Regulation of Spore Formation by the SpoIIQ and SpoIIIA Proteins
The bacterial spore-forming pathogen Clostridium difficile is a leading cause of nosocomial infections in the United States and represents a significant threat to healthcare systems around the world. As an obligate anaerobe, C. difficile must form spores in order to survive exit from the gastrointestinal tract. Accordingly, spore formation is essential for C. difficile disease transmission. Since the mechanisms controlling this process remain poorly characterized, we analyzed the importance of highly conserved secretion channel components during C. difficile sporulation. In the model organism Bacillus subtilis, this channel had previously been shown to function as a “feeding tube” that allows the mother cell to nurture the developing forespore and sustain transcription in the forespore. We show here that conserved components of this structure in C. difficile are dispensable for forespore transcription, although they are important for completing forespore engulfment and retaining the protective spore coat around the forespore, in contrast with B. subtilis. The results of our study suggest that targeting these conserved proteins could prevent C. difficile spore formation and thus disease transmission.
Published in the journal:
. PLoS Genet 11(10): e32767. doi:10.1371/journal.pgen.1005562
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1005562
Summary
The bacterial spore-forming pathogen Clostridium difficile is a leading cause of nosocomial infections in the United States and represents a significant threat to healthcare systems around the world. As an obligate anaerobe, C. difficile must form spores in order to survive exit from the gastrointestinal tract. Accordingly, spore formation is essential for C. difficile disease transmission. Since the mechanisms controlling this process remain poorly characterized, we analyzed the importance of highly conserved secretion channel components during C. difficile sporulation. In the model organism Bacillus subtilis, this channel had previously been shown to function as a “feeding tube” that allows the mother cell to nurture the developing forespore and sustain transcription in the forespore. We show here that conserved components of this structure in C. difficile are dispensable for forespore transcription, although they are important for completing forespore engulfment and retaining the protective spore coat around the forespore, in contrast with B. subtilis. The results of our study suggest that targeting these conserved proteins could prevent C. difficile spore formation and thus disease transmission.
Introduction
A small subset of bacteria can survive adverse environmental conditions by forming a metabolically dormant cell-type known as an endospore (referred to as a “spore” hereafter) [1–3]. Spore formation allows bacteria to survive harsh environmental conditions, such as heat, desiccation, oxygen-rich environments, disinfectants, and antibiotic treatment, since they can “reawaken” when favorable conditions return [1–4]. While spore formation is an ancient and adaptive mechanism for members of the Firmicutes, this developmental process is essential for the survival of many obligate anaerobes that inhabit or transiently live in the gut [5,6].
Clostridium difficile is a spore-forming obligate anaerobe that is a leading cause of nosocomial diarrhea and a major threat to healthcare systems around the world [7–10]. When C. difficile spores are ingested by susceptible hosts, they germinate in the gut and outgrow to form toxin-secreting vegetative cells [7,11,12]. While the toxins produced by C. difficile are responsible for the disease infection symptoms, spores are essential for this obligate anaerobe to transmit disease [6]. Accordingly, during growth in the gastrointestinal tract, C. difficile strongly induces sporulation in order to survive exit from the host [6,13]. Spores complicate C. difficile infection clearance because they are resistant to many disinfectants and inert to antibiotics [4]. As a result, they can persist in the environment for long periods of time and facilitate C. difficile disease recurrence [12,14,15]. Recurrent C. difficile infections are particularly problematic because they can lead to severe complications such as pseudomembranous colitis, toxic megacolon, and death [14–16]. However, despite the importance of spores to the pathogenesis of C. difficile, the molecular mechanisms underlying infectious spore formation remain largely uncharacterized.
Transmission electron microscopy analyses of several spore-forming organisms including C. difficile have shown that sporulation is defined by a series of morphological events starting with the formation of a polar septum, which generates a larger mother cell and smaller forespore [1–3,17]. The mother cell engulfs the forespore to create a protoplast surrounded by two lipid bilayer membranes suspended within the mother cell cytosol. The germ cell wall between the two membranes serves as the template for the synthesis of a thick protective layer of modified peptidoglycan called the cortex, while a series of protective proteinaceous shells called the spore coat is deposited on the outer forespore membrane [2,18]. Once forespore maturation is complete, the mother cell lyses to liberate a highly resistant spore.
Our knowledge of how these morphological events occur derives primarily from studies of the organism Bacillus subtilis. These analyses have revealed that morphological changes during sporulation are coupled to compartment-specific transcriptional changes [1–3]. In particular, the sequential and compartment-specific activation of four conserved sporulation-specific sigma factors, σF, σE, σG, and σK, leads to the activation of transcriptional programs that allow key morphological stages to be completed [1–3,17]. Following asymmetric division, σF and σE are activated early in the forespore and mother cell, respectively; following forespore engulfment, σG and σK are activated in the forespore and mother cell, respectively. These activation events depend upon coordinated intercompartmental signaling events. σF- and σG-dependent signaling in the forespore activates σE and σK in the mother cell, respectively, via regulated intramembrane proteolysis. σF and σE control σG activation in the forespore following engulfment completion by inducing the formation of a channel, also known as the “feeding tube” [19,20]. While the precise composition of this channel has not been determined, “feeding tube” components are thought to physically connect the mother cell to the forespore and transport unknown substrates that are required for σG activity in the forespore [19–21]. The “feeding tube” also controls forespore integrity [20], since the forespore collapses and eventually lyses in mutants lacking channel components [20,22]. σG activity may be further regulated by its apparent dependence on engulfment completion [23–25].
Analyses of sporulation-specific sigma factor function in C. difficile have revealed important differences in the regulatory architecture controlling sporulation [17,26]. While the sigma factors are controlled in a similar compartment-specific manner, σE activation only partially depends on σF; σG activation does not require σE; and σK activation does not depend on σG [27–29]. Since a C. difficile sigE mutant, which is stalled at asymmetric division, still activates σG in the forespore [28], C. difficile σG activity does not appear to be coupled to engulfment completion, in contrast with B. subtilis [23]. In general, activation of C. difficile sporulation-specific sigma factors appears to depend less on intercompartmental signaling and morphological changes than B. subtilis [17,26].
Since genome-wide transcriptional profiling has shown that σG regulon genes are expressed at wildtype levels in a C. difficile sigE−mutant [27,29], the mother cell-to-forespore channel shown to regulate B. subtilis σG activity appears to be dispensable for C. difficile σG activity, at least at early stages of sporulation [30]. Intriguingly, however, the genes encoding B. subtilis channel components, spoIIQ and the eight gene spoIIIA operon, are conserved across all spore-forming bacteria [31,32] and are induced during sporulation in a manner analogous to B. subtilis, with σF activating spoIIQ transcription and σE activating spoIIIA transcription [27,29]. These observations suggest that the mother cell-to-forespore channel may play important but possibly distinct roles during C. difficile spore formation relative to B. subtilis [30].
SpoIIQ has homology to Zn2+-dependent M23 peptidases (LytM domain, [33,34]) and forms a multimeric ring in the inner forespore membrane of B. subtilis [35–38]. The SpoIIIA proteins, SpoIIIAA-SpoIIIAH [39], have homology to secretion system components [19–21,40]. SpoIIIAA appears to function as an ATPase that likely powers the transport of metabolites across the “feeding tube” during B. subtilis sporulation [20]. SpoIIIAH forms a multimeric ring in the mother cell-derived outer forespore membrane that directly binds the SpoIIQ multimeric ring formed in the inner forespore membrane [34,35,37,38]. The SpoIIQ-SpoIIIAH complex alone can drive “zipper-like” engulfment in sporulating B. subtilis lacking a cell wall [41]. Based on these observations, this complex has been proposed to function as a Brownian “ratchet” that helps power engulfment. Consistent with this model, a spoIIQ mutant fails to complete engulfment [33] when sporulation is induced by nutrient starvation, even though “feeding tube” mutants can complete engulfment when sporulation is induced by resuspension [20].
C. difficile SpoIIIAA and SpoIIIAH exhibit 57% and 38% similarity, respectively, to their orthologs in B. subtilis (S1 and S2 Figs), while C. difficile SpoIIQ (CD0125) exhibits only 28% similarity despite also encoding a C-terminal LytM domain ([32], S3 Fig). In contrast with the degenerate active site of B. subtilis SpoIIQ [34], C. difficile SpoIIQ has an intact active site ([30], S3 Fig), suggesting that it may have peptidoglycan endopeptidase activity and thus function differently in C. difficile relative to B. subtilis. Furthermore, residues that directly mediate binding between B. subtilis SpoIIQ and SpoIIIAH are not well conserved in C. difficile (S1 and S2 Figs), raising the question as to whether these proteins interact in C. difficile. Indeed, whether SpoIIQ and/or SpoIIIA proteins regulate forespore integrity and/or have additional functions during C. difficile sporulation remain unknown [30].
To address these questions, we constructed gene disruptions of C. difficile spoIIQ, spoIIIAA, and spoIIIAH and determined their effects on spore formation using microscopic and cell biological assays. We also tested whether C. difficile SpoIIQ and SpoIIIAH interact and whether the predicted ATPase and endopeptidase activities of C. difficile SpoIIIAA and SpoIIQ are required for spore formation. These analyses revealed that SpoIIQ, SpoIIIAA, and SpoIIIAH regulate multiple stages of C. difficile spore formation, including engulfment, proper coat localization around the forespore, and maintenance of the forespore.
Results
SpoIIQ, SpoIIIAA, and SpoIIIAH are required for spore formation
To first determine if C. difficile spore development depends on the SpoIIQ and SpoIIIA proteins, we constructed targeted gene disruptions in the σF-regulated spoIIQ and σE-regulated spoIIIAA and spoIIIAH genes using the ClosTron gene knockout system (S4 Fig, [42]). Since targetron insertion into the spoIIIAA gene likely causes polar effects on the spoIIIA operon, which includes spoIIIAA-spoIIIAH (S4 Fig), the spoIIIAA mutation will be referred to as a spoIIIA mutant from hereon. However, since a second promoter within the spoIIIA operon has been shown to drive expression of spoIIIAG and spoIIIAH ([29], S4 Fig), the spoIIIA mutant likely still produces SpoIIIAH. Microscopic analysis of spoIIQ, spoIIIA, and spoIIIAH mutants during sporulation using the membrane dye FM4-64 and the nucleoid dye Hoechst revealed that these mutants are defective in engulfment (Fig 1). The percentage of cells captured at (i) asymmetric division, (ii) pre-engulfment with FM4-64 staining and Hoechst staining, (iii) post engulfment with FM4-64 staining and Hoechst staining, (iv) post engulfment with FM4-64 staining and Hoechst exclusion, (v) post engulfment with DIC-bright, FM4-64 exclusion and Hoechst exclusion, and (vi) free spore was quantified based on analyses of 100 sporulating cells. Whereas uniform staining of FM4-64 around the entire forespore or the presence of DIC-bright spore compartments was observed in wildtype sporulating cells 73% of the time (blue, green, white, and pink arrows), FM4-64 staining of sporulating spoIIQ and spoIIIAH mutants was restricted to the curved membrane at the mother cell-forespore interface (yellow arrows), and no DIC-bright forespore compartments were observed in these mutants, indicative of an engulfment defect. While the spoIIQ and spoIIIAH mutants both failed to complete engulfment, the spoIIIA and sigG mutants completed engulfment 10% and 24% of the time, respectively, although they did not mature to a stage that excluded Hoechst or FM4-64 (Fig 1). Taken together, these results suggest that SpoIIQ and SpoIIIAH are required for C. difficile forespore engulfment, while the SpoIIIAA-AF complex may be only partially required for engulfment.
