Early concepts of the function of CO2 in bacterial growth can be traced back to as early as a century ago. However, convincing experimental evidence only surfaced in 1935 when Gladstone reported that CO2 is an essential factor in the growth of bacteria1. The growth-promoting effect of CO2 was observed in various bacteria, including Staphylococcus aureus, particularly when glucose was substituted by another carbon source. Many years later, CO2-dependent S. aureus was isolated from abscesses and osteomyelitis2,3. These strains, though very rare, were well documented as dwarf or gonidial (G) strains and usually produced tiny colonies in the absence of additional CO24. Although G strains can be isolated from lesions, their virulence is low in a mouse infection model3. Since the early 1970’s, the CO2 dependence of staphylococci has been largely overlooked due in part to the routine cultivation of clinical isolates in CO2 incubators.

Renewed interest in these so-called dwarf colonies, now referred to as small colony variants (SCVs), was initiated in large part because they were frequently associated with persistent and relapsing infections such as airway infections and osteomyelitis5,6,7. In most cases, SCVs consist of mutants that are frequently affected in respiration comprising thymidine, hemin, or menadione auxotrophs8,9,10. However, unlike the earlier dwarf mutants described by Slifkin3 the respiratory mutants cannot be complemented by elevated CO2. There are several reports where CO2-dependent SCVs of S. aureus have been isolated from patients with catheter-related bacteremia, endocarditis, wound infections, respiratory infections, or nasal colonization11. This shows that CO2-dependent SCVs play a role in certain infections and further studies are necessary to unravel the genetic and biochemical basis of this type of auxotrophy.

We previously investigated whether S. aureus possesses a type 1 electrogenic NADH:quinone oxidoreductase (Ndh1), a proton pump that translocates cations, such as H+ or Na+12. It turned out that such an Ndh1 is not present in staphylococci; however, we found S. aureus has a homolog of the Escherichia coli specific NuoL protein, one of the core components of the proton pumping mechanism in E. coli13. We named the gene mpsA (membrane potential-generating system), because an mpsA mutant was severely defected in membrane potential generation and also grew like an SCV12. This connection and in light of the recent attention on SCVs, we sought to determine the function of the mps operon.

In S. aureus, mpsA is cotranscribed with the mpsB gene, and is separated by a weak transcription terminator from the downstream mpsC. It was unknown at that time whether mpsC contributes to the MpsAB function. MpsA, like the NuoL homolog is a membrane protein with predicted 14 transmembrane domains, while MpsB is a cytoplasmic protein with a predicted metal binding site. While MpsABC lacks NADH oxidation activity, it participates in Na+ transport as mpsABC complemented an Na+/H+ antiporter-deficient E. coli strain, suggesting that MpsABC constitutes a cation-translocating system12.

Here, we extend our previous observations by analyzing the function of MpsABC in greater detail. In principle, this study builds on the work of the 1970s, in which dwarf colonies were found to be complemented by CO2. We show that MpsAB increase the uptake of bicarbonate and represents a new class of dissolved inorganic carbon (DIC) transporter. DIC transporters are responsible for creating an elevated concentration of intracellular bicarbonate and supplying it to carboxysomes and Rubisco. Such transporters are most well studied in cyanobacteria14, but are not fully described in other autotrophic bacteria. In S. aureus, SCV-like mpsAB mutants cannot supply and store sufficient bicarbonate from atmospheric air to feed the important carboxylase reactions in central metabolism. The severe growth defect can only be compensated by increased CO2/bicarbonate supplementation. Importantly, MpsAB homologs are widespread in bacteria and were recently found in autotrophic bacteria functioning as DIC transporters to supply carboxysomes and RubisCO with bicarbonate/CO215,16.


Growth defect of ΔmpsABC is rescued by elevated CO2/NaHCO3

As previously reported, deletion of the mpsABC operon in S. aureus strain SA113 resulted in a severe growth defect, with the typical SCV-like phenotype12. To further characterize this operon, we constructed single deletion mutants of ΔmpsA, ΔmpsB, and ΔmpsC, as well as a deletion of the entire operon, ΔmpsABC, in the agr-positive S. aureus strain HG00117. The mutants were analyzed for growth in liquid culture under atmospheric growth conditions. As shown in Fig. 1a, the mutants ΔmpsA, ΔmpsB, and ΔmpsABC grew slowly and did not achieve the final OD of the wild type (WT) strain HG001, even after 72 h. The growth delay was most pronounced in the first 24 h. In contrast to ΔmpsA and ΔmpsB, the growth of ΔmpsC was not affected, indicating that mpsC does not contribute to the mpsAB activity.

Fig. 1
figure 1

Growth of HG001 ∆mpsABC. a Growth of wild type HG001, ∆mpsA, ∆mpsB, ∆mpsC, and ∆mpsABC in atmospheric (A) conditions. The growth of all mutants except ∆mpsC was significantly lower compared to HG001, **p < 0.01 by unpaired two-sided t-test. ∆mpsC showed no significant difference (ns) in growth compared to HG001. Each point shown in the graph represents the mean value ± standard error mean (SEM) from three independent experiments. Source data are provided as a Source Data file. b Colony appearances of wild type HG001, ∆mpsABC, and its complemented mutant (plasmid pRB473-mpsABC) during 5 days of incubation in atmospheric (A) conditions and 5% CO2. White bar represents a scale of 1 mm

Interestingly, growth of all mutants could be restored to near WT levels under elevated (5%) CO2 concentrations. During the course of 5 days incubation in 5% CO2, the colonies of all mutants were significantly larger than those grown in atmospheric air. Growth of the WT strain was largely uninfluenced by CO2, although the colony size was slightly increased (Fig. 1b and Supplementary Fig. 1). The growth-promoting effect of CO2 was also seen in liquid medium (Fig. 2a and Supplementary Fig. 2). Comparison of the growth in tryptic soy broth (TSB) in the absence or presence of 5% CO2 revealed that growth of the ∆mpsABC mutant was significantly improved in the presence of CO2 (Fig. 2a). This growth tendency is similar in the complemented mutant ∆mpsABC(pRB473-mpsABC) under atmospheric conditions. Given that CO2 and bicarbonate are interconvertible in aqueous solution, we also attempted to complement ∆mpsABC with sodium bicarbonate (NaHCO3). NaHCO3 at concentration ranging from 1 to 50 mM were added to the growth medium and growth of ∆mpsABC was followed for 24 h. At low concentrations (1 mM NaHCO3) no difference in the growth of ∆mpsABC was observed (Fig. 2b). However, with increasing concentrations of up to 50 mM NaHCO3, its growth increased steadily before reaching final OD values comparable with those of 5% CO2. Similar observation was also seen with ∆mpsB (Supplementary Fig. 3a and 3b). The pH of the medium (TSB) increased with the addition of NaHCO3, however the effect of pH of the medium did not play a crucial role on the growth of ΔmpsABC (see Supplementary Note 1, Supplementary Table 3 and Supplementary Fig. 8). The results indicate that the growth deficiency of ∆mpsABC can be largely compensated by the addition of 5% CO2 and high concentrations of NaHCO3.

