The Arsenal of Leptospira Species against Oxidants

Reactive oxygen species (ROS) are byproducts of oxygen metabolism produced by virtually all organisms living in an oxic environment. ROS are also produced by phagocytic cells in response to microorganism invasion. These highly reactive molecules can damage cellular constituents (proteins, DNA, and lipids) and exhibit antimicrobial activities when present in sufficient amount. Consequently, microorganisms have evolved defense mechanisms to counteract ROS-induced oxidative damage. Leptospira are diderm bacteria form the Spirochaetes phylum. This genus is diverse, encompassing both free-living non-pathogenic bacteria as well as pathogenic species responsible for leptospirosis, a widespread zoonotic disease. All leptospires are exposed to ROS in the environment, but only pathogenic species are well-equipped to sustain the oxidative stress encountered inside their hosts during infection. Importantly, this ability plays a pivotal role in Leptospira virulence. In this review, we describe the ROS encountered by Leptospira in their different ecological niches and outline the repertoire of defense mechanisms identified so far in these bacteria to scavenge deadly ROS. We also review the mechanisms controlling the expression of these antioxidants systems and recent advances in understanding the contribution of Peroxide Stress Regulators in Leptospira adaptation to oxidative stress.


Introduction
Leptospira are aerobic diderm bacteria of the Spirochaetes phylum. They are thin, helicalshaped bacteria with a periplasmic endoflagellum, and highly motile organisms. Leptospira genus includes free-living bacteria that can be found in aqueous environments, as well as pathogenic species that can infect and colonize mammalian hosts. They are the causative agent of leptospirosis, a widespread zoonosis [1]. Dissemination of pathogenic Leptospira in the environment depends on reservoir hosts, mainly rodents, which are asymptomatic carriers. Leptospires chronically colonize the proximal renal tubules of these mammals and are excreted in the environment by their urine. Leptospires are transmitted to other animals and humans mostly by exposure to soils and water contaminated by the bacteria. Leptospira penetrate host organisms by abraded skins and mucosa, and they rapidly disseminate via the bloodstream to numerous tissues and organs including kidneys, liver, and lungs. Their remarkable motility, their ability to resist complement killing and avoid recognition by phagocytic cells, as well as a great adaptation to the host environment contribute to a rapid host colonization [1]. The zoonotic transmission also implies that pathogenic Leptospira are able to survive, presumably for a long time, in soils and water.
Leptospirosis symptoms range from a mild flu-like febrile state to more severe and fatal cases leading to hemorrhages and multiple organ failure. Patients with acute leptospirosis experience jaundice and renal failure (Weil's disease), severe pulmonary hemorrhages syndrome (SPHS), and meningitis [2]. The lack of specificity of the clinical manifestations associated with leptospirosis complicates the diagnosis of this disease which is often mistaken with other illnesses and consequently underdiagnosed. One million cases of severe leptospirosis are estimated annually worldwide with about 60,000 deaths [3]. However, Figure 1. Superoxide (O2 •− ), hydrogen peroxide (H2O2), and hydroxyl radical ( • OH) are rea ygen species (ROS) produced by the subsequent reduction in dioxygen (O2). In living or the dismutation or reduction in superoxide, catalyzed by superoxide dismutase (SOD) an tase (SOR), respectively, gives rise to hydrogen peroxide. Peroxidases and catalase catalyz drogen peroxide reduction or dismutation, respectively, into water. Superoxide can react w oxide (NO) to form peroxinitrite (ONO2 − ), and hydrogen peroxide can be transformed in chlorous acid (HOCl) in a reaction catalyzed by myeloperoxidases (MPO). The reactions ( constitute the Haber-Weiss reaction that produces dioxygen and hydroxyl radical from su and hydrogen peroxide, respectively. The reaction (2) is the Fenton reaction. Created with der (BioRender.com).
ROS have different reactivities. Hydroxyl radicals are by far the most reacti They can interact with almost all biomolecules, including proteins, DNAs and lip are believed to have a large spectrum of targets. On the contrary, O2 •− and H2O2 reactive and perform more specific oxidation. It should be noted though that as H2O2 are precursors of • OH, it is difficult to distinguish oxidative damage due to H2O2 from those occurring consequently to the accumulation of • OH. Using bacte tants that accumulate O2 •− and H2O2, it was shown that ROS induce DNA m [15,16]. The deoxyribose and base moieties can be oxidized and 8-oxo 7,8-dihydr sine is the major nucleotide modification observed in DNA in the presence of o [17]. All RNA molecules (rRNA, tRNA, and mRNA) are also vulnerable to oxid ROS and their oxidation reduces translation rate [18,19]. Strand breaks are also o when DNA and RNA are oxidized.
Protein backbones and lateral chains can be oxidized by ROS, which resul creased carbonyl content in proteins, protein-protein crosslinking and protein f tation [20,21]. Sulfur-containing amino acids are particularly susceptible to oxidati age. Disulfide bridges and cysteic acids are formed when cysteines are oxidized; nine sulfoxide and sulfone are products of methionine oxidation [22].
H2O2 interacts with iron located in iron-containing proteins leading to their i tion and fueling the Fenton reaction, the second step of the Haber-Weiss reaction 1, reaction 2) [23]. In addition, superoxide can extract iron from iron-sulfur clust tained in bacterial enzymes, leading to enzyme inactivation [24,25]. . In living organisms, the dismutation or reduction in superoxide, catalyzed by superoxide dismutase (SOD) and reductase (SOR), respectively, gives rise to hydrogen peroxide. Peroxidases and catalase catalyze the hydrogen peroxide reduction or dismutation, respectively, into water. Superoxide can react with nitric oxide (NO) to form peroxinitrite (ONO 2 − ), and hydrogen peroxide can be transformed into hypochlorous acid (HOCl) in a reaction catalyzed by myeloperoxidases (MPO). The reactions (1) and (2) constitute the Haber-Weiss reaction that produces dioxygen and hydroxyl radical from superoxide and hydrogen peroxide, respectively. The reaction (2) is the Fenton reaction. Created with BioRender (BioRender.com).

Endogenous Sources of ROS in Bacteria
Protein backbones and lateral chains can be oxidized by ROS, which results in increased carbonyl content in proteins, protein-protein crosslinking and protein fragmentation [20,21]. Sulfur-containing amino acids are particularly susceptible to oxidative damage. Disulfide bridges and cysteic acids are formed when cysteines are oxidized; methionine sulfoxide and sulfone are products of methionine oxidation [22]. H 2 O 2 interacts with iron located in iron-containing proteins leading to their inactivation and fueling the Fenton reaction, the second step of the Haber-Weiss reaction ( Figure 1, reaction 2) [23]. In addition, superoxide can extract iron from iron-sulfur clusters contained in bacterial enzymes, leading to enzyme inactivation [24,25].