Disruption of C. difficile spoIIQ, spoIIIA, and spoIIIAH resulted in a significant decrease in heat-resistant spore formation relative to wild type. Interestingly, while the C. difficile spoIIQ mutant did not show evidence of mature spore formation by fluorescence microscopy, we observed only a 200-fold defect in heat resistance relative to wild type (Fig 1). Since this defect was not as severe as the ~4–6 log defect reported for B. subtilis spoIIQ mutants [19], we investigated the possibility that the heat-resistant C. difficile spoIIQ mutant cells might arise from a heritable change by testing the heat resistance of subcultured spoIIQ−colonies that arose following heat treatment. The same frequency of heat resistance was observed, indicating that the production of heat-resistant spoIIQ−spores is a stochastic event. In contrast with the C. difficile spoIIQ mutant, no heat-resistant spores were observed for the C. difficile spoIIIA−and spoIIIAH−strains within the limits of detection of our assay (<10−6, Fig 1). The heat resistance defect of the C. difficile spoIIIA−mutant was similar to the defect reported for a B. subtilis ΔspoIIIAA mutant [20], although the C. difficile spoIIIAH−mutant was at least 4-logs more severe than the defect of a B. subtilis ΔspoIIIAH mutant [20].
To confirm that the spoIIQ, spoIIIA, and spoIIIAH gene disruptions abrogated protein production, we analyzed sporulating cell lysates prepared from spoIIQ, spoIIIA, and spoIIIAH mutants by Western blotting using antibodies raised against SpoIIQ and SpoIIIAH. As expected, SpoIIQ and SpoIIIAH were not detected in the spoIIQ and spoIIIAH mutants, respectively, and both proteins were absent in the spo0A mutant, which fails to initiate sporulation altogether (Fig 2A). Consistent with spoIIQ and spoIIIAH regulation by σF and σE, respectively [27,29], SpoIIQ was absent from the sigF mutant, and SpoIIIAH was absent in the sigE mutant. SpoIIIAH was nevertheless detected at wildtype levels in the spoIIIA mutant, since an internal promoter drives expression of spoIIIAG-AH ([29], S4A Fig) similar to the regulation of the B. subtilis spoIIIA operon [43]. Wildtype levels of SpoIIQ were observed in the spoIIIAH mutant, and vice versa, suggesting that loss of the predicted interaction between SpoIIQ and SpoIIIAH did not affect their steady state levels. Wildtype levels of SpoIIQ and SpoIIIAH were also observed in the sigG mutant, suggesting that this mutant’s engulfment defect did not result from the absence of these components. The small amount of SpoIIIAH that was detected in a sigF mutant (Fig 2A) is consistent with the partial activation of σE in a sigF mutant [27,29].
Since we were unable to generate a working antibody for detecting SpoIIIAA, we measured spoIIIAA transcript levels in the same strains. Consistent with the previously reported regulation of spoIIIAA by σE [27,29], statistically significant decreased levels of spoIIIAA transcripts were observed in spo0A, sigF, and sigE mutants relative to wild type (Fig 2B, p < 0.01). spoIIIAA transcript levels were unaffected in the spoIIQ, spoIIIAH, and sigG mutants (Fig 2B), indicating that loss of SpoIIQ or SpoIIIAH does not alter spoIIIAA expression. spoIIIAA transcripts could not be accurately measured in the spoIIIA mutant, since the amplification product is downstream of the targetron insertion.
Plasmid complementation rescues the sporulation defects of spoIIQ, spoIIIA, and spoIIIAH mutants
To validate that the observed mutant phenotypes were due to the targeted insertions, we attempted to complement the mutant strains with a wildtype copy of the disrupted gene(s) expressed from their native promoter using the pMTL83151 multicopy plasmid [44]. The spoIIIA mutant was complemented with the full spoIIIA operon, and the spoIIIAH mutant was complemented with either the full spoIIIA operon, or the spoIIIAH gene alone (S5 Fig). The spoIIQ and spoIIIA complementation constructs all restored production of heat-resistant, DIC-bright spores to their respective mutant backgrounds (S5 Fig). While complementation of the spoIIIAH mutant with either the spoIIIA operon or spoIIIAH gene under the control of the spoIIIA promoter restored heat-resistant spore production, the spoIIIA operon conferred ~8-fold higher heat-resistance to the spoIIIAH mutant relative to complementation with the spoIIIAH gene alone. Western blot analysis revealed that SpoIIIAH levels were elevated in the spoIIIA operon complementation strain relative to spoIIIAH complementation strain and wildtype carrying empty vector (S6 Fig). Complementation of spoIIQ−resulted in ~4-fold greater heat-resistant spore formation than wildtype carrying empty vector. Western blot analysis indicated that SpoIIQ levels were slightly elevated in the spoIIQ complementation strain relative to wildtype carrying empty vector (S6 Fig).
Fluorescence microscopy analyses of the spoIIQ, spoIIIA, and spoIIIAH strains carrying empty vector confirmed that the majority of mutant cells failed to complete engulfment (S5 Fig, yellow arrows). On rare occasions, we observed that the spoIIIA mutant carrying empty vector completed engulfment (S5 Fig, blue arrow), similar to our observations with the spoIIIA mutant alone (Fig 1). Regardless, these results indicate that the gene disruptions in the spoIIQ, spoIIIAA and spoIIIAH genes are responsible for the observed engulfment and heat-resistance defects.
Engulfment defects in the spoIIQ, spoIIIA, and spoIIIAH mutants
To gain further insight into the nature of the engulfment defect in the spoIIQ, spoIIIA, and spoIIIAH mutants, we analyzed each mutant using transmission electron microscopy (TEM). We failed to observe engulfment of spoIIQ and spoIIIAH mutants based on analyses of over 50 cells that had progressed beyond asymmetric division for each mutant, with engulfment being defined as the mother cell-derived membrane surrounding the entire forespore (Fig 3). The spoIIIA mutant was observed to complete engulfment in ~20% of cells analyzed by TEM, even though this mutant failed to produce heat-resistant spores (Fig 1). In contrast, none of the spoIIQ and spoIIIAH mutant cells strains completed engulfment. However, since heat-resistant spoIIQ−spores could be detected at a frequency of 1 in 200 (Fig 1), we extensively analyzed the TEM grids and identified a single spoIIQ−cell that had completed engulfment (S7A Fig). Taken together, these results confirm the live cell microscopy analyses (Fig 1): loss of SpoIIQ and SpoIIIAH causes a severe defect in forespore engulfment, while the apparent loss of SpoIIIAA-AF in the spoIIIA mutant still permits engulfment in 10–20% of cells.
spoIIQ, spoIIIA, and spoIIIAH mutants exhibit defects in adhering coat to the forespore and maintaining forespore integrity
In addition to the engulfment defects observed in the spoIIQ, spoIIIA, and spoIIIAH mutants by TEM, a second “compartment” was often observed to extend from the forespore of the spoIIQ, spoIIIA, and spoIIIAH mutants (Fig 3, white arrows). Closer inspection of these extensions revealed multiple striated lines that were consistent with coat. The mutant coat-like structures appeared to anchor to the leading edge of the engulfing membrane but were not adhered to the mother cell-forespore interface in the majority of cells with engulfment defects. Coat-like structures were present 100% of the time in spoIIQ–, spoIIIA–, and spoIIIAH−strains that had begun engulfment; these structures appeared anchored to the leading edge of the engulfing membrane 94%, 96%, and 66% of the time in spoIIQ–, spoIIIA–, and spoIIIAH−strains, respectively. A similar phenotype was observed in the sigG−strain (Fig 3, [27]). In some instances, the coat-like structures were not associated with the forespore at all and were instead mislocalized to the mother cell cytosol, similar to the previously described coat mislocalization phenotype of a spoIVA mutant ([45], Fig 3, yellow arrows). In particular, mislocalized cytosolic coat was observed with high frequency in the spoIIIAH mutant (51%), regardless of whether the coat was anchored to the leading edge. For the spoIIQ–, spoIIIA–, and spoIIIAH−cells that had coat anchored to the leading edge of the engulfing membrane, 98%, 89%, and 94%, respectively, did not have coat intimately associated with the forespore interface (Fig 3, white arrows). Notably, the rare spoIIIA and spoIIQ mutants that completed engulfment had visible coat surrounding the forespore compartment by TEM (S7A Fig, black arrows). Furthermore, in wildtype cells, coat was only observed after engulfment was complete.
To confirm that the coat-like assemblages observed in the spoIIQ, spoIIIA, spoIIIAH, and sigG mutants were indeed coat, we analyzed the localization of a known coat protein in these mutant backgrounds. In particular, we correlated the localization of the previously reported surface-exposed coat protein CotE fused to a SNAP imaging tag [28] with FM4-64 and Hoechst staining. The CotE-SNAP protein fusion was detected concentrated at both poles of the developing forespore in wild type, with a weaker signal surrounding the forespore (Fig 4) similar to the previously reported localization of this protein fusion around the forespore [28]. Faint CotE-SNAP staining was observed around free spores of wild type, consistent with the surface localization of CotE [46,47]. In contrast, in the spoIIQ, spoIIIA, and spoIIIAH mutants, CotE-SNAP signal was frequently offset from FM4-64 staining of the forespore membrane. The CotE-SNAP signal was also observed mislocalized to the mother cell cytosol in these mutants (Fig 4), similar to the displacement of the CotE-SNAP signal to the mother cell cytosol of the spoIVA mutant, which has previously been shown to mislocalize coat [45]. While the FM4-64 readily stained forespore membranes, it also appeared to associate with mislocalized coat in the spoIVA, spoIIQ, spoIIIA, and spoIIIAH mutants (Fig 4, yellow arrows), making it difficult to assess by light microscopy whether CotE-SNAP was adhered to the forespore membrane. Nevertheless, combined with our TEM data, the CotE-SNAP localization experiments strongly suggest that coat detaches from the forespore and/or completely mislocalizes to the mother cell cytosol in the absence of SpoIIQ and SpoIIIA proteins.