Fig. 2
figure 2

Growth of HG001 ∆mpsABC can be complemented with 5% CO2 and NaHCO3. a Growth of HG001, ∆mpsABC in atmospheric (A)conditions and 5% CO2. The growth of the mutant can also be complemented by plasmid pRB473 carrying mpsABC (compl.). Each point shown in the graph represents the mean value ± standard error mean (SEM) from three independent experiments. b Growth of ∆mpsABC in atmospheric (A) and with additions of NaHCO3 ranging from concentrations of 1 to 50 mM, and 5% CO2. The growth of ∆mpsABC with addition of 50 mM NaHCO3 was similar to that under 5% CO2, as there was no significance difference (ns) between the two conditions (p > 0.05) by unpaired two-sided t-test. Each point shown in the graph represents the mean value ± standard error mean (SEM) from two independent experiments. Source data are provided as a Source Data file

MpsABC increase the uptake of bicarbonate

The diminished ability of the ΔmpsABC mutant to grow under atmospheric conditions as well as the rescue of this defect by CO2 and bicarbonate led us to the suggestion that MpsAB may play a role in CO2 and bicarbonate transport. As the determination of the CO2 transport is very difficult, we compared the bicarbonate uptake activity in the WT strain HG001 and the ∆mpsABC mutant with radiolabeled NaH14CO3. Both strains were grown aerobically in TSB until reaching its respective exponential growth phase before being washed to remove the growth media and resuspended to the same OD578 in Tris buffer. Prior to the addition of NaH14CO3, the cell suspensions were incubated with fluorocitrate and glucose. Fluorocitrate, an aconitase inhibitor, was added to block the TCA cycle so that NaH14CO3 accumulated intracellularly and is not immediately expired by the decarboxylation reactions of the TCA cycle. Glucose was added as energy source because the cells were resuspended in only Tris buffer. After addition of NaH14CO3, samples were rapidly harvested at several time points and the 14C uptake was measured by liquid scintillation counting. The immediate uptake occurred within 120 s until a steady state level was reached (Fig. 3a). Compared with the WT strain HG001, ΔmpsABC showed significantly decreased 14C uptake in the first 120 s. After 15 min, ΔmpsABC showed a 6.6-fold lower radioactivity than the WT strain indicating that the bicarbonate uptake was impaired in the mutant.

Fig. 3
figure 3

Uptake of NaH14CO3 by HG001 and ΔmpsABC, membrane potential determination and mpsA expression. a Cells were preincubated with fluorocitrate for 30 mins prior to the addition of NaH14CO3 (50 μCi). NaH14CO3 was added at time 0 and 1 ml of cell samples collected at times indicated. The H14CO3 uptake was determined by 14C accumulation in cells measured by liquid scintillation counting. The NaH14CO3 uptake in ΔmpsABC was significantly lower than WT HG001; ***p < 0.001 by paired two-sided t-test. Each point shown in the graph represents the mean value ± standard error mean (SEM) from three independent experiments. (CPM = counts per minute). bmpsABC grown in 5% CO2 showed increased membrane potential compared with those grown in atmospheric conditions. Membrane potential was determined by fluorescence intensity measurements using BacLight bacterial membrane potential kit. The values for WT HG001 in atmospheric were set equal to 100%. Cells were grown to exponential growth phase in atmospheric (A) and 5% CO2 (CO2). As a negative control, the H+ ionophore CCCP caused a collapse of the membrane potential in all strains tested both in atmospheric CO2 and in the presence of 5% CO2. When grown under 5% CO2 conditions, HG001 and ∆mpsABC showed significantly higher relative membrane potential (**p < 0.01 and ****p < 0.0001, respectively, as determined by unpaired two-sided t-test) compared with their corresponding strains in atmospheric conditions. Each bar shown in the graph represents the mean value ± standard error mean (SEM) from four independent experiments (three independent experiments for CCCP), each with three technical replicates. c mpsA expression in three wild-type Staphylococcus aureus strains HG001, USA300, and MW2 under atmospheric and 5% CO2 conditions. The relative expression of mpsA under 5% CO2 conditions, normalized to its corresponding strains grown in atmospheric (A) conditions. Only mpsA expression in HG001 is significantly lower in 5% CO2 compared with atmospheric conditions; *p < 0.05 by unpaired two-sided t-test. (ns = not significant). Each bar shown in the graph represents the mean value ± standard error mean (SEM) from four independent experiments, each with three technical replicates. Source data are provided as a Source Data file

mpsAB complements an E. coli CA mutant and vice versa

Previously we described that MpsB contains a metal binding motif (His607, Cys622, and Cys625), which is reminiscent of a carbonic anhydrase (CA) motif12. Therefore, we tried to detect CA activity with purified MpsB alone and cell extracts expressing MpsABC. However, we were unable to detect any CA activity with various methods. In the absence of any detectable enzymatic data, we asked if mpsAB could complement a CO2-dependent E. coli mutant, EDCM63618. EDCM636 is an E. coli K-12 mutant in which the CA gene, can, was deleted. As a result, this strain is unable to grow under atmospheric air, but can grow in the presence of high CO2. This phenotype of EDCM636 is similar to that of HG001ΔmpsABC; hence, we investigated whether mpsAB can restore growth of EDCM636 under atmospheric conditions. To do this, we inserted the S. aureus mpsA, mpsB, mpsAB, and mpsABC genes into E. coli strain EDCM636. The vector alone, pRB473, served as control. Interestingly, neither mpsA nor mpsB alone could restore growth of EDCM636. Plasmids containing mpsAB and mpsABC were able to restore the growth equally well (Fig. 4a), indicating that mpsC was dispensable. As expected, all six strains were able to grow under 5% CO2 conditions (Fig. 4a).

Fig. 4
figure 4

mpsAB(C) complements an E. coli carbonic anhydrase mutant and vice versa. a E. coli carbonic anhydrase mutant (EDCM636) can be complemented with mpsAB and mpsABC using plasmid pRB473 under the control of its native promoter in atmospheric (left) and 5% CO2 (right). Clockwise from the top; EDCM636, EDCM636 pRB473 (empty plasmid), EDCM636 pRB473 mpsA, EDCM636 pRB473 mpsB, EDCM636 pRB473 mpsAB, and EDCM636 pRB473 mpsABC. bmpsABC can be complemented with carbonic anhydrase, can from E. coli MG1655 using pTX30, a xylose-inducible promoter plasmid. Clockwise from the top; wild-type HG001, ∆mpsABC, ∆mpsABC pTX30 (empty plasmid), and ∆mpsABC pTX30 can. Plates were supplemented with xylose (+) or without xylose (−)

Since mpsAB restored the growth of EDCM636, we asked if the CA gene (can) from E. coli could complement the S. aureus ΔmpsABC. To address this question, can from E.coli K-12 was expressed in ΔmpsABC(pTX30-can) under a xylose inducible promoter. As shown in Fig. 4b, without xylose ΔmpsABC(pTX30-can) could not grow under atmospheric air. However, when can expression was induced by xylose, growth was restored. All clones grew in the presence of 5% CO2 (Fig. 4b), suggesting that both the bicarbonate transporter and CA enable growth under atmospheric CO2 level and both are interchangeable. Although the activities of bicarbonate transporters and CA are different, they represent a CO2/bicarbonate concentrating system that can functionally replace each other.