Endogenous Sources of ROS in Bacteria
In bacteria, several flavin-or quinones-containing enzymes from the respiratory chain are potent electron donors that enhance O 2 •− production from electron leaking [26,27]. In addition, superoxide dismutase and reductase enzymes catalyze the dismutation and reduction in superoxide into H 2 O 2 ( Figure 1). Iron released from haem group, iron-sulfur clusters, or mononuclear iron enzymes will be engaged in the Fenton reaction that generates hydroxyl radicals from H 2 O 2 ( Figure 1).
The intracellular concentrations of H 2 O 2 and O 2 •− in E. coli have been estimated to 20-50 nM and 200 nM, respectively [11,28]. Inactivation of several enzymes detoxifying H 2 O 2 can increase the amount of the steady state level of this ROS to 2 µM, resulting in growth defect [28]. One important question is to determine to what extent the level of ROS produced physiologically is harmful for the bacteria or whether ROS might rather act as signaling molecules when present at a tolerable amount as observed in eukaryotes.

Exogenous Sources of ROS Encountered by Bacteria
In addition to ROS produced endogenously, living organisms are exposed to ROS produced in the outside environment by ionizing radiation, UV light, and a large variety of chemicals (e.g., paraquat/methyl viologen) [29,30] (Figure 2).
The intracellular concentrations of H2O2 and O2 •− in E. coli have been estimated to 20-50 nM and 200 nM, respectively [11,28]. Inactivation of several enzymes detoxifying H2O2 can increase the amount of the steady state level of this ROS to 2 μM, resulting in growth defect [28]. One important question is to determine to what extent the level of ROS produced physiologically is harmful for the bacteria or whether ROS might rather act as signaling molecules when present at a tolerable amount as observed in eukaryotes.

Exogenous Sources of ROS Encountered by Bacteria
In addition to ROS produced endogenously, living organisms are exposed to ROS produced in the outside environment by ionizing radiation, UV light, and a large variety of chemicals (e.g., paraquat/methyl viologen) [29,30] (Figure 2).

Figure 2.
Exposition of Leptospira to ROS. Leptospira spp. are potentially exposed to ROS produced endogenously as a result of electron leakage from the respiratory chain. The putative complexes forming the respiratory chain in pathogenic Leptospira, complex I (encoded by LIMLP_00745-00750, LIMLP_03705-03760 in L. interrogans serovar Manilae), complex II (encoded by LIMLP_09980-09990 in L. interrogans serovar Manilae), complex IV (encoded by LIMLP_01080-01085, LIMLP_01375, LIMLP_01100-01110 in L. interrogans serovar Manilae), and complex V (encoded by LIMLP_06045-06080 in L. interrogans serovar Manilae) are represented. Leptospira spp. also face ROS produced in the environment (waters and soils). In addition, pathogenic species are exposed to ROS produced by the host phagocytic cells or tissues. The host mitochondria are one of the main ROS producers. Created with BioRender (BioRender.com).
Commensal, symbiotic, and pathogen bacteria are exposed to ROS produced inside their eukaryotic hosts. Macrophages and neutrophiles contain an inducible NADPH-dependent oxidase (Phox) that produces superoxide in response to the detection of invading pathogens [31,32]. As described above, superoxide can be dismutated to H2O2 through a SOD-catalyzed reaction and H2O2 is further processed in hydroxyl radicals. In neutrophiles, H2O2 reacts with chloride ions to generate hypochlorous acid through a reaction catalyzed by myeloperoxidase (MPO) (Figure 1) [33]. In addition, superoxide can interact with nitric oxide (NO • ) produced in phagocytes by an inducible nitric oxide oxidase to form peroxynitrite (ONO2 − ). Of note, NO • and ONO2 − are reactive nitrogen species (RNS) that are as oxidative as ROS [34].
Phagocytes are not the only eukaryotic cells that produce oxidants. Indeed, NADPH oxidases (Nox and Duox) are also expressed in a variety of other cell types including   Figure 2. Exposition of Leptospira to ROS. Leptospira spp. are potentially exposed to ROS produced endogenously as a result of electron leakage from the respiratory chain. The putative complexes forming the respiratory chain in pathogenic Leptospira, complex I (encoded by LIMLP_00745-00750, LIMLP_03705-03760 in L. interrogans serovar Manilae), complex II (encoded by LIMLP_09980-09990 in L. interrogans serovar Manilae), complex IV (encoded by LIMLP_01080-01085, LIMLP_01375, LIMLP_01100-01110 in L. interrogans serovar Manilae), and complex V (encoded by LIMLP_06045-06080 in L. interrogans serovar Manilae) are represented. Leptospira spp. also face ROS produced in the environment (waters and soils). In addition, pathogenic species are exposed to ROS produced by the host phagocytic cells or tissues. The host mitochondria are one of the main ROS producers. Created with BioRender (BioRender.com).
Commensal, symbiotic, and pathogen bacteria are exposed to ROS produced inside their eukaryotic hosts. Macrophages and neutrophiles contain an inducible NADPHdependent oxidase (Phox) that produces superoxide in response to the detection of invading pathogens [31,32]. As described above, superoxide can be dismutated to H 2 O 2 through a SOD-catalyzed reaction and H 2 O 2 is further processed in hydroxyl radicals. In neutrophiles, H 2 O 2 reacts with chloride ions to generate hypochlorous acid through a reaction catalyzed by myeloperoxidase (MPO) (Figure 1) [33]. In addition, superoxide can interact with nitric oxide (NO • ) produced in phagocytes by an inducible nitric oxide oxidase to form peroxynitrite (ONO 2 − ). Of note, NO • and ONO 2 − are reactive nitrogen species (RNS) that are as oxidative as ROS [34].
Phagocytes are not the only eukaryotic cells that produce oxidants. Indeed, NADPH oxidases (Nox and Duox) are also expressed in a variety of other cell types including epithelium and endothelium. As a matter of fact, H 2 O 2 is detected in lungs [35], kidneys [36], ocular tissues [37], as well as in fluids such as urine [38,39] and blood [37].
Oxidative respiration in mitochondria, present in phagocytic cells or in tissues, is another source of ROS in eukaryotes [40]. Electrons are shuttled through the electron transport chain complexes I-IV located in the mitochondrial inner membrane. Electron leaking from the electron transport chain and their improper transfer to oxygen results in superoxide production. Production of ROS in mitochondrial matrix is stimulated by pathogen-associated molecular patterns (PAMPs) [41].
Attempts to estimate the concentration of oxidants inside a phagosome suggested that 2-50 µM O 2 •− and 1-4 µM H 2 O 2 are produced by macrophages [42] and neutrophils would contain 25 µM O 2 •− [43]. An estimated concentration of 10-200 pM O 2 •− is present in the mitochondrial matrix [40]. ROS produced by the host have bactericidal activities, but they also participate in the activation of other antibacterial pathways of the innate immunity including generation of extracellular traps by the neutrophiles (NETosis) and production of pro-inflammatory molecules.