While the dominant phenotypes observed by TEM for spoIIQ, spoIIIA, and spoIIIAH mutants are shown in Fig 3, 13%, 14%, and 27% of spoIIQ, spoIIIA, and spoIIIAH mutant cells, respectively, harbored forespores that were undergoing forespore collapse. In particular, large invaginations of the forespore membrane were observed in these mutants (S7B Fig, blue arrows), similar to the phenotypes previously described for B. subtilis mutants lacking SpoIIQ or SpoIIIA complex components [20]. These results indicate that these proteins in C. difficile are also required to maintain forespore integrity, similar to B. subtilis [20].
C. difficile σG activity does not depend on SpoIIQ, SpoIIIAA, and SpoIIIAH
In addition to maintaining forespore integrity in B. subtilis, the feeding tube is required to sustain transcription in the forespore [19] and thus is necessary for σG activity [19,20,25,40]. However, previous transcriptional analyses in C. difficile suggested that the “feeding tube” components were dispensable for σG activity, since a C. difficile σG-dependent transcriptional reporter is produced in the forespore of a sigE mutant [28], and the σG regulon is expressed at wildtype levels in the sigE mutant [27,29]. To test whether C. difficile spoIIQ, spoIIIA, and spoIIIAH are required for σG activity, we measured σG-dependent transcript levels in wild type, spoIIQ, spoIIIA and sporulation sigma factor mutants using quantitative RT-PCR. As expected, no statistically significant difference in σG-dependent transcripts spoVT, spoVAD, and CD1430 [27,29], were observed in the feeding tube mutants (S8 Fig). Consistent with the dependence of σG activity on Spo0A and σF, spoVT was significantly decreased in spo0A, sigF, and sigG mutants (p < 0.0005), CD1430 was significantly decreased in spo0A, sigF, and sigG mutants (p < 0.05) and spoVAD was significantly decreased in spo0A, sigF, and sigG mutants (p < 0.01, 0.01, and 0.05, respectively).
Since it is possible that the wildtype levels of σG activity detected in spoIIQ and spoIIIA mutants by qRT-PCR may derive from improper σG activation in the mother cell, we used the σG-dependent SNAP-tag transcriptional reporter to visualize σG activation in spoIIQ and spoIIIA mutants. The promoter region of the σG-dependent sspA gene previously described by Pereira et al. [28] was fused to a codon-optimized SNAP gene and conjugated into wildtype, sigF–, spoIIQ–, sigE–, spoIIIA–, spoIIIAH–, and sigG−strains. Similar to the previous reports [28], SNAP labeling with the TMR-Star substrate (i.e. σG activity) was restricted to the forespore of cells that had completed asymmetric division or engulfment (Fig 5A). No SNAP signal was detectable in either the sigF or sigG mutants (Fig 5A, black arrows), as expected. In contrast, σG-dependent SNAP labeling was detectable in the forespores of cells undergoing sporulation in the spoIIQ–, sigE–, spoIIIA–, and spoIIIAH−strains (Fig 5A, yellow arrows). The prevalence of σG-dependent transcription in cells undergoing sporulation (based on the presence of an asymmetric septum, engulfment initiated, or engulfment completed phenotype) was determined by counting the number of cells exhibiting SNAP labeling. The σG-dependent transcriptional reporter was produced in the forespore of spoIIQ–, spoIIIA–, and spoIIIAH−cells 58%, 57%, and 50%, respectively, of sporulating cells, which was similar to the frequency observed in wild type (57%, Fig 5A). The SNAP signal was observed in the forespore of the sigE mutant in 28% of sporulating cells. Western blot analyses confirmed that wildtype levels of SNAP protein were observed in spoIIQ, sigE, spoIIIA, and spoIIIAH mutants (Fig 5B). Taken together, these results demonstrate that the C. difficile SpoIIQ and SpoIIIA components are dispensable for maintaining transcription in the forespore, in contrast with B. subtilis [19].
SpoIIQ and SpoIIIAH interact
Since these analyses indicated that the C. difficile SpoIIQ and SpoIIIA proteins regulate different cellular processes during sporulation than in B. subtilis, namely σG activity and forespore engulfment, we next sought to investigate how these components regulated these processes. We first tested whether the C. difficile feeding tube components assemble into a complex as has been shown in B. subtilis [34], since the interaction between SpoIIQ and SpoIIIAH is necessary for feeding tube function in B. subtilis [35]. Using a co-affinity purification assay, we determined whether C. difficile SpoIIQ and SpoIIIAH directly interact through their extracellular domains. To this end, we co-expressed His6-tagged SpoIIQ and HA-tagged SpoIIIAH, both lacking their transmembrane domains, in E. coli. Affinity purification of His6-tagged SpoIIQ resulted in the co-purification of HA-tagged SpoIIIAH, whereas HA-tagged SpoVT, which was used as a specificity control, did not co-purify with His6-tagged SpoIIQ when co-expressed (Fig 6). Thus, despite the low degree of sequence homology between B. subtilis and C. difficile SpoIIQ orthologs (S3 Fig), C. difficile SpoIIQ and SpoIIIAH directly interact in vitro through their extracellular domains, consistent with the hypothesis that these proteins form a complex that bridges the intercompartmental space between the mother cell and forespore [34,41].
Mutation of the SpoIIQ LytM catalytic triad does not strongly impact sporulation
Based on these findings, we next tested whether the predicted catalytic activities of SpoIIQ and SpoIIIAA were required for their function. The LytM domain of C. difficile SpoIIQ carries an intact catalytic triad consisting of two conserved motifs: HxxxD and HxH [30]. These motifs coordinate a metal ion (commonly zinc) that is essential for endopeptidase activity, which degrades the peptide linkages that crosslink the glycan strands of peptidoglycan [48]. To determine if C. difficile SpoIIQ’s endopeptidase activity is necessary for sporulation, we complemented the spoIIQ mutant with a spoIIQ variant encoding a histidine 120 to alanine mutation (spoIIQ–/H120A, S3 Fig), which should inactive its predicted endopeptidase activity. Analysis of this strain in the heat resistance assay indicated that the H120A mutation caused an ~50% reduction in heat-resistant spore formation relative to wildtype carrying empty vector (S9 Fig). TEM analyses revealed that 52% of spoIIQ–/H120A cells completed engulfment compared to 88% of the wildtype complementation strain (spoIIQ–/spoIIQ) and 96% of wildtype carrying empty vector (S9 Fig). These results indicate that the endopeptidase activity of SpoIIQ plays a minor role in regulating C. difficile sporulation under the conditions tested.
The Walker A motif of SpoIIIAA is important for C. difficile sporulation
SpoIIIAA is predicted to function as an ATPase, since strains carrying mutations of conserved residues in the Walker A and B boxes (S1 Fig, [49]) in B. subtilis resemble a ΔspoIIIAA mutant [20]. Disruption of the Walker A motif typically prevents ATP binding [50], while disruption of the Walker B motif typically prevents ATP hydrolysis without affecting ATP binding [51,52]. To determine whether the ATPase activity of C. difficile SpoIIIAA is also required for spore formation, we constructed complementation strains encoding SpoIIIAA carrying a Walker A lysine mutation, K167A, a Walker B aspartate mutation, D244A, and a Walker A/Walker B double mutation K167A/D244A (S1 Fig), and tested their ability to complement the heat resistance defect of a spoIIIA mutant. The K167A mutant, expressed from a spoIIIA operon complementation plasmid exhibited ~300-fold defect relative to wildtype carrying empty vector (Fig 7). Interestingly, only 6% of sporulating K167A cells completed engulfment when analyzed by TEM compared to 20% of the parent spoIIIA−strain carrying empty vector (Fig 7), and similar results were observed by FM4-64 and Hoechst staining (S10 Fig). The D244A mutant exhibited close to wildtype levels of heat resistance (~3-fold decrease), consistent with its ability to complete engulfment 35% of the time (Fig 7). The K167A/D244A double mutant resembled the K167A single mutant in exhibiting a three-log decrease in heat resistance and ~4% engulfment efficiency relative to wild type. In contrast, the wildtype complementation strain (spoIIIA–/spoIIIA) exhibited wildtype levels of heat resistance and engulfment completion (Fig 7).
Since we could not test whether the K167A, D244A, or K167A/D244A mutation(s) affected SpoIIIAA protein levels due to the absence of a working antibody, we compared spoIIIAA transcript levels in the K167A mutant, whose heat resistance and engulfment defect was more severe than the D244A mutant and equivalent to the double mutant (Fig 7), relative to wildtype carrying empty vector and the spoIIIA complementation strain. These analyses indicated that spoIIIAA transcript levels in the K167A complementation strain were similar to the spoIIIA complementation strain and wildtype carrying empty vector (S6B Fig). Since the Walker A K167A mutation was considerably more severe than the Walker B D244A mutation, our results suggest that SpoIIIAA function likely depends on its ability to bind, but not necessarily hydrolyze, ATP. Given that B. subtilis SpoIIIAA function completely depends on the presence of intact Walker A and Walker B boxes [20], C. difficile SpoIIIAA appears to have differential requirements for its function relative to B. subtilis.
spoIIQ, spoIIIA, and spoIIIAH mutants actively transform peptidoglycan around the forespore despite their engulfment defects
The engulfment defects of the C. difficile spoIIQ, spoIIIA, and spoIIIAH mutants prompted us to investigate the mechanisms underlying this engulfment defect. In B. subtilis, peptidoglycan hydrolase enzymes that degrade the peptidoglycan layer between the mother cell and forespore drive engulfment [53–55]. Subsequent transformations of this peptidoglycan layer, which involve both the making and breaking of peptide and glycan bonds, essentially “cut” the forespore free of the mother cell until engulfment is complete [56]. Since transpeptidases and/or ligases can incorporate D-alanine into the stem peptide that is conjugated to the glycan strand of peptidoglycan [57], newly remodeled and/or synthesized peptidoglycan can be metabolically labeled using unnatural D-alanine derivatives conjugated to bioorthogonal functional groups [58,59]. To determine if peptidoglycan remodeling and/or synthesis is active during C. difficile forespore engulfment, we incubated sporulating C. difficile cultures with D-alanine bearing an alkyne group and visualized its incorporation into peptidoglycan over time using copper-catalyzed click chemistry [59]. Alkyne D-alanine, referred to as “alkDala,” was labeled through the azide-alkyne cycloaddition of an azide group conjugated to a fluorescein-derivative [60].
Analysis of wildtype sporulating cells using this metabolic labeling assay revealed that fluorescent peptidoglycan signal (PG) was detectable within 10 min of incubating the culture with alkDala (Figs 8 and S11). After 30 min of incubation with alkDala, the peptidoglycan signal was observed surrounding the forespore and, to a lesser extent, the mother cell (Fig 8). In contrast, when the spoIIQ mutant was incubated with alkDala for 10 min or longer, peptidoglycan remodeling and/or synthesis was localized primarily at the curved septa at the mother cell-forespore interface (Fig 8), consistent with the spoIIQ mutant’s engulfment defect (Fig 1). Incubation of the sigE mutant with alkDala resulted in labeling of the polar septa and mother cell peptidoglycan after 20 min of incubation with alkDala. For comparison, B. subtilis engulfment requires ~45 min to complete [61,62], and sporulation occurs more slowly in C. difficile than in B. subtilis [27,28].
