Article

ISSN 0006-2979, Biochemistry (Moscow), 2023, Vol. 88, No. 10, pp. 1504-1512 © Pleiades Publishing, Ltd., 2023.

Published in Russian in Biokhimiya, 2023, Vol. 88, No. 10, pp. 1818-1828.

1504

REVIEW

Generation of Membrane Potential by Cytochrome bd

Vitaliy B. Borisov

Belozersky Institute of Physico-Chemical Biology, Lomonosov Moscow State University, 119991 Moscow, Russia

e-mail: bor@belozersky.msu.ru

Received June 10, 2023

Revised July 8, 2023

Accepted July 11, 2023

Abstract— An overview of current notions on the mechanism of generation of a transmembrane electric potential differ-

ence(Δψ) during the catalytic cycle of a bd-type triheme terminal quinol oxidase is presented in this work. It is suggested

that the main contribution to Δψ formation is made by the movement of H

across the membrane along the intra-protein

hydrophilic proton-conducting pathway from the cytoplasm to the active site for oxygen reduction of this bacterial enzyme.

DOI: 10.1134/S0006297923100073

Keywords: respiratory chain, terminal oxidase, cytochromebd, heme, protonmotive force, membrane potential

Abbreviations: Δψ,transmembrane electrical potential difference; Δp,protonmotive force; τ,time constant, reciprocal of rate

constant(t

1/e

); H

–

,proton/electron stoichiometry which in the case of Escherichia coli respiratory chain means number of pro-

tons released into the periplasm per electron used to reduce oxygen to water; RuBpy,tris(2,2′-bipyridyl)ruthenium(II) chloride.

INTRODUCTION

In 1974, L. A. Drachev and co-authors at the

Belozersky Institute of Physico-Chemical Biology of

Lomonosov Moscow State University developed an

electrometric method for direct measurement of elec-

trical activity of coupling membranes, which provided a

unique opportunity to track intra-protein movements of

electrical charges within one molecular turnover of the

enzyme [1]. Using this method, it was possible to ob-

serve in real time generation of the transmembrane elec-

tric potential difference (Δψ) by bacteriorhodopsin [2],

reaction centers [3], and cytochrome bc

[4] from photo-

synthetic bacteria, as well as terminal cytochrome c oxi-

dase [5-7] and non-canonical retinal-containing bacte-

rial proteins [8, 9]. Two different approaches are used

to study electrogenic mechanism of cytochromec oxi-

dases. The first approach uses photochemical injection

of a single electron into the enzyme embedded in a li-

posome. In this case, tris(2,2′-bipyridyl)ruthenium(II)

chloride (RuBpy) acts as a direct photoactivated reduc-

ing agent, which forms a complex with the cytochrome c

binding site in the oxidase near the input Cu

redox cen-

ter due to electrostatic interactions [5, 6]. As a result of

photoexcitation of RuBpy by a pulsed laser, an electron

is transferred from RuBpy* to Cu

. The oxidized RuBpy

is re-reduced by aniline. This approach makes it possi-

ble to record time-resolved electrogenic charge transfer

during individual one-electron transitions in the cat-

alytic cycle of cytochrome c oxidase [7]. In the second

approach, laser flash photolysis of a complex of car-

bon monoxide (CO) with the oxygen-binding high-spin

hemea

is used to initiate enzymatic reaction in the sin-

gle-turnover mode. Formation of the CO complex with

the partially or completely reduced enzyme occurs un-

der anaerobic conditions. Oxygen(O

) dissolved in water

is then added to the anaerobic cell with the CO-bound

oxidase using rapid mixing technique. During decompo-

sition of the CO-oxidase complex triggered by photolysis,

binds to hemea

and is reduced by electrons pres-

ent in the oxidase that is accompanied by generation of

Δψ[10]. Thus, the second approach uses combination

of the direct electrometric method [1] and the flow-

flash method [11]. Terminal quinol oxidases including

cytochrome bd, which is the subject of this review, do

not have a cytochromec binding site. For this reason,

the first approach is inapplicable for tracking movement

of electric charges inside their protein molecule.