Impaired membrane potential in ΔmpsABC is rescued by 5% CO2

Previously, it was reported that MpsABC represents a membrane potential-generating and cation-translocating system, and that membrane potential was severely affected in the ∆mpsABC mutant12. Because elevated CO2 restores the growth of ∆mpsABC, we wondered whether 5% CO2 also restores the membrane potential in this mutant. The membrane potential of the WT strain, HG001, grown under atmospheric air was set equal to 100% and was used as a comparator for other strains (Fig. 3b). In the ΔmpsABC mutant, the membrane potential was decreased to only 18% of HG001. In contrast, the presence of 5% CO2 increased the membrane potential of the ΔmpsABC mutant and the WT strain up to 164% and 134%, respectively. As a negative control, the H+ ionophore CCCP caused a collapse of the membrane potential in all strains tested both in atmospheric CO2 and in the presence of 5% CO2. Based on these findings, elevated CO2 not only restores growth but also the membrane potential generation in the ΔmpsABC.

mpsA expression was downregulated under 5% CO2 conditions

Since the mps deletion mutants, except ∆mpsC, are responsive to 5% CO2, we postulated that the expression of mpsAB could be affected by CO2. To investigate whether high CO2 levels influence mps transcription, Quantitative Reverse Transcriptase-PCR (qRT-PCR) was performed to determine the transcription of mpsA in atmospheric and 5% CO2 conditions. To exclude strain specific effects, three different WT S. aureus strains were used, namely HG001, USA300 LAC, and MW2 (USA400). RNA was isolated during the exponential growth phase and the mRNA of mpsA from the three strains grown in atmospheric air and in 5% CO2 were compared. Transcript abundance for each strain cultivated in 5% CO2 was normalized to its corresponding strain grown in atmospheric conditions. Relative to the growth in atmospheric air, mpsA in HG001 grown in CO2 was downregulated the most, namely 2.5-fold, in USA300 2-fold, and in MW2 1.7-fold (Fig. 3c). In short, mpsA expression was lower in 5% CO2 compared with atmospheric conditions in all three strains tested; however, only mpsA downregulation in HG001 reached statistical significance (p < 0.05). A downregulation of mpsA (SAOUHSC_00412) by CO2 was also observed under cell culture conditions, as reported in Aureowiki19.

ΔmpsA produces fewer hemolytic toxins and is less pathogenic

Because the CO2/bicarbonate transporter MpsAB is important for growth and membrane potential generation, we predicted that the mutant would have less toxin production and be less virulent. To examine this question, the hemolytic activity of ΔmpsA and HG001 grown in atmospheric and 5% CO2 was tested on sheep blood agar followed by cold shock treatment. Consistent with our hypothesis, no visible hemolytic zone was seen in ΔmpsA when cultivated in atmospheric air, while the presence of 5% CO2 restored toxin production as indicated by a clear halo on blood agar (Fig. 5a). The same result was also observed for the ΔmpsB and ΔmpsABC mutants (Supplementary Fig. 4). The WT strain HG001 formed a hemolysis zone independent of the presence of 5% CO2.

Fig. 5
figure 5

mpsA produces less hemolytic toxin in atmospheric conditions and is less virulent in animal infection models. a Hemolytic toxin production in HG001 and ΔmpsA grown in atmospheric (left) and 5% CO2 (right) at 37 °C after overnight incubation (above) and after cold shock treatment (below). b Kaplan–Meier plot of the survival of Galleria mellonella larvae infected with HG001 and ΔmpsA. Larvae injected with PBS were used as control. Larvae infected with ΔmpsA showed significantly better survival rate compared with the larvae infected with wild-type HG001; ****p < 0.0001 as determined by Log-rank (Mantel–Cox) test. Results are representative of four independent experiments. c Comparison of wild-type HG001 and ΔmpsA in a 48 h intranasal mouse infection model (pneumonia model) in the lung, kidneys, and liver. The bacterial burden of ΔmpsA in the lung was significantly lower (*p = 0.036) compared with HG001. There was no significant difference (ns) in bacterial burden in the kidney and liver between the two strains. The number of bacteria per organ based on determination of CFU in n = 8 (WT HG001) and n = 9 mice (ΔmpsA) is shown. The vertical line indicates the median. The detection limit was 10 CFU per organ. Data were analyzed using two-tailed Mann–Whitney test. Source data are provided as a Source Data file

Following the finding of decreased toxin production from ΔmpsA, we were interested to find out if this effect is relevant in vivo. To characterize the role of mps on virulence, Galleria mellonella larvae were used as an invertebrate infection model. The survival rate of larvae injected with WT HG001, ΔmpsA, and PBS as control were observed over the course of 5-day period (Fig. 5b). In the PBS control group, 95% of the larvae were alive at the end of the 5-day period. In contrast, larvae infected with HG001 showed a survival rate of only 13% after the 5-day period, while 53% of the larvae survived when infected with ΔmpsA. These results indicate that deletion of mpsA rendered S. aureus less virulent in an invertebrate infection model.

To assess the contributions of mpsAB to S. aureus pathogenesis using an intranasal mouse infection model (pneumonia model), female Balb/c mice were intranasally infected with HG001 and ΔmpsA. After 48 h, mice were sacrificed and the lungs, kidneys, and livers were recovered to determine the bacterial burden. Although the ΔmpsA generally exhibited a lower bacterial burden in all three organs, only the bacterial load in the lung was significantly lower compared with its WT strain HG001 (Fig. 5c). These results indicate that the ΔmpsA is attenuated in pathogenicity compared with its WT strain in this mouse infection model. Taken together, these findings suggest that a functional bicarbonate transport system (mps) is required for fitness and pathogenicity in vivo.

Phylogenetic distribution of mpsAB homologs

Considering the significant effect of mpsAB in S. aureus, we examined the phylogenetic distribution of both genes. Searching the RefSeq database revealed genes homologous to mpsA and mpsB were found in a number of species that span the Firmicutes phylum (Fig. 6). These included bacteria from the genus Staphylococcus, Bacillus and a few from Alicyclobacillus, Geobacillus, Parageobacillus, Sulfobacillus, and Thermaerobacter (Fig. 6 and Supplementary Fig. 6). Furthermore, homologs of mpsAB were also widespread in genomes from multiple phyla of prokaryotes (Supplementary Fig. 7). Among those which were well depicted in the phylogenetic tree are from the phyla Proteobacteria, Actinobacteria, and Bacteroidetes. MpsAB are highly conserved in the genus Staphylococcus and to a lesser extent in Bacillus and other Firmicutes (Supplementary Fig. 5). Apart from few exceptions in Actinobacteria and Proteobacteria, in most genomes mpsA and mpsB homologs are always adjacent. In Acidimicrobium ferrooxidans, a ferrous-iron-oxidizing bacterium, mpsA and mpsB homologs exist as a single fused gene (Supplementary Fig. 5).