To determine the optimal length of time for measuring alkDala incorporation during sporulation, we analyzed the distribution of the alkDala label in sporulating wild type cells 10’, 20’, 30’, and 40’ after alkDala addition. Sporulating wildtype cells with visible peptidoglycan labeling were binned into the following categories: (i) no staining of the forespore, (ii) labeling of the polar septum, (iii) partial labeling of the forespore on the mother cell distal side (i.e. labeling after engulfment has initiated), (iv) partial labeling around the middle of the forespore, (v) partial labeling of the forespore on the mother cell proximal side, (vi) labeling around the entire forespore (S11 Fig). Based on these analyses, we chose to label cells after a 30 minute incubation with alkDala, since this was the earliest time point at which full labeling of the forespore was detected in the majority of wildtype sporulating cells (S11 Fig).
As expected, the alkDala probe labeled division septa in all strains (S12A Fig), and fluorescent labeling was not observed in wildtype cells incubated with D-alanine, which cannot undergo cycloaddition (S12B Fig), or at time 0 min, even though the samples were exposed to the azido-fluorophore probe (Fig 9). To ensure that alkDala specifically labeled newly transformed PG, we incubated WT cells with the cell wall synthesis inhibitors vancomycin and imipenem prior to addition of alkDala and evaluated alkDala incorporation by flow cytometry. Vancomycin inhibits cell wall synthesis by preventing both transpeptidation and transglycosylation [63], and imipenem covalently inhibits the penicillin binding proteins required for transpeptidation [64]. Incubation of wildtype cells with alkDala resulted in a statistically significant increase in median fluorescent intensity (MFI) relative to the MFI of WT cells incubated with Dala (S13 Fig; p < 0.0001). While vancomycin treatment did not reduce alkDala labeling relative to the positive control in a statistically significant manner, imipenem treatment decreased alkDala label incorporation ~5-fold relative to the positive control (p < 0.0001). Taken together, these results suggest that the alkDala probe specifically labels newly synthesized and/or remodeled peptidoglycan, and peptidoglycan continuously surrounds the C. difficile forespore throughout engulfment as previously observed in B. subtilis [65].
Since the metabolic labeling time course demonstrated that the fluorescent signal was maximal after 30 min of alkDala incorporation, we used this labeling period to assess whether C. difficile mutants defective in engulfment could remodel and/or synthesize peptidoglycan around the forespore. Although the metabolic label was evenly distributed around the entire perimeter of wildtype forespores, the label was only partially distributed around the mother cell proximal side of the forespore in engulfment-defective spoIIQ, spoIIIA, spoIIIAH, and sigG mutants (Fig 9). These results suggest that the engulfment defect of the spoIIQ, spoIIIA, spoIIIAH, and sigG mutants is not due to a failure to activate peptidoglycan remodeling and/or synthesis. Instead, the active peptidoglycan transformations observed in the spoIIQ, spoIIIA, and spoIIIAH mutants appear to be insufficient to drive engulfment to completion.
Discussion
Since the SpoIIIAA-AH components of the B. subtilis “feeding tube” channel are universally conserved in spore-forming organisms [31,32], and a SpoIIQ-like ortholog is conserved in the Clostridia [32], we hypothesized that these proteins would play a critical role in regulating C. difficile spore formation. In this study, we have demonstrated that C. difficile SpoIIQ and SpoIIIA proteins control forespore engulfment and integrity and the intimate association of the coat with the forespore (Figs 3, 4 and S7). Although SpoIIQ and SpoIIIAH are strongly required for engulfment, the SpoIIIAA-AF proteins appear to be only partially required for engulfment completion in C. difficile, since the spoIIIA mutant completes engulfment ~10–20% of the time (Figs 1, 7, and S7). Given that this mutant produces wildtype levels of SpoIIQ and SpoIIIAH (Fig 2), and SpoIIQ and SpoIIIAH directly interact at least in vitro (Fig 6) similar to their B. subtilis counterparts [34], C. difficile SpoIIQ and SpoIIIAH would appear to be sufficient to complete engulfment in some spoIIIA mutant cells.
While it remains possible that SpoIIIAG also regulates C. difficile forespore engulfment in the spoIIIA mutant, our observations are nevertheless consistent with the proposal that SpoIIQ-SpoIIIAH complex functions like a “Brownian” ratchet to allow for “zipper-like” engulfment [41]. Indeed, the finding that the SpoIIQ H120A mutant exhibits only a partial defect in engulfment completion and heat-resistant spore formation relative to wild type (~50%, S9 Fig) implies that SpoIIQ-SpoIIIAH complex formation is more important for engulfment completion than the putative endopeptidase activity of C. difficile SpoIIQ. In contrast, B. subtilis SpoIIQ lacks endopeptidase activity, and the SpoIIQ-SpoIIIAH complex is dispensable for engulfment when sporulation is induced by the re-suspension method [20,41,66]. However, when sporulation is induced by nutrient exhaustion, B. subtilis SpoIIQ is required to complete engulfment [22,33,41]. This observation suggests that media composition causes changes within sporulating cells such that some sporulation proteins are differentially required for engulfment. Since the 70:30 media used to induce C. difficile sporulation in this study resembles the nutrient exhaustion media used in B. subtilis [67], it will be interesting to test whether differences in media compositions and sporulation conditions (e.g. broth vs. plate-based induction) will lead to differential requirements for C. difficile SpoIIQ and SpoIIIAH during engulfment. Indeed, C. difficile sigG mutants appear to exhibit differences in engulfment completion when sporulation is induced in broth vs. on plates, although slight differences in strain background could be responsible for this difference [27,28]. Regardless, the engulfment defects of C. difficile spoIIQ and spoIIIAH mutants suggest that the ancestral function of the SpoIIQ-SpoIIIAH complex is to control engulfment during sporulation [68].
Even though SpoIIQ and SpoIIIAH appear to be sufficient to mediate engulfment in ~15% of C. difficile spoIIIA−cells, the spoIIIA−mutant nevertheless failed to produce heat-resistant spores. Since the spoIIIA−mutant is likely defective in producing the SpoIIIAA-AF proteins (S4 Fig), these proteins would appear to regulate steps beyond engulfment during C. difficile sporulation (Fig 1). Indeed, our mutational analyses implicate SpoIIIAA’s predicted ability to bind ATP as being critical for engulfment completion, since mutation of the Walker A ATP binding motif (K167A) results in an ~300-fold defect in heat-resistant spore formation relative to wild type (Fig 7). Interestingly, ATP hydrolysis would appear to be less important for SpoIIIAA’s function during spore formation, since the Walker B mutant (D244A) exhibits only a 3-fold defect in engulfment and heat-resistant spore formation (Fig 7). Given that the phenotype of the K167A/D244A double mutant resembles that of the K167A single mutant, nucleotide binding by SpoIIIAA may induce a conformational change within the protein that is necessary for its function. Consistent with this hypothesis, B. subtilis SpoIVA Walker A ATP binding mutants exhibit different phenotypes from Walker B ATPase mutants [52]. Alternatively, a different aspartate residue may substitute for the predicted role of D244 in catalyzing C. difficile SpoIIIAA’s ATPase activity. While this functional redundancy is formally possible, we note that the equivalent Walker B mutation in B. subtilis SpoIIIAA (D224A) causes a heat-resistant spore formation defect equivalent to a ΔspoIIIAA mutant [20]. It will be important in future studies to determine whether C. difficile SpoIIIAA binds and hydrolyzes ATP, and whether these activities are necessary to power transport of proteins and/or metabolites from the mother cell to the forespore similar to B. subtilis SpoIIIAA [19–21].
While the C. difficile spoIIIA mutant completed engulfment in ~10–20% of cells yet failed to produce heat-resistant spores, the C. difficile spoIIQ mutant exhibited a severe engulfment defect and produced heat-resistant spores 0.5% of the time relative to wild type. The mechanism by which spoIIQ−cells form functional spores remains mysterious given that SpoIIIAH likely binds SpoIIQ during C. difficile sporulation (Fig 6) and is required for heat-resistant spore formation. Interestingly, a differential requirement for SpoIIIAH is observed in B. subtilis, since a spoIIIAH mutant has a 1000-fold less severe phenotype relative to other spoIIIA mutants [20]. While a mechanism underlying these differential phenotypes remains unclear for both C. difficile and B. subtilis, functionally redundant mechanisms appear to exist in both organisms. Testing this hypothesis in C. difficile would be greatly aided by analyses of C. difficile SpoIIQ and SpoIIIA protein complex formation during sporulation.
Although the SpoIIQ and SpoIIIA proteins regulate C. difficile forespore engulfment, these proteins appear dispensable for σG activity in the forespore (Figs 5 and S8) as predicted [27,29]. Despite these observations, it nevertheless remains possible that these proteins are needed to sustain σG activity after engulfment is complete. Contrary to this model, the number of spoIIIA−cells that activated σG was identical to wild type (Fig 5). Nevertheless, since we cannot assess the duration of σG activity in the forespore due to the inability to synchronize sporulation in C. difficile [27,28,45], it remains possible that the forespore may require resources from the mother cell in a SpoIIQ- and SpoIIIA-dependent manner during late stages of sporulation.
Our analyses also uncovered a surprising role for C. difficile SpoIIQ and SpoIIIA proteins in regulating the adherence of the spore coat to the engulfing forespore. TEM analyses revealed that the spore coat appears to localize and anchor to the leading edge of the engulfing membrane but sometimes sloughs away from the mother cell-forespore interface (Fig 3). Unfortunately, little is known about the mechanisms by which the spore coat localizes around the forespore in C. difficile, since few coat morphogenetic proteins are conserved between C. difficile and B. subtilis [18]. SpoIVA and the clostridial-specific SipL have been shown to function as coat morphogenetic proteins by localizing the coat to the forespore in C. difficile [45], but how these proteins are recruited to the forespore membrane is unclear. Our results suggest an intriguing link between engulfment completion and adhering coat around the forespore, since the minority of spoIIIA−and spoIIQ−cells that completed engulfment produced coat surrounding the forespore (S7 Fig). Perhaps proteins localized to the leading edge of the engulfing membrane recruit C. difficile coat proteins but are insufficient to adhere the coat to the forespore in the absence of engulfment completion, or mechanical forces that drive engulfment to completion are also required to intimately associate the coat with the forespore.
