Bioenergetics and Reactive Nitrogen Species in Bacteria

The production of reactive nitrogen species (RNS) by the innate immune system is part of the host’s defense against invading pathogenic bacteria. In this review, we summarize recent studies on the molecular basis of the effects of nitric oxide and peroxynitrite on microbial respiration and energy conservation. We discuss possible molecular mechanisms underlying RNS resistance in bacteria mediated by unique respiratory oxygen reductases, the mycobacterial bcc-aa3 supercomplex, and bd-type cytochromes. A complete picture of the impact of RNS on microbial bioenergetics is not yet available. However, this research area is developing very rapidly, and the knowledge gained should help us develop new methods of treating infectious diseases.


Introduction
Primary bacterial pathogens are infectious agents responsible for severe and often deadly diseases in humans. In addition, commensal bacteria can produce opportunistic infections in immunosuppressed patients. Disease-causing bacteria are becoming resistant to most commonly available antibiotics, which poses a threat to global public health. The production of reactive nitrogen species (RNS) by the innate immune system is part of the host's defense against invading microbes. RNS refers to various nitrogenous products including nitric oxide ( • NO), peroxynitrite anion (ONOO -), nitroxyl (HNO), dinitrogen trioxide (N 2 O 3 ), nitrite (NO 2 -), nitrogen dioxide ( • NO 2 ), nitronium cation (NO 2 + ), nitrosonium cation (NO + ), nitrosoperoxycarbonate anion (ONOOCO 2 -), nitryl chloride (Cl-NO 2 ), S-nitrosothiols (RSNOs) [1]. • NO, along with carbon monoxide and hydrogen sulfide, is considered an endogenous gaseous signaling molecule [2][3][4][5]. • NO is the main RNS produced by the host and the main source for the generation of the other RNS. This small diatomic molecule is a free radical, i.e., with one unpaired electron, and can diffuse easily through biological membranes. The enzymes that produce • NO are NO synthases (NOS). They convert L-arginine and O 2 into L-citrulline and • NO using NADPH as the electron donor. There are three NOS isoforms: neuronal (nNOS), endothelial (eNOS), and inducible (iNOS). nNOS and eNOS are constitutively expressed whereas iNOS expression is induced by immunological stimuli. The latter occurs predominantly in macrophages and plays an essential role in immune defense. • NO can combine with superoxide radical (O 2 •− ) produced by the NADPH oxidase at diffusion-controlled rates yielding another RNS, ONOO − . Under physiological conditions, ONOO − is in equilibrium with peroxynitrous acid, ONOOH (pK a = 6.8), and local pH affects peroxynitrite reactivity. Both ONOO − and ONOOH are able to cross biological membranes. Peroxynitrite is a potent oxidant and nitrating agent, with a very important role in the destruction of invading pathogens by macrophages, as ONOOH spontaneously homolyzes to hydroxyl radical ( • OH) and • NO 2 [6,7]. As they are within bacteria-containing phagolysosomes in macrophages, RNS creates a hostile In order to transfer electrons from NADH to quinone, bacteria use three different families of NADH:quinone reductases (dehydrogenases)-NDH-1, NDH-2, and NQR (Table 2). NDH-1 reductases are closely related to the mitochondrial complex I and function as redoxdriven proton pumps [24,25]. Both NDH-2 and NQR are unrelated to the canonical complex I. NDH-2 enzymes are non-electrogenic and therefore unable to support PMF [26,27]. NQR reductases operate as redox-driven sodium pumps, i.e., they generate a sodium ion motive force rather than PMF [28][29][30]. The sodium ion motive force, along with PMF and ATP, is the third energy currency used by a few bacteria [31]. Bacteria with more than one NADH:quinone reductase show a preference for one or another enzyme depending on the growth conditions. Bacterial complex III, also termed cytochrome bc 1 complex, transfers electrons from quinol to ferricytochrome c. This redox reaction is coupled with the production of PMF via the Q-cycle (Mitchellian redox-loop) mechanism [32,33]. The presence of complex III in bacterial respiratory chains is optional. Some bacteria, e.g., Escherichia coli, have no cytochrome c at all, and hence no cytochrome bc 1 [34]. Cytochrome c of other bacteria is not water-soluble but fused either to complex III or complex IV. This leads to the formation of a supercomplex between complex III and complex IV (Table 2). Accordingly, the cytochrome bcc-aa 3 (III 2 -IV 2 ) supercomplex was discovered in Mycobacterium smegmatis and Corynebacterium glutamicum [35][36][37]. A supercomplex composed of cytochrome bc 1 and aa 3 -type cytochrome c oxidase was also identified in Rhodobacter sphaeroides [38]. Figure 1 shows examples of three different types of branched bacterial respiratory chains in which the complex III is absent (E. coli [34]), present as a separate enzyme (Pseudomonas aeruginosa [29]), or forms a tight supercomplex with the aa 3 -type cytochrome c oxidase (M. tuberculosis [39,40]). Figure 1. Aerobic respiratory chains of Escherichia coli, Pseudomonas aeruginosa, and Mycobacterium tuberculosis. In E. coli, two NADH dehydrogenases, NDH-1 and NDH-2, and succinate dehydrogenase (SDH) transfer electrons to ubiquinone (UQ)/menaquinone (MQ) pool. Three quinol oxidases, cytochromes bo3, bd-I, and bd-II, oxidize ubiquinol/menaquinol with the concomitant reduction of O2 to 2H2O. P. aeruginosa has three NADH dehydrogenases, NDH-1, NDH-2, NQR, and SDH. The electrons from ubiquinol are further transferred to O2 either directly via two quinol oxidases, cytochrome bo3 and bd-type cyanide insensitive oxidase (CIO), or via the bc1 complex to three cytochrome c oxidases, caa3, cbb3-1, and cbb3-2. M. tuberculosis possesses three NADH dehydrogenases, one NDH-1, two NDH-2, and two succinate dehydrogenases, SDH-1 and SDH-2. The electrons from menaquinol are then transferred to O2 via cytochrome bd or cytochrome bcc-aa3 supercomplex.
