Streptococcus agalactiae is a major neonatal pathogen whose infectious route involves septicemia. This pathogen does not synthesize heme, but scavenges it from blood to activate a respiration metabolism, which increases bacterial cell density and is required for full virulence. Factors that regulate heme pools in S. agalactiae are unknown. Here we report that one main strategy of heme and protoporphyrin IX (PPIX) homeostasis in S. agalactiae is based on a regulated system of efflux using two newly characterized operons, gbs1753 gbs1752 (called pefA pefB), and gbs1402 gbs1401 gbs1400 (called pefR pefC pefD), where pef stands for ‘porphyrin-regulated efflux’. In vitro and in vivo data show that PefR, a MarR-superfamily protein, is a repressor of both operons. Heme or PPIX both alleviate PefR-mediated repression. We show that bacteria inactivated for both Pef efflux systems display accrued sensitivity to these porphyrins, and give evidence that they accumulate intracellularly. The ΔpefR mutant, in which both pef operons are up-regulated, is defective for heme-dependent respiration, and attenuated for virulence. We conclude that this new efflux regulon controls intracellular heme and PPIX availability in S. agalactiae, and is needed for its capacity to undergo respiration metabolism, and to infect the host.
The infectious route of numerous bacterial pathogens includes septicemia, where bacteria are exposed to heme-rich blood. Heme (iron protoporphyrin IX) is generally considered a bacterial iron source. However, while some pathogens do not biosynthesize heme, they use environmental heme to activate key functions. For example, incorporation of heme by the major neonatal pathogen Streptococcus agalactiae activates a latent respiration chain. Respiration metabolism stimulates S. agalactiae growth and survival in blood, and is needed for virulence. While the importance of heme in S. agalactiae behavior is documented, how it manages its intracellular heme pools remains unknown. We discovered a novel regulon, called Pef for “porphyrin-regulated efflux”, that modulates S. agalactiae intracellular availability of heme and protoporphyrin IX. A single transcriptional regulator, PefR, represses two distinct efflux transport operons. Regulator-mediated repression is alleviated by heme or protoporphyrin IX. Importantly, over-expression of Pef efflux transporters led to intracellular heme insufficiency, and consequent respiration and virulence defects. Inversely, when Pef efflux transporters were inactivated, results indicated an increased intracellular accumulation of heme and protoporphyrin IX. These studies point to the important role of regulated efflux transport systems in bacterial pathogens for maintaining intracellular heme at levels sufficient to stimulate growth and promote infection.
Citation: Fernandez A, Lechardeur D, Derré-Bobillot A, Couvé E, Gaudu P, Gruss A (2010) Two Coregulated Efflux Transporters Modulate Intracellular Heme and Protoporphyrin IX Availability in Streptococcus agalactiae. PLoS Pathog 6(4): e1000860. https://doi.org/10.1371/journal.ppat.1000860
Editor: Michael R. Wessels, Children's Hospital Boston, United States of America
Received: November 23, 2009; Accepted: March 16, 2010; Published: April 22, 2010
Copyright: © 2010 Fernandez et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: Research was funded by the Institut National de la Recherche Agronomique, and a grant, for the StrepRespire project, from the French research agency ‘Agence Nationale de la Recherche’. A.F. was a recipient of a post-doctoral fellowship from the ANR StrepRespire Project. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Heme (iron protoporphyrin IX) is a redox-active molecule, and a cofactor for numerous cell functions used in oxygen sensing and signal transmission, metabolism, and metal homeostasis ,[–],. In addition to its varied activities as a cofactor, heme promotes toxic oxygen radical production . The duality between heme as a multifunctional cofactor, and a potentially toxic molecule, suggests the need for strict limitation of its intracellular levels. Metal-free protoporphyrin IX (PPIX) is also found intracellularly, as a heme precursor in bacteria that synthesize heme, and as an intermediate during iron recovery from heme, as shown in Escherichia coli . Thus, cells might have to deal with both heme and PPIX intracellular pools.
While most studied organisms synthesize heme to ensure activity of hemoproteins under the appropriate conditions, numerous bacteria lack heme biosynthesis genes, making heme-catalyzed processes fully dependent upon external heme supplies. For example, Haemophilus influenzae, Bacteroides sp., and several Firmicutes, including Lactococcus lactis, Enterococcus faecalis, Streptococcus agalactiae, and numerous Lactobacillus sp., require heme to activate a respiration metabolic pathway ,. Some of these bacteria (e.g., H. influenzae, E. faecalis, Bacteroides sp., Lactobacillus brevis and Lactobacillus plantarum) also encode heme-dependent catalases, which rely on exogenous heme for both their stability and activity . Thus, heme supplied by the environment can have a determining effect on the metabolic and enzymatic capacities in organisms lacking the heme biosynthetic pathway.
All bacteria, regardless of their heme biosynthesis capacities, need to manage their intracellular heme pools. Regulation may be exerted at the levels of biosynthesis, uptake, degradation, and possibly efflux, which is in some cases coordinated with the cell iron status ,. The use of efflux as a means of heme homeostasis remains in question. The sole candidate, HrtAB, a heme-regulated transporter, was first reported as having a role in heme toxicity in Staphylococcus aureus; orthologs of this system were also described in L. lactis and Bacillus anthracis , ,[–],. HrtAB in S. aureus, B. anthracis, and likely several Gram-positive pathogens responds to an extracytoplasmic heme sensor, HssS (part of HssSR two-component system) to activate expression , .
S. agalactiae is an important human pathogen that does not synthesize its own heme. Nevertheless, infection by this bacterium involves compulsory passage through the bloodstream, causing septicemia and subsequent meningitis , . We showed previously that although S. agalactiae generally grows by a fermentation metabolism, it can also use heme, present in blood, to activate the terminal cytochrome bd quinol oxidase for respiration metabolism. Thus, beyond the potential use of heme uptake to acquire iron, the use of heme to activate the energetically favorable respiration metabolism confers a significant gain in cell density, and is required for full bacterial virulence in a septicemia model , .