A link between SpoIIQ and coat localization around the forespore has been described in B. subtilis, since SpoIIQ is required for many coat proteins, including the σE-dependent coat protein CotE (unrelated to C. difficile CotE [47]), to surround the forespore in a process known as “encasement” [69]. Since B. subtilis CotE localizes properly in a sigG mutant [69], the B. subtilis spoIIQ mutant’s ~30-fold encasement defect suggests that components of the coat indirectly interact with the forespore-localized SpoIIQ. It should be noted, however, that CotE in a B. subtilis spoIIQ mutant appears to track along the mother cell-forespore interface [69], in contrast with C. difficile spoIIQ, spoIIIA, and spoIIIAH mutants in which coat is located some distance from this interface due to an apparent defect in adhering to the forespore (Figs 3 and 4). Furthermore, the B. subtilis ΔspoIIQ mutant completes engulfment in the conditions used for the coat localization studies, whereas the C. difficile spoIIQ mutant largely fails to complete engulfment (Figs 3, S7 and S9). Since B. subtilis CotE localization around the forespore depends upon earlier morphogenetic proteins SpoVM, SpoIVA, and SpoVID [69], it would be interesting to determine whether B. subtilis “feeding tube” components affect the localization of these earlier morphogenetic proteins, and vice versa. Similarly, C. difficile CotE is a σK-regulated protein that appears to localize to the outermost layers of C. difficile spores [46], so determining the localization patterns of SpoIVA and/or SipL in the spoIIQ, spoIIIA, and spoIIIAH mutants may provide insight into whether SpoIIQ and/or SpoIIIAA-AH regulate the localization of these coat morphogenetic proteins. Future studies evaluating whether these proteins form a channel in C. difficile, why these proteins are important for forespore integrity, and how these proteins regulate engulfment and coat association with the forespore will provide much-needed insight into how these cellular processes are controlled in C. difficile and potentially other spore-forming organisms.
Materials and Methods
Bacterial strains and growth conditions
All C. difficile strains are listed in Table 1 and derive from the parent strain JIR8094, an erythromycin-sensitive derivative [70] of the sequenced clinical isolate 630 [71]. C. difficile strains were grown on solid brain heart infusion media supplemented with yeast extract (BHIS: 37 g brain heart infusion, 5 g yeast extract, 0.1% (w/v) L-cysteine, 15 g agar per liter) [72]. Taurocholate (TA; 0.1% w/v), thiamphenicol (5–10 μg/mL), kanamycin (50 μg/mL), cefoxitin (16 μg/mL), FeSO4 (50 μM), and/or erythromycin (10 μg/mL) were used to supplement the BHIS media as indicated. Cultures were grown at 37°C, under anaerobic conditions using a gas mixture containing 85% N2, 5% CO2, and 10% H2.
Sporulation was induced on media containing BHIS and SMC (90 g BactoPeptone, 5 g protease peptone, 1 g NH4SO4, 1.5 g Tris base, 15 g agar per liter) [73], at 70% SMC and 30% BHIS (70:30 media, 63 g BactoPeptone, 3.5 g Protease Peptone, 11.1 g BHI, 1.5 g yeast extract, 1.06 g Tris base, 0.7 g NH4SO4, 15 g agar per liter) [45]. 70:30 agar (supplemented as appropriate with thiamphenicol at 10 μg/mL) was inoculated from a starter culture grown on solid media. 70:30 broth was made as stated above omitting the agar.
HB101/pK424 strains were used for conjugations and BL21(DE3) strains were used for protein expression. E. coli strains were routinely grown at 37°C, shaking at 225 rpm in Luria-Bertani broth (LB). Media was supplemented with chloramphenicol (20 μg/mL), ampicillin (100 μg/mL), or kanamycin (30 μg/mL) as indicated.
E. coli strain construction
All strains are listed in S1 Table; all plasmids are listed in S2 Table; and all primers used are listed in S3 Table. For disruption of spoIIQ, spoIIIAA, and spoIIIAH, a modified plasmid containing the retargeting group II intron, pCE245 (a gift from C. Ellermeier, University of Iowa), was used as the template. Primers used to amplify the targeting sequence from the template carried flanking regions specific for each gene target and are listed as follows: spoIIQ (#1052, 1053, 1054 and 532, the EBS Universal primer as specified by the manufacturer (Sigma Aldrich)), spoIIIAA (#1049, 1050, 1051 and 532), and spoIIIAH (#1264, 1265, 1266, and 532). The resulting retargeting sequences were digested with BsrGI and HindIII and cloned into pJS107 (a gift from J. Sorg, University of Texas A&M), a derivative of pJIR750ai (Sigma Aldrich). The ligations were transformed into DH5α and confirmed by sequencing. The resulting plasmids were used to transform HB101/pK424.
To construct the spoIIQ complementation construct, primers #1177 and 1178 were used to amplify spoIIQ containing 106 bp of the upstream region using 630 genomic DNA as the template. To construct the spoIIQ H120A complementation construct, SOE primers #1177 and #1851 were used to generate a 5’ fragment (590 bp) containing the H120A mutation; primers #1850 and #1178 were used for the 3’ SOE product using the IIQ complementation construct as a template. To construct the spoIIIA operon complementation construct, primers #1174 and 1175 were used to amplify 211 bp upstream of spoIIIAA and 9 bp downstream of spoIIIAH using 630 genomic DNA as the template. The spoIIIAH complementation construct was made using PCR splicing by overlap extension (SOE, [74]). Primer pair #1174 and 1618 was used to amplify the 5’ SOE product, while primer pair #1617 and 1239 was used to amplify the 3’ SOE product. The resulting fragments were mixed together, and flanking primers #1174 and #1239 were used to generate a fragment corresponding to 211 bp of the spoIIIA upstream region fused to the spoIIIAH gene (PspoIIIA-spoIIIAH). To construct the spoIIIA operon K167A complementation construct, SOE primers #1174 and #1432 were used to generate a 5’ fragment (590 bp) containing the K167A mutation; primers #1431 and #1175 were used for the 3’ SOE product. The flanking primers #1174 and #1175 were used to amplify the K167A IIIA complementation construct. To construct the spoIIIA operon D244A complementation construct, SOE primers #1174 and #1853 were used to generate a 5’ fragment (590 bp) containing the D244A mutation; primers #1852 and #1854 were used for the 3’ SOE product using the IIIA complementation construct as a template. The flanking primers #1174 and #1854 were used to amplify the D244A IIIA mutation insert, digested with NotI and SalI. The plasmid carrying the IIIA complementation construct was also digested with NotI/SalI and then gel purified to separate the plasmid backbone from the wildtype fragment. The D244A IIIA NotI/SalI fragment was ligated to the gel-purified cut vector. To construct the spoIIIA operon K167A/D244A complementation construct, SOE primers #1174 and #1853 were used to generate a 5’ fragment (590 bp) containing the D244A mutation; primers #1852 and #1854 were used for the 3’ SOE product using the K167A complementation construct as a template. The flanking primers #1174 and #1854 were used to amplify the D244A IIIA mutation insert, digested with NotI and SalI, and ligated to the IIIA complementation construct digested with NotI/SalI as described earlier. All complementation constructs except for the D244A and K167A/D244A were digested with NotI and XhoI and ligated into pMTL83151 [44] digested with the same enzymes.
To construct strains producing recombinant N-terminally truncated SpoIIQ and N-terminally truncated SpoIIIAH for antibody production, primer pairs #1568 and 1569 and #1566 and 1567, respectively were used to amplify codon optimized spoIIQ and spoIIIAH genes lacking stop codons off template synthesized by Genscript. The spoIIQ expression construct deletes the sequence encoding the first 30 amino acids of SpoIIQ, while the spoIIIAH expression construct deletes the sequence encoding the first 33 amino acids of SpoIIIAH, which removes the membrane-tethering domains and improves the solubility of the proteins in E. coli. The resulting PCR products were digested with NdeI and XhoI, ligated to pET22b, and transformed into DH5α. The resulting pET22b-spoIIQ and pET22b-spoIIIAH plasmids were used to transform BL21(DE3) for protein expression.
To construct the pET28a-HA-spoIIIAH construct for the affinity co-purification studies, primer pair #1665 and 1614 was used on the codon-optimized spoIIIAH template synthesized by Genscript. To construct the pET28a-HA-spoVT construct for the affinity co-purification studies, primer pair #1691 and 1313 was used to amplify spoVT encoding an N-terminal HA-tag using C. difficile genomic DNA as the template. The resulting PCR products were digested with NcoI and XhoI, ligated to pET28a digested with the same enzymes, and transformed into DH5α. The pET28a-HA-spoIIIAH construct was transformed into BL21(DE3) to construct strain #1378. The pET28a-HA-spoIIIAH construct was transformed into BL21(DE3) to construct strain #1404.
To construct the σG-dependent transcriptional reporter, the σG-regulated promoter of sspA (PsspA) was fused to a C. difficile codon optimized SNAP-tag [75] to generate PsspA-SNAP (Genscript) with flanking restriction sites. This promoter region has previously been described [28]. The plasmid was transformed into E. coli DH5α, isolated, and digested with NotI and XhoI then cloned into the complementation plasmid pMTL84151, transformed into E. coli HB101 (S1 Table) and subsequently conjugated into C. difficile strains.
C. difficile strain construction
C. difficile strains were constructed using TargeTron-based gene disruption as described previously (S4 Fig, [27]). TargeTron constructs in pJS107 were conjugated into C. difficile using an E. coli HB101/pK424 donor strain. HB101/pK424 strains containing the appropriate pJS107 construct were grown aerobically to exponential phase in 2 mL of LB supplemented with ampicillin (50 μg/mL) and chloramphenicol (10 μg/mL). Cultures were pelleted, transferred into the anaerobic chamber, and resuspended in 1.5 mL of late-exponential phase C. difficile JIR8094 cultures (grown anaerobically in BHIS broth). The resulting cell mixture was plated as seven 100 μL spots onto pre-dried, pre-reduced BHIS agar plates. After overnight incubation, all growth was harvested from the BHIS plates, resuspended in 2.5 mL pre-reduced BHIS, and twenty-one 100 μL spots per strain were plated onto three BHIS agar plates supplemented with thiamphenicol (10 μg/mL), kanamycin (50 μg/mL), and cefoxitin (16 μg/mL) to select for C. difficile containing the pJS407 plasmid. After 24–48 hrs of anaerobic growth, single colonies were patched onto BHIS agar supplemented with thiamphenicol (10 μg/mL), kanamycin (50 μg/mL), and FeSO5 (50 μM) to induce the ferredoxin promoter of the group II intron system. After overnight growth, patches were transferred to BHIS agar plates supplemented with erythromycin (10 μg/mL) for 24–72 hrs to select for cells with activated group II intron systems. Erythromycin-resistant patches were struck out for isolation onto the same media and individual colonies were screened by colony PCR for a 2 kb increase in the size of spoIIQ (primer pair #1074 and 1075), spoIIIAA (primer pair #1302 and 1176), and spoIIIAH (primer pair #1301 and 1239) (S4 Fig).