GENERAL CHARACTERISTICS

OF CYTOCHROME bd

Membrane-bound terminal oxidases of the aerobic

respiratory chains of organisms are classified as translo-

cases (enzymes in class EC7). They catalyze four-electron

ELECTROGENIC CYTOCHROME bd 1505

BIOCHEMISTRY (Moscow) Vol. 88 No. 10 2023

reduction of molecular oxygen to water by ferrocyto-

chromec or quinol (ubiquinol, menaquinol, and possi-

bly plastoquinol) [12,13]. The catalyzed redox reaction

is coupled with generation of Δp (protonmotive force).

Δp is an “energy currency” and is used by the cell to syn-

thesize ATP through the mechanism of oxidative phos-

phorylation [14]. Terminal oxidases are divided into two

evolutionarily unrelated superfamilies: heme/Cu-con-

taining oxidases and bd-type oxidases also called cyto-

chromes bd [15-18]. Unlike the heme-copper oxidases,

all biochemically characterized cytochromes bd are qui-

nol oxidases, do not contain Cu, and are found only

in bacteria and archaea, including pathogens [19-21].

The latter circumstance makes it possible to consider

bd enzymes as promising therapeutic targets [21, 22].

Since generation of Δψ in the single-turnover mode has

been studied so far only in the terminal bd oxidases from

Escherichia coli, we should consider these enzymes in

more detail.

Like the electron transport chains of many bac-

teria, aerobic respiratory chain of E. coli is branched.

Its terminal region is generally represented by three qui-

nol oxidases: heme-copper cytochromebo

and two cy-

tochromes bd, bd-I and bd-II [23,24]. Unlike bd-type

oxidases, cytochrome bo

forms Δp by the proton pump

mechanism that makes it possible to double pump-

ing stoichiometry: proton/electron (H

–

) [25, 26].

Cytochromes bo

, bd-I, and bd-II are encoded by the

cyoABCDE, cydABX, and appCBX operons, respectively.

cyoABCDE is predominantly expressed under high O

partial pressure, while cydABX is predominantly ex-

pressed under microaerobic conditions. The appCBX

expression is induced during anaerobic growth of E. coli,

entry of the culture into the stationary phase of growth,

and phosphate starvation [24]. Recently, there has been

more and more evidence reported that, in addition

to functioning as molecular energy transducers, bd-type

oxidases are involved in other vital processes in the bac-

terial cell [27-30]. Cytochromebd-I is involved in for-

mation of disulfide bonds during protein folding [31],

heme biosynthesis [32], and mechanisms of bacterial

resistance to antibiotics [33], peroxynitrite [34], nitro-

gen monoxide [35-41], and ammonia [42]. Both bd oxi-

dases (bd-I and bd-II) also endow E. coli with resis-

tance to cyanide [43], sulfide [43-45], and hydrogen

peroxide [46-54].

Three-dimensional structures of both E. coli bd en-

zymes have recently been published (Figs. 1 and2) [55-58].

Cytochrome bd-I was found to contain four subunits

(CydA, CydB, CydX, CydY), while cytochrome bd-II

only three (AppC, AppB, AppX). The CydA, CydB, and

CydX subunits are homologous to the AppC, AppB, and

AppX subunits, respectively. Two large subunits, CydA/

AppC and CydB/AppB, form structural core of the pro-

tein. Of the other structural differences between the two

bd oxidases, it should be noted that the bd-II protein in-

corporated into amphipoles is mainly in the form of a

dimer (Fig. 2), while the bd-I enzyme exists only as a

monomer [57] (Fig. 1). Oxygen channel in cytochrome

bd-II has a smaller diameter compared to that of cyto-

chrome bd-I [57]. In addition, the putative proton-con-

ducting pathway in the bd-II enzyme is shorter than in

the bd-I oxidase [57]. CydA/AppC contains three dif-

ferent hemes acting as redox cofactors: one low-spin

hexacoordinate, b

558

, and two high-spin pentacoordi-

nate, b

595

and d. The heme axial ligands are amino acid

Fig. 1. Three-dimensional structure of E. coli cytochrome bd-I with

3.3 Å resolution (pdb ID 6RX4). In addition to hemesb

558

, b

595

, andd

associated with the CydA subunit, ubiquinone-8 (Q8) and glycero-

phospholipid (shown as spherical symbols) associated with the CydB

subunit are found in the protein structure. Reprinted from Theßeling

et al. [55] under the terms of the Creative Commons Attribution4.0

International Public License.

