(Received for publication, December 3, 1996, and in revised form, April 14, 1997)
From the Department of Public Health, Graduate School of Medicine, Kyoto University, Kyoto 606, Japan
Stopped-flow rapid-scan spectrophotometry was employed to study complicated oxidation processes of ubiquinol-cytochrome c reductase (QCR) that was purified from bovine heart mitochondria and maximally contained 0.36 mol of ubiquinone-10/mol of heme c1. When fully reduced QCR was allowed to react with dioxygen in the presence of cytochrome c plus cytochrome c oxidase, the oxidation of b-type hemes accompanied an initial lag, apparently low potential heme bL was oxidized first, followed by high potential heme bH. Antimycin A inhibited the oxidation of both b-type hemes. The oxidation of heme c1 was triphasic and became biphasic in the presence of antimycin A. On the other hand, starting from partially reduced QCR that was poised at a higher redox potential with succinate and succinate-cytochrome c reductase, the b-type hemes were oxidized immediately without a lag. When the ubiquinone content in QCR was as low as 0.1 mol/mol heme c1 the oxidation of the b-type hemes was almost suppressed. As the Q-deficient QCR was supplemented with ubiquinol-2, the rapid oxidation of b-type hemes was restored to some extent. These results indicate that a limited amount of ubiquinone-10 found in purified preparations of QCR is obligatory for electron transfer from the b-type hemes to iron-sulfur protein (ISP) and heme c1.
The characteristic oxidation profiles of heme bL, heme bH, and heme c1 were simulated successfully based on a mechanistic Q cycle model. According to the simulations the two-electron oxidation of ubiquinol-10 via the ISP and heme c1 pathway, which is more favorable thermodynamically than the bifurcation of electron flow into both ISP and heme bL, does really occur as long as heme bL is in the reduced state and provides ubiquinone-10 at center i. Mechanistically this process takes time, thus explaining the initial lag in the oxidation of the b-type hemes. With the partially reduced QCR, inherent ubisemiquinone at center i immediately oxidizes reduced heme bH thus eliminating the lag.
The mechanistic Q cycle model consists of 56 reaction species, which
are interconnected by the reaction paths specified with microscopic
rate constants. The simulations further indicate that the rate
constants for electron transfer between the redox centers can be from
105 to 103 s1 and are rarely
rate-limiting. On the other hand, a shuttle of ubiquinone or ubiquinol
between center o and center i and the oxidation
of heme c1 can be rate-limiting. The interplay
of the microscopic rate constants determines the actual reaction
pathway that is shown schematically by the "reaction map." Most
significantly, the simulations support the consecutive oxidation of
ubiquinol in center o as long as both heme
bL and heme bH are in
the reduced state. Only when heme bL is
oxidized and ISP is reduced can SQo donate an electron to heme
bL. Thus, we propose that a kinetic control
mechanism, or "a kinetic switch," is significant for the bifurcation of electron flow.
Ubiquinol-cytochrome c oxidoreductase (QCR1; bc1 complex or complex III) is one of the three sites for energy conservation in the mitochondrial respiratory chain. This mitochondrial enzyme consisting of 11 subunits (1) translocates protons from the matrix side of mitochondrial inner membranes toward the cytoplasmic side coupled with electron transfer from ubiquinol to cytochrome c (2, 3). QCR contains four redox centers, two b-type hemes (heme b562/bH and heme b566/bL), a c-type heme (heme c1), and a 2Fe-2S cluster (ISP) (3). In mitochondria, low potential heme bL is located near the outside surface of the inner membrane, whereas high potential heme bH is situated inside the membrane about 20 Å away from heme bL. ISP and heme c1 are largely extramembranous on the cytoplasmic side of the inner membrane (4). In addition to these four prosthetic groups, ubiquinone-10 is usually found in purified QCR prepared from mammalian mitochondria (5, 6).