Despite the importance of growth in heme-rich blood as an initial step of S. agalactiae infection, the functions involved in regulating intracellular heme levels are unknown. Homologs of HrtAB and HssSR exist in S. agalactiae, and might participate in modulating heme toxicity upon sensing of extracellular heme. However, the mechanism by which HrtAB modulates heme toxicity is unknown, and the question remains whether other systems are needed to regulate heme pools. Here we report the existence of a novel regulon comprising two efflux operons and a single repressor that senses intracellular heme and PPIX, and is needed to maintain their homeostasis. This newly described system is shown to impact on S. agalactiae respiration capacity and virulence.
Identification of gbs1753 gbs1752 as a putative heme- and PPIX- induced locus in S. agalactiae
Transcriptome studies, comparing S. agalactiae gene expression under respiration (i.e., aerobic growth in the presence of exogenous heme and menaquinone) versus aerobic fermentation (i.e., no addition) conditions, initially revealed that gbs1753 gbs1752 was 2.4 to 5.1 fold higher under respiration conditions (AD, PG, EC, and P. Glaser [Pasteur Institute]; Table S1). The gbs1753 ORF encodes an integral membrane protein of the drug:H+ antiporter family, belonging to the major facilitator superfamily (MFS) . The gbs1752 ORF encodes an unknown protein with 2 transmembrane domains. We chose this locus for study, as it was conserved among Gram-positive bacteria that lack a complete heme biosynthesis pathway, but encode cytochrome bd quinol oxidases, indicating a capacity for respiration metabolism (Fig. 1 and Table S2).
A, gbs1753 gbs1752 (pefA pefB) and B, gbs1402 gbs1401 gbs1400 (pefR pefC pefD) loci. Bent arrows and lollipops indicate the mapped or putative promoters, and rho-independent terminators, respectively.
The +1 transcriptional start of gbs1753 gbs1752 was located by 5′-RACE PCR mapping at 134 nucleotides upstream of the gbs1753 start codon at a cytosine (Fig. 2A). The gbs1753 promoter region was fused to a lacZ reporter, referred to as Pgbs1753-lacZ, and expressed on a low copy number plasmid (Fig. 2A) . In the absence of added heme, Pgbs1753-lacZ displayed basal level expression in static and aerobic growth conditions (possibly reflecting trace amounts of heme in BHI medium). Cultures grown with added heme (from 0.1 µM to 10 µM) displayed up to 9-fold higher Pgbs1753-lacZ expression compared to controls without heme, even in non-respiration-permissive conditions (Fig. 2B), indicating that heme, and not the state of respiration, was the inducing factor for the gbs1753 promoter. Significant Pgbs1753-lacZ induction was observed at heme concentrations of 0.3 µM and above. Similarly, PPIX, gallium protoporphyrin (GaPPIX), and zinc mesoporphyrin (ZnMPIX) also induced Pgbs1753-lacZ, while free iron had no inducing effect. These initial results indicate that gbs1753 expression is induced by different porphyrin molecules, regardless of their metal core status.
A. Schematic map of the transcriptional fusion PpefA-lacZ (same as Pgbs1753-lacZ). Sequence of the pefAB promoter region is displayed. The +1 transcriptional start and −10 and −35 motifs are in bold blue characters. B. Expression analysis of PpefA-lacZ by determination of β-galactosidase activity in early stationary phase. S. agalactiae was grown in BHI liquid medium in the presence of the indicated amount of candidate inducers. Strains harboring the pTCV-lac vector (promoterless negative control) did not show β-galactosidase activity during growth (0.4±0.1 Miller Units). Measurements were performed at least three times.
Identification of Gbs1402 as a putative regulator of gbs1753 gbs1752 expression
A random mutagenesis approach was used to identify genetic factors that affect gbs1753 gbs1752 expression. A transposon-generated mutant library was screened for clones in which expression of the Pgbs1753-lacZ fusion was up-regulated, as detected by deep blue colony color. Several mutations mapped in a single ORF, gbs1402. The gbs1402 gene encodes a multiple antibiotic resistance MarR-like regulator (for review see ), and is located just upstream of gbs1401 gbs1400, encoding a putative ABC-type multidrug transport complex (Fig. 1B). Sequence analysis predicted that the Gbs1401 and Gbs1400 proteins both contain a transmembrane domain and an ATPase signature. These observations led us to formulate a working hypothesis that both gbs1753 gbs1752 and gbs1401 gbs1400 loci are involved in PPIX and metalloporphyrin efflux, and are regulated by a single protein, Gbs1402. The genes were renamed as pef genes, for porphyrin-regulated efflux. gbs1753 gbs1752 are renamed pefA pefB; gbs1401 gbs1400 are renamed pefC pefD; and the gbs1402 gene for the potential regulator is renamed pefR (Fig. 1).
PefR binds specifically to pefAB and pefRCD promoter regions and represses their transcription
Proteins of the MarR family characteristically bind to DNA inverted repeat motifs (IR) . Sequence analysis revealed the presence of a near-perfect 18-nucleotide IR within a 23 bp consensus, (5′-TAAAATAGTTCTCACGATAACTA-3′) present once upstream of pefA pefB, and twice (one identical sequence, and one inexact copy with 3 nucleotide substitutions in italics) upstream of pefR pefC pefD (Fig. 3A). The IR is not present elsewhere on the S. agalactiae genome. This 23-nucleotide sequence contains the −10 region (TAAAAT) of a putative promoter and constituted a candidate target site for PefR binding to pefAB and pefRCD promoter regions. Mobility shift assays were performed using a purified PefR His-fusion protein, in combination with DNA fragments comprising the IRs of pefAB or pefRCD promoter regions, plus a fragment without an IR as negative internal control (Fig. 3B). PefR caused a mobility shift of both the pefAB and pefRCD fragments in a protein concentration-dependent manner. No shift was observed with the control DNA fragment.
A. A conserved 23-nucleotide motif is present once upstream of pefAB, and twice upstream of pefRCD and is highlighted. The IR present in each of the motifs is marked by arrows. The −10 and −35 motifs, and the mRNA pefAB and putative pefRCD start sites are in blue. Start codons and RBS sequence are in italics. One motif upstream of pefRCD (dotted arrows) differs from the other motifs by 3 nucleotides, which are in gray italics. B. PefR binds the pefAB and pefRCD promoter regions in gel shift assays. Two pmoles of pefAB or pefRCD promoter fragment were incubated in the presence of 0, 4, 17, 34, 63 pmoles of PefR (lanes 1 to 5) and 4.6 pmoles control fragment, corresponding to an 116-bp fragment of the pefA gene. C. Northern blot analyses of pefAB and pefRCD mRNA in the WT and pefR strains, using locus-specific probes (see Materials and Methods). As probe efficiencies and times of exposure differ for each target RNA, differences between pefAB and pefRCD levels are not comparable. ldhL mRNA (‘ctrl’) was used to control for RNA quantity.