The membrane-bound terminal oxidases are divided into two superfamilies: hemecopper oxidases and bd-type cytochromes [41][42][43]. The active site of a heme-copper oxidase termed the binuclear center (BNC) is composed of a high-spin heme (a3, o3, or b3) and a copper ion (CuB). The enzyme catalyzes the transfer of electrons from cytochrome c or quinol to O2 with the production of 2H2O. The reaction is coupled to the generation of PMF using the mechanism of redox-coupled proton pumping across the membrane Figure 1. Aerobic respiratory chains of Escherichia coli, Pseudomonas aeruginosa, and Mycobacterium tuberculosis. In E. coli, two NADH dehydrogenases, NDH-1 and NDH-2, and succinate dehydrogenase (SDH) transfer electrons to ubiquinone (UQ)/menaquinone (MQ) pool. Three quinol oxidases, cytochromes bo 3 , bd-I, and bd-II, oxidize ubiquinol/menaquinol with the concomitant reduction of O 2 to 2H 2 O. P. aeruginosa has three NADH dehydrogenases, NDH-1, NDH-2, NQR, and SDH. The electrons from ubiquinol are further transferred to O 2 either directly via two quinol oxidases, cytochrome bo 3 and bd-type cyanide insensitive oxidase (CIO), or via the bc 1 complex to three cytochrome c oxidases, caa 3 , cbb 3 -1, and cbb 3 -2. M. tuberculosis possesses three NADH dehydrogenases, one NDH-1, two NDH-2, and two succinate dehydrogenases, SDH-1 and SDH-2. The electrons from menaquinol are then transferred to O 2 via cytochrome bd or cytochrome bcc-aa 3 supercomplex.
The membrane-bound terminal oxidases are divided into two superfamilies: hemecopper oxidases and bd-type cytochromes [41][42][43]. The active site of a heme-copper oxidase termed the binuclear center (BNC) is composed of a high-spin heme (a 3 , o 3 , or b 3 ) and a copper ion (Cu B ). The enzyme catalyzes the transfer of electrons from cytochrome c or quinol to O 2 with the production of 2H 2 O. The reaction is coupled to the generation of PMF using the mechanism of redox-coupled proton pumping across the membrane [21,22,[44][45][46][47][48][49][50][51][52][53][54][55][56][57][58][59]. A heme-copper oxidase that uses cytochrome c as an electron donor (cytochrome c oxidase) has the second copper site, Cu A . Cu A directly accepts electrons from cytochrome c. If the The catalytic cycle of bd-type oxidases is deduced from the studies on the E. coli cytochrome bd-I [90,103-106] (Figure 2). It includes the intermediates termed O 1 , A 1 , A 3 , P, F*, F, and takes into account that the quinol substrate is a two-electron donor. In the O 1 → A 1 transition, an electron transfers from heme b558 to heme d and the latter binds O2. In the next A 1 → A 3 transition, two electrons from a quinol reduce heme b558 and heme b595. In the A 3 → P transition, a true transient peroxy complex of ferric heme d is formed concomitant The catalytic cycle of bd-type oxidases is deduced from the studies on the E. coli cytochrome bd-I [90,103-106] (Figure 2). It includes the intermediates termed O 1 , A 1 , A 3 , P, F*, F, and takes into account that the quinol substrate is a two-electron donor. In the O 1 → A 1 transition, an electron transfers from heme b 558 to heme d and the latter binds O 2 . In the next A 1 → A 3 transition, two electrons from a quinol reduce heme b 558 and heme b 595 . In the A 3 → P transition, a true transient peroxy complex of ferric heme d is formed concomitant with oxidation of heme b 595 . The O-O bond cleavage occurs in the next, P→ F* transition in which the ferric heme d is further oxidized to the ferryl form with a porphyrin π-cation radical (Por •+ ). Then in the F*→ F transition, the radical is quenched by an electron from the ferrous heme b 558 . The F→ O 1 transition, in which two electrons from a second quinol reduce the ferryl heme d (to the ferric form) and heme b 558 , completes the cycle. The P/F*→ F and F→ O 1 transitions were reported to be electrogenic [88][89][90][91]107].

