permissive conditions. Surprisingly, only B. subtilis noc was able to complement the growth defect of the double mutant at 42°C (). Similarly, we took advantage of the synthetic lethal phenotype of Δnoc Δrbd in S. aureus. We introduced the same his6 fusions under the control of an aTc-inducible (P) promoter into the double mutant at the L54a phage attachment site. Again, only the native noc allele supported growth under the non-permissive condition (). Furthermore, not only was B. subtilis noc incapable of supporting growth of the S. aureus Δnoc Δrbd mutant, it was unable to correct the over-initiation defect of the S. aureus Δnoc mutant (). Importantly, immunoblot analysis using anti-6xHis antibodies indicated that in both complementation tests, the heterologous Noc proteins were produced at comparable or even higher levels than the native proteins (). Furthermore, as has been observed previously with Noc [9], a YFP fusion to Noc expressed in B. subtilis localized in foci along the cell periphery indicative of it associating with membranes surrounding the nucleoid in addition to binding DNA (). Finally, ChIP-seq experiments using anti-6xHis antibodies revealed that both His6-Noc fusions bound to virtually all the same chromosomal sites in B. subtilis and S. aureus (). Thus, merely binding to the NBS sites throughout the chromosome is not sufficient for Noc function, suggesting that the Noc orthologs require species-specific contacts with replication and/or division factors and that these interaction interfaces are not conserved between the two proteins (See Discussion).

Noc and Noc are not functionally interchangeable.

(A) Spot-dilutions of B. subtilis strain PY79 (wt) and the indicated derivatives harboring his-tagged noc fusions from either B. subtilis (noc) or S. aureus (noc) expressed from the IPTG-inducible P promoter. Cells were grown overnight and the resulting cultures were normalized to an OD600 of 0.2 and serially diluted. 5 μl of each dilution were spotted onto LB agar with or without inducer and the plates were incubated overnight at the indicated temperatures. (B) Spot-dilutions of S. aureus HG003 (wt) and its indicated derivatives. Cells were grown, serially diluted, and plated as described in (A). In these strains the noc fusions were expressed from the aTc-inducible P promoter. (C) Marker-frequency analysis of the indicated S. aureus strains was performed as in Fig 4. The results shown are the average ± standard deviation (n = 3). Results for wt and Δnoc cells are replotted from Fig 4. p > 0.05 (ns), p ≤ 0.01 (**). (D) Immunoblot analysis of Noc protein levels in the indicated strains. Cell extracts representing equivalent culture OD600 were prepared from B. subtilis and S. aureus strains grown in LB or TSB, respectively at 37°C with or without inducer. Proteins were separated by SDS-PAGE, transferred to PVDF membrane, and probed with an anti-6xHis antibody. A cross-reacting protein (asterisk) serves as a loading control. (E) Noc-YFP and Noc-YFP localize to the peripheral membranes above the nucleoid in B. subtilis. Representative images of Δnoc B. subtilis cells expressing noc-yfp or noc-yfp under the control of the P promoter. Cells were induced at OD600 = 0.01 with 0.5% xylose and analyzed by fluorescence microscopy at OD600 = 0.25. Noc-YFP, DAPI-stained DNA and merged images with Nile Red-stained membranes (Mem) are shown. Scale bar indicates 1 μm. Larger fields can be found in S6 Fig. (F) Noc and Noc have largely overlapping binding sites in S. aureus. ChIP-seq using the anti-6xHis antibodies was performed on S. aureus Δnoc cells expressing noc or noc under the control of the P promoter. Wild-type and Δnoc cells lacking a his-tagged noc fusion were used as negative controls. Data presented were first normalized to the total number of reads then relative to the input for each strain and finally relative to that of the relevant control sample (wild-type cells for noc and Δnoc cells for noc). The data are plotted in 1 kb bins. The higher background and higher peaks in the Noc ChIP-seq profile are due to fewer and sparser sequencing reads in this sample and the normalization process used. Genome positions are labeled as in Fig 5A. Insets show a close-up view of the origin region including a minor Noc binding site adjacent to the dnaA gene (gray bar). The data are plotted in 10 bp bins.

Fig 4

Over-replication phenotype of Δnoc mutants.

Fig 5

Identification of Noc binding sites.