Are Leptospira Exposed to ROS in Their Different Ecological Niches?
Leptospira species are aerobic bacteria that possess a pathway for oxidative phosphorylation ( Figure 2). Genes encoding putative NADH dehydrogenase (LIMLP_00745-00750, LIMLP_03705-03760), succinate dehydrogenase (LIMLP_09980-09985), cytochrome C oxidases (LIMLP_01080-01085, LIMLP_01375, LIMLP_01100-01110), and a F1 ATP-synthase complex (LIMLP_06045-06080) are annotated in the pathogen L. interrogans genomes (serovar Manilae strain UP-MMC-NIID LP) [44]. The endogenous production of ROS has never been measured in Leptospira, but it is very likely that these bacteria also produce oxidants as a result of electron leaking from the respiratory chain.
Most Leptospira species are free-living organisms that can be isolated from soils, freshwaters, stagnant waters, sewage, and even drinking water [45][46][47][48]. Surface soils and waters are well-oxygenated and exposed to sunlight energy. All these aquatic and soil microcosms contain ROS arising from abiotic reactions and from soil microbiome and plants [49,50]. Studies establishing a correlation between Leptospira survival and soil composition are scarce. Lall et al. [51] have shown that the presence of Leptospira correlates with the presence of iron, copper, and manganese, metals that exacerbate ROS production. Even though there are no studies that have measured the level of ROS in microcosmos-containing Leptospira, it is reasonable to conjecture that leptospires are exposed to oxygen byproducts in their freeliving lifestyle ( Figure 2). Furthermore, Leptospira have been shown to form aggregates [52] and biofilms [45,53] in aquatic environments and to what extent these lifestyles protect them from oxidative stress, remains to be evaluated.
Pathogenic Leptospira species are mainly extracellular bacteria that escape phagocytosis by host immune cells. They colonize different tissues including lung, kidney, and liver, that are highly oxygenated and therefore ROS producers [54] (Figure 2). Several studies have evaluated whether leptospirosis correlated with an increased oxidative stress in the host. Blood of leptospirosis patients contains a higher amount of ROS and NO • , and a lower amount of gluthathione (GSH), an anti-oxidant, than healthy individuals [55,56]. A correlation between leptospirosis and oxidative stress has also been observed in infected animals [57,58].
A higher number of circulating neutrophiles has been reported during human leptospirosis [59] and NETosis has been implicated in leptospires killing [60,61], but pathogenic Leptospira remain at the surface of neutrophiles without triggering ROS production by MPO [62]. Interestingly, the non-pathogenic strain, L. biflexa, exhibit a different behavior in the same condition as they were found inside phagocytic vacuoles of neutrophiles and they triggered ROS production [62]. This might indicate that pathogenic Leptospira species are able to efficiently detoxify extracellular ROS whereas saprophytes do not.
Establishing a correlation between ROS production and infection by leptospires does not necessarily prove that the level of ROS produced by the host threatens Leptospira survival. Instead, the demonstration that these pathogens are confronted to deadly ROS during infection is founded on a study by Eshghi et al. [70], showing that catalase mutants of L. interrogans are avirulent. There is, therefore, compelling evidence that pathogenic Leptospira are exposed to a host-triggered oxidative stress during infection and that their ability to withstand this stress is important for their virulence.

Defenses against ROS
Defenses against ROS include non-enzymatic low molecular weight molecules which act as thiol-redox buffers, detoxification enzymes that breakdown ROS and repair machineries that reverse oxidative damage to molecules.

Catalase and Peroxidases
Catalases and peroxidases are oxidoreductases that catalyze H 2 O 2 breakdown. Catalase degrades two molecules of H 2 O 2 into H 2 O and O 2 through a dismutation reaction ( Figure 3). They are classified in three main groups: monofunctional catalases, bifunctional catalase-peroxidases, and manganese-containing catalases (reviewed in [71]). Mono-and bifunctional catalases use heme prosthetic group as a cofactor for oxidoreduction whereas manganese-containing catalases are non-heme enzymes that use manganese ions for oxidoreduction. In addition to classical catalase activity, bifunctional catalases also bear a peroxidase activity.
have shown that macrophages infected with leptospires produced a higher amount of ROS [68,69].
Establishing a correlation between ROS production and infection by leptospires does not necessarily prove that the level of ROS produced by the host threatens Leptospira survival. Instead, the demonstration that these pathogens are confronted to deadly ROS during infection is founded on a study by Eshghi et al. [70], showing that catalase mutants of L. interrogans are avirulent. There is, therefore, compelling evidence that pathogenic Leptospira are exposed to a host-triggered oxidative stress during infection and that their ability to withstand this stress is important for their virulence.

Defenses against ROS
Defenses against ROS include non-enzymatic low molecular weight molecules which act as thiol-redox buffers, detoxification enzymes that breakdown ROS and repair machineries that reverse oxidative damage to molecules.