• NO and Bacterial Heme-Copper Terminal Oxidases
With the exception of the mycobacterial aa 3 -type oxidase (see Section 3.1.1), the bacterial heme-copper oxidases tested to date, such as the cbb 3 -type oxidases from Vibrio cholerae and Rhodobacter sphaeroides, and the aa 3 -type oxidase from R. sphaeroides, are rapidly and strongly inhibited by • NO [135], similar to their mitochondrial homolog, cytochrome c oxidase [136]. The reaction of the mitochondrial enzyme with • NO was studied in more detail. It was shown that low, nanomolar levels of • NO reversibly inhibit the enzyme activity [136] whereas high, micromolar levels of • NO cause irreversible damage to the enzyme [137]. The reversible inhibition occurs via two pathways. At high reductive pressure (high turnover conditions) and low O 2 tensions, the O 2 -competitive inhibition pathway prevails. It occurs through the reaction of • NO with the two-electron reduced (and possibly one-electron reduced) BNC leading to the production of the nitrosyl derivative of the enzyme. At low reductive pressure (low turnover conditions) and high O 2 tensions, the noncompetitive pathway prevails. The latter proceeds via reaction of • NO with the catalytic intermediates that have Cu B oxidized, resulting in the generation of the nitrite-bound enzyme [138][139][140][141]. It is reasonable to assume that the bacterial heme-copper oxidases studied [135] are inhibited by • NO through similar mechanisms.

• NO-Metabolizing Activity of the Mycobacterial bcc-aa 3 Supercomplex in Turnover
Mycobacteria contain no water-soluble cytochrome c. Probably for this reason their aa 3 -type cytochrome oxidase needs to be in a tight supercomplex with cytochrome bcc, a homolog of the mitochondrial cytochrome bc 1 [35,36]. Forte et al. reported that a purified chimeric supercomplex composed of M. tuberculosis cytochrome bcc and M. smegmatis aa 3type oxidase resists inhibition by • NO [57]. The effect of • NO on the O 2 consumption by the bcc-aa 3 supercomplex in the presence of excess dithiothreitol (DTT) and menadione (MD) was evaluated amperometrically. A very small, short-term decrease in the O 2 consumption induced by • NO is followed by quick and complete restoration of the initial enzyme's activity (Figure 3, inset). Surprisingly, the • NO decay allowing for the activity recovery occurs much faster than one would expect. The reason for this turned out to be the ability of the bcc-aa 3 supercomplex to degrade • NO under turnover conditions. The rate of • NO decay in the presence of the enzyme and reductants is significantly higher than in the presence of the reductants only ( Figure 3, top panel). Furthermore, in the absence of DTT and MD, the kinetic profiles of • NO decay in aerobic solution with and without the bcc-aa 3 are identical ( Figure 3, bottom panel). The latter two observations support the conclusion that the • NO decomposition is indeed catalyzed by the purified bcc-aa 3 supercomplex in turnover with O 2 and the electron donors. The maximum • NO-consuming activity of the enzyme measured following the addition of 30 µM • NO appeared to be about 300 mol • NO × (mol bcc-aa 3 ) −1 × min −1 [57] (Table 3).
the ability of the bcc-aa3 supercomplex to degrade  NO under turnover conditions. The rate of  NO decay in the presence of the enzyme and reductants is significantly higher than in the presence of the reductants only ( Figure 3, top panel). Furthermore, in the absence of DTT and MD, the kinetic profiles of  NO decay in aerobic solution with and without the bcc-aa3 are identical ( Figure 3, bottom panel). The latter two observations support the conclusion that the  NO decomposition is indeed catalyzed by the purified bcc-aa3 supercomplex in turnover with O2 and the electron donors. The maximum  NO-consuming activity of the enzyme measured following the addition of 30 µM  NO appeared to be about 300 mol  NO × (mol bcc-aa3) −1 × min −1 [57] (Table 3).   Table 3. Overview of • NO interactions with mycobacterial cytochrome bcc-aa 3 supercomplex and E. coli cytochrome bd-I, respiratory enzyme complexes which contribute to mechanisms of bacterial resistance to • NO.

Enzyme Complex
Inhibition by • NO • NO Degradation in Turnover [142,143] Possible mechanisms for this reaction catalyzed by the bcc-aa 3 are worth discussing. Earlier, it was reported that in the mitochondrial cytochrome oxidase, • NO can react with the catalytic intermediates O, P, and F, each according to a 1:1 stoichiometry [138,140]. One could suggest that in the bcc-aa 3 • NO also reacts with these species populated at a steady-state. In view of the fact that in the bcc-aa 3 the • NO/O 2 stoichiometry was estimated to be 2.65 [57] i.e., >1, we assume that in this enzyme • NO can react with more than one intermediate during the catalytic cycle. Figure 4 shows possible reaction pathways for the bcc-aa 3 taking into account modern views on the structures of intermediates O, F, and P. As in the mitochondrial enzyme [138,140], in the reactions with O, F, and P, • NO is thought to donate one electron to Cu B 2+ yielding nitrosonium ion (NO + ) and Cu B 1+ . This results in the oxidation of • NO to NO 2 and the conversion of a corresponding intermediate into the succeeding one along the catalytic cycle of the bcc-aa 3 ( Figure 4, reactions 1, 2, 3, see also Figure 2). In other words, following the reaction with one molecule of • NO, O is converted into E, F-into O, and P-into F. In the mitochondrial cytochrome oxidase, NO 2 produced from • NO binds with a relatively high affinity to the oxidized heme a 3 (or Cu B ) in the BNC [140]. This impedes the complete reduction of the BNC and, hence, its ability to bind and further reduce O 2 . As a result, O 2 consumption is halted. We hypothesize that in the case of the bcc-aa 3 NO 2 generated from • NO does not bind to the BNC with high affinity. Instead, NO 2 is quickly ejected into the bulk phase from the supercomplex without affecting the catalytic O 2 consumption.  Since the bcc-aa3 is an O2-binding heme protein, it cannot be ruled out that the enzyme is also capable of acting as a  NO dioxygenase. A possible mechanism of such reaction similar to that reported for the truncated hemoglobin N of M. tuberculosis [144] is shown in Figure 4 (reaction 4). According to the proposed pathway, the reaction of the catalytic intermediate A with  NO yields nitrate (NO3 -) that should leave the BNC rapidly in order to avoid inhibition of the main O2 reductase activity. All proposed reaction mechanisms ( Figure 4, reactions 1-4) await experimental confirmation.