To determine whether PefR impacts on pefA pefB and pefR pefC pefD expression in vivo, Northern blot experiments were performed on the WT strain and an in-frame ΔpefR mutant, using pefAB and pefC as probes (Fig. 3C). The deduced transcript sizes were compatible with organization of the pefA and pefB genes as one operon, and of pefR, pefC, and pefD genes as another. Compared to the WT strain, expression of both pefAB and pefRCD operons was strongly increased in the ΔpefR mutant. We also evaluated expression of the PpefA-lacZ transcriptional fusion in the WT and ΔpefR mutant strains. β-galactosidase expression in the ΔpefR background was 12 times higher than in the WT strain (Miller Units were 62.9±9.2 in ΔpefR versus 5.1±1.7 in the WT strain).
The above in vitro and in vivo results indicate that PefR is a transcriptional repressor of both the pefAB and the pefRCD operons, by binding directly to the operator regions.
PefR is an intracellular heme and PPIX sensor and regulator of pef expression
A characteristic of MarR family regulators is their binding to effector molecules, which leads to induction or repression of their target genes –. Transcriptional fusions showed that the pefAB operon was induced in the presence of metalloporphyrins or PPIX (Fig. 2B). As PefR binds the two pef promoter regions, and appears to repress transcription, we hypothesized that PefR binding and repression are modulated by heme and PPIX. To test this in vitro, mobility shift assays between PefR and the pefAB or pefRCD promoter region DNA fragments were performed with and without heme or PPIX. For both DNA targets, PefR–DNA binding was alleviated in a heme or PPIX concentration-dependent manner (Fig. 4A, Fig. S1A). Iron had no effect on PefR-DNA binding (Fig. S1B).
A. Gel mobility shift analysis of the effect of heme on PefR binding to pefAB (right) and pefRCD (left) promoter regions. 2 pmoles of PpefAB or PpefRCD fragments and 30 pmoles of PefR were mixed. Increased concentrations of heme were added in ratios indicated (keeping PefR constant). Assays were also performed with PPIX (Fig. S1A), giving similar results. On the two top panels, lanes 1–3 were juxtaposed to lanes 4–5, which were separated on the initial same gel. B. Northern blot analyses of pefAB and pefRCD expression in the presence of heme or PPIX in WT NEM316. Cultures were grown in the presence of 0, 1, 5 and 10 µM heme or PPIX, and harvested for total RNA extraction in early stationary phase. As probe efficiencies and times of exposure differ for each target RNA, differences between pefAB and pefRCD levels are not comparable. ldhL (gbs0947; ‘ctrl’) mRNA was used to control for RNA quantities.
Transcriptional fusion data showed that heme and PPIX up-regulate pefAB expression. To further confirm these results, we performed Northern blot experiments in the absence and presence of these molecules, using pefAB and pefC DNA as probes. Both heme and PPIX induced expression of the two pef operons (Fig. 4B). These in vivo results are in keeping with in vitro gel shift data showing that PefR repression is alleviated in the presence of these porphyrins. We conclude that heme and PPIX both modulate PefR repression of the pefAB and pefRCD operons.
Expression of hrtAB as a function of heme and PPIX levels in S. agalactiae
Genomic studies of S. agalactiae revealed the existence of an analog of HrtAB, a heme-regulated transport system initially characterized in S. aureus and shown to be involved in heme toxicity . Gbs0119 and Gbs0120 showed 45% and 29% identity with HrtB and HrtA of S. aureus respectively. We used Northern blot experiments (Fig. 5A) and a lacZ promoter fusion, Pgbs0119-lacZ (Fig. 5B), to assess the heme and PPIX concentrations needed to induce the hrtAB locus. Interestingly, hrtAB expression was low at heme concentrations below 1 µM, with strong induction at 10 µM; PPIX did not induce its expression, as was observed in S. aureus. Importantly, no hrtAB induction was observed at heme levels where pefAB was induced, i.e., between 0.1 and 0.5 µM heme (Fig. 2B). We conclude that the pef regulon is induced at heme concentrations below those needed for hrtAB induction, indicating that these functions are active under different conditions.
A. Northern blot analyses of gbs0119 expression in the presence of heme or PPIX in WT NEM316. Cultures were grown in the presence of 0, 1, 5 and 10 µM heme or PPIX, and harvested for total RNA extraction in early stationary phase. ldhL (gbs0947; ‘crtl’) mRNA was used as RNA quantity control. The hybridization was performed on the same membrane as that used in Fig. 4B. B. Expression analysis of Pgbs0119-lacZ by determination of β-galactosidase activity in early stationary phase. S. agalactiae was grown in BHI liquid medium in the presence of different heme concentrations. Measurements were performed three or more times.
Role of pefAB and pefRCD operons in porphyrin sensitivity
The above results led us to ask whether pefAB and pefRCD loci are involved in porphyrin efflux. Several in vivo approaches were developed to explore this question. We constructed in-frame pefA (encoding a putative drug:H+ antiporter) and pefB (encoding a membrane protein of unknown function) deletion mutants; as the two components of pefCD are predicted to encode a single ATP-dependent transporter, we generated a deletion removing both ORFs. Mutations were combined to inactivate both pef operons. Tests were also performed with the ΔpefR deletion mutant, in which expression of both pef loci were highly induced (Fig. 3C).