Catalase and Peroxidases
Catalases and peroxidases are oxidoreductases that catalyze H2O2 breakdown. Catalase degrades two molecules of H2O2 into H2O and O2 through a dismutation reaction ( Figure 3). They are classified in three main groups: monofunctional catalases, bifunctional catalase-peroxidases, and manganese-containing catalases (reviewed in [71]). Mono-and bifunctional catalases use heme prosthetic group as a cofactor for oxidoreduction whereas manganese-containing catalases are non-heme enzymes that use manganese ions for oxidoreduction. In addition to classical catalase activity, bifunctional catalases also bear a peroxidase activity. The dismutation of H2O2 into water and dioxygen (O2) by heme-using catalases is a two-step reaction. In a first step (1), one molecule of H2O2 is reduced into water in a reaction where the heme ferric porphyrin (Por-Fe 3+ ) acts as an electron donor and is oxidized into an oxoferryl porphyrin cation radical (Por •+ -Fe 4+ =O). In a second step (2), a second molecule of H2O2 is oxidized into O2, allowing the regeneration of the ferric porphyrin. (c) Glutathione peroxidases (GPx) and glutaredoxin (Grx), which are oxidized during peroxide reduction or glutathionylation, use glutathione (GSH) as cofactors to regenerate their reduced forms, whereas the oxidized peroxiredoxin (PrXox) is reduced by thioredoxin (Trx). The glutathione    Pathogenic Leptospira species express a monofunctional heme-containing catalase (encoded by LIMLP_10145, katE, in L. interrogans) (Figure 4). the glutathione reductase (GR) and thioredoxin reductase (TrxR), respectively. The NADPH/NAD is the redox couple involved in these reactions. (d) A simplified H2O2 reduction reaction by cy chrome C peroxidase (CCP) is represented. The CCP-bound heme is first reduced by the cytochro C (CytC-Fe 2+ ). The activated CCP reduces H2O2 into 2 molecules of H2O using the electron of reduced heme.
Far ahead the availability of Leptospira genomes, two studies demonstrated that a catalase activity can be detected in several strains of pathogenic Leptospira [78,79]. This catalase is localized in the periplasm of Leptospira and its inactivation showed that not only this catalase is the major H 2 O 2 detoxification enzyme but its activity is required for virulence in L. interrogans [70]. KatE is the second gene of an operon with LIMLP_10150 which encodes an ankyrin repeat-containing protein [80]. This operon is up-regulated in the presence of H 2 O 2 [80], at 37 • C [81,82], and when Leptospira are cultivated within a dialysis membrane chamber implanted in rat peritoneal cavities [83,84]. The function of the LIMLP_10150-encoding protein is unknown but similar ankyrin repeat-containing proteins have been shown to interact with and promote the catalase activity in other bacteria [85][86][87]. It has been proposed that the ankyrin domain-containing protein stabilizes the catalase in a proper conformation or orientation to promote H 2 O 2 entry in the active site [85] or heme binding [86]. Corin et al. [88] showed that saprophytes such as L. biflexa did not exhibit a detectable catalase activity even though genome sequencing showed the presence of a bifunctional catalase-peroxidase encoded by katG (LEPBIa2495) in saprophytes.
Peroxidases reduce H 2 O 2 into H 2 O using an electron donor (thioredoxin, NADH, and NADPH) (Figure 3) (reviewed in [89]). They have a larger spectrum of substrates than catalases and they also reduce organic hydroperoxides (RO 2 H) into their corresponding alcohols (ROH). They are classified into two families, i.e., thiol peroxidases and cytochrome C peroxidases. Thiol peroxidases reduce H 2 O 2 and organic hydroperoxides by a mechanism involving the oxidation of catalytic cysteine residues (formation of a cysteine sulfenic acid and disulfide bond). They are further subclassified in different families according to the disulfide reductase system that regenerates the oxidized peroxidase into an active reduced peroxidase. For instance, the bacterial alkylhydroperoxidase, AhpC, most often uses AhpF, a NADH:disulfide oxidoreductase flavoprotein, as reductase. However, in some bacteria (Mycobacterium tuberculosis and Helicobacter pylori), AhpF is absent and AhpC is reduced by a thioredoxin (Trx) and a thioredoxin reductase (TrxR) (Figure 3). Both AhpF and the TrxR are finally reduced by NADPH.
An AhpC-encoding ORF has been identified in L. interrogans (LIMLP_05955, AhpC1) but this species belongs to the category of bacteria that do not possess AhpF whereas L. biflexa genome encodes two AhpC paralogs (AhpC1, LEPBIa1358 and AhpC2, and LEPBIa3009) and one AhpF (LEPBIa3008) (Figure 4). A role of L. interrogans AhpC1 in degrading peroxides was first shown in vitro using a recombinant protein and by overexpressing leptospiral ahpC1 in E. coli [90]. The Trx/TrxR system that reduces AhpC1 has not been identified in L. interrogans; however, the system encoded by trxA (thioredoxin LIMLP_09870) and trxRB (thioredoxin reductase LIMLP_07165) was shown to have a reducing activity in vitro in the presence of NADPH, suggesting that its function can be to reduce AhpC1 in vivo. Inactivation of ahpC1 in L. interrogans impaired their ability to grow in the presence of paraquat, a superoxide-generating compound, but it did not in the presence of H 2 O 2 [80]. This was surprising as ahpC1, as well as trxA and trxRB, are up-regulated in the presence of H 2 O 2 [80]. This can be explained by the fact that H 2 O 2 produced exogenously would be mainly reduced by the periplasmic catalase present in pathogenic Leptospira before it can reach the cytoplasm. In this scenario, AhpC1 would reduce H 2 O 2 present in Leptospira cytoplasm, as arising for instance by superoxide reduction.
The bacterioferritin comigratory protein (BCP), thiol peroxidase (Tpx), and Glutathione peroxidase (Gpx) have peroxidase activities demonstrated in vitro against H 2 O 2 and organic peroxide, even though the physiological reducing systems devoted to their regeneration is not always known [91][92][93][94]. These enzymes contribute to some extent to peroxide breakdown in vivo in several bacteria [91,93,[95][96][97][98][99] but in which exact particular condition they fulfill their function is a matter of discussion [100]. Leptospira genomes contain ORFs annotated as BCP (LIMLP_18310), Tpx (LIMLP_03630), and Gpx (LIMLP_13255, LIMLP_17550). Neither the enzymatic activities nor the functions of the proteins encoded by these ORFs have been characterized. However, the up-regulation of BCP and Gpx-encoding ORFs in the presence of H 2 O 2 in L. interrogans suggests a role in defense against ROS [80].
The second main family of peroxidases are cytochrome C peroxidases (CCP) that catalyze the reduction in H 2 O 2 using electrons from cytochrome C. In bacteria, CCPs are dimeric proteins where each monomer contains two, or more rarely three, heme binding domains (reviewed in [101]). They are located in the periplasm and can be soluble or anchored to inner or outer membranes. Electrons are first transferred from cytochrome C to the high potential (hp) heme-binding domain, at the C-terminus of the protein. Then, the electrons are transferred from the reduced hp heme-binding domain to the low potential (lp) heme-binding domain located at the N-terminus of the protein. The lp heme-binding domain contains the binding site for H 2 O 2 . After two consecutive electron transfers from the hp heme-binding domain, H 2 O 2 is reduced into two molecules of water (Figure 3d). One role of CCPs is to detoxify exogenous H 2 O 2 that have accumulated in the periplasm. Recently, Khademian and Imlay [102] proposed that CCP can also be a reductase allowing H 2 O 2 to act as final electron acceptor under anaerobic condition.
L. interrogans and biflexa each encode 4 ORFs annotated as CCP (LIMLP_02795, LIMLP_04655, LIMLP_05260 and LIMLP_14625; LEPBIa1208, LEPBIa2430, LEPBIa2855, and LEPBIa5260). However, two of them (LIMLP_05260 and LIMLP_14325; LEPBIa3120 and LEPBIa1208) are probably MauG-like proteins involved in the methylamine metabolism pathway, as suggested by the presence of a specific Tyr residue (Y338 in LIMLP_05260, Y291 in LIMLP_14325, Y351 in LEPBIa3120, Y339 in LEPBIa1208). The LIMLP_02795 ORF is dramatically up-regulated in the presence of H 2 O 2 [80], which suggests a role of the CCP encoded by this ORF either in detoxifying H 2 O 2 or using H 2 O 2 as electron acceptor. Yet, such a role remains to be experimentally demonstrated either by a biochemical characterization of the protein or phenotypic studies of a mutant inactivated in LIMLP_02795.