Previous work on the mechanism of electron transfer and proton translocation by QCR revealed characteristic features that lead to various hypothetical mechanisms (7, 8). To date, the protonmotive Q cycle, originally proposed by Mitchell (2), has become the generally accepted hypothesis. The central idea of the cyclic model is "branching" of electron flow from ubiquinol that delivers an initial electron to ISP at center o on the cytoplasmic side, one of the assumed Q-reactive centers. This electron is transferred from ISP to heme c1 and then to cytochrome c. Ubisemiquinone (SQ) thus generated is an intermediate and subsequently donates an electron to low potential heme bL at center o yielding quinone in turn. Then, quinone is translocated to center i, another Q-reactive site on the matrix side, and reduced to SQi by accepting an electron from high potential heme bH to which the electron has been transferred from heme bL (3, 9, 10). Ubiquinone at center o or i is usually referred to as Qo or Qi, respectively. These reactions constitute the first half of the Q cycle. In the second half, the oxidation of another molecule of quinol at center o proceeds following the same processes as before and provides a second electron at center i to reduce SQi to quinol. The quinol then goes back to center o completing the protonmotive Q cycle. Thus bifurcation of electron flow from ubiquinol into ISP and heme bL at center o as well as electrogenic electron transfer from heme bL to heme bH is most pivotal in the energy conservation mechanism because this supports proton translocation across the membrane.
Despite a considerable experimental support for the protonmotive Q cycle, there are still some observations that are not necessarily compatible with this model (11-15). The oxidation of reduced QCR purified from yeast or bovine heart mitochondria by oxidants has been reported to occur even when the endogenous ubiquinone is depleted from the enzyme complex (11, 12). This result is apparently inconsistent with the proposed functional role of Q not only as a proton translocator but also as an electron mediator between b-type hemes and ISP. Also, it has been reported that no lag appears in the oxidation of b-type hemes when fully reduced yeast QCR is oxidized by ferricyanide (12), or of heme b in rat liver mitochondria by ferricyanide plus air (13). The latter result forms the basis for a proposed semiquinone cycle that assumes a shuttle of ubisemiquinone between center o and center i (8). According to the Q cycle mechanism, the oxidation of the b-type hemes initiated by pulsing an oxidant to the fully reduced QCR does not occur immediately; Q that is required to oxidize heme bH at center i is lacking because further oxidation of an intermediate SQo by heme bL at center o is blocked as this heme is in the reduced state initially. Therefore, it is important to confirm experimentally whether the oxidation of b-type hemes accompanies a lag or not and to examine the obligatory role of ubiquinone in this oxidation (16-18).
In previous studies (11-13), nonphysiological oxidants such as ferricyanide and a cobalt chelate were used mostly as an electron acceptor for QCR. Although precautions to eliminate their direct interactions especially with the b heme(s) in QCR were taken, the possibility has been pointed out that ferrous heme b is accessible to ferricyanide at the outer side of submitochondrial particles (19). This problem would be resolved if we use cytochrome c plus cytochrome c oxidase (CCO) as the oxidizing system. On the other hand, spectral complexities that are introduced by use of this system and accordingly may hamper the data analyses will be lessened by recording all the spectral changes with rapid-scan spectrophotometry. A series of absorption spectra collected during a reaction and displayed in a way to disclose their characteristic features in detail are useful not only in manifesting the full aspect of the spectral changes at a glance but also in detecting and characterizing reaction intermediates of hitherto unknown nature, if any (20-22). A deliberate choice of experimental conditions to shift the rate-limiting step would be advantageous to increase an occupancy of a certain spectral species and thus to identify its nature.
Here, we employ a stopped-flow and rapid-scan technique to establish whether the oxidation of b-type hemes in fully reduced QCR exhibits a lag or not. The oxidation is initiated by mixing reduced QCR with dioxygen in the presence of cytochrome c and CCO. The QCR preparations purified from bovine heart muscle usually contain a varying amount of ubiquinone, mostly substoichiometric to heme c1, and consequently the preparations seem to be a mixture of QCR with a full set of redox centers and an incomplete set. Especially the QCR preparation with the lowest content of ubiquinone is suitable to examine its putative obligatory role in reoxidation, and in fact it is shown that ubiquinone is absolutely necessary for the oxidation of b-type hemes. These results have led us to interpret our results in the context of a "Q pocket" model that contains centers i and o, as assumed by Wikström and Krab (8). Such a pocket may be provided by a dimeric structure of this complex revealed by the structural studies (4, 23) even if it is lacking in the monomeric structure. It is also possible that ubiquinone and ubiquinol make contact alternatively with o and i domain in the Q pocket without being released from QCR.