C. difficile complementation
HB101/pK424 donor strains carrying the appropriate complementation construct were grown in LB containing ampicillin (50 μg/mL) and chloramphenicol (20 μg/mL) at 37°C, 225 rpm, under aerobic conditions, for 6 hrs. C. difficile recipient strains spoIIQ–, spoIIIAA–, and spoIIIAH−containing group II intron disruptions, were grown anaerobically in BHIS broth at 37°C with gentle shaking for 6 hrs. HB101/pK424 cultures were pelleted at 2500 rpm for 5 min and the supernatant was removed. Pellets were transferred to the anaerobic chamber and gently resuspended in 1.5 mL of the appropriate C. difficile culture. The resulting mixture was inoculated onto pre-dried, pre-reduced BHIS agar plates, as seven 100 μL spots for 12 hrs. All spots were collected anaerobically and resuspended in 1 mL PBS. The resulting suspension was spread onto pre-dried, pre-reduced BHIS agar plates supplemented with thiamphenicol (10 μg/mL), kanamycin (50 μg/mL), and cefoxitin (10 μg/mL) at 100 μL per plate, five plates per conjugation. Plates were monitored for colony growth for 24–72 hrs. Individual colonies were struck out for isolation and analyzed for complementation by phase contrast microscopy, Western blot analysis and transmission electron microscopy. A minimum of two independent clones from each complementation strain was phenotypically characterized.
For the SNAP-tag expression constructs, a pMTL84151 [44] or pMTL84121 [28] plasmid backbone was used. The complementation protocol was followed as described except that after spots were collected from overnight growth on BHIS plates, 100 μL of the resulting PBS suspension was spotted 7 times onto a BHIS agar plate supplemented with thiamphenicol (10 μg/mL), kanamycin (50 μg/mL), and cefoxitin (16 μg/mL). This procedure was repeated for three plates.
Sporulation assay
C. difficile strains were grown from glycerol stocks on BHIS plates supplemented with TA (0.1% w/v), or with both TA and thiamphenicol (5–10 μg/mL) for strains with pMTL83151-derived or pMTL84151-derived plasmids (as previously described [27]). Cultures grown on BHIS agar plates were then used to inoculate 70:30 agar plates (with thiamphenicol at 5–10 μg/mL as appropriate) for 17–24 hrs depending on the assay. Sporulation induced lawns were harvested in PBS, washed once, resuspended in PBS, visualized by phase contrast microscopy, and/or further processed for analysis by transmission electron microscopy, Western blotting, or fluorescence microscopy.
Heat resistance assay
C. difficile strains were induced to sporulate as described above, and cells were harvested in 1.0 mL PBS, and split into two tubes. One tube was heat shocked at 60–65°C for 25 minutes. Both heat-shocked and non-heat shocked cells were serially diluted, and cells were plated on pre-reduced BHIS-TA plates. After 20 hrs on BHIS-TA, colonies were counted, and cell counts were determined. The percent of heat-resistant spores was determined based on the ratio of heat-resistant cells to total cells, and sporulation efficiencies were determined based on the ratio of heat-resistant cells for a strain compared to wild type. Results are based on a minimum of three biological replicates.
Electron microscopy
One hundred microliters of bacterial cell suspension samples from sporulation assays were prepared as previously described [45].
Antibody production
The anti-SpoIIQ and anti-SpoIIIAH antibodies used in this study were raised in rabbits by Cocalico Biologicals (Reamstown, PA). The antigens SpoIIQ-His6 and SpoIIIAH-His6 were purified on Ni2+-affinity resin from E. coli strains #1301 and 1302 as described above. Cultures were grown and protein expression was analyzed as previously described [27].
Western blot analyses
Sporulation assay C. difficile cells (50 μL of PBS suspension) were freeze-thawed three times, diluted in 100 μL EBB buffer (8 M urea, 2 M thiourea, 4% (w/v) SDS, 2% (v/v) β-mercaptoethanol), and incubated at 95°C for 20 min with vortexing every 5 min. Samples were centrifuged for 5 min at 15,000 rpm, and 7 μL of 4X sample buffer (40% (v/v) glycerol, 1 M Tris pH 6.8, 20% (v/v) β-mercaptoethanol, 8% (w/v) SDS, and 0.04% (w/v) bromophenol blue), was added. Protein samples were incubated again at 95°C for 15 minutes with vortexing followed by centrifugation for 5 min at 15,000 rpm. SDS-PAGE gels (12%–15%) were loaded with 5 μL of the sample. Gels were transferred to Bio-Rad PVDF membrane and blocked in 50% PBS:50% Odyssey Blocking Buffer with 0.1% (v/v) Tween for 30 min at RT. Polyclonal rabbit anti-SpoVT ([27] anti-SpoIIQ and anti-SpoIIIAH, antibodies were used at a 1:1,000 dilution. Monoclonal mouse anti-Spo0A [27] was used at a 1:10,000 dilution. Monoclonal mouse anti-SNAP (NEB) was used at a 1:2,000 dilution. IRDye 680CW and 800CW infrared dye-conjugated secondary antibodies were used at a 1:20,000 dilutions. The Odyssey LiCor CLx was used to detect secondary antibody fluorescent emissions for Western blots.
RNA processing
RNA from WT, spo0A–, sigF–, spoIIQ–, sigE–, spoIIIA–, spoIIIAH–, and sigG−strains grown for 17 hrs on 70:30 sporulation media was extracted for qRT-PCR analyses of spoIIIAA transcript. RNA from WT, spo0A–, sigF–, spoIIQ–, sigE–, spoIIIA–, and sigG−strains grown for 25 hr on 70:30 sporulation media was extracted for qRT-PCR analyses of spoVT, CD1430, and spoVAD transcripts. RNA from WT/EV, spo0A–/EV, spoIIIAA–/EV, spoIIIA–/spoIIIA operon, and spoIIIA–/spoIIIAK167A operon complementation strains grown for 17 hr on 70:30 sporulation media was extracted for qRT-PCR analyses of spoIIIAA transcript. RNA was extracted using a FastRNA Pro Blue Kit (MP Biomedical) and a FastPrep-24 automated homogenizer (MP Biomedical). Contaminating genomic DNA was depleted using three successive DNase treatments and mRNA enrichment was done using an Ambion MICROBExpress Bacterial mRNA Enrichment Kit (Invitrogen). Samples were tested for genomic DNA contamination using quantitative PCR for rpoB. Enriched RNA was reverse transcribed using Super Script First Strand cDNA Synthesis Kit (Invitrogen) with random hexamer primers.
Quantitative RT-PCR
Transcript levels of spoIIIAA and rpoB (housekeeping gene) were determined from cDNA templates prepared from 3 biological replicates of WT, spo0A–, sigF–, spoIIQ–, sigE–, spoIIIA–, spoIIIAH–, and sigG−and three biological replicates of WT/EV, spo0A–/EV, spoIIIA–/EV, spoIIIA–/spoIIIA operon, and spoIIIA–/spoIIIAK167A operon. Gene-specific primer pairs for spoIIIAA and rpoB have been previously described [29,75]. Transcript levels of spoVT, CD1430, spoVAD, and rpoB were determined from cDNA templates prepared from three biological replicates of WT, spo0A–, sigE–, spoIIIA–, and sigG–. Transcript levels of CD1430 and spoVAD were analyzed using gene-specific primer pairs #1458 and 1459, #1708 and 1709, respectively. Gene-specific primers for measuring spoVT transcript levels have been previously described [27]. Quantitative real-time PCR was performed (as described by [75]). Briefly, using SYBR Green JumpStart Taq Ready Mix (Sigma), 50 nM of gene specific primers, and an ABI PRISM 7900HT Sequence Detection System (Applied Biosystems). Transcript levels were normalized to the housekeeping gene rpoB using the standard curve method and calculated relative to either the spo0A– strain or spo0A– strain carrying empty pMTL83151 vector.
SNAP-tag reporter construction
The CotE-SNAP previously described by Pereira et al. [28] was transformed into E. coli HB101/ pK424 and conjugated into the indicated C. difficile strains to analyze coat localization in spoIIQ and spoIIIA mutants.
C. difficile strains containing SNAP-tag reporters were grown on 70:30 media to induce sporulation. Cells were grown as a lawn for 21 hours on solid 70:30 media and harvested as described by Pereira et al. [28]. Briefly, cells were harvested in PBS and pelleted (4,000 rpm for 3 min), washed once with PBS, reconstituted in 100 μL of PBS. TMR-star SNAP substrate (NEB) was added to a final concentration of 3 μM to each tube and cells were incubated for 30 min at 37°C. Cells were pelleted, washed 3 times with PBS, and resuspended in PBS. Hoechst 33342 (10 mg/ml) was added to a final concentration of 15 μg/ml and FM4-64 (200 μg/ml) was added to a final concentration of 1 μg/mL.
Peptidoglycan labeling assay
Strains were harvested from 70:30 plates after 14 hours of growth as a bacterial lawn and re-suspended in 3 mL of 70:30 liquid media. For each strain used, the culture was split into 2 tubes for two conditions, each containing 1.5 mL of culture. Alkyne D-alanine or D-alanine (ACROS Organics) was added to each tube, respectively, at a final concentration of 2.5 mM and incubated at 37°C for 30 min. with mild shaking. After incubation, cells were pelleted (8000 rpm for 3 min.) and washed 3x with PBS. Cells were resuspended in 0.7 mL of 2% formaldehyde diluted in PBS and incubated for 10 min on the nutator. Cells were then pelleted and washed 2x with 1 mL PBS. Cells were incubated with 5 mg/mL lysozyme, 37°C, 45 min., pelleted, washed 2x with 1 mL PBS, and washed once with 3% BSA (in PBS). For the click chemistry reaction, a Click-iT Plus Alexa Fluor 488 Picolyl Azide Toolkit (Molecular Probes) was used according to the manufacturer’s instructions. After incubation with Click-iT reagents, samples were pelleted and washed 1x with 3% BSA and 1x with PBS. Samples were resuspended and Hoechst 33342 (10 mg/ml) was added to a final concentration of 15 μg/ml.
For the peptidoglycan labeling timecourse, cells were harvested into 5.5 ml of 70:30 broth after 14 hours of growth on 70:30 plates, and either alkyne D-alanine or D-alanine (ACROS Organics) was added to each tube. One mL samples of each culture was taken at every timepoint (0, 10, 20, 30, and 40 min) and processed as described above.
For evaluation of peptidoglycan labeling after treatment with antibiotics, 1 ml of WT cells in BHIS broth were harvested at late exponential phase for each treatment condition. 2X MIC of antibiotics (2 μg/ml vancomycin and 8 μg/ml imipenem) was added to designated cells and mixed with mild shaking. Dala and alkDala was added immediately after to designated cells and incubated for 30 minutes with mild shaking in the anaerobic chamber. Cells were processed for peptidoglycan labeling as described above.