Low Molecular Weight (LMW) Thiol Redox Buffers
The best characterized LMW thiol molecule is glutathione (GSH), a tripeptide composed of glutamate, cysteine, and glycine. The glutamate and cysteine are linked by a peptide bound between the gamma-carboxyl of glutamate and the amino group of cysteine. The synthesis of GSH is catalyzed by gamma-glutamylcysteine ligase (GCL) and glutathione synthetase (GS) in E. coli, and GSH can reach a concentration estimated in the millimolar range [103]. This tripeptide bears a reactive sulfhydryl group that can maintain the redox of cells [104]. GSH can be oxidized into a disulfide-bonded form (GSSG). GSH and GSSG form a redox pair acting as an electron donor and acceptor in redox reactions. One role of GSH is to regenerate the reduced state of thiol enzymes such as glutathione peroxidase, peroxiredoxin, and glutaredoxin. GSH is also a cofactor of protein disulfide isomerases (PDIs) which catalyze the isomerization and reduction in disulfides. During these reactions, GSH is oxidized into GSSG (Figure 3c). To recover the pool of GSH and restore the redox buffer of bacteria, GSSG is reduced into GSH by the glutathione reductase.
Cysteine residues are particularly prone to oxidation giving rise to disulfide bonds and sulfenic acid (Cys-SOH). These oxidations are reversible but overoxidation into sulfunic and sulfonic acids (Cys-SO 2 H and Cys-SO 3 H) irreversibly modifies and damages proteins. To avoid this, GSH can form transient disulfide bridges with cysteines in proteins exposed to ROS. This modification is known as S-glutathionylation and is catalyzed by the glutathione S transferase (GST). Glutaredoxins catalyze the deglutathionylation to restore reduced cysteines.
Many enzymes of the GSH synthesis and metabolism can be identified in Leptospira genomes. Indeed, LIMLP_08995 and LIMLP_ 08990 encode putative GCL and GS, respectively, in L. interrogans. GST-encoding ORFs are also annotated in Leptospira genomes (LIMLP_02530, LIMLP_06655, and LIMLP_13670), so are glutaredoxins (LIMLP_08980, LIMLP_08985), GSH hydrolase (LIMLP_09000) that catalyzes GSH breakdown into cysteinylglycine and glutamate, and glutathione peroxidases (LIMLP_13255, LIMLP_17550). Importantly, GCL, GS, and glutaredoxin activities can be measured in L. interrogans lysates, demonstrating the existence of a GSH synthesis and metabolism in these bacteria [105]. Despite the absence of an ORF encoding a GR, such activity can be also detected in Leptospira lysates, but the redox system responsible for reducing GSSG is unknown. LIMLP_08950 is the phylogenetically closest ORF that can fulfill a GR function.
In Sasoni et al. [105], a much lower GSH content was detected in L. interrogans than in E. coli (60 and 1300 fmol for 10 7 L. interrogans and E. coli, respectively). The exact contribution of GSH in maintaining Leptospira redox is thus unclear. It is worth mentioning that the two glutaredoxins and one GST (LIMLP_13670) are up-regulated in Leptospira upon oxidative stress [80]. Another evidence of a participation of glutathionylation and deglutathionylation in the oxidative stress response of Leptospira is the finding that the two leptospiral glutaredoxins (encoded by LIC11809 and LIC11810, the homologs of LIMLP_08980 and LIMLP_08985 in L. interrogans serovar Copenhageni strain Fiocruz L1-130, respectively) can complement the growth defect of Saccharomyces cerevisiae mutants lacking the endogenous glutaredoxin in the presence of H 2 O 2 [106].

Superoxide Dismutase and Reductase
Superoxide is the precursor of many ROSs (including H 2 O 2 and • OH, see Figure 1) and defenses against superoxide are vital for many bacteria to survive. It is generally believed that all living organisms own systems for superoxide detoxification [107]. The most common enzymes in charge of superoxide removal are superoxide dismutase (SOD) and superoxide reductase (SOR). SOD are metalloenzymes that use a metal (Fe, Mn, Cu, Zn, or Ni) as electron acceptor and donor to catalyze the dismutation reaction of superoxide into H 2 O 2 and O 2 ( Figure 5). these bacteria [105]. Despite the absence of an ORF encoding a also detected in Leptospira lysates, but the redox system respons unknown. LIMLP_08950 is the phylogenetically closest ORF tha In Sasoni et al. [105], a much lower GSH content was dete in E. coli (60 and 1300 fmol for 10 7 L. interrogans and E. coli, respe bution of GSH in maintaining Leptospira redox is thus unclear. I the two glutaredoxins and one GST (LIMLP_13670) are up-reg oxidative stress [80]. Another evidence of a participation of glu tathionylation in the oxidative stress response of Leptospira is th tospiral glutaredoxins (encoded by LIC11809 and LIC1 LIMLP_08980 and LIMLP_08985 in L. interrogans serovar Copen 130, respectively) can complement the growth defect of Saccha lacking the endogenous glutaredoxin in the presence of H2O2 [1