Fig. 2. Three-dimensional structure of E. coli cytochrome bd-II dimer

with 3.0Å resolution (pdbID 7OSE). In addition to hemesb

558

, b

595

andd associated with the AppC subunit, ubiquinone-8 (shown in red)

associated with the AppB subunit is found in the protein structure.

Reprinted from Grauel et al. [57] under the terms of the Creative Com-

mons Attribution4.0 International Public License.

BORISOV1506

BIOCHEMISTRY (Moscow) Vol. 88 No. 10 2023

Fig. 3. Triangular arrangement of hemesb

558

, b

595

, andd in the CydA

subunit of E.coli cytochromebd-I. Periplasm: top of the picture, cy-

toplasm: bottom of the picture. Reprinted from Theßeling et al. [55]

under the terms of the Creative Commons Attribution4.0 International

Public License.

residues of the CydA/AppC subunit. These are His186

and Met393 for heme b

558

and Glu445 for heme b

595

[55-58]. In cytochromebd-II, the axial ligand of hemed

is His19 [57-58]. In the case of cytochrome bd-I, data

on the nature of the hemed axial ligand are contradic-

tory. Safarian etal. [56] state that this is also His19, but

according to the model of Theßeling etal. [55], such a

ligand is Glu99. The hemes in the protein are arranged

in a triangle (Fig. 3). Additional structural element in

CydA/AppC is the so-called Q-loop. It is located near

heme b

558

and is directly involved in binding of quinol,

a lipophilic electron donor. The other large subunit,

CydB/AppB, does not contain any metal-containing co-

factors. Instead, it carries a tightly bound ubiquinone-8

or demethylmenaquinone-8. This quinone occupies posi-

tion equivalent to the heme-binding site in CydA/AppC

and, probably, plays a role in the protein structure sta-

bilization. Heme b

558

is the primary electron acceptor

upon quinol oxidation. Heme d serves as a site for O

binding and its subsequent reduction to 2H

O [59,60].

Hemed in cytochromebd-I has an unusually high affin-

ity for O

, and the resulting oxygenated complex is very

stable [61-64]. Functions of hemeb

595

are poorly under-

stood. Excessive distance between the central Fe atoms

of hemesb

595

andd (10.9-11.3Å) most likely does not

allow them to form a structural binuclear center similar

to that of heme-copper oxidases. However, van der Waals

contacts between these hemes are possible since the dis-

tance between their edges is much smaller (3.5-3.8 Å)

[55-58]. The latter circumstance suggests the possibility

of a very fast electron transfer between hemesb

595

andd

that was experimentally confirmed [65,66]. Therefore,

these hemes could potentially form a functional diheme

center. This assumption is consistent with the data of a

number of studies [67-79]. An electron that came from

quinol to hemeb

558

is apparently transferred to hemeb

595

and next to hemed.

ELECTROGENIC REACTIONS

AND CATALYTIC CYCLE

OF CYTOCHROME bd-I FROM E. coli

Use of optical and electrometric methods in com-

bination with flow-flash method made it possible to

observe in real time transient formation and decay of

the individual intermediates of the catalytic cycle of

E. coli cytochrome bd-I at 21°C [26, 80-83]. The pro-

posed scheme of the catalytic cycle is shown in Fig.4.

In spectroscopic studies, hemoprotein was in detergent

micelles, and in electrometric studies, it was incorporated

into liposomes. In the experiment, the enzyme was ini-

tially converted into a completely reduced state in which

heme d was bound to CO (R

–CO, b

558

595

–CO).