Sensitivity of ΔpefR, ΔpefA ΔpefCD, and ΔpefB ΔpefCD mutants to metalloporphyrins was evaluated by plate inhibition tests (Fig. S2). Both ΔpefA ΔpefCD and ΔpefB ΔpefCD mutants showed greater sensitivity than the WT strain to 1 nmole heme (Fig. S2A). Similar results were obtained using Gallium PPIX (GaPPIX; tested at 50 nmoles, Fig. S2B). We noted that ΔpefA ΔpefCD was more sensitive than ΔpefB ΔpefCD; this phenotypic difference might suggest an accessory role of PefB in PefA PefB function. The single ΔpefA, ΔpefB, ΔpefC or ΔpefD mutants gave little or no inhibition by these porphyrins (data not shown), suggesting a functional redundancy between the efflux systems encoded by these loci. Sensitivity of the ΔpefR mutant to heme and GaPPIX did not differ significantly from the WT. We further tested heme-mediated inhibition in liquid medium by growing WT and pef single and double mutants, and the ΔpefR mutant, in 0 or 1 µM heme (Fig. 6A and data not shown). The ΔpefA ΔpefCD and ΔpefB ΔpefCD mutants, but not the other tested strains, displayed a slight growth inhibition in the presence of heme. Addition of 2 µM or 4 µM heme exacerbates growth retardation of these mutants (data not shown). These results indicate the need for at least one of the Pef efflux systems to avoid heme toxicity.
A. Growth curves of WT and mutant strains in the presence of heme. Cells were grown aerobically in M17G medium supplemented with 0 or 1 µM heme. WT (black circle), WT +1 µM heme (black square), ΔpefA ΔpefCD (red circle), ΔpefA ΔpefCD +1 µM heme (red square), ΔpefB ΔpefCD (gray circle, dashed line) and ΔpefB ΔpefCD +1 µM heme (gray square, dashed line). Results shown are representative of 3 experiments. Growth retardation of ΔpefA ΔpefCD or ΔpefB ΔpefCD was more pronounced with 2 and 4 µM heme. B. Photosensitivity of WT and mutant S. agalactiae strains grown in the presence of PPIX. Cells were grown until early stationary phase in M17G medium supplemented or not with 10 µM PPIX. Serial 10-fold dilutions (exponent is indicated) were exposed to 0, 10, or 50 minutes visible light. Plates were photographed after 24 h incubation.
To evaluate PPIX accumulation in S. agalactiae WT and mutant cells, we exploited its reactivity upon exposure to visible light; when excited by light, PPIX generates reactive oxygen species ,. The WT strain, and ΔpefAB ΔpefCD single and combined mutants, and the ΔpefR mutant, were grown with 10 µM PPIX and exposed to visible light for 0, 10 or 50 minutes. Viability of cells grown without PPIX and exposed to light was equivalent for all strains (Fig. 6B). Strikingly, inactivation of both putative pumps led to total mortality upon short light exposure (Fig. 6B). These results suggested that PPIX accumulates in S. agalactiae when pefAB and pefCD systems are inactivated. There were also marked differences between WT and ΔpefR sensitivity to PPIX after a longer (50 minute) light treatment. The ΔpefR mutant, which is up-regulated for pefAB and pefCD expression, showed essentially full viability, compared to a >10-fold drop for the WT strain. These data, showing heme and PPIX sensitivities of ΔpefAB ΔpefCD mutants, and lower PPIX sensitivity of the ΔpefR mutant give strong evidence for a role of the pef regulon in porphyrin efflux and intracellular homeostasis.
Intracellular porphyrin availability in S. agalactiae WT and ΔpefA ΔpefCD strains
We used two approaches to evaluate differences in intracellular porphyrin in the WT versus ΔpefA ΔpefCD strain. First, we exploited the fact that heme- and PPIX- induce PpefA-lacZ (same as Pgbs1753-lacZ above), to compare induction levels in the WT and ΔpefA ΔpefCD double mutant strains (Fig. 7A). In response to heme and PPIX addition, β-galactosidase activity was respectively about 2-fold and 3-fold increased in the ΔpefA ΔpefCD mutant compared to WT, suggesting that more heme and PPIX are available to activate the pefA (gbs1753) promoter in this mutant.
A. Expression analysis of PpefA-lacZ by β-galactosidase activity determinations was performed in early stationary phase cells of WT and ΔpefA ΔpefCD strains. S. agalactiae and derivatives were grown in BHI liquid medium. Results represent the mean ± standard deviation from triplicate experiments. Asterisks denote statistically significant differences as determined by Student's t-test (p≤0.05). B. PPIX- or heme-dependent production of the E. faecalis catalase KatA in S. agalactiae WT, and ΔpefA ΔpefCD mutant strains. Cells were grown in M17G supplemented or not with 1 µM of PPIX or heme. The loading of equivalent amounts of protein was verified by Coomassie stained gels performed in parallel. KatA was detected in total S. agalactiae protein extracts by immunoblot assays. Results shown are representative of 3 experiments.
Second, we used an in vivo “heme and PPIX sensor”: the E. faecalis catalase KatA is degraded if not bound to a porphyrin molecule . Intracellular availability of heme or PPIX was evaluated by comparing the relative stability of the E. faecalis KatA expressed in the WT strain and ΔpefA ΔpefCD and ΔpefR mutants (Fig. 7B and data not shown). Cells were grown without porphyrins or in 1 µM heme or PPIX, and KatA levels were followed in Western blots on cell lysates. Amounts of KatA in the WT and ΔpefR mutant strains were not significantly different (data not shown), which might reflect the limits of this reporter system. However, in the ΔpefA ΔpefCD mutant to which heme or PPIX was added, KatA showed pronounced stabilization, as expected for higher intracellular porphyrin levels in that strain. Results of both in vivo systems used above point to greater availability of porphyrins in the ΔpefA ΔpefCD mutant.
Physiological impact of pefAB and pefRCD activities on S. agalactiae respiration and virulence
S. agalactiae takes up exogenous heme, which activates its membrane cytochrome bd quinol oxidase, and is needed for respiration metabolism; the shift to respiration increases cell density by at least 20% compared to aerobic fermentation growth . We compared WT, ΔpefR, ΔpefA ΔpefCD, ΔpefB ΔpefCD, and the ΔpefR strain complemented by a plasmid-carried pefR gene (ppefR) for their capacity to grow in respiration conditions (Fig. 8A). The WT, ΔpefA ΔpefCD, ΔpefB ΔpefCD, and the complemented ΔpefR strain showed increased growth densities, indicative of respiration growth in these conditions. In contrast, the ΔpefR mutant was not augmented, suggesting a respiration defect of this strain. The pefR::ISS1 insertional mutant gave the same results as the ΔpefR deletion strain (data not shown).