Fig. 6
figure 6

mpsAB homologs are widespread in the Firmicutes phylum. Maximum likelihood phylogenetic analysis of concatenated alignments of mpsA and mpsB homologs amongst the phylum Firmicutes. Node support is indicated by bootstrap values from 100 resamplings of the alignment when they exceeded 70%. Collapsed clades are labeled by the genus of associated taxa. The number of taxa belonging to the respective clade is indicated in brackets. Source data are provided as a Source Data file

Apart from S. aureus, mpsAB homologs were found in a few human pathogens such as Bacillus anthracis, Legionella pneumophila, and Vibrio cholerae (Table 1). Interestingly, all these three pathogens also carry genes encoding protein with CA domain in addition to mpsAB homologs. In the family of Staphylococcaceae, only Macrococcus caseolyticus JCSC5402, Staphylococcus carnosus TM300, and Staphylococcus pseudintermedius ED99 do not have mpsAB homologs. Instead, they carry genes with CA homologs. This surprising observation also extend to a number of human pathogens; Listeria monocytogenes, Streptococcus pyogenes, Enterococcus faecalis, Enterococcus faecium, Mycobacterium tuberculosis, Helicobacter pylori, Escherichia coli, and Pseudomonas aeruginosa (Table 1). All these important pathogens have CA homologs instead of mpsAB homologs, emphasizing the importance of bicarbonate/CO2 supply to the microorganisms.

Table 1 Distribution of MpsAB and carbonic anhydrase (CA) homologs in various species


Despite an almost 50-year-old observation of CO2-dependent S. aureus growth, little is known about the genetic basis of S. aureus regarding its response to changes in CO2 availability. In the present work, we demonstrate that the growth defect of the ΔmpsABC mutant under atmospheric CO2 levels could be largely rescued by 5% CO2 (Fig. 2a) or by ≥ 50 mM bicarbonate (Fig. 2b). Uptake studies with radiolabeled NaH14CO3 indicates that MpsABC contributed to a significant accumulation of H14CO3 in the cytoplasm of the WT strain (Fig. 3a). The bicarbonate uptake experiment is tricky because we had to prevent CO2 evaporation as much as possible. This is most likely the reason why we observed increased variations after 5 min. However, one should consider that for substrate uptake, the first 2 min are crucial. During this time range, the standard error mean (SEM) values were really small. We assume that the addition of fluorocitrate was probably not inhibiting the TCA cycle completely; we do not dare to increase the concentration any higher because of the side effects it may cause (we used 10 mM fluorocitrate and the normal concentration used for aconitase enzyme assay is 100 μM).

Deletion of the mpsC gene showed no phenotypic alterations or growth defect, suggesting it is not a functional part of the mpsAB operon. Furthermore, the E. coli CA mutant could be complemented with only mpsAB, and the gene synteny revealed that mpsC is not collocated with mpsAB homologs in other bacteria than staphylococci. Taken together, these observations speak in favor of MpsAB representing a bicarbonate or DIC transporter with the ability to accumulate intracellular DIC.

CAs are Zn2+ metalloenzymes, which catalyze the reversible hydration of CO2 (CO2 + H2O ↔ HCO3 + H+). For this reason, we hypothesized that a CA mutant in E. coli (EDCM636) could be complemented by mpsAB. The E. coli can gene encodes a β-class CA, which is essential under atmospheric but not at 5% CO218. As expected, the E. coli can mutant could be complemented by mpsAB and vice versa; the S. aureus mpsABC mutant could be complemented by E. coli specific can (Fig. 4). Due to the mutual complementation, we thought that MpsB, MpsAB, or MpsABC might have CA activity. Unfortunately, we were unable to detect CA activity using purified proteins or with whole cell extracts. The absence of CA activity in MpsAB suggests that MpsAB and CA have different enzymatic mechanisms, yet they serve the same function; namely, preventing evaporation of CO2 by trapping it as bicarbonate for anaplerotic metabolism. Although a considerable amount of CO2 is produced by a functional TCA cycle, this CO2 will be lost in the cytoplasm due to an insufficient concentration for anaplerotic reactions. To prevent this from happening, CA catalyzed the formation of bicarbonate from CO2, which significantly delays the release of intracellular CO2 and providing bicarbonate required for carboxylation reactions20.

The observation that EDCM636 could only be complemented by both MpsAB suggests they function together as a transporter. This is also supported by the collocation of mpsAB homologs in many microorganisms across multiple phyla (Fig. 6, Supplementary Figs. 5 and 7). Furthermore, MpsA belongs to PFam0036121, which consists of a diverse family of proton-conducting membrane transporters, including NADH:quinone oxidoreductase subunits (complex I)22. In this regard, we demonstrated that MpsABC constitutes a cation-translocating system, capable of Na+ transport similar to the observation regarding NuoL12. MpsB on the other hand belongs to PFam10070, a family of conserved proteins in bacteria of unknown function. Based on these observations, we propose a model that MpsAB is a sodium bicarbonate cotransporter (NBC) as illustrated in Fig. 7. Such NBC transporters are prevalent in mammals23, having important functions in maintaining intracellular and whole-body pH, as well as contributing to the transepithelial transport processes. The bicarbonate cotransporters are composed of 13 transmembrane domains24, similar to MpsA which has 14. It is unknown whether mammals also require an MpsB homolog; although the NBC stoichiometry in Xenopus oocytes is 1 Na+: 2 HCO3, indicating a possible accessory protein interaction25. As CO2 is volatile, transporting bicarbonate or DIC helps to “trap” it in the cytoplasm for the carboxylation reactions of anaplerotic metabolism. In Firmicutes, these include pyruvate carboxylase fuelling the TCA cycle, acetyl-CoA-carboxylase as the first enzyme of fatty acid synthesis, or phosphoribosylaminoimidazole carboxylase involved in purine biosynthesis.

Fig. 7
figure 7

Proposed function for MpsAB. We proposed that MpsAB represents a sodium bicarbonate cotransporter (NBC). These transporters are prevalent in mammalians and are expressed throughout the body. Unlike CO2 which can diffuse passively in and out of the cells, bicarbonate (HCO3) needs to be transferred into the cells via a transporter. In S. aureus, MpsAB most likely function together as cotransporter to transport Na+ and HCO3. Me2+ indicates a metal binding site in MpsB

Phylogenetic analysis revealed that mpsAB are widespread, not only among Firmicutes, but also across multiple phyla (Fig. 6 and Supplementary Fig. 7). Bacteria that possess homologs of MpsAB have diverse lifestyles; for example hyperthermophilic (e.g., Aquifex aeolicus), thermophilic and acidophilic (e.g., Acidimicrobium ferrooxidans and Acidithiobacillus caldus), CO2 fixing bacteria (e.g., Chloroflexus aurantiacus), and nitrogen-fixing bacteria (e.g., Bradyrhizobium oligotrophicum and Frankia sp). In addition, MpsAB homologs were also described in the gammaproteobacterial chemolithoautotroph Thiomicrospira crunogena15. Similar to S. aureus, the T. crunogena genes Tcr_0853 (mpsA homolog) and Tcr_0854 (mpsB homolog) were cotranscribed, constitute a probable DIC transporter, and its mutants required elevated DIC for growth15. Although T. crunogena has CO2 concentrating mechanisms (CCMs), its DIC uptake process is unclear due to the lack of cyanobacterial transporter homologs. That being said, it is assumed that in autotrophic bacteria, a DIC concentrating system is necessary to ensure that Rubisco is saturated with CO2, so that carboxylation proceeds at its maximum rate.