Evidence that S. aureus Noc acts post-translationally to restrain replication initiation

The Noc enrichment profile from the ChIP-seq experiment contained a small peak of enrichment within the promoter region of the dnaA gene (Figs ). Although Noc expressed in S. aureus contained a similar enrichment peak, we wondered whether Noc functions in replication control by regulating dnaA expression. Accordingly, we compared the relative levels of DnaA and the house-keeping sigma factor SigA by immunoblot analysis using anti-DnaA and anti-SigA antibodies. Both antibodies were raised against the B. subtilis proteins but cross-reacted with their S. aureus orthologs. Intriguingly, we detected a 1.7-fold increase in DnaA levels in cells lacking Noc compared to wild-type (). Furthermore, the dnaA suppressor mutations reduced the levels of DnaA in the Δnoc mutant to a level slightly below wild-type. To directly test whether the over-initiation phenotype in cells lacking Noc was due to this increase in DnaA levels, we compared the ori:ter ratio in a strain harboring an aTc-inducible promoter fusion to dnaA. Consistent with previous results, we did not observe a correlation between mild DnaA overproduction and over-initiation of DNA replication in S. aureus [33]. In the absence of inducer, the leaky expression from this plasmid-borne dnaA allele resulted in DnaA levels comparable to the Δnoc mutant (). However and importantly, the ori:ter ratio in this strain was similar to wild-type and a matched empty vector control strain. Furthermore, even higher levels of DnaA in the presence of inducer did not cause over-initiation compared to the control strain (). As a positive control for these experiments we used a strain harboring the same aTc-inducible promoter fused to an ATPase defective allele of dnaA (dnaAR318H). As reported previously [33], induction of DnaAR318H caused a severe growth defect and led to dramatic over-initiation of replication (). We conclude that Noc directly or indirectly affects DnaA levels but these changes are not the major determinant of the observed effects on DNA replication.

Noc and DnaA have opposing activities.

(A). Marker-frequency analysis of the indicated strains. Cultures were grown to OD600 = 0.4 and then processed to determine ori:ter ratios by qPCR (top panel) as in Fig 4 or to quantify DnaA protein levels by immunoblot (bottom panel). In induced cultures, 1 ng/ml aTc was added at OD600 = 0.05. oriC-to-terminus (ori:ter) ratios are shown as the average ± standard deviation (n = 3). p > 0.05 (ns), p ≤ 0.05 (*), p ≤ 0.01 (**), p ≤ 0.001 (***), p ≤ 0.0001 (****). To quantify DnaA levels, the immunoblot signal was normalized to SigA and reported relative to the wild-type strain that was designated as having a signal of 1. Standard deviation was indicated as SD (n = 3). (B). Marker-frequency analysis of the indicated strains. Overnight cultures of Δnoc cells carrying either an empty vector (vector) or a plasmid containing dnaA under P control were diluted to an OD600 = 0.01, then grown to an OD600 of 0.05 at which time the indicated amount of inducer was added. Cells were then harvested at OD600 = 0.4 and the ori:ter ratios were determined as in Fig 4. Results shown are the average ± standard deviation (n = 3). Results for wt cells carrying empty vector or the dnaA-containing plasmid are replotted from (A). (C). Spot-dilutions of wild-type S. aureus HG003 and its Δnoc derivative carrying plasmids as in (B). Cultures were diluted to an OD600 of 0.15, serially diluted, and plated on the indicated medium as in Fig 1. Plates were incubated overnight at 37°C and photographed. If, as our data suggest, Noc negatively regulates replication initiation at the post-translational level, then overproduction of DnaA in a Δnoc mutant should exacerbate the over-initiation phenotype. As can been seen in , overexpression of dnaA in cells lacking Noc dramatically increased replication initiation with an ori:ter ratio approaching the levels reached upon DnaAR318H production in wild-type cells. Furthermore, similar to what has been reported previously for the ATPase deficient DnaA variant [33], this level of over-replication led to a dramatic growth defect () and a significant increase in cell size () (see below). Altogether these data argue that Noc exerts its control on replication initiation through a post-translational mechanism.