A. Impact on respiration metabolism of deregulating pefAB pefCD expression by pefR inactivation. S. agalactiae WT, ΔpefA ΔpefCD, ΔpefB ΔpefCD, ΔpefR and ΔpefR transformed with vector containing a wild-type copy of pefR (ΔpefR + ppefR) strains were grown in respiration-permissive conditions (i.e., 1 µM heme and 10 µM menaquinone). S. agalactiae respiration growth is characterized by a gain in cell density . Absorbance (OD600) is shown on cultures after 22 h growth. Errors bars represent the standard deviation of three independent experiments. B. Impact on virulence of deregulating pefAB pefCD expression by pefR inactivation. Survival curves in adult mice infected with S. agalactiae WT (black square), ΔpefA ΔpefCD (red diamond), ΔpefB ΔpefCD (gray triangle, dashed line) or ΔpefR (blue triangle) strains. Differences in mortality between mice infected with the WT versus the ΔpefR mutant were statistically significant (p<0.001).
To confirm that the growth difference observed above was due to respiration metabolism, we performed the same growth experiments in the presence of 2-n-heptyl-4-hydroxyquinoline N-oxide (HQNO), which inhibits respiration but allows fermentation growth (data not shown; ). All tested strains except ΔpefR displayed lower growth densities in HQNO, which were comparable to those in aerobic fermentation; HQNO had no effect on cell density of the ΔpefR mutant. These results confirm that all strains tested above (Fig. 8A), except ΔpefR, activated respiration growth.
Respiration growth provokes an increase in oxygen consumption . This property was examined to confirm the respiration-defect of ΔpefR. Oxygen consumption in aerobic fermentation growth by the WT, ΔpefR, and ΔpefR (ppefR) strains was measured as 20.3, 21.0, and 31.1 µM.min−1 per OD600 = 1 cells (Table 1), which in these conditions reflects cytoplasmic NADH oxidase activity . In respiration-permissive conditions, oxygen consumption by the WT and ΔpefR (ppefR) strain was markedly higher (44.2 and 51.6 µM.min−1 respectively), but only moderately higher for the ΔpefR mutant (30.2 µM.min−1) (Table 1), further indicating the respiration-defect in the ΔpefR mutant. These results, together with the above studies, indicate that high PefAB and PefCD efflux activities impact on respiration by diminishing heme availability.
WT, ΔpefAB ΔpefCD and ΔpefR strains were tested in a mouse infection model (Fig. 8B). Virulence of the parental strain, and the ΔpefA ΔpefCD or ΔpefB ΔpefCD mutants was essentially the same. In contrast, the ΔpefR mutant (as well as the pefR::ISS1 insertional mutant; data not shown) showed markedly attenuated virulence. Earlier findings showed that a S. agalactiae respiration-defective mutant is attenuated for virulence . Reduced intracellular heme of pefR leads to a respiration deficiency, which can explain virulence attenuation of this mutant.
The present study uncovers a previously unknown system of porphyrin homeostasis in S. agalactiae, comprising two operons encoding distinct efflux pumps, controlled by a single intracellular regulator. Our results indicate that PefR, like numerous MarR-type proteins, acts as an intracellular sensor to regulate efflux of its ligands , , in this case, porphyrins. The range of PefR regulation is confined to the pefAB and pefRCD operons, as deduced from the presence of an IR within a 23 bp sequence uniquely upstream of these operons. This configuration is typical of MarR binding sites , , . Expression of the pefAB and pefCD efflux loci limits S. agalactiae intracellular porphyrin availability; at high pef expression levels, S. agalactiae may be unable to activate respiration metabolism, and to cause septicemic infection in the animal host. The management of intracellular porphyrin levels by efflux pumps, and regulation by an intracellular sensor in S. agalactiae constitutes new information on heme and PPIX homeostasis strategies.
Homology searches revealed that 9 out of 10 species carrying pefAB genes also encode cytochrome bd quinol oxidases, and thus are genetically equipped (like S. agalactiae) to activate a respiration metabolism in the presence of heme, or heme and a menaquinone (Table S2). In contrast, the pefRCD operon seems to be specific to the Streptococcus genus, and is also present in species lacking the respiration genes. Among conditionally respiring bacteria, most characterized S. agalactiae isolates , and Streptococcus uberis encode the complete pef regulon. Since members of both these species share the same ecological niche (both are responsible for bovine intramammary infection , ), the presence of the complete pef regulon might conceivably arise from a genetic transfer event. However, this possibility is unlikely, as the identity between their pef ORFs (73% to 49%) is not higher than the 72% identity between these species at the genome level (Average Nucleotide Identity; calculated as in ). Conservation of the pef regulon may indicate a role in survival and/or infection in the particular biotopes of both these species.
Results of this study add heme and PPIX to the inventory of MarR interactants. Several MarR proteins were previously shown to bind to, and regulate efflux of lipophilic and planar molecules, such as antibiotics, aromatic aldehydes or fatty acids, usually as a means to limit cellular toxicity ,. PefR activity would expectedly be tuned to retain sufficient intracellular heme for functions such as respiration. Indeed, pefAB expression in cells grown with porphyrins is induced to only half the levels compared to a fully induced ΔpefR mutant (data not shown). This, and the fact that the ΔpefR mutant is respiration defective, supports the need for basal levels of intracellular heme. Moreover, the presence of two putative PefR binding sites upstream of pefRCD (versus one upstream of pefAB) might influence the differential regulation of the two loci; possibly, lower levels of pefCD expression could participate in limiting intracellular heme depletion.
PefAB and PefCD add to a handful of other systems described as being involved in porphyrin efflux. The PefAB and PefCD systems share common features with two efflux systems in eukaryotes that control porphyrin pools: Feline leukemia virus receptor C, FLVRC, is an MFS-family protein (like PefA) that exports cytoplasmic metalloporphyrins across an ion-proton gradient , . The breast cancer resistance protein Bcrp/ABCG2 in humans is an ABC family transporter (like PefCD) that regulates eukaryotic intracellular heme levels under hypoxic conditions , . Just two possible porphyrin efflux systems were described in bacteria, neither of which is an analog of PefAB or PefCD: In E. coli, TolC effluxes PPIX, possibly to facilitate its turnover after iron extraction from heme; neither its regulation, nor its capacity to efflux heme have been reported , . In S. aureus, the hrtAB locus is regulated by heme, but not PPIX, and its inactivation provokes accrued heme sensitivity , . The S. agalactiae hrtAB homologous system (gbs0120 gbs0119) is likely to have a similar role in limiting heme toxicity. In contrast, the pef regulon is activated by PPIX, and at heme concentrations that do not induce hrtAB.