Superoxide Dismutase and Reductase
Superoxide is the precursor of many ROSs (including H2O and defenses against superoxide are vital for many bacteria to lieved that all living organisms own systems for superoxide deto common enzymes in charge of superoxide removal are superox superoxide reductase (SOR). SOD are metalloenzymes that use or Ni) as electron acceptor and donor to catalyze the dismutati into H2O2 and O2 ( Figure 5).  In the superoxide dismutation reaction, one molecule of superoxide is oxidized into O 2 by transferring one electron to the SOD-bound metal. A second molecule of superoxide is then reduced into H 2 O 2 by gaining electron from the reduced SOD, restoring the initial state of the enzyme with no external reducer [108]. SODs are divided into three families according to the metals used for catalysis: Fe/MnSODs (SodB/SodA), Cu/ZnSODs (SodC), and NiSODs [107]. Fe-and MnSODs are closely related. Some members of this family strictly depend on either Fe 2+ or Mn 2+ , whereas others (the cambialistic SODs) can coordinate and be active with both metals. SODs are located in the cytosol (Fe/MnSOD, NiSOD) or in the periplasm (Cu/ZnSOD).
As opposed to the double reduction-oxidation mechanism catalyzed by SODs, ironbinding SOR enzymes only catalyze the reduction in the O 2 •− radical into H 2 O 2 ( Figure 5). This is a fundamental difference with SODs since oxidized SORs need to be reduced back to their initial state by a reducer. Rubredoxins have been identified as electron donors for SORs in the anaerobes Archaeoglobus fulgidus [109] and Desulfovibrio vulgaris [110].
Most bacteria possess one or several isoforms of SODs and/or SORs. Anaerobes would preferentially contain SORs since these enzymes allow removal of superoxide without producing oxygen. Saprophytic L. biflexa encode a Fe/MnSOD (LEPBIa0027) that shares 71% identity with the E. coli SodB ( Figure 4) and exhibits the amino acids required for Fe 2+ /Mn 2+ coordination (H27, H74, D157, and H161). Biochemical characterization is needed to determine whether L. biflexa SodB uses preferentially Fe 2+ or Mn 2+ for catalyzing superoxide removal or whether the two metals are interchangeable.
Surprisingly, neither SOD nor SOR orthologs have been identified in pathogenic Leptospira spp. [111]. These observations are also supported by a study showing absence of detectable SOD activity in L. interrogans cultures as opposed to L. biflexa [112]. It is interesting to note that SOR-like enzymes have been described in other pathogenic spirochetes such as Treponema spp. (TP0823) [113] and a functional MnSOD has been described in Borrelia spp. (BB0153) whose role is essential for virulence [114,115]. Therefore, pathogenic Leptospira spp. remain an enigma concerning their mechanism of superoxide tolerance, if any. It should be noted that only very few bacterial species are known to lack any enzymatic superoxide removal mechanism, one of them being Lactobacillus plantarum, which uses manganese as a superoxide scavenger [116,117]. SOD/SOR-independent mechanism of superoxide scavenging relying on manganese has also been observed in Neisseria gonorrhoeae [118], but this has never been explored in pathogenic Leptospira.

Regulation of the Oxidative Stress Response
Defenses against accumulation of deadly ROS in bacteria are tightly regulated transcriptionally in order to maintain intracellular ROS homeostasis adapted to the environment the bacteria are facing. There are several transcriptional regulators involved in the regulation of the adaptive response to oxidative stress, including OxyR, PerR, OhrR, and SoxRS. All these regulators have in common an ability to sense the presence of ROS through aminoacid oxidation and to trigger the appropriate transcriptional response, i. e., "oxidative stress regulon", that confers a better ability to survive under oxidative stress. Thus, ROS can also function in bacteria as signaling molecules to activate or derepress expression of target genes.
OxyR, PerR, OhrR, and SoxRS are not present in all bacteria but several of them can co-exist within the same bacterial species and their respective regulon may overlap to some extent.

OxyR
OxyR is a 34 kDa protein of the LysR transcriptional regulator family that selfassociates into a tetramer ( Figure 6). It is activated when an intramolecular disulfide bond is formed between two cysteine residues (C199 and C208, according to E. coli OxyR sequence) in the presence of H 2 O 2 or upon modification of the redox status of bacteria [119,120]. This leads to a conformational switch resulting into a higher affinity for DNA and favoring thereby the interaction of the RNA polymerase with DNA [121]. Oxidation of OxyR is reversible and the disulfide bridge is reduced by the glutaredoxin and thioredoxin systems [120]. When bound to DNA, oxidized OxyR mostly activates the expression of genes encoding proteins involved in H 2 O 2 removal (catalase, and alkyl hydroxyperoxidase), and in maintaining the thiol redox (glutathione oxidoreductase, glutaredoxin, thioredoxin, and thioredoxin reductase) [122,123]. OxyR regulon also encompasses genes involved in lowering the content of free iron (fur, dps, yaaA) in heme biosynthesis (hemH), and in iron-sulfur cluster assembly (sufABCDE, sufS) [124]. Similar to any canonical LysR transcriptional regulator, OxyR represses its own expression. Mutants inactivated in oxyR are generally more sensitive to H 2 O 2 than the WT strain [125,126]. transcriptional regulator, OxyR represses its own expression. Mutants inactivated in oxyR are generally more sensitive to H2O2 than the WT strain [125,126].

PerR
Peroxide stress regulator (PerR) belongs to the Fur transcriptional repressor family. PerR was first identified and described in Bacillus subtilis [127,128]. It is a dimer of two 17 kDa protomers with each protomer having an amino-terminal DNA binding domain and a carboxy-terminal dimerization domain. PerR has a regulatory metal binding site composed of three histidines and two aspartates (H37, H91, H93, D104, and D85 according to the PerR sequence in B. subtilis) located at the hinge between the two domains and that controls DNA binding. When the regulatory metal (Fe 2+ or Mn 2+ ) occupied the metal binding site, PerR adopts a conformation with a high affinity to DNA, leading to repression of PerR-controlled genes [129][130][131]. In the presence of H2O2, H37 and H91 in iron-bound PerR are oxidized into 2-oxohistidines [132]. This oxidation is mediated by hydroxyl radicals produced by H2O2 and the Fe 2+ coordinated in the regulatory metal-binding through a Fenton reaction [132]. Therefore, Mn 2+ can function as a surrogate regulatory metal for DNA binding, but not as a H2O2 sensing metal. PerR oxidation induces a conformational switch leading to PerR dissociation from DNA and derepression of the PerR regulon [132,133] (Figure 6).
PerR oxidation is irreversible and, in B. subtilis, oxidized PerR is degraded by Lon protease [134]. PerR generally regulates its own expression and the expression of oxidative stress-related genes. In B. subtilis, genes encoding catalase, AhpCF, and CCP are repressed by PerR as well as genes coding for MrgA, a Dps analog, Fur, and the heme biosynthesis machinery (hemAXCDBL) [128,135,136]. Inactivation of perR leads to a greater tolerance to H2O2 in many bacteria [128,[137][138][139].
OxyR and PerR are evolutionarily distinct, but they are functional homologs as they both control genes involved in defenses against peroxide stress. OxyR mostly exists in