dnaA suppressors partially suppress the cell division defect in Δnoc mutants

Previous studies indicate that S. aureus cells lacking Noc display division defects including oblique FtsZ-rings, an increase in cell size, and the production of anucleate cells [17] (). Here, we have shown that the Δnoc mutant also over-initiates DNA replication. To investigate the contribution of over-initiation to the division defects in cells lacking Noc, we took advantage of the suppressor mutations isolated in dnaA. We analyzed cell size and FtsZ localization by fluorescence microscopy in the Δnoc mutant and in the Δnoc mutant harboring dnaA(sup1) or dnaA(sup2). Consistent with our observation that over-initiation leads to an increase in cell size (), both dnaA mutations partially suppressed the large cell phenotype of the Δnoc mutant (). To monitor FtsZ localization we used an FtsZ-GFP fusion as a merodiploid [34] in the same set of strains. Interestingly, the suppressors reduced the percentage of cells with abnormal Z-rings (). In particular, we observed a reduction in oblique Z-rings and in the percentage of cells with diffuse FtsZ-GFP fluorescence. Furthermore, we also found that ~10% of cells lacking Noc exhibited extremely strong DAPI staining (). We suspected this phenotype was due to increased cell envelope permeability in the mutant, and staining cells with the membrane-impermeable dye propidium iodide (PI) confirmed this (). Importantly, the dnaA suppressors alleviated this hyper-staining/membrane permeability phenotype such that it was comparable to wild-type cells (). Collectively, these data suggest that the cell division problems experienced by S. aureus cells lacking Noc are partially due to the over-initiation of DNA replication.

The cell division phenotypes in cells lacking Noc are partially due to over-initiation of replication.

(A) Representative images of HG003 (wt) and derivatives harboring the plasmid pLOW-ftsZ-gfp. Cells were grown to an OD600 ~ 0.01 and FtsZ-GFP production was induced with 10 μM IPTG. When cultures reached an OD600 ~ 0.4, cells were resuspended in 1XPBS and visualized using phase contrast and fluorescence microscopy. Scale bar indicates 1 μm. (B) The same set of strains, but without the pLOW-ftsZ-gfp plasmid, were grown to an OD600 = 0.4, resuspended in 1XPBS, stained with BODIPY-Vancomycin (Van-FL) and propidium iodide (PI), and visualized by fluorescence microscopy. Examples of multiple FtsZ-rings (single arrow), diffuse FtsZ signal (double arrow), and PI-positive cells (arrowhead) are indicated. (C) Quantification of the FtsZ-ring formation phenotypes, frequency of PI staining, and cell size in the indicated strains.

Discussion

The initial goal of this study was to identify additional regulators of division site placement in S. aureus by screening for synthetic lethal partners of the nucleoid occlusion factor Noc. The Tn-Seq analysis successfully identified Rbd and ComEB, annotated as a rhomboid-family protease and a deoxycytidylate deaminase, respectively as being essential upon Noc inactivation. Although we intended to use the synthetic lethal phenotype of Noc- Rbd- or Noc- ComEB- mutants to learn more about Rbd and ComEB function, our genetic analysis led to the surprising discovery that Noc plays a role in controlling the initiation of DNA replication as well as functioning as a nucleoid occlusion factor. We therefore shifted our focus to studying this newfound function for Noc instead of further investigating the activities of Rbd and ComEB. Consequently, the underlying cause(s) of the synthetic lethal phenotypes we observe for Δnoc Δrbd or Δnoc ΔcomEB strains remain unclear. Defects in Rbd or ComEB were not found to increase the ori:ter ratio of wild-type or Δnoc cells, indicating that the synthetic lethality in combination with Δnoc is not due to additional problems constraining replication initiation. However, the possible role of ComEB in nucleotide metabolism may exacerbate the phenotype of Δnoc cells by limiting the availability of nucleotides needed to fuel the elevated level of DNA replication. Potential explanations for the Δnoc Δrbd phenotype are more numerous. Aggravation of the replication, division, or both phenotypes of Noc- cells is possible upon rbd inactivation, and in either case the added problems may be due to a failure in substrate processing by Rbd rather than a direct role in these processes for Rbd itself. Further studies of Rbd function aided by the strong growth phenotype of Δnoc Δrbd cells identified here should shed light on the physiological role of rhomboid-like proteases in bacteria, which is poorly understood in general.