Photolysis of CO from this state of the oxidase leads to

the transient appearance of the form of cytochromebd-I

not bound to CO (R

, b

558

595

). This transition

–CO→R

) is not resolved in time in both spectro-

photometric and electrometric measurements. In the

presence of O

, a molecule of this diatomic gas binds

to heme d. As a result, the oxygenated complex, inter-

mediate A

558

595

–O

), is formed. The rate of

formation of A

is directly proportional to concentra-

tion of O

, with the second-order rate constant to be

about 2 × 10

–1

[64, 82]. The R

→A

transition

is not accompanied by generation of Δψ [26, 82, 83].

is quickly (τ ~ 4.5 μs) converted into an intermediate,

which Belevich et al. first discovered, described, and

named as compoundP [82]. It was found that the A

→P

transition is also not coupled with generation of Δψ [26,

82, 83]. In contrast to the production of A

from R

the rate of formation of compoundP does not depend

on concentration of O

. During the A

→P transition,

hemeb

595

undergoes oxidation, hemeb

558

remains in the

reduced state, and new oxygen intermediate of heme d

reveals an unusual absorption maximum at 635 nm[82].

There is still no consensus on chemical structure of

the compound P. In the original work [82], Belevich

et al. suggested that P is a true peroxide complex, ei-

ther a ferryl intermediate with an amino acid radical or

a cation radical of the porphyrin ring. According to the

more recent report by Paulus etal. [84], compound P

is a ferryl form of hemed with π-cation radical on the

porphyrin ring, which is in magnetic interaction with

heme b

595

. It is important to emphasize that Paulus etal.

[84] observed formation of compound P at 1°C, i.e.,

under non-physiological conditions. It is possible that the

spectral intermediateP, appearance of which was regis-

tered in real time by Belevich et al. [82], is a mixture

of a true peroxide complex (b

558

595

–O–O–(H))

and a ferryl π-cation radical (b

558

595

=O

2–

), pro-

vided that they have similar absorption spectra. At the

next stage, P is converted (with τ ~ 47 μs) into a non-rad-

ical form of the ferryl complex of heme d (compound F)

that is accompanied by oxidation of heme b

558

. Cat-

ELECTROGENIC CYTOCHROME bd 1507

BIOCHEMISTRY (Moscow) Vol. 88 No. 10 2023

Fig. 4. Catalytic cycle of the E.coli cytochromebd-I. Compounds A

P, F, O

, A

are catalytic intermediates of the enzyme. Compounds

and R

–CO are not part of the oxidase catalytic cycle, but can be

obtained artificially. Red “arrows of coupling” indicate generation of

Δψ at P→F and F→A

transitions. Structures of the compounds are dis-

cussed in the main text.

Fig. 5. Proposed proton-conducting pathway in E.coli cytochrome bd-I.

The pathway is lined with side chains of several hydrophilic amino

acids and allows transfer of protons from the cytoplasmic side of the

membrane to hemed propionate. It also contains numerous water mol-

ecules (indicated by blue spherical symbols). Reprinted from Friedrich

et al. [22] under the terms of the Creative Commons Attribution4.0

International Public License.

alytic intermediate F, most likely, has the structure of

558

595

= O

2–

. The P→F transition is associated

with generation of Δψ [26, 82, 83].

The bd-type oxidase contains three hemes. There-

fore, if the isolated enzyme does not contain a bound

quinol, then it can be expected that in the completely

reduced state it carries three electrons(R

). In this case,

the reaction of R

with O

stops at formation of com-

pound F [80]. If cytochrome bd-I contains a molecule

of bound quinol, which is a two-electron donor, its oxi-

dation in the presence of O

makes it possible to convert

F into intermediate A

with τ ~ 0.6-1.1 ms [81, 82]. A

is,

probably, the one-electron form of the oxidase with the

heme d oxycomplex (b

558

595

–O

). The F→A

tran-

sition, like the previous P→F transition, is accompanied

by generation of Δψ [81, 82]. Whether Δψ is formed at

one more particular stage of the catalytic cycle, in the

→A

transition (Fig.4), is still unknown.

It was found that under the steady-state conditions

in the presence of O

and ubiquinol-1, F and A

are main

catalytic intermediates of the cytochrome bd-I (about

40% each) [60]. About 20% of the oxidase is probably in

the O

state that is a one-electron form with the oxidized

heme d (b

558

595

–OH). The O

state has not been

observed in the single-turnover experiments using the

flow-flash method [80, 82, 83]. However, it is currently

recognized that O

is apparently also a catalytic interme-

diate of the cytochrome bd-I (Fig.4). It should also be

noted that the R

form of the enzyme is most likely not

its catalytic intermediate [59,60], however, for the needs

of experiment, it can be easily produced artificially.