PerR
Peroxide stress regulator (PerR) belongs to the Fur transcriptional repressor family. PerR was first identified and described in Bacillus subtilis [127,128]. It is a dimer of two 17 kDa protomers with each protomer having an amino-terminal DNA binding domain and a carboxy-terminal dimerization domain. PerR has a regulatory metal binding site composed of three histidines and two aspartates (H37, H91, H93, D104, and D85 according to the PerR sequence in B. subtilis) located at the hinge between the two domains and that controls DNA binding. When the regulatory metal (Fe 2+ or Mn 2+ ) occupied the metal binding site, PerR adopts a conformation with a high affinity to DNA, leading to repression of PerR-controlled genes [129][130][131]. In the presence of H 2 O 2 , H37 and H91 in iron-bound PerR are oxidized into 2-oxohistidines [132]. This oxidation is mediated by hydroxyl radicals produced by H 2 O 2 and the Fe 2+ coordinated in the regulatory metal-binding through a Fenton reaction [132]. Therefore, Mn 2+ can function as a surrogate regulatory metal for DNA binding, but not as a H 2 O 2 sensing metal. PerR oxidation induces a conformational switch leading to PerR dissociation from DNA and derepression of the PerR regulon [132,133] (Figure 6).
PerR oxidation is irreversible and, in B. subtilis, oxidized PerR is degraded by Lon protease [134]. PerR generally regulates its own expression and the expression of oxidative stress-related genes. In B. subtilis, genes encoding catalase, AhpCF, and CCP are repressed by PerR as well as genes coding for MrgA, a Dps analog, Fur, and the heme biosynthesis machinery (hemAXCDBL) [128,135,136]. Inactivation of perR leads to a greater tolerance to H 2 O 2 in many bacteria [128,[137][138][139].
OxyR and PerR are evolutionarily distinct, but they are functional homologs as they both control genes involved in defenses against peroxide stress. OxyR mostly exists in Gram-negative bacteria whereas PerR is generally found in Gram-positive bacteria. There are exceptions as OxyR homologs can be found in some actinobacteria (Mycobacterium leprae, Corynebacterium glutamicum, Streptomyces coelicolor) [140] and PerR homologs exist in some proteobacteria [137]. OxyR and PerR rarely coexist within the same bacterial species; however, they can be both found in Deinococcus radiodurans and Neisseria gonorrhoeae [141].

OhrR
Organic hydroperoxide resistance regulator) (Ohrh) is a transcriptional repressor of the MarR family well-distributed in bacteria. Similar to PerR, OhrR binds DNA when in its reduced form, resulting in gene repression ( Figure 6). It senses organic hydroperoxides (RO 2 H) through a single cysteine residue (C15 in B. subtilis OhrR) which is oxidized into cysteine sulfenic acid (Cys-SOH) [142,143]. This OhrR derivative remains bound to promoters until it undergoes further modifications into disulfide bond (Cys-S-S-R) or sulfenyl amide (Cys-SN) if reacting with a reduced cellular thiol or an amino group, respectively [144]. This results in the dissociation of OhrR from DNA and repression alleviation. The different OhrR cysteine derivatives can be reduced into thiol groups, allowing the regeneration of a reduced OhrR. Soonsanga et al. [145] also demonstrated the existence of an irreversible form of OhrR when the cysteine sulfenic acid derivative is further oxidized into cysteine sulfinic acid (Cys-SO 2 H). In that case, the cysteine sulfinic acid OhrR derivative is thought to be degraded.
It should be noted that another family of OhrR in which two cysteine residues are involved in organic hydroperoxides sensing has been described in Xanthomonas campestris [146]. In that case, the second cysteine residue provides the reduced thiol group to form the disulfide bond necessary to promote OhrR dissociation from DNA.
OhrR was first identified as a repressor of its own expression and of ohrA, which encodes a peroxiredoxin that scavenges organic peroxide [142,147,148]. Determination of the genome wide OhrR regulon performed in Chromobacterium violaceum indicated that the OhrR regulon encompasses, in fact, only a very limited number of genes in addition to ohrA and ohrR. In this bacterium, OhrR represses a putative diguanylate cyclase and activates indirectly three virulence-related genes [149]. OhrR mutants are generally more resistant to organic peroxide than their WT parental strain [150][151][152][153][154].

SoxRS
SoxRS control the expression of genes encoding defenses against superoxide. In E. coli, it is encoded by two adjacent and divergently transcribed genes, soxR and soxS. SoxR is a 17 kDa homodimer that belongs to the MerR transcriptional regulator family and SoxS is a 12 kDa transcriptional regulator of the AraC family. Each SoxR protomer contains an iron-sulfur cluster [2Fe-2S] that is oxidized by superoxide as well as by redox compounds [155,156]. The binding of oxidized SoxR to the soxS promoter activates soxS expression ( Figure 6). Oxidized SoxR is reduced by NADPH-dependent Rsx/Rse enzymes [157].
The two proteins SoxRS are present together in proteobacteria and in actinomycetes [164]. Some bacteria, such as Pseudomonas aeruginosa, only contain SoxR and are devoid of SoxS. Other species, including the Bacteroidetes Porphyromonas ginvivalis, contain neither SoxR, nor SoxS.