 NO Reductase Activity of Heme-Copper Oxidases
The amperometric studies showed that a few bacterial heme-copper oxidases are able to decompose  NO under reducing anaerobic conditions at  NO concentrations in the solution in the range of 5 to 10 µM. Figure 5 demonstrates such activity of the purified mycobacterial bcc-aa3 supercomplex [57]. The pre-reduced enzyme was anaerobically added to an O2-free solution of  NO in the presence of excess DTT and MD. The addition of the enzyme was shown to increase the rate of the decomposition of  NO. It has to be noted that the slow  NO decay observed before the addition of the bcc-aa3 is due to the non-enzymatic reaction of  NO with the reductants. Additionally, the initial fast drop in the  NO concentration detected immediately after the addition of the enzyme is probably due to  NO binding to the bcc-aa3. The  NO-consuming activity of the bcc-aa3 under anaerobic conditions at ~8 µM  NO added appeared to be about 3 mol  NO × (mol bcc-aa3) −1 × min −1 [57] (Table 3). As one can see, this is ~100 times lower than that observed under Since the bcc-aa 3 is an O 2 -binding heme protein, it cannot be ruled out that the enzyme is also capable of acting as a • NO dioxygenase. A possible mechanism of such reaction similar to that reported for the truncated hemoglobin N of M. tuberculosis [144] is shown in Figure 4 (reaction 4). According to the proposed pathway, the reaction of the catalytic intermediate A with • NO yields nitrate (NO 3 -) that should leave the BNC rapidly in order to avoid inhibition of the main O 2 reductase activity. All proposed reaction mechanisms ( Figure 4, reactions 1-4) await experimental confirmation.

• NO Reductase Activity of Heme-Copper Oxidases
The amperometric studies showed that a few bacterial heme-copper oxidases are able to decompose • NO under reducing anaerobic conditions at • NO concentrations in the solution in the range of 5 to 10 µM. Figure 5 demonstrates such activity of the purified mycobacterial bcc-aa 3 supercomplex [57]. The pre-reduced enzyme was anaerobically added to an O 2 -free solution of • NO in the presence of excess DTT and MD. The addition of the enzyme was shown to increase the rate of the decomposition of • NO. It has to be noted that the slow • NO decay observed before the addition of the bcc-aa 3 is due to the non-enzymatic reaction of • NO with the reductants. Additionally, the initial fast drop in the • NO concentra-tion detected immediately after the addition of the enzyme is probably due to • NO binding to the bcc-aa 3 . The • NO-consuming activity of the bcc-aa 3 under anaerobic conditions at~8 µM • NO added appeared to be about 3 mol • NO × (mol bcc-aa 3 ) −1 × min −1 [57] ( Table 3). As one can see, this is~100 times lower than that observed under aerobic turnover conditions. A similar activity was also reported previously for such heme-copper oxidases as the ba 3 and caa 3 from Thermus thermophilus [145], the bo 3 from E. coli [146], the cbb 3 from Pseudomonas stutzeri [147] and R. sphaeroides [148]. Notably, the mitochondrial beef heart aa 3 -type oxidase does not catalyze the anaerobic degradation of • NO [149]. For the ba3 oxidase from T. thermophilus it was directly shown by gas chromatography that the end product of the catalytic  NO decay under reducing anaerobic conditions is nitrous oxide (N2O), i.e., the  NO reductase activity takes place [145]. It is reasonable to suggest that this is also the case for the other bacterial oxidases, which were reported to degrade  NO under the same conditions [57,146,148]. The reaction mechanism could resemble that used by native bacterial  NO reductases. Both mechanisms, however, are still under debate [150,151]. In general, two  NO molecules react with the fully reduced BNC of the oxidase yielding one molecule of N2O as the end product, with the formation of the hyponitrite species as a transient intermediate. For more details, see Figure 23 in [151].
Since the  NO reductase activity measured in some bacterial oxidases is not too high and the conditions requested hardly often occurs in vivo, we do not expect that this contributes significantly to microbial defense mechanisms against  NO-induced stress.

bd-Type Oxidases Confer Bacterial Resistance to  NO
Evidence is accumulating that in at least some pathogenic bacteria, cytochrome bd is involved in their defense against  NO-induced stress. Jones-Carson et al. examined the role of the two major terminal oxidases of Salmonella Typhimurium, the heme-copper cytochrome bo3 (encoded by the cyoABCD operon) and cytochrome bd (encoded by the cydAB operon), in its antinitrosative defensive system [152]. The authors compared growth rates of the wild-type strain, ΔcyoABCD, and ΔcydAB mutants in LB broth supplemented with 5 mM DETA NONOate. The latter is the  NO donor that at the added concentration produced a stable flux of 5 µM  NO during the experiment. In contrast to the wild-type and ΔcyoABCD strains, the ΔcydAB mutant appeared to be hypersusceptible to  NO as manifested by the extended lag phase following the DETA NONOate addition. Jones-Carson et al. also compared the rates of respiration in the wild-type, ΔcyoABCD, and ΔcydAB bacterial cultures treated with 50 µM spermine NONOate. The O2 consumption activity of the ΔcydAB mutant was much more sensitive to spermine NONOate as compared to that For the ba 3 oxidase from T. thermophilus it was directly shown by gas chromatography that the end product of the catalytic • NO decay under reducing anaerobic conditions is nitrous oxide (N 2 O), i.e., the • NO reductase activity takes place [145]. It is reasonable to suggest that this is also the case for the other bacterial oxidases, which were reported to degrade • NO under the same conditions [57,146,148]. The reaction mechanism could resemble that used by native bacterial • NO reductases. Both mechanisms, however, are still under debate [150,151]. In general, two • NO molecules react with the fully reduced BNC of the oxidase yielding one molecule of N 2 O as the end product, with the formation of the hyponitrite species as a transient intermediate. For more details, see Figure 23 in [151].