As PefAB efflux relies on proton motive force (PMF) to export substrates, we speculate that activity would be stimulated by the greater PMF generated under respiration conditions, as shown in L. lactis , , . Indeed, the PefAB system is conserved in streptococci and lactobacilli having the capacity to activate a respiration metabolism. As PefCD requires ATPase activity, its activity likely varies according to growth conditions , . The need for both PefAB and PefCD activities in S. agalactiae may accommodate the different metabolic states encountered in vivo, e.g., anaerobic fermentation in abscess, aerobic fermentation in lungs, and respiration in sepsis.
A model for heme and PPIX homeostasis in S. agalactiae, based on the newly characterized Pef operons, is proposed (Fig. 9): PefR represses expression of pefAB and pefRCD operons. Heme and PPIX are assimilated by unknown mechanisms. Once intracellular, these molecules interact with PefR, which detaches from its binding sites to activate PefAB and PefCD efflux pumps. Activities of the two Pef systems may assure rapid adjustment of intracellular heme levels under different cell physiological conditions. Whether PPIX efflux by pefAB pefCD has a biological role in S. agalactiae as an enzymatic byproduct of iron capture as in E. coli  remains to be determined. At higher heme concentrations, HrtAB homologs Gbs0120 and Gbs0119 could be activated via the putative two-component system Gbs0122 (heme sensor) and Gbs0121 (regulator), as was demonstrated for HssRS in S. aureus . This system would have a dominant role in protecting cells in a heme-rich environment, e.g., in conditions of massive degradation of host red blood cells; such a role is consistent with the strong induction of hrtAB (>200-fold) when heme levels are high (Fig. 5). Inactivation of pefAB and pefCD loci results in increased intracellular heme and PPIX pools, with consequences on growth and on heme-dependent enzyme activities; constitutive activity of these operons by pefR inactivation depletes these intracellular pools, resulting in respiration and virulence defects.
Extracellular heme and PPIX may be internalized by as yet unknown transporters. By homology with a recently described system in S. aureus , heme, but not PPIX, may bind to a putative external two-component receptor protein Gbs0122, the homolog of S. aureus HssS, resulting in gbs0119 gbs0120 (hrtAB) induction. Once inside the cell, free porphyrin molecules may encounter different binding proteins, including PefR. Apo-PefR binds to pefAB and pefRCD promoter regions to repress their expression. PefR-porphyrin binding releases PefR from DNA, to enable pefAB and pefRCD expression. The PefAB and PefCD loci mediate efflux of free heme and PPIX to avoid toxicity. Overexpression of PefAB and PefCD leads to heme depletion and respiration and virulence defects. Phenotypes of ΔpefR versus ΔpefAB ΔpefCD mutants are shown in the Table below.
A role for respiration functions in virulence has been reported for diverse bacterial pathogens, including Brucella abortus, Shigella flexnei, S. aureus and Mycobacterium tuberculosis; unlike S. agalactiae, these bacteria biosynthesize heme and are autonomous for respiration ,. In S. agalactiae, respiration is part of the metabolic reprogramming that occurs during the requisite septicemic phase of infection, in heme-rich blood . We suggest that a correlation between unavailability of heme due to high pefAB and pefCD activity, and the respiration defect explains virulence attenuation in the ΔpefR mutant. The use of efflux to regulate metabolic activity of a major bacterial pathogen has not been previously reported, and will lead to a better understanding of how bacteria deal with heme and other porphyrins in the variable conditions they encounter during infection.
Materials and Methods
All animal experiments were performed in strict accordance with INRA institutional guidelines of good animal practice (Jouy-en-Josas, France), and approved by the Direction des Services Vétérinaires (accreditation number 78-63).
Bacterial strains, growth conditions and plasmids
Strains and plasmids used in this study are described in Tables 2 and 3. NEM316, a S. agalactiae capsular serotype III strain was used as wild type (referred to as WT) and was isolated from a fatal case of septicemia . S. agalactiae and its derivatives were cultivated at 37°C in M17 medium (Oxoid) supplemented with glucose (0.2% for pre-cultures and 1% for test cultures [referred to as M17G]). For β-galactosidase assays, S. agalactiae was grown in BHI (brain heart infusion, Difco Laboratories) supplemented with 0.8% glucose. Aerated cultures were grown under agitation at 200 rpm in a ratio of air space to liquid of approximately 5/1. Respiring cultures were grown under agitation in the presence of 1 µM hemin (from a stock solution of 10 mM hemin chloride, Fluka) and 10 µM vitamin K2 (a menaquinone; Sigma). E. coli was cultivated in LB medium (Luria-Bertani, Difco Laboratories) at 37°C with aeration by shaking at 180 rpm. Antibiotics were used as needed at the following concentrations: for S. agalactiae, 5 µg/ml erythromycin, 1000 µg/ml kanamycin, 4 µg/ml chloramphenicol, 5 µg/ml tetracycline; for E. coli, 100 µg/ml erythromycin, 20 µg/ml chloramphenicol.
RNA extraction, Northern blot and RACE PCR
RNA was extracted from S. agalactiae cultures as described . Cells from 20 ml culture with an OD600 of 0.5∼0.8 (exponential growth phase) or OD600∼1.5 were harvested by centrifugation at 6000×g during 10 min. Total RNA was extracted with a guanidine isothycionate and phenol-chloroform step , using the TRIzol Reagent (Invitrogen).
For Northern blot analysis, RNA samples (30 µg) were mixed with an equal volume of glyoxal load dye (Ambion) and were electrophoretically separated on a 0.9% agarose glyoxal gel . RNA samples were transferred to a Biodyne B membrane (Pall) according to manufacturer's instructions. Hybridization and detection were performed using ECL direct nucleic acid labeling and detection systems (Amersham). A ∼500 base pair (bp) DNA labeled fragment of each ORF tested was used as probe. Primers used for probe generation are shown in Table S3.