We also simulate the behavior of the redox centers based on a proposed kinetic model, in which starting from the fully reduced state of QCR the reaction intermediates proliferate as the reaction proceeds in accordance with the multiplicity of an intermediate containing a specified number of reducing equivalents, and then converge to final products. One of the advantages of this approach is to allow us to test alternative mechanistic possibilities by incorporating the thermodynamic and kinetic parameters that define the reaction into computer simulations. Consequently, a kinetic control mechanism for the bifurcation of electron flow will be proposed that contrasts with the thermodynamic barrier hypothesis proposed by Ding et al. (24) but bears some resemblance to the "catalytic switch" mechanism proposed by Brandt et al. (25, 26).
Succinate-cytochrome c reductase (27),
ubiquinol-cytochrome c reductase (6), and cytochrome
c oxidase (20) were purified from beef heart muscle
according to previously reported methods and stored at 80 °C until
used. Succinate-cytochrome c reductase (SCR) contained about
3.5 nmol of heme b/mg of protein and exhibited the electron
transfer activity of 70-90 nmol of cytochrome c
reduced·s
1·(mg protein)
1 in a medium
containing 0.1 M sodium phosphate buffer (pH 7.4), 0.3 mM EDTA, 20 mM succinate, and 100 µM cytochrome c (28, 29). Purified
preparations of ubiquinol-cytochrome c reductase (QCR) contained 4.2-4.5 nmol of heme c1/mg of protein
and exhibited the catalytic activity of 330-410 mol of cytochrome
c reduced·s
1·(mol heme
c1)
1 when measured in an assay
mixture containing 50 mM sodium phosphate buffer (pH 7.0),
0.3 mM EDTA, 50 µM cytochrome c,
and 25 µM Q2H2 at 20 °C (6,
30). The initial rate of cytochrome c reduction was
corrected against nonenzymatic reduction of cytochrome c by ubiquinol in the absence of QCR. The Q10 content of QCR
varied with enzyme preparations ranging from 0.1 to 0.36 mol of
Q10/mol of heme c1. The purity and
the enzyme activity of cytochrome c oxidase (CCO) were the
same as reported previously (20).
Cytochrome c (horse heart, type III) and antimycin A were purchased from Sigma. Cholic acid was obtained from Wako Pure Chemicals (Tokyo, Japan). Other chemicals were obtained commercially at the highest purity.
Stopped-flow rapid-scan recordings with and without a laser flash were carried out on an apparatus as described previously (20-22). With this apparatus the recording time of a spectrum over a 200-nm wavelength range was 12 ms, and usually 100 spectra were recorded with a minimal time interval of 30 ms including the recording time. The dead time of the apparatus under the present experimental conditions was around 10 ms, and the end of this period was chosen as time 0 for displaying spectral changes.
Two different methods were employed to prepare sample solutions for stopped-flow and rapid-scan measurements as follows. Method 1: purified QCR was diluted with 50 mM sodium phosphate buffer (pH 7.4) containing 0.25% sodium cholate to give a final concentration of 6-7 µM heme c1 and placed in one of the reservoirs of the stopped-flow apparatus. The solution was bubbled with N2 gas for 15 min at 20 °C to attain anaerobic conditions. The fully reduced form of QCR was prepared by addition of a slight excess of sodium dithionite, and allowed to stand for another 15 min at 20 °C under N2 atmosphere. Then the temperature was lowered to 10 °C. The other reservoir contained cytochrome c (1.0 µM) and CCO (6-7 µM aa3) in an air-saturated solution consisting of 50 mM sodium phosphate buffer (pH 7.4) and 0.25% sodium cholate. After incubation for 10 min at 10 °C, the solutions in both reservoirs were mixed at a 1:1 ratio to start the reaction, and spectral changes were recorded by rapid-scan spectrophotometry at an appropriate time interval. Method 2: a mixture containing QCR (6-7 µM cytochrome c1), 1 µM cytochrome c, and CCO (6-7 µM aa3) in 0.25% sodium cholate, 50 mM sodium phosphate buffer (pH 7.4) was placed in one reservoir and bubbled with a gas mixture of CO and N2 (1:4) for 10 min at 20 °C. A slight excess of sodium dithionite was added to reduce all redox components before further incubation for 15 min at 20 °C. Then the temperature was brought to 10 °C. In the other reservoir, an air-saturated solution containing 50 mM sodium phosphate buffer (pH 7.4), 0.25% sodium cholate, and no protein components was placed, and the temperature was equilibrated at 10 °C. The two solutions in the reservoirs were mixed to flow at a 1:1 ratio into the observation cell of the stopped-flow apparatus, and the mixture in the cell was irradiated with a laser flash of 587 nm to initiate the redox reaction by photolyzing the cytochrome c oxidase-CO complex. The two methods gave essentially the same result in terms of the oxygen reaction.