Control of DNA replication by Noc

The elevated ori:ter ratio observed in Δnoc cells and its suppression by mutations in dnaA are consistent with a model in which Noc controls replication initiation. Further support for this idea comes from our findings that cells lacking Noc have elevated DNA content relative to cell volume and cells with increased Noc protein levels have a reduction in the ori:ter ratio relative to wild-type. Finally, the synthetic growth phenotype and increased ori:ter ratio in Δnoc mutant cells that over-expresses DnaA also argue for a role in replication initiation. However, because of the limited tools available to study replication in S. aureus, we cannot rule out the possibility that Noc also functions in replication elongation [35]. How Noc controls replication initiation remains unclear. Our finding that overexpression of dnaA does not lead to increased replication initiation unless Noc is inactivated indicates that Noc is unlikely to be regulating origin firing by affecting dnaA expression. Furthermore, the failure of Noc to functionally substitute for Noc even though it binds to almost all the same chromosomal sites as Noc suggests that site-specific DNA-binding activity alone is unlikely to account for replication control. However, we note that our ChIP-seq analysis identified two small enrichment peaks for Noc surrounding the dnaA gene while expression of Noc in S. aureus only had one of these small peaks (). Intriguingly, the predicted DnaA binding sites required for origin unwinding are located in these two regions [33, 36]. Accordingly, it is formally possible that Noc binding to these sites occludes DnaA and inhibits origin firing. Alternatively, this second enrichment peak could be reporting on an interaction between Noc and DnaA bound to the origin (see below). Because this intergenic region is critical for origin firing [37], we were unable to investigate whether or not Noc binding at this position is important for its role in replication control. We hypothesize that Noc recognizes a specific molecular target to mediate its effect on replication initiation and that the interaction interface with this target is not conserved in Noc. DnaA is an obvious candidate as a direct regulatory target of Noc, but so far we have not been able to detect a Noc-DnaA interaction. Further work will therefore be required to determine the precise mechanism by which Noc controls initiation. Nevertheless, the discovery that Noc controls replication initiation in addition to its role in nucleoid occlusion provides a striking example of a single protein that can coordinate cell division and DNA replication by affecting both major cell-cycle processes. It is noteworthy that mutations in dnaC encoding the replicative helicase were also identified as suppressors of Δnoc Δrbd and Δnoc ΔcomEB (). Furthermore, at least one of these mutations (dnaC) was able to suppress the over-initiation phenotype of the Δnoc Δrbd mutant (). Since DnaC is required for both replication initiation and elongation [38] the molecular basis of suppression remains unclear. In the context of the model that Noc negatively regulates initiation, we hypothesize that these DnaC variants are specifically impaired in initiation function, however, further analysis will be required to establish the defects in these mutants.

Mechanism of cell division regulation by Noc proteins

The mechanism by which Noc proteins block cell division over the nucleoid has remained unclear for many years. Attempts at identifying a specific component of the divisome targeted by Noc have been unsuccessful [10]. However, this protein was recently shown to have an amino-terminal amphipathic helix that recruits DNA-bound Noc complexes to the membrane [10]. Based on this result, it has been proposed that, rather than interacting with a specific component of the division apparatus, Noc nucleoprotein complexes at the membrane physically occlude the assembly of the division machinery in areas occupied by the origin-proximal portion of the chromosome [10]. If true, the only activities of Noc required for its control of cell division are its association with Noc-binding sites on the chromosome and their recruitment to the membrane. Given that Noc binds to the same sites as Noc, forms higher order nucleoprotein complexes and, like Noc, appears to associate with the membrane in addition to DNA, the physical occlusion model would predict that Noc should be able to substitute for Noc. However, we find that Noc fails to support growth of Min- Noc- B. subtilis cells under non-permissive conditions, suggesting that physical occlusion of divisome assembly is unlikely to be the sole mechanism by which Noc proteins mediate division inhibition. Our results suggest that an additional species-specific interaction between Noc and a divisome protein is also likely to be required for its activity. The search for this elusive interaction partner should therefore continue.