Flow cytometry
The median fluorescent intensity (MFI) of alkDala incorporation was determined using a MACSQuant VYB flow cytometer. MACSQuantify software was used for data collection and FlowJo V.10.0.8 was used for data analysis. Cells that incorporated Hoechst dye 33342 (Molecular Probes) were evaluated for alkDala staining based on fluorescence in the FITC channel.
His6-tag pulldowns
E. coli BL21(DE3) strains were grown to mid-log phase in 2YT (5 g NaCl, 10 g yeast extract, and 15 g tryptone per liter), 225 rpm, at 37°C. 250 μM isopropyl-β-D-1-thiogalactopyranoside (IPTG) was added to induce the cells followed by an overnight incubation at 18°C. Cultures were pelleted, resuspended in low-imidazole buffer (500 mM NaCl, 50 mM Tris [pH 7.5], 15 mM imidazole, 10% [vol/vol] glycerol), and lysed by freeze-thawing and sonication. The insoluble material was pelleted, and the soluble fraction (Input) was batch affinity purified using Ni2+ affinity resin and eluted with high-imidazole buffer (500 mM NaCl, 50 mM Tris [pH 7.5], 150 mM imidazole, 10% [vol/vol] glycerol). The resulting eluates were run on SDS-PAGE gels (12%) and transferred onto a PVDF membrane for Western blot analysis, as described above.
Fluorescence microscopy
For live cell fluorescence microscopy studies, C. difficile strains were harvested in PBS, pelleted, and resuspended in PBS. For initial characterization of mutant phenotypes, cells were resuspended in PBS containing 1 μg/mL FM4-64 (Molecular Probes) and 15 μg/mL Hoechst 33342 (Molecular Probes). All live bacterial suspensions (4 μL) were added to a freshly prepared 1% agarose pad on a microscope slide, covered with a 22 x 22 mm #1 coverslip and sealed with VALAB (1:1:1 of vaseline, lanolin, and beeswax) as previously described [27].
DIC and fluorescence microscopy was performed using a Nikon PlanApo Vc 100x oil immersion objective (1.4 NA) on a Nikon Eclipse Ti2000 epifluorescence microscope. Multiple fields for each sample were acquired with an EXi Blue Mono camera (QImaging) with a hardware gain setting of 1.0 and driven by NIS-Elements software (Nikon). Images were subsequently imported into Adobe Photoshop CS6 for minimal adjustments in brightness/contrast levels and pseudocoloring.
DIC and fluorescence microscopy for cells that were processed for peptidoglycan labeling experiments were performed and processed with the same equipment as described above with the following differences: a Nikon PlanApo Vc 60x oil immersion objective (1.4 NA) was utilized, hardware gain setting 2.0, and fields were imaged with Z-spacing of 0.15 μm followed by deconvolution using AutoQuant 3x software (MediaCybernetics).
Quantification of total cells undergoing sporulation was determined by analyzing multiple fields for each strain at random. At least 50 cells were enumerated for each strain. Sporulating cells were identified as either having a polar septum with or without DNA staining in the forespore, a DIC-dark forespore with or without DNA staining in the forespore compartment, a DIC-bright forespore without DNA staining, or a free spore (no mother cell compartment).
Supporting Information
Zdroje
1. Higgins D, Dworkin J (2012) Recent progress in Bacillus subtilis sporulation. FEMS Microbiol Rev 36: 131–148. doi: 10.1111/j.1574-6976.2011.00310.x 22091839
2. McKenney PT, Driks A, Eichenberger P (2012) The Bacillus subtilis endospore: assembly and functions of the multilayered coat. Nat Rev Microbiol. doi: 10.1038/nrmicro2921 23202530
3. Tan IS, Ramamurthi KS (2014) Spore formation in Bacillus subtilis. Environ Microbiol Rep 6: 212–225. doi: 10.1111/1758-2229.12130 24983526
4. Setlow P (2006) Spores of Bacillus subtilis: their resistance to and killing by radiation, heat and chemicals. Journal of applied microbiology 101: 514–525. 16907802
5. Angert ER, Losick RM (1998) Propagation by sporulation in the guinea pig symbiont Metabacterium polyspora. Proc Natl Acad Sci U S A 95: 10218–10223. 9707627
6. Deakin LJ, Clare S, Fagan RP, Dawson LF, Pickard DJ, et al. (2012) The Clostridium difficile spo0A gene is a persistence and transmission factor. Infect Immun 80: 2704–2711. doi: 10.1128/IAI.00147-12 22615253
7. Carroll K, Bartlett J (2011) Biology of Clostridium difficile: implications for epidemiology and diagnosis. Annual review of microbiology 65: 501–521. doi: 10.1146/annurev-micro-090110-102824 21682645
8. Eyre DW, Wilcox MH, Walker AS (2014) Diverse sources of C. difficile infection. N Engl J Med 370: 183–184. doi: 10.1056/NEJMc1313601 24401066
9. Gupta A, Khanna S (2014) Community-acquired Clostridium difficile infection: an increasing public health threat. Infect Drug Resist 7: 63–72. doi: 10.2147/IDR.S46780 24669194
10. Rupnik M, Wilcox M, Gerding D (2009) Clostridium difficile infection: new developments in epidemiology and pathogenesis. Nature reviews Microbiology 7: 526–536. doi: 10.1038/nrmicro2164 19528959
11. Howerton A, Patra M, Abel-Santos E (2013) Fate of ingested Clostridium difficile spores in mice. PLoS One 8: e72620. doi: 10.1371/journal.pone.0072620 24023628
12. Seekatz AM, Young VB (2014) Clostridium difficile and the microbiota. J Clin Invest 124: 4182–4189. doi: 10.1172/JCI72336 25036699
13. Janoir C, Deneve C, Bouttier S, Barbut F, Hoys S, et al. (2013) Adaptive strategies and pathogenesis of Clostridium difficile from in vivo transcriptomics. Infect Immun 81: 3757–3769. doi: 10.1128/IAI.00515-13 23897605
14. Johnson S (2009) Recurrent Clostridium difficile infection: a review of risk factors, treatments, and outcomes. J Infect 58: 403–410. doi: 10.1016/j.jinf.2009.03.010 19394704
15. Maroo S, Lamont J (2006) Recurrent Clostridium difficile. Gastroenterology 130: 1311–1316. 16618421
16. Kelly C (2012) Can we identify patients at high risk of recurrent Clostridium difficile infection? Clinical microbiology and infection: the official publication of the European Society of Clinical Microbiology and Infectious Diseases 18 Suppl 6: 21–27.
17. Fimlaid KA, Shen A (2015) Diverse Mechanisms Regulate Sporulation Sigma Factor Activity in the Firmicutes. Current Opinion in Microbiology. doi: 10.1016/j.mib.2015.01.006 25646759
18. Henriques AO, Moran CP Jr. (2007) Structure, assembly, and function of the spore surface layers. Annu Rev Microbiol 61: 555–588. 18035610
19. Camp AH, Losick R (2009) A feeding tube model for activation of a cell-specific transcription factor during sporulation in Bacillus subtilis. Genes Dev 23: 1014–1024. doi: 10.1101/gad.1781709 19390092
20. Doan T, Morlot C, Meisner J, Serrano M, Henriques A, et al. (2009) Novel secretion apparatus maintains spore integrity and developmental gene expression in Bacillus subtilis. PLoS genetics 5. doi: 10.1371/journal.pgen.1000566 19609349
21. Meisner J, Wang X, Serrano M, Henriques A, Moran C (2008) A channel connecting the mother cell and forespore during bacterial endospore formation. Proceedings of the National Academy of Sciences of the United States of America 105: 15100–15105. doi: 10.1073/pnas.0806301105 18812514
22. Sun YL, Sharp MD, Pogliano K (2000) A dispensable role for forespore-specific gene expression in engulfment of the forespore during sporulation of Bacillus subtilis. J Bacteriol 182: 2919–2927. 10781563
23. Regan G, Itaya M, Piggot P (2012) Coupling of σG Activation to Completion of Engulfment during Sporulation of Bacillus subtilis Survives Large Perturbations to DNA Translocation and Replication. Journal of bacteriology 194: 6264–6271. doi: 10.1128/JB.01470-12 22984259
24. Rudner DZ, Losick R (2001) Morphological coupling in development: lessons from prokaryotes. Dev Cell 1: 733–742. 11740935
25. Partridge SR, Errington J (1993) The importance of morphological events and intercellular interactions in the regulation of prespore-specific gene expression during sporulation in Bacillus subtilis. Mol Microbiol 8: 945–955. 8355618
26. Saujet L, Pereira FC, Henriques AO, Martin-Verstraete I (2014) The regulatory network controlling spore formation in Clostridium difficile. FEMS Microbiol Lett 358: 1–10. doi: 10.1111/1574-6968.12540 25048412
27. Fimlaid KA, Bond JP, Schutz KC, Putnam EE, Leung JM, et al. (2013) Global Analysis of the Sporulation Pathway of Clostridium difficile. PLoS Genet 9: e1003660. doi: 10.1371/journal.pgen.1003660 23950727
28. Pereira FC, Saujet L, Tome AR, Serrano M, Monot M, et al. (2013) The Spore Differentiation Pathway in the Enteric Pathogen Clostridium difficile. PLoS Genet 9: e1003782. doi: 10.1371/journal.pgen.1003782 24098139
29. Saujet L, Pereira FC, Serrano M, Soutourina O, Monot M, et al. (2013) Genome-wide analysis of cell type-specific gene transcription during spore formation in Clostridium difficile. PLoS Genet 9: e1003756. doi: 10.1371/journal.pgen.1003756 24098137
30. Crawshaw AD, Serrano M, Stanley WA, Henriques AO, Salgado PS (2014) A mother cell-to-forespore channel: current understanding and future challenges. FEMS Microbiol Lett 358: 129–136. doi: 10.1111/1574-6968.12554 25105965
31. Abecasis AB, Serrano M, Alves R, Quintais L, Pereira-Leal JB, et al. (2013) A genomic signature and the identification of new sporulation genes. J Bacteriol 195: 2101–2115. doi: 10.1128/JB.02110-12 23396918
32. Galperin MY, Mekhedov SL, Puigbo P, Smirnov S, Wolf YI, et al. (2012) Genomic determinants of sporulation in Bacilli and Clostridia: towards the minimal set of sporulation-specific genes. Environ Microbiol 14: 2870–2890. doi: 10.1111/j.1462-2920.2012.02841.x 22882546