Regulation of Oxidative Stress Defenses in Leptospira
A protein exhibiting the four characteristic cysteines and homology with typical SoxR is found only in some Leptospira spp. and not distributed widely in the whole genus ( Figure 4). Identification of a canonical SoxS in Leptospira spp. is unclear. A protein exhibiting 33% of homology with E. coli SoxS has been found in Leptospira saprophytes (LEPBIa2624); however, this ORF contains extra domains that are not the landmarks of canonical SoxS. Whether LEPBIa2624-encoding regulator is a bona fide SoxS that controls the expression of sodB remains to be demonstrated. Neither SoxR, nor SoxS are found in L. interrogans.
Unlike most diderm bacteria, no OxyR has been reported so far in L. interrogans. A far ortholog of an OxyR-like LysR regulator has been annotated in L. biflexa (LEPBIa3010) and appears to be present in some but not all saprophytic species of Leptospira. However, there are no reports to date showing that it is a bona fide OxyR. Further studies are needed to determine whether this LysR regulator has a role in controlling the oxidative stress response in saprophytic Leptospira spp.
Two PerR-like regulators have been identified in L. Interrogans. PerRA (encoded by LIMLP_10155) was first identified as a Fur regulator whose inactivation elicits the up-regulation of catalase and peroxidase-encoding genes [165]. The second PerR, named PerRB (encoded by LIMLP_05620), was identified among the ORFs up-regulated when L. interrogans were exposed to H 2 O 2 [80,166]. The distribution of PerRA and PerRB strikingly differs between saprophytes and pathogenic species. Homologs of PerRA and PerRB are present in all pathogenic species of the P1 clades sequenced so-far. However, PerRA is present in all saprophytes whereas homologs of PerRB cannot be found in non-pathogenic Leptospira species. Conversely, PerRB homologs are found in the P2 clade species where PerRA is generally missing [166,167] (Figure 4).
The respective function of PerRA and PerRB seems more complementary than redundant. Phenotypic and transcriptomic studies led to the conclusion that PerRA functions as a bona fide PerR in L. interrogans. PerRA inactivation leads to a higher survival in the presence of H 2 O 2 than the WT [165,168]. Identification of the PerRA regulon indicates that not only PerRA represses the ank-katE operon (LIMLP_10145-10150) and genes encoding AhpC1 (LIMLP_05955) and CCP (LIMLP_02795), but it also activates a gene locus encoding a TonB-dependent transporter and the two-component system VicKR [165][166][167]. The main function of PerRA is therefore to control expression of defenses against H 2 O 2 .
The up-regulation of perRB in the presence of H 2 O 2 suggests that, similarly to PerRA, PerRB is an ROS sensor. Indeed, classical PerRs, which generally self-repress their expression, dissociate from DNA in the presence of ROS, leading to their up-regulation. A perRB mutant has a comparable resistance to H 2 O 2 as the WT strain. However, it exhibits a higher survival when exposed to paraquat [166]. From this phenotype, one can infer that L. interrogans PerRB represses genes involved in superoxide detoxification. RNASeq analyses of a perRB mutant when L. interrogans are cultivated in the EMJH culture medium or in dialysis membrane chamber did not provide an obvious explanation for this phenotype [166,167]. Indeed, the PerRB regulon encompasses either genes with unknown or poorly characterized function, or genes encoding factors involved in regulation (transcriptional regulators, c-di-GMP metabolism, and sigma factors). The putative mechanisms whose expression is controlled by PerRB and allowing to better tolerate deadly concentrations of superoxide are thus not understood. In the model that can be presently drawn, the main functions of PerRA and PerRB are to control expression of defenses against H 2 O 2 and superoxide, respectively. As mentioned earlier, since no SoxRS system has been identified in L. interrogans, it is unknown how these bacteria orchestrate the response to superoxide. It is therefore tempting to speculate that PerRB fulfills the function of SoxRS in these bacterial species.
Interestingly, a limited number of genes, including the TonB-dependent transporter cluster, were found deregulated in both the perRA and perRB mutants, suggesting a certain level of redundancy in their regulon [166,167]. A double perRAperRB mutant is more resistant to both H 2 O 2 and O 2 •− , indicating that the double mutant exhibits the respective phenotype of the single perRA and perRB mutants [166]. This double mutant was shown to be avirulent in the hamster and mice models and several virulencerelated genes (including ligA, ligB, lvrA, lvrB, and clpB) were down-regulated in this mutant [166,167]. The exact role of PerRA and PerRB in the regulation of a virulenceassociated network needs to be deciphered.
An ORF is annotated as a putative OhrR regulator in both pathogenic and saprophytes clades (LIMLP_17545 and LEPBI_I0798, respectively) ( Figure 4) but no studies that characterized these proteins have been performed yet.
The transcriptional response to H 2 O 2 has been characterized in L. interrogans [80]. Catalase and peroxidase-encoding genes (katE, ccp and ahpC) of the PerRA regulon were among the highest H 2 O 2 -responsive genes (i.e., genes rapidly up-regulated with sublethal doses of H 2 O 2 ). Detoxification enzymes are therefore the first line of defense when pathogenic Leptospira are exposed to H 2 O 2 . The catalase is located in the periplasm in L. interrogans and is probably the main enzyme which allows a rapid elimination of H 2 O 2 [70,80].
When L. interrogans are exposed to higher doses of H 2 O 2 , additional oxidative stress and redox-related genes are up-regulated including genes encoding thiol peroxidases, thioredoxin disulfide reductase, DsbD, Bcp, and Dps, as well as molecular chaperones from the heat shock response (DnaK/DnaJ/GrpE, GroEL/GroES, the small HSPs, and ClpB) and DNA repair proteins from the SOS response (RecA, RecN, DNA Pol IV, and LexA). Pathogenic Leptospira species have evolved to be very effective in rapidly breaking down H 2 O 2 before it metabolizes into the very reactive • OH. In addition, these bacteria are also well-equipped with a variety of repair mechanisms to heal oxidative damage to proteins and DNA occurring when H 2 O 2 detoxifying enzymes are overwhelmed by the amount of ROS. Unlike what has been observed in other bacteria, genes encoding methionine sulfoxide reductases (that reduce methionine sulfoxide arising upon methionine oxidation), the iron-sulfur cluster synthesis and assembly SUF machinery, and the specific oxidative stress-related chaperone Hsp33 are not significantly up-regulated upon oxidative stress in L. interrogans, at least in the conditions that were tested.

Concluding Remarks and Perspectives
Understanding how Leptospira adapt to an oxidative environment, whether in the environmental niche or within the host, is far from being completely deciphered. The main limitation is the restricted number of laboratories that conduct research on Leptospira and leptospirosis, a neglected bacterium and disease. Another limitation is the difficulty to genetically manipulate these bacteria and to inactivate genes by allelic exchange, particularly in the pathogenic species. It is therefore not always possible to demonstrate the direct involvement of a particular factor in the oxidative stress response. Moreover, the mechanisms and pathways participating in the defense against oxidative stress are numerous and a certain level of redundancy and overlap is expected, whose study would require obtaining multiple mutants. The recent development of a new approach using the CRISPR/Cas9 system for inactivating genes in Leptospira [9,10,169] probably permits advancing our knowledge on the physiology of these bacteria and in particular on the different factors participating in the oxidative stress response. For instance, a mutant inactivated in ccp (LIMLP_02795), one of the most up-regulated ORF upon exposure of L. interrogans to H 2 O 2 , is not available. Determining the exact contribution of leptospiral CCPs in H 2 O 2 detoxification would certainly benefit from having an effective method to generate mutants.
To date, most of our understanding of the oxidative stress response of Leptospira has focused on one particular ROS, H 2 O 2 , and how defenses against this oxidant are repressed by PerRA. Much less is known on how Leptospira adapt to the presence of other important ROS such as O 2 •− or HOCl and what regulators control these adaptations, if any. In addition, important ROS detoxification machineries such as SOD/SOR are absent in pathogenic Leptospira species, which is unusual for aerobic bacteria. Do pathogenic Leptospira possess mechanisms to detoxify O 2 •− , a very important ROS produced by the host during infection, or do they rely exclusively on repair mechanisms against superoxidemediated oxidative damage? Are Leptospira exposed to neutrophil-generated HOCl? These are among the important questions that would need to be answered in the future and require further investigation.
Pathogenic Leptospira and saprophytes have different repertoires of enzymes to detoxify ROS. Notably, pathogenic species have shown a strong catalase activity mediated by KatE, who is among the most expressed proteins in L. interrogans, while the saprophyte species did not have any detectable catalase activity even though their genome encodes a catalase of a different family (KatG). The specific role of KatG in the saprophytic species of Leptospira also remains to be elucidated.
In addition, as mentioned above, saprophytes possess an SOD, whereas pathogenic species do not. These observations indicate that Leptospira species might have evolved their antioxidant mechanisms according to their respective ecological niches and the nature of the ROS they are exposed to. Deciphering the evolution of the oxidative stress response within the different Leptospira clades will also be of great interest to reconstruct the evolutionary history of adaption to oxidative stress in this genus.
Finally, due to the importance of defenses against H 2 O 2 for Leptospira virulence, it is tempting to propose that targeting the KatE catalase can be a successful therapeutic strategy. This requires to identify a specific inhibitor of the leptospiral KatE that does not affect the activity of human catalases, an important impediment in developing such drugs.