Partially reduced QCR was prepared by using a catalytic amount of SCR (0.5 µM cytochrome b) and 10 mM sodium succinate as a reducing system. After reduction of QCR with succinate for 30 min at 20 °C, sodium malonate was added (12 mM, final) to block electron transfer from succinate to QCR catalyzed by SCR. The reaction of partially reduced QCR with cytochrome c and CCO was followed by Method 1.
Optical measurements to determine the electron transfer activity of
respiratory enzymes and the concentration of cytochrome components were
carried out with a Unisoku multi-wavelength spectrophotometer equipped
with a thermostatted cell holder. The ubiquinone-10 content of purified
QCR was estimated according to the reported method (31) by using an
extinction coefficient of 12.25 mM1·cm
1 for the difference
between the oxidized and reduced quinone at 275 nm (12). Cytochrome
c (6), cytochrome c1 (32), cytochrome b in SCR (33), and heme a in CCO (20) were
determined according to the reported methods. The concentration of CCO
was expressed in terms of cytochrome aa3.
Protein was estimated according to Lowry et al. (34).
The spectral data collected by rapid-scan spectrophotometry were processed by using either a home-built computer program as described previously (35) or MATLAB (The MathWorks, Inc., Natick, MA). Numerical calculations for solving the differential equations that represent a reaction model were performed by using MATLAB on a desktop computer (Dell, OptiPlex XMT 5133).
Fig. 1A shows
three-dimensional display of spectral changes recorded on mixing
dithionite-reduced QCR (0.36 mol of Q10/mol of heme
c1) with an air-saturated solution containing
cytochrome c and CCO in the stopped-flow rapid-scan
apparatus. The concentration of cytochrome c was 6-7-fold
lower than that of CCO or of QCR to minimize its spectral contribution
to the absorbance change of heme c1 around 553 nm and to control the rate of its oxidation. An excess of CCO is
expected to keep cytochrome c almost in the oxidized state
during the redox reaction. The first spectrum taken immediately after
the mixing, or at time 0, shows that QCR is almost in the reduced state
with a peak of heme b components at 562 nm and a shoulder of
heme c1 at 553 nm. A broad absorption band
around 600 nm is due to the oxidized form of CCO. As the reaction
proceeds, the 562-nm peak becomes smaller after a short lag period with
a growth of the 604-nm peak. This result indicates that mixing of fully
reduced QCR with cytochrome c and CCO under the air brought
about the oxidation of hemes b in QCR and electron transfer
to CCO. It should be noted that a fairly large portion of heme
b still remained in the reduced state at 3 s (Fig. 1, A and B).