In 2005, Belevich et al. [81] postulated based on

the obtained results existence of an intra-protein pro-

ton-conducting pathway for the transfer of H

from cyto-

plasm to the oxygen reductase center of cytochrome bd-I.

The authors suggested that such movement of H

across

the membrane, associated with the transfer of an electron

from hemeb

558

to hemesb

595

andd, is accompanied by

generation of Δψ observed in the experiments [26, 80-83].

Release of H

into the periplasmic space during oxida-

tion of quinol by the enzyme also contributes to cre-

ation ofΔp. 3D structures of the bd-I oxidase published

in 2019, with resolution of 2.68Å (pdb ID 6RKO) [56]

and 3.3Å (pdbID 6RX4) [55], confirmed the hypothesis

suggested by Belevich etal. [81]. The structures show a

chain of water molecules stretching along a hydrophilic

proton-conducting pathway that starts at the cytoplasmic

interface between the CydA and CydB subunits and runs

perpendicular to the membrane plane towards heme d.

This proton-conducting pathway includes several hydro-

philic amino acid residues (Fig. 5). From the cytoplas-

mic side, the pathway begins with Asp119

CydA

, then, ap-

parently, it includes Lys57

CydA

, Lys109

CydA

, Asp105

CydA

Tyr379

CydB

, and, finally, Asp58

CydB

, from which protons

are likely delivered to the propionate group of heme d [55].

It has been suggested that the conserved hydrophilic resi-

dues Ser108

CydA

, Glu107

CydA

, and Ser140

CydA

also belong

to this pathway, facilitating transfer of H

from Asp58

CydB

to the hemed propionate [56].

BORISOV1508

BIOCHEMISTRY (Moscow) Vol. 88 No. 10 2023

Belevich et al. [81] also hypothesized that the bd-I

molecule contains two amino acid residues with pro-

tonated groups, which are sensitive to the redox state of

the high-spin pentacoordinate hemesb

595

andd. Studies

of the Glu445Ala and Glu107Leu mutant forms of the

E. coli cytochrome bd-I by electrometry and absorp-

tion spectroscopy with microsecond resolution indi-

cate that exactly these highly conserved Glu445

CydA

and

Glu107

CydA

residues are functionally important [81,83].

As noted above, Glu445

CydA

is the axial ligand of the

hemeb

595

iron [55, 56]. Its replacement with Ala in the

CydA subunit leads to the enzyme inactivation. At the

same time, hemeb

595

is retained in the protein but loses

its ability to be reduced even in the presence of a strong

electron donor, dithionite, added in excess [81]. As in

the case of the wild-type cytochrome bd-I, the reaction

of the reduced Glu445Ala mutant enzyme with oxygen

exhibits an initial non-electrogenic stage consisting of

the R

→A

and A

→P transitions. However, in contrast

to the wild-type enzyme, the microsecond phase is not

detected in the mutant during Δψ generation. Instead,

the mutant form exhibits a slower, smaller electrogen-

ic phase (τ ~ 1.3 ms; amplitude –0.36 mV) followed by

a much larger electrogenic transition (τ ~ 12.5 ms; am-

plitude –1.7 mV). Both electrogenic phases, most likely,

reflect the P→F transition in different subpopulations

of the Glu445Ala enzyme [81]. Thus, the substitu-

tion of Glu445 for Ala strongly inhibits the transmem-

brane charge transfer associated with oxidation of cyto-

chromebd-I by oxygen.

Similarly, substitution of Glu107 for Leu in the

CydA subunit leads to the loss of quinol oxidase ac-

tivity by cytochrome bd-I. The fully reduced mutant

form of the Glu107Leu protein (R

) binds O

at about

the same rate as the wild-type enzyme. However, for-

mation of the ferryl intermediate(F) in the mutant ox-

idase is believed to be significantly slower compared to

the wild-type enzyme. This is evidenced by the results

of spectrophotometric experiments, according to which

production of the compound F has not been observed

within the 100-μs time interval in the mutant oxidase,

in contrast to the wild-type protein [83]. This conclu-

sion is consistent with the fact that the rate of generation

ofΔψ (the main phase) by the mutant oxidase is about

350times slower than the rate measured for the wild-type

enzyme [83].