Coordinating DNA-replication and cell division

To ensure faithful inheritance of genetic material, cell division must be coordinated with DNA replication and segregation. Noc is thought to contribute to this coordination by blocking cell division over the origin-proximal region of the chromosome where its binding sites are distributed [9]. This division inhibition activity is the only known function of B. subtilis Noc. However, as we have shown here, S. aureus Noc has the additional activity of restricting the initiation of DNA replication, thus further integrating the processes of division and DNA replication/segregation in this organism. To our knowledge, this activity for Noc is the first example of a ParB-like protein controlling replication initiation. ParB proteins typically bind centromeric parS sequences and work with ParA partner proteins to promote origin segregation [39]. In B. subtilis, the ParA protein Soj has also been shown to both inhibit and activate DNA replication initiation by DnaA in a manner modulated by the ParB protein Spo0J [29]. S. aureus lacks a ParA homolog, indicating that the effects on replication observed in mutants defective for Noc are not an indirect consequence of a misregulated ParA protein partner as is the case for B. subtilis mutants inactivated for Spo0J (ParB). Although we favor the idea that Noc directly modulates DnaA activity in S. aureus additional work is required to establish the mechanism of replication control. Irrespective of the precise mechanism, our results raise the question of why S. aureus utilizes a Noc protein with the added activity of controlling the initiation of DNA replication whereas B. subtilis does not. Differences in cell morphology and the geometries of chromosome segregation and cell division in these organisms might explain the distinct Noc regulatory activities used by these organisms. In rod-shaped cells, chromosome segregation proceeds along the long cell axis. The spatial cues do not change from one cell cycle to the next. Therefore, even if replication were to outpace division, the pattern of chromosome segregation would remain the same. The situation in spherical cells like S. aureus is very different. Just as division alternates between three perpendicular planes, so too must the orientation of chromosome segregation. Thus, if replication were initiated prematurely relative to the progress of division, the appropriate spatial cues might not be in place to direct segregation in an orientation compatible with that of the next division plane. Furthermore, Noc-dependent inhibition of division due to the segregation of these prematurely replicated origins would be more difficult to overcome given the reduced spatial resolution in these small spherical cells. Consistent with this idea, we note that a significantly larger portion of the terminus region in S. aureus lacks Noc binding sites compared to B. subtilis. The dual function of Noc in nucleoid occlusion and replication control may therefore serve to maintain a tighter coupling between division and replication to keep the geometries of chromosome segregation in step with that of the division plane and/or to ensure that division is not impaired by prematurely segregated origins. The challenge for the future will be to determine how Noc restrains replication and how its apparent inhibitory effects are relieved in response to cell cycle signals to facilitate proper coordination between replication initiation and cell division.

Materials and methods

General methods

S. aureus strains were grown in tryptic soy broth (TSB) at 30°C or 37°C with aeration, unless otherwise indicated. The medium was supplemented with erythromycin (5 μg/ml for chromosomal insertions and 10 μg/ml for plasmids), chloramphenicol (5 μg/ml for chromosomal insertions, 10 μg/ml for plasmid), spectinomycin (100 μg/ml), kanamycin and neomycin (25 μg/ml each), 5-bromo-4-chloro-3-indolyl ß-D-galactopyranoside (X-Gal, 250 μg/ml), or anhydrotetracycline (aTc, 100 ng/ml unless otherwise indicated). B. subtilis strains were derived from the prototrophic strain PY79 [40]. Cells were grown in Luria Broth (LB) or Casein Hydrolysate (CH) medium [41] at 37°C with aeration, unless otherwise indicated. The medium was supplemented with tetracycline (10 μg/ml), spectinomycin (100 μg/ml), kanamycin 10 μg/ml), chloramphenicol (5 μg/ml), xylose (0.5% w/v) or isopropyl ß-d-thiogalactopyranoside (IPTG, 0.5 mM). Lists of oligonucleotide primers, strains, plasmids, and descriptions of their construction can be found in Supplemental Material.

Transposon insertion library construction and sequencing

Transposon libraries of S. aureus strains TM18 (wt) and Δnoc::spec were constructed according to Wang et al. [19], except that the donor strain TM17 contained the transposon plasmid pTP77. Each library had >70,000 insertions. Transposon-sequencing (Tn-seq) was adapted from Zhang et al. [42]. Briefly, genomic DNA isolated from each library was sonicated (using Q800R2 QSONICA) to 200–400 bp fragments. Nicked ends were repaired (Quick Blunt kit, NEB), and dA-tails were added with Taq polymerase (NEB), followed by ligation of adapters using T4 ligase (NEB). Transposon-junctions were PCR-amplified using primers oTP182 and oTP183. PCR products were purified and incubated with the endonuclease NotI (NEB) to remove any contaminating DNA derived from the transposon plasmid. Finally, a second round of PCR was performed on 100 ng of each sample, using primers oTP184-187 and oTP188-191. A 200–400 bp product was gel-purified and sequenced on the Illumina HiSeq 2500 platform (Biopolymers Facility at Harvard Medical School). The sequencing reads were mapped to each TA site on the S. aureus NCTC8325 genome (NCBI NC_007795.1). Genes in which reads were statistically underrepresented in Δnoc compared to wild-type were identified by the Mann Whitney U test. Visual inspection of transposon insertion profiles was performed with the Sanger Artemis Genome Browser and Annotation tool. Tn-seq datasets are accessible through NCBI's Gene Expression Omnibus under accession number GSE101335.