Since the • NO reductase activity measured in some bacterial oxidases is not too high and the conditions requested hardly often occurs in vivo, we do not expect that this contributes significantly to microbial defense mechanisms against • NO-induced stress.

bd-Type Oxidases Confer Bacterial Resistance to • NO
Evidence is accumulating that in at least some pathogenic bacteria, cytochrome bd is involved in their defense against • NO-induced stress. Jones-Carson et al. examined the role of the two major terminal oxidases of Salmonella Typhimurium, the heme-copper cytochrome bo 3 (encoded by the cyoABCD operon) and cytochrome bd (encoded by the cydAB operon), in its antinitrosative defensive system [152]. The authors compared growth rates of the wild-type strain, ∆cyoABCD, and ∆cydAB mutants in LB broth supplemented with 5 mM DETA NONOate. The latter is the • NO donor that at the added concentration produced a stable flux of 5 µM • NO during the experiment. In contrast to the wild-type and ∆cyoABCD strains, the ∆cydAB mutant appeared to be hypersusceptible to • NO as manifested by the extended lag phase following the DETA NONOate addition. Jones-Carson et al. also compared the rates of respiration in the wild-type, ∆cyoABCD, and ∆cydAB bacterial cultures treated with 50 µM spermine NONOate. The O 2 consumption activity of the ∆cydAB mutant was much more sensitive to spermine NONOate as compared to that of the wild-type bacteria. Additionally, unlike the wild-type and ∆cyoABCD cells, the O 2 consuming activity of the ∆cydAB cells did not improve over time following the addition of spermine NONOate. Cytochrome bd was reported to add to the • NO-detoxifying activity of the flavohemoglobin Hmp that converts • NO into NO 3 − . Both Hmp and the bd oxidase contribute to similar extents to S. Typhimurium pathogenesis. Furthermore, there is a substantial degree of independence between these two proteins in S. Typhimurium pathogenesis. It is suggested that low O 2 levels in mice favor • NO detoxification by cytochrome bd whereas high O 2 tension favor Hmp as the • NO-detoxifier. Bacteria may experience different O 2 and • NO levels as the inflammatory response evolves over time during the infection. Therefore, S. Typhimurium may preferentially use Hmp or the bd oxidase according to the availability of O 2 and • NO. Thus, cytochrome bd, along with Hmp, is an important component of the antinitrosative defensive system of S. Typhimurium [152].
Shepherd et al. examined the relative contribution of cytochrome bd-I (CydAB), Hmp, the flavorubredoxin NorVW, the nitrite reductase NrfA, and the iron-sulfur cluster repair protein YtfE to the • NO-tolerance mechanisms in a multidrug-resistant uropathogenic E. coli (UPEC), strain EC958 [153]. For this purpose, the authors mutated the cydAB, hmp, norVW, nrfA and ytfE genes in EC958. Growth rates of wild-type EC958, and cydAB, hmp, norVW, nrfA and ytfE mutants were measured following the addition of the • NO-releaser NOC-12 under microaerobic conditions. It turned out that mutation of cydAB and hmp confers the highest sensitivity to • NO. Furthermore, the ∆cydAB mutant displayed increased sensitivity to neutrophil killing, reduced survival within primed macrophages, and an attenuated colonization phenotype in the mouse bladder. The fact that deletion of cydAB impairs survival in a mouse model suggests that the bd oxidase-dependent respiration under nitrosative stress conditions is a key factor for host colonization. Thus, the UPEC cytochrome bd-I provides the greatest contribution to • NO tolerance and host colonization at low O 2 tensions and is of major importance for the accumulation of high microbial loads in the course of infection of the urinary tract [153].
Beebout et al. reported that cytochrome bd of UPEC (E. coli cystitis isolate UTI89) is highly expressed in biofilms and that loss of the bd-oxidase-expressing subpopulation impairs barrier function and reduces the abundance of extracellular matrix [154]. The authors hypothesized that cytochrome bd is preferentially expressed in the UPEC biofilm because the enzyme provides protection against nitrosative stress. The addition of the • NO donor NOC-12 to planktonic cultures was found to significantly reduce the growth rate of the ∆cydAB mutant: the doubling time increased from 37 to 106 min after the treatment. This finding suggests that during aerobic growth the bd oxidase serves as an • NO sink that reversibly sequesters • NO. This protects respiration mediated by cytochrome bo 3 which is a proton pump that is more efficient at transducing energy but susceptible to irreversible inhibition by • NO. Beebout et al. proposed that cytochrome bd-expressing subpopulations in UPEC are critical for withstanding such harmful metabolic by-products as • NO while in the biofilm state [154].