Glu445

CydA

appears to be protonated during the

transition of heme b

595

from the oxidized to the re-

duced form, i.e., it serves to compensate for the nega-

tive charge of the electron that came to the heme. In the

case of heme d, Glu107

CydA

probably plays the same role.

According to the published three-dimensional struc-

ture of the E.coli cytochrome bd-I, heme b

595

is located

near the periplasmic surface [55, 56]. Therefore, if H

is

transferred to Glu445

CydA

from the periplasmic side of

the membrane during the heme b

595

reduction, this pro-

ton is unlikely to be used in the oxygen reductase reac-

tion catalyzed by the enzyme.

CAN CYTOCHROME bd-II

FROM E. coli GENERATE Δψ?

Functional studies of the E.coli cytochromebd-II

are still at the very early stages. Becker etal. [85] report-

ed that the H

–

ratio for the bd-II enzyme is 0, i.e.,

it is an uncoupled quinol oxidase. It is known that cy-

tochromes bd-I and bo

from E.coli are coupled quinol

oxidases, with the H

–

values of 1 and 2, respective-

ly[25, 26]. Becker et al. constructed the mutant strain

of E. coli, MB37, in the respiratory chain of which cy-

tochrome bd-II was present but all the primary proton

potential generators known at that time, NADH de-

hydrogenase 1 (NDH-1), cytochrome bo

, and cyto-

chrome bd-I, were absent. The authors calculated H

–

by comparing the values for the specific rates of oxygen

consumption and ATP synthesis observed for the MB37

strain and other E. coli mutant strains for which the

–

values had already been measured [85]. Bacterial

cells of all the strains were grown under the same condi-

tions, and the rate of ATP synthesis was calculated taking

into account the rates of formation of metabolic prod-

ucts– CO

, acetate, ethanol, and lactate. Unexpectedly,

the MB37 strain, which, according to the authors’ sug-

gestion, should have the completely uncoupled aerobic

respiratory chain, was capable of growing under aerobic

conditions on non-fermentable substrates. However, the

question arises: how is ATP synthesis ensured in this

case? Becker et al. hypothesized [85] that ATP in the

MB37 strain is produced exclusively via substrate phos-

phorylation. In the more recent work, Shepherd et al.

[86] suggested that in this mutant strain the proton po-

tential is formed due to functioning of an electrogenic

antiporter, which transports an anion of glutamic acid

(glutamate) into the cell in exchange for the release of

a neutral γ-aminobutyric acid (GABA) from the cell.

In this case, GABA in the cell is synthesized from glu-

tamate, and an intracellular proton is consumed during

the process.

Borisov et al. [26] found the conclusions of the

authors of those two studies [85, 86] unconvincing and

experimentally tested whether cytochrome bd-II gen-

erates Δp. It was found that, under the steady state

conditions, both components of Δp – Δψ and ΔpH –

are formed due to quinol oxidase activity of cyto-

chromebd-II [26]. The H

–

ratio was measured. As in

the case of cytochrome bd-I, it turned out tobe1[26].

It was also shown that the bd-II oxidase is able to gen-

erate Δψ during a single molecular turnover of the en-

zyme, presumably, during the P→F and F→A

tran-

sitions [26]. Thus, one can conclude that the E. coli

cytochrome bd-II is the primary generator of Δp.

ELECTROGENIC CYTOCHROME bd 1509

BIOCHEMISTRY (Moscow) Vol. 88 No. 10 2023

Therefore, to explain the growth of the E. coli MB37

cells under aerobic conditions, alternative mechanisms

of ATP formation proposed in [85,86] are not required.

Funding. This work was financially supported by the

Russian Science Foundation (project no.22-24-00045,

https://rscf.ru/en/project/22-24-00045/).

Acknowledgments. The author would like to express

his deepest gratitude to M. I. Verkhovsky (passed away),

I. N. Belevich, N. P. Belevich, D. A. Bloch (passed away),

and A. Jasaitis for wonderful time spent measuring elec-

trogenic activity of the enigmatic cytochromebd.

Ethics declarations. The author declares no conflict

of interest in financial or any other sphere. This article

does not contain any studies involving animals or hu-

man participants performed by author.

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