Based on the ubiquinone content of the samples employed, we simply assume that maximally 36% QCR in the purified preparation contains a full set of redox centers; that is 1 mol each of Q10-(2), heme bL-(1), heme bH-(1), heme c1-(1), and ISP-(1). In parentheses the maximal number of reducing equivalent that can be retained is given. Accordingly, fully reduced QCR contains six reducing equivalents. It is proposed that center o accommodates two ubiquinone molecules at domains Qos and Qow that have a strong and weak interaction with ubiquinone, respectively (24, 36). The stoichiometry of the present preparation shows that only one of them is retained probably at Qos. On reaction with the oxidizing system, QCR equipped with a full set of redox centers can be oxidized rapidly compared with the incomplete complex. This is in accord with the experimental result indicating that a fairly large portion of heme b remains in the reduced state after the rapid oxidation (Fig. 1, A and B) as described above. According to the Q cycle mechanism ubiquinone is supposed to be released from QCR to move from center o to center i or vice versa (2, 3). But it is less likely that a limited amount of ubiquinone-10 found in the purified preparation of QCR swims around in a detergent medium to mediate translocation of protons between centers o and i. Rather, it is more likely for ubiquinone to mediate proton translocation without being released from the QCR complex. Therefore, we postulate in QCR a big ubiquinone pocket that contains centers i and o, as assumed by Wikström and Krab (8). Ubiquinone and ubiquinol (not ubisemiquinone) may be able to make contact alternatively with o and i domain in the ubiquinone pocket through a "flip-flop" motion. Such a pocket may be provided by a dimeric structure of this complex as described previously. Further studies are required to find out whether this kind of mechanism is functioning in the catalytic reaction of QCR in phospholipid membranes. Also the x-ray crystallographic studies that are in progress will soon reveal these essential features (4, 37-39).
The time courses of absorbance difference at 566-575 nm, 554-540 nm, and 604-630 nm that monitor the redox change of hemes b, heme c1, and CCO, respectively (Fig. 1B), were derived from the data shown in Fig. 1A. Heme b components in QCR were oxidized with an initial lag, and a half-time for the oxidation was about 150 ms. Electron transfer to CCO occurred in the same time range as shown by an initial absorbance increase at 604-630 nm. The oxidation of heme c1 was triphasic; the rapid oxidation and re-reduction that occurred within 300 ms after initiation of the reaction was followed by a slow decrease in absorbance for heme c1. A decline of the absorbance of CCO was slower than heme c1. As the oxidation of heme b with a lag and the triphasic oxidation of heme c1 were already observed by de Vries et al. (40) who employed yeast mitochondrial membranes, the present result confirms their finding.
Fig. 1C shows the time difference spectra derived from the data in Fig. 1A. A difference spectrum between 0 and 150 ms shows a peak at 565 nm and a deep trough at 605 nm (spectrum 1 in Fig. 1C), indicating that heme bL in QCR is oxidized first accompanying electron transfer to CCO. Tsai et al. (12) demonstrated, by using a rapid freezing EPR technique, that low potential heme bL was oxidized more rapidly than high potential heme bH during reaction of fully reduced yeast QCR with Q1. The peak of heme b shifts to 563 nm in the difference spectra of 0.15-0.3 and 0.3-0.6 s (spectra 2 and 3), indicating that the oxidation of heme bH dominates after heme bL has been oxidized to an appreciable extent. The oxidation of heme c1 in a later stage is apparent as indicated by the peak at 553 nm in the difference spectra of 0.6-1.5 and 1.5-3 s (spectra 4 and 5).
Fig. 2 shows the effect of antimycin A on the oxidation
of QCR (0.36 mol of Q10/mol of heme
c1). Fully reduced QCR was prepared in the
presence of antimycin A and mixed with an air-saturated solution
containing cytochrome c plus CCO to initiate the reaction. There was no sign for the oxidation of b-type hemes, and the
oxidation of heme c1 was biphasic. When the
reduction of hemes b was incomplete by chance, an
oxidant-induced reduction of heme bL occurred
although its extent relative to the total heme b was less
than 5% (Fig. 2). An absorbance increase of CCO at 604 nm due to
electron transfer from QCR proceeded along with the oxidation of heme
c1, followed by its gradual decay as in Fig.
1.
Oxidation of QCR with a Low Q10 Content
Fig.