Consistently, • NO caused more significant growth inhibition in non-pathogenic E. coli strains lacking cytochrome bd as compared to cytochrome bo 3 -deficient ones [155]. In Shewanella oneidensis, the bd oxidase provides tolerance to nitrite rather than • NO, but this is an exceptional case [156]. A protective role of cytochrome bd against • NO stress also agrees with the expression of this enzyme in E. coli [154,157,158], S. Typhimurium [152], Staphylococcus aureus [159], Bacillus subtilis [160], and M. tuberculosis [161] in response to • NO. Interestingly, in M. tuberculosis, the bd oxidase was reported to be necessary for optimal respiration at acidic pH as the bcc-aa 3 supercomplex is markedly inhibited under these conditions [162].
Like most heme-copper oxidases tested (see Section 3.1), the bd-type oxidases from non-pathogenic E. coli and A. vinelandii are rapidly inhibited by • NO [142]. This was demonstrated on the level of both the purified enzymes from these bacteria [142] and the E. coli cells lacking cytochrome bo 3 [155,163]. The inhibition is reversible with the IC 50 value of 100 nM • NO for the purified bd oxidases from E. coli and A. vinelandii at 70 µM O 2 in the assay medium [142] (Table 3). Unlike some heme-copper oxidases (see Section 3.1.2), cytochrome bd does not exhibit a measurable • NO reductase activity under anaerobic conditions. The question arises as to if cytochrome bd is quickly inhibited by submicromolar concentrations of • NO and unable even scavenge this RNS via • NO reductase-like reaction, how can it serve as one of the key mechanisms for protecting bacteria against nitrosative stress? Phenomenologically, the answer to this question can be obtained by comparing the kinetic profiles of activity recovery from • NO inhibition following the addition of the • NO scavenger oxyhemoglobin (HbO 2 ) for the bd oxidase and the mitochondrial cytochrome c oxidase ( Figure 6). Upon • NO depletion in solution by HbO 2 , the recovery is significantly faster in cytochrome bd than in the mitochondrial oxidase under similar experimental conditions [142,164]. However, what molecular mechanisms underlie such a rapid recovery of activity in the case of the bd oxidase? Studies of the interaction of • NO with different cytochrome bd species made it possible to shed light on the molecular mechanisms [142,143,165,166]. • NO binds at the level of the heme d active site. The reaction occurs if heme d is in the ferrous, ferryl, or ferric state. The rate of • NO binding to the ferrous uncomplexed heme d (R species) has never been measured. One may expect that its value (k on ) is comparable with those for the binding of CO and O 2 to the fully reduced enzyme, i.e., in the range of 10 8 to 10 9 M −1 ·s −1 [101]. The reaction yields the nitrosyl ferrous heme d adduct (Figure 7, reaction 1) [72]. It turned out that the rate of • NO dissociation from heme d 2+ (k off ) in the purified fully reduced cytochrome bd-I of E. coli is unusually high, 0.133 s −1 [143] (Table 3). A similar value (0.163 s −1 ) was later reported for membrane preparations of E. coli mutant strain RKP4544 devoid of cytochrome bo 3 [155]. This k off value is about 30 times higher than that for • NO dissociation from ferrous heme a 3 in the mitochondrial cytochrome c oxidase [164]. Furthermore, the • NO off-rate for cytochrome bd is faster than that detected for almost all heme proteins. Such a high • NO dissociation rate obviously explains why after • NO-inhibition the activity of cytochrome bd is restored much faster than that of the mitochondrial oxidase ( Figure 6). The reaction of • NO with the A. vinelandii cytochrome bd in the ferryl state (F species) is fast (~10 5 M −1 ·s −1 ) and likely produces the oxidized enzyme with nitrite bound at ferric heme d (Figure 7, reaction 2) [165]. This is about 10 times faster than the same reaction for the mitochondrial cytochrome c oxidase (~10 4 M −1 ·s −1 ) [138,167]. Then, NO 2 likely escapes from heme d 3+ to the bulk phase, but the off rate for nitrite has to be determined. Since intermediate F is highly populated in turnover [105], we think that the rapid oxidation of • NO into NO 2 by cytochrome bd also contributes to the mechanisms of bacterial resistance to • NO. The reaction of • NO with ferric heme d in the purified fully oxidized cytochrome bd-I of E. coli (O species) proceeds with k on of~10 2 M −1 ·s −1 yielding a nitrosyl adduct, d 3+ -NO or d 2+ -NO + (Figure 7, reaction 3) [166]. The reaction is rather slow and the O species is not a catalytic intermediate of cytochrome bd [168] therefore it barely contributes to mechanisms of • NO-inhibition or • NO tolerance. Thus, we can conclude that the bd oxidase confers • NO resistance to bacteria due to (i) extraordinary high • NO off-rate and (ii) the ability to rapidly convert • NO into NO 2 in turnover.
cies) proceeds with kon of ~ 10 2 M −1 ·s −1 yielding a nitrosyl adduct, d 3+ -NO or d 2+ -NO + ( Figure  7, reaction 3) [166]. The reaction is rather slow and the O species is not a catalytic intermediate of cytochrome bd [168] therefore it barely contributes to mechanisms of  NO-inhibition or  NO tolerance. Thus, we can conclude that the bd oxidase confers  NO resistance to bacteria due to (i) extraordinary high  NO off-rate and (ii) the ability to rapidly convert  NO into NO2 -in turnover.