Another problem with the “ancient” Rubisco is that it also reacts with oxygen26. In this respect, the atmospheric CO2 content in ancient times was high, while that of O2 was low. In a CO2-rich environment, the CO2-fixing enzymes in autotrophic bacteria, such as Rubisco could work properly despite its low affinity and limited discrimination between CO2 and O2. However, due to oxygenic photosynthesis in the subsequent 2.5 billion years, the atmosphere became O2 rich and CO2 poor27. As a consequence, the cytoplasmic CO2 levels became too low for proper CO2 fixation and assimilation28,29. Therefore, it is assumed that autotrophic bacteria that grow in atmosphere appear to uniformly have CCMs27. Bacterial CCM involves two main functions: (a) active transport of inorganic carbon species (HCO3 and CO2) to concentrate HCO3 within the cell, and (b) the pool of HCO3 is then utilized to provide elevated CO2 concentrations around primary CO2 fixing enzyme, Rubisco, encapsulated in carboxysomes which also contain CA14. Recently, DIC transporters from four evolutionary distinct families were described in several genera of sulfur-oxidizing chemolithoautotrophs16. Two of these DIC transporters demonstrate DIC uptake even though they share low protein identity with the well-characterized cyanobacterial transporters, SbtA- and SuIP-family bicarbonate transporters. SbtA is an inducible, high-affinity Na+-dependent HCO3 transporter30, while BicA, a member of the SuIP family, is a low-affinity, high-flux Na+-dependent HCO3 transporter31. Heterologously expressed chromate ion transporter from Hydrogenovibrio thermophilus JR2 is also capable of DIC uptake16. The fourth type of transporter is a two component DIC transporter encoded by the genes Tcr_0853 and Tcr_0854 in Hydrogenovibrio crunogenus (previously known as T. crunogena) as discussed previously15,16. Another well-characterized DIC transporter expressed in cyanobacteria is BCTI, encoded by the cmpABCD operon is an inducible, high-affinity HCO3 transporter belonging to the ATP binding cassette transporter family32. It is thought that these transporters differ in their affinities and mechanisms for transport (as cation symporter or anion antiporter), which provide advantages under specific growth conditions16. Out of all these distinct transporters families, MpsAB belongs to the same type as encoded by Tcr_0853 and Tcr_0854 from H. crunogenus in terms of function and homology; MpsAB is 29–30% identical to Tcr_0853 and Tcr_0854. Such transporters and their function were so far not described in Firmicutes.

Staphylococci, like most other Firmicutes, are neither autotrophic nor do they possess typical carboxysome structures or Rubisco. The question is, therefore, why do they need MpsAB as a DIC concentrating system. The most rational answer would be that enzymes involved in substrate carboxylation are not sufficiently supplied with HCO3 under atmospheric CO2, thus require a higher HCO3 concentration for proper activity. For example, the biotin-dependent pyruvate carboxylase has a central function in fueling the TCA cycle with oxaloacetate. If this reaction is impaired, not only the TCA cycle but also respiration and the membrane potential would be impaired. This is exactly the observed phenotype of the mpsABC mutant, which exhibited the typical features of SCV in atmospheric CO2 and similar to the S. aureus hemB mutant10,12. It is also tempting to speculate that MpsAB serve to prevent the depletion of cellular DIC, a role which is conventionally played by CA or other known cyanobacterial bicarbonate transporter. S. aureus has neither of them, however since CO2 or HCO3 is crucial for many cellular processes, a DIC concentrating mechanism is likely to be important for its growth and survival. As a major pathogen S. aureus needs to adapt to different niches; as commensal inhabitant on environmentally exposed skin and mucosal surfaces to colonization and infection inside the mammalian host. Variations of CO2 levels are one of the evident conditions it would encounter in this process, and having a DIC concentrating mechanism would ensure its sufficient supply intracellularly. Collectively, these hypotheses could explain the role of MpsAB beyond the known carbon-fixing bacteria.

Due to the interchangeable role of MpsAB and CA, we sought to compare the occurrence of both the genes in Firmicutes. In this phyla, there is tendency that either one of them is present; in some cases both genes are present in one strain/species, for example in B. anthracis and B. subtilis (Table 1). This same observation appears to hold true for selected species of Gram-positive and Gram-negative pathogens (Table 1). Interestingly, highly pathogenic species for example Legionella pneumophila and Vibrio cholera have MpsAB homologs as well as at least two CA homologs, while Mycobacterium tuberculosis, Helicobacter pylori, E. coli O157:H7, and Pseudomonas aeruginosa have two or even three CAs. The importance of the distribution of MpsAB and CA in the respective strains or species is not yet clear. Nevertheless, the occurrence of two and even three CA genes, and/or MpsAB suggests that DIC concentrating mechanism play an important role in fitness and pathogenicity. We assume that the decreased virulence of the mpsA mutant is due to the very low intracellular bicarbonate levels. Bicarbonate is the substrate for biotin carboxylase that produces carboxybiotin, the substrate for other carboxylases, such as PEP−, or pyruvate carboxylase that feed the TCA cycle. For example, the Km value for bicarbonate of the E. coli biotin carboxylase is comparatively high at 16 mM33, indicating that the enzyme has a very low affinity for bicarbonate. This suggests that a high level of intracellular bicarbonate is needed to fuel the TCA cycle, respiration, fatty acid biosynthesis, and membrane potential. ATP and membrane potential are important for toxin secretion.

The virulence attenuation of the ΔmpsA was also seen in vivo. In the Galleria mellonella larvae survival model, the killing rate by the mutant was significantly decreased (Fig. 5b). In the intranasal S. aureus mouse infection model (pneumonia model), the CFU/lung was also significantly decreased with ΔmpsA (Fig. 5c). We have chosen a lung infection model because the CO2 content in the lung is higher and we expect that the mpsA mutant might have a better chance to grow. CO2 is produced during respiration and is carried by the blood through the venous system to the lungs, where it is exhaled with a concentration of ~3.8% in the tidal air or 450 l of CO2 per day34. There was no statistically significant difference in bacterial burden in the kidney and liver between HG001 and the mpsA mutant. This can be explained that the lung was the primary organ that was infected with S. aureus. From there, S. aureus spreads to other organs during the course of infection. Spreading is a complex process as the bacteria have several barriers to pass: first the lung epithelium and endothelium of blood vessels, and then again the endothelium of blood vessels to establish infections in other organs. Thus, infection burden in kidneys and liver was lower than in the lung, as it has also been observed by Lee et al.35.