Identification of permissive growth conditions

Noc depletion strains harboring Δrbd or ΔcomEB (strains aTP431 and aTP508) were streaked on plates containing 0.5 X LB No NaCl, LB No NaCl, LB 0.5% NaCl, or LB 1% NaCl, and incubated at 30˚, 37˚ or 42˚C. The colony size of each strain was compared with the Noc depletion strain aTP359 grown under the same conditions. The growth conditions in which colonies from aTP431 and aTP508 were comparable in size to aTP359 were considered permissive. LB 0.5% NaCl at 37°C did not allow growth for either aTP431 or aTP508 and was considered non-permissive.

ChIP-Seq

ChIP was performed as described previously [43] with modification. Briefly, cells were grown in TSB medium to OD600 = 0.4 for S.aureus, and in CH medium to OD600 = 0.25 for B. subtilis, and incubated with 3% formaldehyde for 30 min at room temperature. Formaldehyde was quenched and the cells washed, and lysed. Lysates were sonicated using a Q800R2 sonicator (QSONICA) to generate 300–500 bp randomly sheared chromosomal DNA fragments. The lysates were then incubated with anti-Noc or anti-6xHis antibodies (Genscript) overnight at 4°C. The sample was then processed as described previously and sequenced using the Illumina MiSeq platform. The sequencing reads were mapped to the S. aureus NCTC8325 genome (NCBI NC_007795.1) or B. subtilis PY79 genome (NCBI NC_022898.1) using CLC Genomics Workbench software (Qiagen). ChIP-seq datasets are accessible through Gene Expression Omnibus under accession number GSE93264.

Whole genome sequencing

Whole genome sequencing was performed according to Baym et al. [44]. 1.5 ng genomic DNA from each strain was used in a 2.5 μl Nextera Tagmentation reaction (Illumina). After incubation at 37°C for 5 minutes, the reaction was immediately placed on ice. Tagmented DNA was then mixed with 11 μl KAPA Library Amplification Kit master mix (Kapa Biosystems), 4.4 μl of each indexing primer (5 μΜ) followed by PCR amplification. Amplified DNA was then purified from 15 μl of each reaction with 12 μl of Agencourt AMPure XP beads (Beckman Coulter) and resuspended in 30 μl buffer containing 10 mM Tris-Cl (pH 8.0), 1 mM EDTA (pH 8.0), and 0.05% Tween-20. The concentration of each sample was measured by Qubit (Thermo Fisher Scientific Inc.) and equivalent amounts of DNA were pooled, analyzed on TapeStation (Agilent Technologies) for quality control, and sequenced using the Miseq platform (Illumina). Sequencing reads were analyzed on CLC Genomics Workbench. Single nucleotide polymorphisms (SNP) and deletions were identified by comparing the sequence of the suppressors to the parental strains. Raw data are accessible through NCBI's Sequence Read Archive under accession number SRP111468.

Fluorescence microscopy

Cells at OD600 ~ 0.4 were pelleted by centrifugation at 3,300 xg for 2 min, and immobilized on 2% (wt/vol) agarose pads containing M9 salts solution. Cell walls were stained with 0.5 μg/ml BODIPY FL vancomycin (Van-FL, ThermoFisher) and 0.5 μg/ml Vancomycin-HCl. Cell membranes were stained with 1 μg/ml Nile Red (ThermoFisher). DNA was stained with DAPI (Molecular Probes) at 2 μg/ml, or with Propidium Iodide (Molecular Probes) at 5 μM. To quantitatively characterize DNA content, cells were immediately fixed with ethanol followed by staining with Propidium iodide. Fluorescence microscopy was performed using a Nikon TE2000 inverted microscope with a Nikon CFI Plan Apo VC 100X objective lens. Images were cropped and adjusted using MetaMorph software (Molecular Devices). Final figures were prepared using Adobe Illustrator (Adobe Systems). Image analyses were performed using MATLAB. All cells were segmented using phase-contrast images. Well-separated cells that were not undergoing cytokinesis were manually selected and used for analysis. Cell volume and intensity of fluorescence signals were determined using the built-in functions in MATLAB.