Peroxynitrite and Bacterial Terminal Oxidases
The study of the interaction of peroxynitrite with bacterial terminal oxidases is at the very initial stage. To date, the only bacterial oxidase that has been studied for the reaction with this highly reactive toxic compound is cytochrome bd-I from E. coli [109,169]. Earlier, the interaction of the eukaryotic heme-copper oxidase, the aa3-type cytochrome c oxidase isolated from bovine heart mitochondria, with ONOO − was investigated [170]. It was shown that the mitochondrial enzyme when solubilized or in proteoliposomes is irreversibly damaged by ONOO − (Table 4). At concentrations of less than 20 µM ONOO − significantly raises the enzyme's Km for O2. This effect was tentatively explained by the nitration of some tyrosine residues [137]. At higher concentrations ONOO − was reported to decrease the Vmax. The ONOO − -induced lowering of the Vmax could be due to both the destruction of the CuA site in cytochrome c oxidase, and the irreversible loss of the 830-nm absorption band characteristic of the oxidized CuA was observed [170], and the degradation of hemes a and a3.

Peroxynitrite and Bacterial Terminal Oxidases
The study of the interaction of peroxynitrite with bacterial terminal oxidases is at the very initial stage. To date, the only bacterial oxidase that has been studied for the reaction with this highly reactive toxic compound is cytochrome bd-I from E. coli [109,169]. Earlier, the interaction of the eukaryotic heme-copper oxidase, the aa 3 -type cytochrome c oxidase isolated from bovine heart mitochondria, with ONOO − was investigated [170]. It was shown that the mitochondrial enzyme when solubilized or in proteoliposomes is irreversibly damaged by ONOO − (Table 4). At concentrations of less than 20 µM ONOO − significantly raises the enzyme's K m for O 2 . This effect was tentatively explained by the nitration of some tyrosine residues [137]. At higher concentrations ONOO − was reported to decrease the V max . The ONOO − -induced lowering of the V max could be due to both the destruction of the Cu A site in cytochrome c oxidase, and the irreversible loss of the 830-nm absorption band characteristic of the oxidized Cu A was observed [170], and the degradation of hemes a and a 3 . Borisov et al. studied amperometrically the effect of ONOO − on the O 2 consumption by the E. coli cytochrome bd-I at the level of the isolated detergent-solubilized enzyme and the bd-I overexpressing bacterial cells [169]. It turned out that in both cases, the O 2 consumption by the bd-I oxidase is not inhibited by up to 0.1 mM ONOO − (Figure 8, Table 4). The effect of higher ONOO − concentrations was not tested. After the addition of ONOO − a slight short-term generation of O 2 was observed ( Figure 8). This is likely due to the catalase-like activity of cytochrome bd-I that scavenges H 2 O 2 , a contaminant in the commercial ONOO − or a product of the peroxynitrite degradation [109,113,114]. Furthermore, using the stopped-flow rapid mixing technique it was shown that the bd-I oxidase is able to catalyze scavenging of ONOO − . The kinetics of this reaction was measured [169]. In these experiments, the enzyme pre-reduced anaerobically with excess reducing agents, N,N,N',N'-tetramethyl-p-phenylenediamine (TMPD), and ascorbate, was mixed with an air-equilibrated solution of ONOO − . The ONOO − decomposition rate was determined at 310 nm. It was found that ONOO − disappears with an observed rate constant that is proportional to the cytochrome bd-I concentration and increases with the TMPD concentration. Importantly, in control experiments, neither the protein nor the reductants tested independently reveal the decay of ONOO − to a significant extent. The apparent turnover rate at which the bd-I oxidase, in turnover with O 2 and excess TMPD and ascorbate, decomposes ONOO − , was estimated to be~600 mol ONOO − × (mol enzyme) −1 × min −1 [169] (Table 4). Since the rate constant was found to increase with the enzyme activity (the electron flux), in the bacterial cell in which cytochrome bd-I utilizes ubiquinol as the substrate, the peroxynitrite-decomposing activity may be even higher. For instance, a turnover number of cytochrome bd-I is about seven times higher when the reducing system is ubiquinone-1 plus DTT as compared to that for TMPD plus ascorbate [168]. If the peroxynitrite-neutralizing activity of the bd-I oxidase is proportional to the electron flux, its apparent turnover rate in the E. coli cell could be as high as~4200 mol ONOO − × (mol enzyme) −1 × min −1 . To summarize, the E. coli cytochrome bd-I in the catalytic steady state is not only resistant not ONOO − , but also capable of decomposing this highly reactive cytotoxic effector, thus serving as an important detoxifier of ONOO − in vivo.
A possible mechanism of the peroxynitrite decomposition catalyzed by the bd-I enzyme has never been proposed. We assume that the most likely site for the reaction is the highspin heme d. We may suggest at least four possible reaction mechanisms. The fact that the addition of ONOO − to the isolated bd-I protein in turnover with O 2 and reductants resulted in the production of • NO [169] (Table 4) points out that • NO could be the main product. If this is the case, a one-electron reduction of ONOO − to • NO and H 2 O 2 by the ferrous heme d may occur (Figure 9, reaction 1). If so, at least part of the H 2 O 2 transiently generated following the addition of ONOO − to the enzyme is also the main reaction product. There are two observations that are not consistent with the mechanism proposed. According to the reaction scheme ( Figure 9, reaction 1), the decay of one molecule of ONOO − added should generate one molecule of • NO. In the experiments, however, the amount of • NO produced was approximately 12 times less than the amount of ONOO − added. In addition, no • NO production was detected with the ONOO − -treated cells while the short-term generation of H 2 O 2 is in place (Figure 8). The latter two findings indicate that the • NO produced in the case of the isolated enzyme might be a secondary product, possibly non-enzymatic because the formation of • NO was also observed in the absence of the protein, albeit to a lesser extent [169].  [169] with permission.