33. Londono-Vallejo JA, Frehel C, Stragier P (1997) SpoIIQ, a forespore-expressed gene required for engulfment in Bacillus subtilis. Mol Microbiol 24: 29–39. 9140963
34. Meisner J, Moran CP Jr. (2011) A LytM domain dictates the localization of proteins to the mother cell-forespore interface during bacterial endospore formation. J Bacteriol 193: 591–598. doi: 10.1128/JB.01270-10 21097616
35. Blaylock B, Jiang X, Rubio A, Moran CP Jr., Pogliano K (2004) Zipper-like interaction between proteins in adjacent daughter cells mediates protein localization. Genes Dev 18: 2916–2928. 15574594
36. Rubio A, Pogliano K (2004) Septal localization of forespore membrane proteins during engulfment in Bacillus subtilis. EMBO J 23: 1636–1646. 15044948
37. Levdikov VM, Blagova EV, McFeat A, Fogg MJ, Wilson KS, et al. (2012) Structure of components of an intercellular channel complex in sporulating Bacillus subtilis. Proc Natl Acad Sci U S A 109: 5441–5445. doi: 10.1073/pnas.1120087109 22431604
38. Meisner J, Maehigashi T, Andre I, Dunham CM, Moran CP Jr. (2012) Structure of the basal components of a bacterial transporter. Proc Natl Acad Sci U S A 109: 5446–5451. doi: 10.1073/pnas.1120113109 22431613
39. Illing N, Errington J (1991) The spoIIIA operon of Bacillus subtilis defines a new temporal class of mother-cell-specific sporulation genes under the control of the sigma E form of RNA polymerase. Mol Microbiol 5: 1927–1940. 1766372
40. Camp AH, Losick R (2008) A novel pathway of intercellular signalling in Bacillus subtilis involves a protein with similarity to a component of type III secretion channels. Mol Microbiol 69: 402–417. doi: 10.1111/j.1365-2958.2008.06289.x 18485064
41. Broder DH, Pogliano K (2006) Forespore engulfment mediated by a ratchet-like mechanism. Cell 126: 917–928. 16959571
42. Heap J, Kuehne S, Ehsaan M, Cartman S, Cooksley C, et al. (2010) The ClosTron: Mutagenesis in Clostridium refined and streamlined. Journal of microbiological methods 80: 49–55. doi: 10.1016/j.mimet.2009.10.018 19891996
43. Guillot C, Moran CP Jr. (2007) Essential internal promoter in the spoIIIA locus of Bacillus subtilis. J Bacteriol 189: 7181–7189. 17693505
44. Heap J, Pennington O, Cartman S, Minton N (2009) A modular system for Clostridium shuttle plasmids. Journal of microbiological methods 78: 79–85. doi: 10.1016/j.mimet.2009.05.004 19445976
45. Putnam EE, Nock AM, Lawley TD, Shen A (2013) SpoIVA and SipL are Clostridium difficile spore morphogenetic proteins. J Bacteriol 195: 1214–1225. doi: 10.1128/JB.02181-12 23292781
46. Permpoonpattana P, Phetcharaburanin J, Mikelsone A, Dembek M, Tan S, et al. (2013) Functional characterization of Clostridium difficile spore coat proteins. Journal of bacteriology 195: 1492–1503. doi: 10.1128/JB.02104-12 23335421
47. Permpoonpattana P, Tolls E, Nadem R, Tan S, Brisson A, et al. (2011) Surface layers of Clostridium difficile endospores. Journal of bacteriology 193: 6461–6470. doi: 10.1128/JB.05182-11 21949071
48. Firczuk M, Bochtler M (2007) Folds and activities of peptidoglycan amidases. FEMS Microbiol Rev 31: 676–691. 17888003
49. Walker JE, Saraste M, Runswick MJ, Gay NJ (1982) Distantly related sequences in the alpha- and beta-subunits of ATP synthase, myosin, kinases and other ATP-requiring enzymes and a common nucleotide binding fold. EMBO J 1: 945–951. 6329717
50. Story RM, Steitz TA (1992) Structure of the recA protein-ADP complex. Nature 355: 374–376. 1731253
51. Bell CE (2005) Structure and mechanism of Escherichia coli RecA ATPase. Mol Microbiol 58: 358–366. 16194225
52. Castaing J-P, Nagy A, Anantharaman V, Aravind L, Ramamurthi K (2013) ATP hydrolysis by a domain related to translation factor GTPases drives polymerization of a static bacterial morphogenetic protein. Proceedings of the National Academy of Sciences of the United States of America 110: 60.
53. Gutierrez J, Smith R, Pogliano K (2010) SpoIID-mediated peptidoglycan degradation is required throughout engulfment during Bacillus subtilis sporulation. J Bacteriol 192: 3174–3186. doi: 10.1128/JB.00127-10 20382772
54. Meyer P, Gutierrez J, Pogliano K, Dworkin J (2010) Cell wall synthesis is necessary for membrane dynamics during sporulation of Bacillus subtilis. Mol Microbiol 76: 956–970. doi: 10.1111/j.1365-2958.2010.07155.x 20444098
55. Morlot C, Uehara T, Marquis KA, Bernhardt TG, Rudner DZ (2010) A highly coordinated cell wall degradation machine governs spore morphogenesis in Bacillus subtilis. Genes Dev 24: 411–422. doi: 10.1101/gad.1878110 20159959
56. Sogaard-Andersen L (2013) Stably bridging a great divide: localization of the SpoIIQ landmark protein in Bacillus subtilis. Mol Microbiol 89: 1019–1024. doi: 10.1111/mmi.12365 23944268
57. Turner RD, Vollmer W, Foster SJ (2014) Different walls for rods and balls: the diversity of peptidoglycan. Mol Microbiol 91: 862–874. doi: 10.1111/mmi.12513 24405365
58. Kuru E, Hughes HV, Brown PJ, Hall E, Tekkam S, et al. (2012) In Situ probing of newly synthesized peptidoglycan in live bacteria with fluorescent D-amino acids. Angew Chem Int Ed Engl 51: 12519–12523. doi: 10.1002/anie.201206749 23055266
59. Siegrist MS, Whiteside S, Jewett JC, Aditham A, Cava F, et al. (2013) (D)-Amino acid chemical reporters reveal peptidoglycan dynamics of an intracellular pathogen. ACS Chem Biol 8: 500–505. doi: 10.1021/cb3004995 23240806
60. Breinbauer R, Kohn M (2003) Azide-alkyne coupling: a powerful reaction for bioconjugate chemistry. Chembiochem 4: 1147–1149. 14613105
61. Pogliano J, Osborne N, Sharp MD, Abanes-De Mello A, Perez A, et al. (1999) A vital stain for studying membrane dynamics in bacteria: a novel mechanism controlling septation during Bacillus subtilis sporulation. Mol Microbiol 31: 1149–1159. 10096082
62. Sharp MD, Pogliano K (1999) An in vivo membrane fusion assay implicates SpoIIIE in the final stages of engulfment during Bacillus subtilis sporulation. Proc Natl Acad Sci U S A 96: 14553–14558. 10588743
63. Courvalin P (2006) Vancomycin resistance in gram-positive cocci. Clin Infect Dis 42 Suppl 1: S25–34. 16323116
64. Rodloff AC, Goldstein EJ, Torres A (2006) Two decades of imipenem therapy. J Antimicrob Chemother 58: 916–929. 16997845
65. Tocheva EI, Lopez-Garrido J, Hughes HV, Fredlund J, Kuru E, et al. (2013) Peptidoglycan transformations during Bacillus subtilis sporulation. Mol Microbiol 88: 673–686. doi: 10.1111/mmi.12201 23531131
66. Sun DX, Cabrera-Martinez RM, Setlow P (1991) Control of transcription of the Bacillus subtilis spoIIIG gene, which codes for the forespore-specific transcription factor sigma G. J Bacteriol 173: 2977–2984. 1902213
67. Sterlini JM, Mandelstam J (1969) Commitment to sporulation in Bacillus subtilis and its relationship to development of actinomycin resistance. Biochem J 113: 29–37. 4185146
68. Ojkic N, Lopez-Garrido J, Pogliano K, Endres RG (2014) Bistable forespore engulfment in Bacillus subtilis by a zipper mechanism in absence of the cell wall. PLoS Comput Biol 10: e1003912. doi: 10.1371/journal.pcbi.1003912 25356555
69. McKenney PT, Eichenberger P (2012) Dynamics of spore coat morphogenesis in Bacillus subtilis. Mol Microbiol 83: 245–260. doi: 10.1111/j.1365-2958.2011.07936.x 22171814
70. O'Connor J, Lyras D, Farrow K, Adams V, Powell D, et al. (2006) Construction and analysis of chromosomal Clostridium difficile mutants. Molecular microbiology 61: 1335–1351. 16925561
71. Sebaihia M, Wren B, Mullany P, Fairweather N, Minton N, et al. (2006) The multidrug-resistant human pathogen Clostridium difficile has a highly mobile, mosaic genome. Nature genetics 38: 779–786. 16804543
72. Sorg JA, Dineen SS (2009) Laboratory maintenance of Clostridium difficile. Curr Protoc Microbiol Chapter 9: Unit 9A 1.
73. Wilson KH, Kennedy MJ, Fekety FR (1982) Use of sodium taurocholate to enhance spore recovery on a medium selective for Clostridium difficile. J Clin Microbiol 15: 443–446. 7076817
74. Horton R, Hunt H, Ho S, Pullen J, Pease L (1989) Engineering hybrid genes without the use of restriction enzymes: gene splicing by overlap extension. Gene 77: 61–68. 2744488
75. Pishdadian K, Fimlaid KA, Shen A (2014) SpoIIID-mediated regulation of sigma function during Clostridium difficile sporulation. Mol Microbiol.
76. Pishdadian K, Fimlaid KA, Shen A (2015) SpoIIID-mediated regulation of sigma(K) function during Clostridium difficile sporulation. Mol Microbiol 95: 189–208. doi: 10.1111/mmi.12856 25393584
77. Doan T, Coleman J, Marquis KA, Meeske AJ, Burton BM, et al. (2013) FisB mediates membrane fission during sporulation in Bacillus subtilis. Genes Dev 27: 322–334. doi: 10.1101/gad.209049.112 23388828
78. Yutin N, Galperin MY (2013) A genomic update on clostridial phylogeny: Gram-negative spore formers and other misplaced clostridia. Environ Microbiol 15: 2631–2641. doi: 10.1111/1462-2920.12173 23834245
79. Finn RD, Clements J, Eddy SR (2011) HMMER web server: interactive sequence similarity searching. Nucleic Acids Res 39: W29–37. doi: 10.1093/nar/gkr367 21593126
Štítky
Genetika Reprodukční medicínaČlánek vyšel v časopise
PLOS Genetics
2015 Číslo 10
Nejčtenější v tomto čísle
- Single Strand Annealing Plays a Major Role in RecA-Independent Recombination between Repeated Sequences in the Radioresistant Bacterium
- The Rise and Fall of an Evolutionary Innovation: Contrasting Strategies of Venom Evolution in Ancient and Young Animals
- Genome Wide Identification of SARS-CoV Susceptibility Loci Using the Collaborative Cross
- DCA1 Acts as a Transcriptional Co-activator of DST and Contributes to Drought and Salt Tolerance in Rice