Electron microscopy

Cells were harvested at OD600 ~ 0.4, resuspended into LB medium, and fixed overnight at 4°C with 2.5% Glutaraldehyde, 1.25% Paraformaldehyde and 0.03% picric acid in 0.1 M sodium cacodylate buffer (pH 7.4). Fixed cells were washed in 0.1M cacodylate buffer and incubated with 1% Osmium Tetroxide (OsO4)/1.5% Potassium Ferrocyanide (KFeCN6) for 1 hour. Samples were then washed twice with ddH2O, washed once with Maleate buffer (MB), and incubated in 1% uranyl acetate in MB for 1 hour. Samples were washed twice with ddH2O, followed by dehydration in increasing concentration of alcohol (10 min each with 50%, 70%, 90%, twice with 100%). The samples were then incubated in propyleneoxide for 1 hour and infiltrated overnight in a 1:1 mixture of propyleneoxide and TAAB Epon (Marivac Canada Inc. St. Laurent, Canada). The samples were then embedded in TAAB Epon and polymerized at 60°C for 48 hrs. Ultrathin sections (~60 nm) were cut on a Reichert Ultracut-S microtome, mounted onto copper grids stained with lead citrate, and examined in a JEOL 1200EX Transmission electron microscope. Images were recorded with an AMT 2k CCD camera.

Marker frequency analysis

S. aureus cells were grown in LB 0.5% NaCl medium at 37°C, except Δnoc Δrbd, which was first grown under permissive conditions (0.5X LB no NaCl, 30°C) to OD600 ~0.4, then back diluted into nonpermissive conditions (LB 0.5% NaCl medium, 37°C) at an OD600 ~0.04. Sodium azide was added to cells at OD600 ~0.4 to prevent further growth and chromosomal DNA was then isolated using DNeasy Blood and Tissue Kit (Qiagen). To obtain cells with an ori:ter ratio of 1, exponentially growing cells (OD600 = 0.15) were treated with 50 μg/ml rifampicin for 1 hour at 37°C before harvesting. Quantitative PCR was performed using the SYBR FAST qPCR Kits (Kapa Biosystems) on a StepOne Plus Real-Time PCR System (Applied Biosystems). Primer sets oTP478/oTP479 and oTP480/oTP481 were used to amplify the S. aureus oriC and ter regions, respectively. The 2-ΔΔCt method was used to quantify the relative ori:ter ratio, where chromosomal DNA sample from rifampicin-treated wild-type cells was used for normalization. Marker-frequency analysis of B. subtilis strains was the same as S. aureus, except that cells were grown in CH medium at 30°C until OD600 ~ 0.25. Primer sets oTP482/oTP483 and oTP484/oTP485 were used to amplify the B. subtilis oriC and ter regions, respectively. Cell growth and chromosomal DNA preparation were the same for genome-wide marker frequency analysis. Whole genome sequencing was performed as described above. The sequencing reads from all strains were normalized to 51 million and the data were plotted in 30 kb bins. The smoothed conditional means were determined by LOESS method using ggplot2 in R [45]. The fraction of points used to fit each local regression (spanS) was 0.08. WGS data for marker frequency analysis are accessible through Gene Expression Omnibus under accession number GSE100776.

Immunoblot analysis

Whole cell lysates from exponentially growing cultures (OD600 = 0.4) were prepared as previously described [46]. Samples were heated at 100°C for 5 min prior to loading. Equivalent amount of cells based on OD600 at the time of harvest were separated by SDS-PAGE on Tris-Glycine gels, and transferred to PVDF membrane (EMD Millipore). Membranes were blocked in 5% nonfat milk with 0.5% Tween-20 for 1 h. Blocked membranes were probed with anti-6xHis (1:4000) (Genscript), anti-Noc (B. subtilis) (1:10,000), anti-DnaA (B. subtilis) (1:10,000) [47], or anti-σA (B. subtilis) (1:10,000) [48] antibodies. Primary antibodies were detected with horseradish-peroxidase conjugated anti-mouse (for anti-His) or anti-rabbit (for anti-Noc, anti-DnaA and anti-σA) antibodies (BioRad) and detected with Western Lightning ECL reagent as described by the manufacturer. Images were obtained by using the Molecular Imager Gel Doc XR system (Bio-Rad) and analyzed by ImageJ [49]. S. aureus immunoblots were performed in a strain lacking the spa gene encoding Surface Protein A.

Supplemental materials and methods.