A possible mechanism of the peroxynitrite decomposition catalyzed by the bd-I enzyme has never been proposed. We assume that the most likely site for the reaction is the high-spin heme d. We may suggest at least four possible reaction mechanisms. The fact that the addition of ONOO − to the isolated bd-I protein in turnover with O2 and reductants resulted in the production of  NO [169] (Table 4) points out that  NO could be the main product. If this is the case, a one-electron reduction of ONOO − to  NO and H2O2 by the ferrous heme d may occur (Figure 9, reaction 1). If so, at least part of the H2O2 transiently generated following the addition of ONOO − to the enzyme is also the main reaction product. There are two observations that are not consistent with the mechanism proposed. According to the reaction scheme ( Figure 9, reaction 1), the decay of one molecule of ONOO − added should generate one molecule of  NO. In the experiments, however, the amount of  NO produced was approximately 12 times less than the amount of ONOO − added. In addition, no  NO production was detected with the ONOO − -treated cells while the shortterm generation of H2O2 is in place (Figure 8). The latter two findings indicate that the  NO produced in the case of the isolated enzyme might be a secondary product, possibly non-enzymatic because the formation of  NO was also observed in the absence of the protein, albeit to a lesser extent [169]. It was reported that ONOO − generates Compound II (Fe 4+ = O 2− ) in myeloperoxidase, lactoperoxidase, and catalase, and Compound I (Fe 4+ = O 2− Por + , where Por + is a porphyrin radical) in horseradish peroxidase [171,172]. Since these are ferriheme (Fe 3+ ) enzymes, in these reactions ONOO − serves as a one-electron and two-electron oxidant, respectively. We, therefore, suggest that in cytochrome bd-I ONOO − also could react with the ferric heme d, (e.g., to the O 1 catalytic intermediate, see Figure 2). In the case of one-electron oxidation heme d 3+ is converted to Compound F (analog of Compound II, see Figure 2)  − Figure 9. Possible mechanisms of the peroxynitrite decomposition catalyzed by cytochrome bd-I from E. coli.
It was reported that ONOO − generates Compound II (Fe 4+ = O 2− ) in myeloperoxidase, lactoperoxidase, and catalase, and Compound I (Fe 4+ = O 2− Por •+ , where Por •+ is a porphyrin radical) in horseradish peroxidase [171,172]. Since these are ferriheme (Fe 3+ ) enzymes, in these reactions ONOO − serves as a one-electron and two-electron oxidant, respectively. We, therefore, suggest that in cytochrome bd-I ONOO − also could react with the ferric heme d, (e.g., to the O 1 catalytic intermediate, see Figure 2). In the case of oneelectron oxidation heme d 3+ is converted to Compound F (analog of Compound II, see Figure 2) with the concomitant release of • NO 2 from ONOO − (Figure 9, reaction 2).
It is also possible that the ferric heme d catalyzes the isomerization of peroxynitrite to nitrate (NO 3 -). If so, Compound F and • NO 2 are transient reaction intermediates, not the final products (Figure 9, reaction 3). The fact that certain iron (III) porphyrins are capable of catalyzing the isomerization of ONOO − to NO 3 - [173] is in agreement with this hypothesis. In the case of two-electron oxidation heme d 3+ is converted to Compound F* (analog of Compound I, see Figure 2) with the co-production of NO 2 − from ONOO − (Figure 9, reaction 4). It is worth noting that microbial and mammalian peroxiredoxins catalyze detoxification of peroxynitrite via its two-electron reduction to nitrite [174,175].

Concluding Remarks
Usually, terminal oxygen reductases of bacterial respiratory chains are strongly inhibited by nitric oxide and peroxynitrite. However, some of the respiratory enzymes, such as the mycobacterial bcc-aa 3 supercomplex and bd-type oxidases, confer resistance to RNS, thereby contributing to microbial pathogenicity. An understanding of the molecular mechanisms of bacterial pathogenicity is essential for the development of new strategies to combat infectious diseases. In this regard, it would be interesting to figure out the reaction mechanisms underlying bcc-aa 3 supercomplex-mediated • NO detoxification and importantly, whether this unique property of the mycobacterial enzyme is shared by other aa 3 -type oxidases, eventually complexed with the bc 1. The interest in bd-type oxidases is increasing due to their peculiar enzymatic abilities, stress tolerance, and importance to pathogensfeatures that merit more in-depth functional and structural studies. Determination of cytochrome bd structure from different microorganisms would help in the characterization and rational design of selective inhibitors of these oxidases. Based on already published 3D structures of bd-type oxidases, one of the main challenges in the structure-driven design of quinone substrate-like inhibitors is expected to be the high flexibility of the N-terminal part of the quinol binding site called the Q-loop. Another promising direction for future research is the study of the effect of RNS on the anaerobic terminal reductases and other bioenergetic enzymes in anaerobic pathogenic bacteria. All in all, the development of next-generation antibiotics selectively targeting the RNS-insensitive respiratory complexes in pathogens may reduce their impact on human health and social development.

Conflicts of Interest:
The authors declare no conflict of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript, or in the decision to publish the results.