In conclusion, we propose that MpsAB constitutes a DIC transporter that is important for growth of S. aureus under low, atmospheric CO2 conditions. This transporter system underlies the importance of CO2/bicarbonate in the fitness and pathogenicity of S. aureus and may help shed some light on earlier observations about CO2-dependent variants. Furthermore, mpsAB homologs are widespread in diverse groups of microorganisms that adopt different lifestyles and occupy a wide range of niches. In contrast to the dogma of DIC transporters, MpsAB plays an important function even in non-autotrophic bacteria by concentrating bicarbonate for anaplerotic pathways that are relevant across most microorganisms. An interesting finding in our study was that MpsAB and CA could functionally replace one another in our mutual complementation experiments, further supporting the essentiality of bicarbonate. Within this context, a number of the pathogenic species have either MpsAB or CA, whereas both are present in some of these species, suggesting their roles in growth and virulence.


Bacterial strains and growth conditions

The strains used in this study are listed in Supplementary Table 1. For cloning procedures, all staphylococcal and E. coli strains were cultivated at 37 °C with shaking at 150 rpm in basic medium (BM) (1% soy peptone, 0.5% yeast extract, 0.5% NaCl, 0.1% glucose, and 0.1% K2HPO4, pH 7.2), unless specified otherwise. All cultures were grown in 10 ml medium using baffled 100 ml shake flasks (flask-to-medium ratio 10:1) as recommended36, with the exception of growth studies, which were grown in 15 ml medium (flask-to-medium ratio 7:1). The medium was supplemented with the following antibiotics, where applicable at the indicated final concentrations: chloramphenicol at 10 μg ml−1, tetracycline at 25 μg ml−1, for staphylococcal strains and 100 μg ml−1 ampicillin and 30 μg ml−1 kanamycin for E. coli strains.

Growth studies of staphylococcal strains

TSB (Sigma-Aldrich) and TSA plates (Sigma-Aldrich) were used for growth studies involving S. aureus. For growth characterization on solid medium, S. aureus strains were precultured for 24 h at 37 °C under continuous shaking starting from a single colony. Cultures were then diluted to 10−5–10−7 and an aliquot of 100 μl was plated on TSA plates. The plates were incubated for 5 days at 37 °C under atmospheric and 5% CO2 conditions. The 5% CO2 level was achieved in a CO2 incubator (Heraeus Instruments). The colony size and appearance on TSA was observed every 24 h for 5 days and documented with a Leica M125 stereomicroscope. For growth characterization in liquid medium, S. aureus cells were precultured in TSB as described above. S. aureus strains involved were WT HG001, ΔmpsA, ΔmpsB, ΔmpsC, and ΔmpsABC that were transformed with pRB473-mpsA, pRB473-mpsB, pRB473-mpsC, and pRB473-mpsABC, respectively. Main cultures were inoculated to OD578 = 0.05 and grown under atmospheric and 5% CO2 conditions at 37 °C under continuous shaking. Aliquots were taken at 2, 4, 6, 8, 10, 12, 24, 48, and 72 h for OD578 measurements.

Growth studies of ΔmpsABC with bicarbonate supplemented media

Media were supplemented with NaHCO3. Precultures were grown as described above. Main cultures were cultivated as described above as well, but with the addition of the supplements at final concentrations of 1, 5, 10, and 50 mM and grown under atmospheric conditions. ΔmpsABC grown under atmospheric and 5% CO2 conditions were used as controls.

Complementation experiments of ΔmpsABC and EDCM636

With regards to S. aureus ΔmpsABC complemented with can from E. coli, the cultures were inoculated and were adjusted to OD578 = 5, then the strains were streaked on agar plates containing no xylose or 0.5% xylose (filter sterilized). Complementation of EDCM636 with pRB473-mpsA, pRB473-mpsB, pRB473-mpsAB, and pRB473-mpsABC, were also performed as described above, with the exception that BM and BMA were used instead of TSB and TSA.

Construction of the S. aureus deletion mutants

All oligonucleotides used in this study are listed in Supplementary Table 2. Nucleotide and amino acid sequences were obtained from the Kyoto Encyclopedia of Genes and Genomes (KEGG). The deletion mutants S. aureus HG001 ΔmpsB (KEGG accession no. SAOUHSC_00413) and ΔmpsC (SAOUHSC_00414) were constructed as markerless deletions using allelic replacements as described by Bae and Schneewind37. Briefly, 1 kb upstream and 1 kb downstream of mpsB and mpsC, respectively were amplified from the chromosomal DNA of S. aureus HG001. The fragments were assembled with linearized (Bg1II restriction enzyme) plasmid pBASE638 by Gibson assembly39 using Hi-Fi DNA Assembly Master Mix (New England Biolabs). The resulting plasmids were first introduced into E. coli DC10B40 and then into S. aureus RN4220 via electroporation before transformation of S. aureus HG001. Deletion of the genes were confirmed by PCR and sequence analysis. For S. aureus HG001 ΔmpsA and ΔmpsABC, pKOR137 carrying up- and downstream flanking regions of 2 kb each for both deletions12 were used.

Construction of complementation vectors

Complementation of ΔmpsB was carried out with plasmid pCtufamp41 and ΔmpsC with plasmid pRB47342. For construction of complementation vector for mpsB, mpsB was amplified and then assembled into linearized pCtufamp plasmid (HindIII and PacI restriction enzyme) by Gibson assembly. As for construction of complementation vector for mpsC, the putative native promoter sequence for mpsABC as well as mpsC were amplified and then inserted into linearized pRB473 (EcoRI restriction enzyme). The putative promoter regions were determined by DNA sequence analysis. The constructed plasmids were first introduced into E. coli DC10B then into S. aureus RN4220 before being transformed into S. aureus HG001 ΔmpsB and ΔmpsC, respectively. For complementation of ΔmpsA and ΔmpsABC, recombinant vector plasmids pRB473-mpsA and pRB473-mpsABC from previous study12 were isolated and the corresponding deletion mutants were transformed as described above. In addition, all constructed pRB473 derivatives were transformed into EDCM636, an E. coli MG1655 derivative harboring a kanamycin resistance marker replacing a deletion of the CA encoding gene can. It was purchased from E. coli Genetic Stock Center, Yale University. Additional complementation vectors pRB473-mpsB and pRB473-mpsAB were constructed and transformed into EDCM636, including the empty vector.

Construction of pTX30-can

The xylose inducible plasmid pTX3043 was used for expression of can (KEGG accession no. b0126). Therefore, can was amplified from the chromosomal DNA of E. coli MG1655. The insert was inserted into the linearized pTX30 (BamH1 and EcoR1 restriction enzymes) using T4 DNA ligase (Thermo Scientific). The resulting plasmids was transformed into S. aureus RN4220 via electroporation before being transformed into ΔmpsABC.

Quantitative RT-PCR

qRT-PCR was carried out to determine the gene expression of mpsA in three WT S. aureus strains, namely HG001, USA30044, and MW245 under atmospheric and 5% CO2 conditions. All bacteria precultures were precultivated in atmospheric and 5% CO2 conditions, respectively, for 24 h. Main cultures were inoculated at an OD578 = 0.1 for each strain and grown in its respective growth conditions for 3 hrs. Subsequently an aliquots of OD578 = 2.0 were harvested. RNA isolation was carried out using a RNeasy Mini kit (Qiagen) according to manufacturer’s instructions. The resulting RNA was treated with RQ1 RNase-Free DNase (Promega). Subsequently, the RNA was analyzed for DNA contamination using ReproFast DNA Polymerase (Genaxxon Bioscience) with no-RT control PCR. Power SYBR® Green RNA-to-CT™ 1-Step Kit (Applied Biosystems) was used in AviaMx Real-Time PCR System (Agilent Technologies) with primers directed to mpsA using 50 ng of RNA as template in each reaction. DNA gyrase subunit B (gyrB) was used as housekeeping gene control. The RNA used in qRT-PCR was isolated from four independent experiments. The relative expression of mpsA under 5% CO2 was normalized to its corresponding strains grown in atmospheric conditions.