The pefA transcriptional start was mapped using a 5′/3′ rapid amplification cDNA ends (RACE) kit, second generation (Roche Applied Science) according to supplier's instructions. Mapping was realized with RNA extracted from respiring cells, using primers: 5′TAGATGTAGGTGCTAACGTCG3′ and 5′CTTGTTGAGCCGTTGACAACG3′.
Plasmid pTCV-lac is a low copy number plasmid used to evaluate promoter activities in S. agalactiae . A DNA fragment containing gbs1753 promoter was PCR-amplified with primers 5′GCGTAGAATTCATTAAATGGAG3′, containing an EcoRI site (underlined) and 5′TATCTCGGATCCCTATTTCTGAT3′, containing a BamHI site (underlined). After digestion of the amplified fragment by EcoRI and BamHI, the gbs1753 promoter was cloned into plasmid pTCV-lac, resulting in plasmid pTCV-J11 carrying the Pgbs1753-lacZ (or PpefA-lacZ) fusion. The plasmids pTCV-lac and pTCV-J11 were subsequently transformed into S. agalactiae by electroporation and recombinant clones were obtained by erythromycin selection. The same strategy was performed to generate a Pgbs0119-lacZ fusion using the primers 5′ATACGCCAGAATTCTCGGCGAC3′ and 5′CCTTGGATCCTTTGATGTGAAC3′, giving rise to plasmid pTCV-J21.
Mutagenesis and screening conditions
Random insertional mutagenesis was performed on S. agalactiae with pG+host8::ISS1 basically as described . Both Pgbs1753-lacZ (reporter for gbs1753 transcription) and pG+host8::ISS1 plasmids were established in S. agalactiae. The strain was grown at 30°C with kanamycin for 2.5 h. The temperature was then shifted to 37°C for 2.5 h and plated on M17G with erythromycin, kanamycin and 80 µg/ml X-gal (5-bromo-4-chloro-3-indolyl-beta-D-galactopyranoside, BioMerieux), to obtain ∼100 CFU per plate. After 24 h incubation at 37°C, deep blue colonies were selected. Stable ISS1 mutants were isolated by growth at 30°C without erythromycin as described . The flanking chromosomal DNA was sequenced using primer 5′AGGGCATGGAAACAATTCGAGG3′. From the 5000 mutants we screened, 7 were in the pefR locus. Stable ISS1 mutants were then retested for gbs1753 up-regulation.
Gbs1402 (PefR) overexpression and purification
The gbs1402 ORF was amplified by PCR from S. agalactiae NEM316 using primers 5′CACCATGGAGAATCCTCTTCAAAA3′ and 5′TAATCAAAATCTTCCATCGCC3′. This amplified fragment was cloned into the E. coli expression plasmid Champion pET100 directional TOPO vector (Invitrogen) and transformed into E. coli TOP10. After plasmid verification by sequencing, the plasmid pET100-J14 was electroporated in E. coli BL21 (DE3). Protein expression was induced at an OD600 = 0.6 by addition of 1 mM IPTG for 2 h. Cells were harvested by centrifugation at 6000 rpm for 10 min and resuspended in 10 ml binding buffer (Tris HCl 50 mM pH 8, NaCl 300 mM, Imidazole 50 mM). Cells were broken by shaking with glass beads in a Fast Prep apparatus (MP Biomedicals). The lysate was centrifuged at 14000 rpm for 15 min at 4°C. The recombinant His-tagged fusion protein was purified by nickel affinity chromatography using His-Select affinity (Sigma) equilibrated with binding buffer according to supplier's instructions. The elution was carried out with binding buffer containing 300 mM imidazole. All fractions were collected and analyzed by SDS-PAGE. Purified proteins were dialyzed against 50 mM Tris HCl pH 8, 80 mM NaCl and 6.25% glycerol. Protein concentrations were determined by the Lowry assay (Bio-Rad).
Strains harboring PaphA-3-katA-His6 plasmid were incubated overnight under static conditions with or without 1 µM heme or PPIX. Cell growth was harvested by centrifugation at 6000×g during 10 min. Cells were broken by shaking with glass beads in a Fast Prep apparatus (MP Biomedicals). Immunoblotting analysis was done with rabbit anti-KatA antiserum as described, and kindly provided by Dr. L. Hederstedt . Detection was performed using ECL Plus Western blotting detection reagents (GE Healthcare).
Electrophoretic mobility shift assay (EMSA)
A 281 bp DNA fragment containing the gbs1753 promoter region and a 248 bp DNA fragment containing the gbs1402 promoter region were generated by PCR from genomic DNA of S. agalactiae and purified using the PureLink PCR Purification Kit (Invitrogen). Binding assays with PefR were carried out using a binding buffer (5% glycerol, 20 mM Tris HCl pH 8, 50 mM KCl, 0.2 mM MgCl2, 1 mM EDTA, 0.2 mM DTT, 0.3 µM BSA) in a final volume of 15 µl at 37°C. Reaction mixtures were incubated at 37°C for 20 min, after which they were analyzed by gel electrophoresis on an 8% polyacrylamide gel in TBE 1× buffer, stained with ethidium bromide. Reactions were carried out in the presence of a 116 bp non-specific competitor DNA (internal coding gbs1753 sequence) where specified. Where tested, heme or PPIX were added 20 min after protein and DNA components. Gel shift experiments were performed with two independent batches of purified PefR.
Construction of Δgbs1753 (ΔpefA), Δgbs1752 (ΔpefB), Δgbs1401 Δgbs1400 (ΔpefCD) and Δgbs1402 (ΔpefR) mutants and ppefR plasmid construction
In-frame pefA, pefB, pefCD, and pefR deletion mutants were constructed using the strategy described below. Briefly, the two regions flanking the locus to be deleted were independently amplified by PCR (see Table S3 for primers). Amplified fragments were digested by HindIII or EcoRV enzyme and ligated to each other. The resulting fragments were amplified by PCR, digested by EcoRI enzyme and cloned into the thermosensitive shuttle plasmid pG+host5. Electroporation of S. agalactiae strains and allelic exchange were done as described . In-frame deletions were confirmed by PCR and sequence analysis. The pefR gene was amplified (Table S3 for primers), and cloned using EcoRI and BamHI on fragment ends, onto plasmid pRC2 cut with the same enzymes; the resulting plasmid, pRC2-J14, is referred to as ppefR in Results.
PPIX and metalloporphyrin sensitivity tests
Stock solutions (10 mM) of PPIX, GaPPIX, ZnPPIX, and ZnMPIX (Frontier Scientific) were prepared in DMSO. PPIX sensitivity of S. agalactiae NEM316 and its derivatives was examined on early stationary growing cells (OD600 = 1.6). For PPIX light sensitivity tests, serial dilutions were spotted on plates and exposed to visible light for 0, 10 or 50 minutes. A 500 W halogen lamp with a glass lid placed at a distance of 55 cm was used as light source. Metalloporphyrin sensitivity tests on plates were performed as described : Briefly, 1∶100 dilutions of stationary-phase cultures were prepared in M17G soft (0.7%) agar, and poured over M17G plates. Metalloporphyrin (heme, 5 µl of a 0.2 mM solution; GaPPIX, 5 µl of a 10 mM solution) was spotted onto the plates. All plates were incubated for 20 h at 37°C and then photographed.
Oxygen consumption was determined as described . Briefly, S. agalactiae WT and ΔpefR late exponential phase cultures, prepared in aerobic fermentation or respiration conditions, were washed twice with PBS at 4°C and resuspended in the same buffer to obtain a 1 ml bacterial suspension at OD600 = 1.0. Oxygen consumption was followed with a Clark-type oxygen electrode (Liquid-Phase Oxygen electrode unit DW1, Hansatech instruments). The maximum oxygen consumption rate was measured following the addition of 10 mM glucose.
Mouse virulence assay
Pathogen-free 6 week-old Swiss CD1 mice (Charles River laboratories) were infected intravenously with S. agalactiae NEM316 or derivatives. Groups of 7–8 mice were anesthetized with ketamine (100 µg/g, Merial) and xylazine (12 µg/g, Bayer) and were inoculated in the eye vein with 108 CFU. Bacterial counts were determined in parallel by plating serial dilutions in saline buffer on M17G. Cells were harvested from mid-log phase and washed in a solution of NaCl 0.9%. Mortality was observed over a 10-day period. Animal experiments were performed in triplicate.
To find the conserved sequence between pef promoter regions, sequence were aligned with ClustalW and manually refined. A search for the 23 bp consensus in S. agalactiae NEM316 genome was done by visual inspection, and using BlastN program with EXPECT threshold set at 100. Pef protein homologs were identified using Genome Region Comparison, http://cmr.jcvi.org/cgi-bin/CMR/CmrHomePage.cgi, and/or were retrieved from genomic Blast databases, http://blast.ncbi.nlm.nih.gov/Blast.cgi/, using BlastP program with an E-value threshold set at 0.01.
A. PPIX displaces PefR from its DNA target. Gel mobility shift analysis of the effect of PPIX on PefR binding to the pefAB (right) and pefRCD (left) promoter regions. Samples contained 2 pmoles of PpefAB or PpefRCD fragment and 30 pmoles of PefR, to which were added either sample buffer, 120 pmoles (left) or 240 pmoles (right) of PPIX. On the two top panels, lanes 1–2 were juxtaposed to lane 3, which were separated on the initial same gel. B. Heme, but not iron, displaces PefR from its DNA target. Samples contained 2 pmoles of PpefAB fragment and 32 pmoles of PefR, to which were added either sample buffer, 160 pmoles heme, or 160 pmoles iron. Lanes 1–2 were juxtaposed to lane 3–4, which were separated on the initial same gel.
(1.51 MB EPS)
Differential heme (FePPIX) and GaPPIX sensitivity of the pef mutants. Stationary phase cultures of WT, ΔpefR, ΔpefA ΔpefCD or ΔpefB ΔpefCD strains were spread on M17G plates and 1 nmole of heme (A) or 50 nmoles of GaPPIX (B) were pipetted directed onto plates. Plates were incubated 24 hours, and then photographed. Representative results of at least 3 experiments are shown.
(1.40 MB EPS)
Transcriptome analysis in respiration versus aerobic fermentation conditions. Cells were grown in M17 medium with 1% glucose, supplemented or not with a mixture of 10 µM vitamin K2 (a menaquinone) and 48 µg/ml hemoglobin as heme source. Cells were harvested at OD600 = 0.3 for RNA extraction. Total RNA was extracted and analyzed by hybridization on NEM316 derived whole genome DNA macroarray as described . Fold change in expression is the mean of two independent macroarray experiments. Shown are results of S. agalactiae genes whose expression was induced or repressed at least 2-fold in respiration compared to aeration conditions. Genes further studied in this work are in bold. Gene assignments are according to the Sagalist web site (http://genolist.pasteur.fr/SagaList/) and BLAST searches (http://blast.ncbi.nlm.nih.gov/Blast.cgi/).
(0.09 MB DOC)
Distribution of pef regulon and cytochrome genes among Lactobacillales. * Reorganization of gene or domain order; # frameshift mutation in pefA homologous gene. In bold, species containing the complete pef regulon; ** Imperfect repeats, characteristic of MarR DNA binding sites, are present in respective pefAB and pefRCD promoter regions of this strain; *** gbs1401 and gbs1400 ORFs are missing in S. agalactiae 2603V/R .
(0.06 MB DOC)
We are grateful to IERP for technical assistance in animal studies. We thank Lars Hederstedt (Lund University, Sweden) for the generous gift of plasmid and anti-KatA antibody. We are grateful to Marie-Agnès Petit for application of ANI program and for critical and thoughtful reading of the manuscript, Gilles Lamberet for precious help in oxygen uptake determinations and Olivier Son and Isabelle Poquet for advice in gel shift assays (Micalis). We thank Cécile Wandersman, Patrick Trieu-Cuot, and Philippe Glaser (Institut Pasteur), Claire Poyart (Hôpital Cochin), and Philippe Bouloc (Institut de Génétique et Microbiologie) for stimulating discussions, and the members of the Micalis ‘Batiment 222’ lab for their support in the course of this study.
Conceived and designed the experiments: AF DL PG AG. Performed the experiments: AF DL ADB EC. Analyzed the data: AF DL PG AG. Wrote the paper: AF AG.
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