Bicarbonate uptake analysis

Main cultures were inoculated to an OD578 = 0.1 and grown until exponential growth phase for 3 h (S. aureus HG001) and 18 h (ΔmpsABC). Cells were then centrifuged and washed with 10 mM Tris buffer at pH 7. Cells were resuspended in Tris buffer and adjusted to OD578 of 1 in a final volume of 10 ml. Fluorocitrate and glucose at a final concentration of 10 mM and 5 mM, respectively, were added to both cell suspensions before incubated at room temperature with magnetic stirring for 30 min. After that, 50 μCi of NaH14CO3 (specific activity 58 mCi mmol−1, Hartmann Analytic) was added. One milliliter of samples was collected at time 0 (before the addition of NaH14CO3), 0.5, 1, 2, 4, 6, 8, 10, and 15 min. After each sample was collected, cells were immediately filtered by vacuum filtration onto membrane filters (WhatmanTM ME 25 mixed cellulose ester membrane filters 0.45 μm) and washed with 10 ml of Tris NaCl buffer (10 mM Tris with 100 mM NaCl). The membrane filters were then placed in a vial containing 10 ml of liquid scintillation cocktail (Ultima Gold, PerkinElmer). Radioactivity retained on the membrane filters was taken as H14CO3 uptake which was determined by 14C accumulation in cells, measured by liquid scintillation counting (LKB Wallac 1209 RackBeta liquid scintillation counter). Results were recorded as counts per minute (CPM).

Hemolysis assay

To analyze hemolytic toxin production, overnight cultures of HG001 ΔmpsA, ΔmpsB, and ΔmpsABC grown in 5% CO2 were used. Each bacterial strain was adjusted to an OD578 of 2 and streaked onto blood agar (Oxoid). In addition, to better visualize the hemolysin halo zones, cultures were grown in atmospheric (16 h for HG001 and 48 h for ΔmpsA) and in 5% CO2 conditions (16 h for both HG001 and ΔmpsA). An aliquot of same OD578 was collected for each strain before being centrifuged to remove the cell pellets. The remaining supernatant was filtered and concentrated with SpeedVac. The concentrated supernatant was then dropped into blood agar. All plates were incubated at 37 °C under atmospheric and 5% CO2 conditions respectively for 24 h before subjected to cold shock treatment for 72 h.

Galleria mellonella larvae infection model

Final-stage instar larvae of G. mellonella were purchased from, Germany. Ten larvae weighing between 300 and 600 mg were infected with S. aureus HG001 and ΔmpsA, respectively. Bacteria were grown in TSB at 37 °C with shaking for 24 h (HG001) and 48 h (ΔmpsA). Cells were washed twice and resuspended in Dulbecco’s Phosphate-Buffered Saline (DPBS) (GibcoTM) before being adjusted to an OD578, which corresponds to 5 × 108 colony-forming unit (CFU) for each strain. Each larva was injected with 5 × 106 cells. Larvae injected with DPBS served as control group. The larvae were incubated at 37 °C for 5 days after infection and surviving larvae were counted every day starting from 24 h after infection. The experiments were replicated four times. Data collected from each independent experiment were pooled for statistical analysis, resulting in n= 40 for every strain.

Membrane potential measurement

Main cultures were grown to exponential growth phase for HG001 (3 h in atmospheric and 5% CO2, respectively) and also for ΔmpsABC (18 h in atmospheric and 3 h in 5% CO2 conditions). Cells were washed once in phosphate-buffered saline (PBS) before adjusted to an OD578 of 0.4. Membrane potential was determined using BacLight bacterial membrane potential kit (Invitrogen) according to the manufacturer’s protocol. Briefly, 10 μl of the dye 3,3′-diethyloxacarbocyanine iodide (DiOC2[3]) was added to the bacterial suspension samples and incubated for 30 min. Then, 200 μl of the stained or unstained sample was applied to a black, flat-bottomed 96-well plate to determine the red and green fluorescence intensity using a microplate reader (Tecan Infinite M200). Excitation and emission wavelengths were chosen as recommended by the kit’s protocol. The fluorescence intensities of wild-type HG001 grown in atmospheric was set equal to 100%.

Mouse infection experiments

Overnight cultures of HG001 and ΔmpsA in Brain Heart Infusion Broth (BHI) medium were diluted to a final OD600 of 0.05 in 50 ml fresh BHI medium and grown until exponential growth phase (3.5 h for HG001 and 6 h for ΔmpsA) at 37 °C with 5% CO2. After centrifugation, the cell pellet was resuspended in BHI with 20% glycerol, aliquoted and stored at −80 °C. For the generation of in vivo infection, aliquots were thawed and washed twice with PBS. The infectious dose used for infection was very similar for both strains (2.1 × 108 CFU/HG001 and 1.7 × 10 CFU/ΔmpsA in 20 μl). A sample of the infection inoculum was plated on TSB agar plates in order to control the infection dose. For the intranasal S. aureus infection model (pneumonia model) we used female Balb/c mice (8 or 9 per group, 6 weeks, Janvier Labs, Le Genest-Saint-Isle, France). They were intranasally infected with 2.1 × 108 CFU of HG001 and with 1.7 × 108 CFU of ΔmpsA. During infection, mice were scored twice a day and the severity of infection was determined accordingly to recognize if humane endpoint was reached. After 48 h of infection, mice were sacrificed, the lungs, kidneys, and livers recovered, homogenized and plated in serial dilutions on TSB agar plates incubated overnight at 37 °C with 5% CO2 in order to determine the bacterial burden. Significant difference in the CFU counts in the organs between the two groups was determined with Mann–Whitney test.

Ethics statement

All of the animal studies were approved by the local government of Lower Franconia, Germany (approval number 55.2-2532-2-155) and performed in strict accordance with the guidelines for animal care and experimentation of German Animal Protection Law and the DIRECTIVE 2010/63/EU of the EU. The mice were housed in individually ventilated cages under normal diet in groups of four to five throughout the experiment with ad libitum access to food and water.

Phylogenetic analysis of mpsA and mpsB homologs

Homologs of mpsA (YP_498998.1) and mpsB (YP_498999.1) from S. aureus were identified from the RefSeq database46 using Microbial Protein BLAST. All searches were either conducted within the whole Bacteria domain, or restricted to the bacterial phylum Firmicutes or the bacterial genus Staphylococcus. Since several species have more than one putative homologs of mpsA and mpsB, we restricted the hits only to those protein pairs of mpsA and mpsB, whose coding sequences, extracted from the respective GenBank files, are in immediate proximity in the genome. The protein sequences of mpsA and mpsB homologs were aligned separately using Clustal Omega (version 1.2.1)47. The multiple sequence alignments (MSAs) were subsequently concatenated into one single MSA comprising 350 taxa (Bacteria), 83 taxa (Firmicutes), and 29 (Staphylococcus), respectively. Phylogenetic trees were constructed using maximum likelihood (ML) analysis provided by the program RAxML (version 8.2.9)48. The GAMMA Model of rate heterogeneity was used and all model parameters were estimated by RAxML. LG (Bacteria, Staphylococcus) and JTT (Firmicutes) with empirical base frequencies were determined to be the best-scoring (likelihood score) protein substitution model. Results were assessed using 100 bootstrap replicates. The best tree was visualized using TreeGraph2 (version 2.14.0–771 beta)49.

Occurrence of MpsAB and CA homologs based on PFam domains

The occurrence of MpsAB and CA homologs were inferred based on PFam domains21 search from finished bacterial genomes in Integrated Microbial Genomes & Microbiomes (IGM/G) database50. MpsA, MpsB, prokaryotic type-CA, and eukaryotic-type CA belongs to PFam00361, PFam10070, PFam00484, and PFam00194, respectively. Results were presented as the presence (if yes, the frequency it was found in a particular species) or absence of the respective PFam domains.

CA assays

CA assay was performed using purified N-terminal strep-tagged MpsB protein. Two methods were used to detect CA activity, electrometric and colorimetric methods. The electrometric method refers to enzymatic assay of CA for Wilbur-Anderson Units (EC, as listed in the website of Sigma-Aldrich (document CR BIOT-MAJ-1013), based on cited references51,52,53. One Wilbur-Anderson unit will cause the pH of a 20 mM Trizma buffer to drop from 8.3 to 6.3 per minute at 0 °C. The assay is briefly described here and the full protocol can be found on Sigma-Aldrich’s website54. Assay buffer was prepared at 20 mM using Trizma Base and purified water (Milli-Q) and the pH was adjusted to 8.3 with 2 N Sulfuric Acid. CO2 saturated solution was used as substrate and was prepared by placing a small piece of dry ice into cold Milli-Q water for at least 30 min prior to the experiment. CA enzyme standard solution was used as control. It was prepared fresh prior to the experiment by dissolving 2 mg of CA from bovine erythrocytes lyophilized powder, ≥2000 W-A units mg−1 protein (Sigma-Aldrich, Germany). Then the concentrated standard solution was diluted to 60–90 U ml−1. This concentration corresponds to a reaction time between 10 and 20 s. The buffer reference standards (pH 4,7, and 10) and pH electrode to equilibrate to <3 °C before calibrating the pH meter with each of the reference buffer. All solutions and dram vials were kept cold on ice prior to use. To perform the blank reaction, 3 ml of ice cold assay buffer and 0.05 ml of ice cold purified water were pipetted into a dram vial with a micro stir bar. The temperature of the reaction mixture was checked with thermometer and proceed to the next step if the temperature was <3 °C, by placing the pH electrode in the solution, with stirring. After the pH had reached >8.5, 2 ml of ice cold CO2 saturated solution was added. The time required for the pH to change from 8.3 to 6.3 was recorded. This step was repeated a few times and once the blank time of 65 s was reached, the experiment proceeded immediately with CA control. For control, 3 ml of ice cold assay buffer was added to the dram vial and if the temperature was <3 °C and subsequently when the pH > 8.5, 2 ml of ice cold CO2 saturated solution was added to the reaction mixture. When the pH reached 8.4–8.5, 0.05 ml of CA standard solution was added. The time required for the pH to change from 8.3 to 6.3 was recorded. If the time is not in the 10–20 s range, a more concentrated enzyme standard must be prepared. If the blank average time (from a minimum of five blank values) was in the range of 70–100 s, the experiment could proceed with purified MpsB protein. The steps for MpsB protein were the same as control, in which 0.05 ml of MpsB was used instead of CA standard solution. The CA U ml−1 is determined as:

$${\mathrm{Units}}\;{\mathrm{ml}}^{ - 1}\;{\mathrm{enzyme}}:\frac{{\left( {{{T}}_{{\mathrm{blank}}\,{\mathrm{average}}}-{{T}}_{{\mathrm{sample}}\,{\mathrm{average}}}} \right){\mathrm{/df}}}}{{\left( {{{T}}_{{\mathrm{sample}}\;{\mathrm{average}}}} \right)\left( {0.05} \right)}}$$

where df = Dilution factor

T = Time (in seconds) required for the pH to change from 8.3 to 6.3 as per the Unit Definition

0.05 = Volume (in milliliter) of enzyme used

We found that this method is unreliable because of the difficulty in maintaining the temperature at <3 °C. Therefore, inconsistencies in the pH readings and subsequently the deviations in the time for the pH change from 8.3 to 6.3 resulted in inaccurate and non-reproducible readings. Therefore, we attempted another assay using colorimetric method. The colorimetric method to detect CA activity was performed according to previous studies20,55 with slight modifications. The assay was based on changing-pH/dye indicator method using a Tecan Infinite M200 injector system. Briefly, two reaction buffers were prepared: (a) a buffer using phenol red as indicator (200 mM), 50 mM HEPES, and 200 mM Na2SO4 at pH 6.5, 7, and 7.5, (b) a buffer using m-cresol purple as indicator (200 mM), 50 mM TAPS, and 200 mM Na2SO4 at pH 7.5 and 8.4. CO2 saturated water was prepared by placing a small piece of dry ice in Milli-Q water for at least 30 mins prior to the experiment. Purified MpsB protein was diluted in buffers and the reaction was initiated by adding an equivalent amount of CO2 saturated water with the Tecan injector system. The subsequent color changes of the pH-sensitive dye indicators were monitored by Tecan microplate reader every 0.2 s for 1 min at 558 nm (pH 6.5–7.5) or 578 nm (pH 7.5–8.4). All reactions were performed at room temperature (~25 °C) and in a final volume of 1 ml. The CA activities (if any) of MpsB protein and positive control CA from bovine erythrocytes lyophilized powder (Sigma-Aldrich, Germany) were measured at final concentrations of 100 and 0.1 μg ml−1, respectively. A total of 50 mM Tris-HCl at corresponding pH of the buffers was used as nonenzymatic controls. Due to the nondetectable CA activity, we repeated the assay with whole cell lysate of wild-type HG001, ΔmpsB, and ΔmpsABC with and without addition of NADH and finally with resting cell suspensions of the three strains. However, no detectable CA activity was observed.

Statistical analyses

Data are presented as mean values and SEM from at least three independent biological replicates unless specified otherwise. Data from the mouse experiment are presented as median values. Normal distributions were analyzed by Student's t-test. The larvae infection model was analyzed using Log-rank (Mantel–Cox) test. For the mouse infection experiments, two-tailed Mann–Whitney-test was employed to compare the difference of CFU counts in the organs between the mutant clones with the WT HG001. All statistical analyses were performed using GraphPad Prism 6.0 software. A p value of <0.05 was considered to be statistically significant, with n represents independent biological replicates.

Reporting summary

Further information on research design is available in the Nature Research Reporting Summary linked to this article.