3A shows the redox behavior of fully reduced
QCR (0.1 mol of Q10/mol of heme c1)
upon reaction with oxygen in the presence of cytochrome c
and CCO. When the reaction was initiated by the flow-flash method (20,
41), CCO was oxidized completely within a few milliseconds at 10 °C
(20). Since this oxidation is much faster than that of fully reduced
QCR so far examined, no change was seen in QCR during the complete
oxidation of CCO. Then, the shoulder at 553 nm disappeared accompanying
an increase in absorbance at 604 nm, whereas the peak at 562 nm
remained unchanged (Fig. 3A). This result indicates that
hemes b in QCR with a low Q10 content were not
oxidized by the cytochrome c/CCO system in the time range
examined. However, it should be noted that QCR with the low
Q10 content is catalytically active enough to exhibit the
electron transfer activity of about 350 nmol of cytochrome c
reduced·s1·(mol heme
c1)
1 when assayed in the presence
of 25 µM Q2H2 and 50 µM cytochrome c as described under
"Experimental Procedures." In accordance with this, when QCR (0.1 mol of Q10/mol of heme c1) was
supplemented with exogenous ubiquinone-2 (Q2) prior to
reduction with sodium dithionite, the oxidation of hemes b
was restored to some extent (Fig. 3B). At the same time,
re-reduction of heme c1 was recognized in a
later stage. Antimycin A inhibited this oxidation. Therefore, it seems
that the exogenous Q2 fulfills the role of intrinsic Q10 to a certain extent. These results clearly indicate
that ubiquinone is an essential component for electron transfer from
hemes b of QCR to CCO via cytochrome c.
Previously, we reported that in ascorbate-reduced QCR reconstituted
into potassium-loaded phospholipid vesicles, a potassium diffusion
potential induced the reduction of heme b components and
that ubiquinone was required for reversed electron transfer from heme
c1 to heme b (42). These findings
were confirmed recently (43), again supporting this essential role of
ubiquinone.
The above conclusion is inconsistent with the previous reports that the oxidation of fully reduced QCR by oxidants was not affected even when the endogenous ubiquinone was depleted from the enzyme (11, 12). It should be noted, however, that either ferricyanide or cobalt chelate was used in these studies. In fact, using the QCR preparation that contained 0.1 mol of Q10/mol of heme c1 we also observed that both heme b and heme c1 were oxidized rapidly when the fully reduced form was reacted with 250 eq of ferricyanide (data not shown). This result contrasts with the non-oxidizability of hemes b when cytochrome c plus CCO was the oxidizing system (Fig. 3A) but agrees with the oxidation of these components in yeast QCR that was brought about by 500 eq of ferricyanide (12). Thus, the discrepancy between our results and previous ones (11, 12) would be ascribed to the direct oxidation of heme b components in QCR by nonphysiological oxidants, as pointed out previously (19).
Oxidation of Partially Reduced QCRFig.
4A illustrates the redox behavior of
partially reduced QCR (0.36 mol of Q10/mol of heme
c1) upon reaction with cytochrome c
plus CCO under aerobic conditions. Partially reduced QCR was prepared
by incubation of QCR with succinate in the presence of a catalytic
amount of succinate-cytochrome c reductase (SCR). Under this
condition heme c1, iron-sulfur protein, and most
of heme bH were reduced but not heme
bL as reported previously (44). No initial lag
was observed during oxidation of heme bH as
shown by a trace at 562-575 nm, and a triphasic redox behavior of heme c1 was also discerned (Fig. 4B). As a
reference, the partially reduced QCR was reduced completely by adding a
small amount of dithionite and allowed to react with oxygen catalyzed
by cytochrome c and CCO. This time, the oxidation of hemes
b clearly accompanied an initial lag that became more
apparent compared with the result shown in Fig. 1 (data not shown). The
triphasic behavior of heme c1 was more apparent,
too. This oxidation profile was not affected by addition of
Q2 (data not shown). These results indicate that even with
the present preparation of QCR (0.36 mol of Q10/mol of heme
c1) the immediate oxidation of heme b
occurs as long as the oxidation starts from the partially reduced
state.
Summary of Experimental Observations
Stopped-flow rapid-scan spectrophotometric studies on the oxidation kinetics of reduced QCR have revealed characteristic behavior of the redox components in the complex as follows. (i) Starting from the fully reduced QCR the oxidation of b-type hemes accompanies an initial lag; apparently heme bL is oxidized first, followed by heme bH. Antimycin A inhibits the oxidation. The oxidation of heme c1 is triphasic and becomes biphasic in the presence of antimycin A. (ii) Q10 is essential for electron transfer from b-type hemes to heme c1 and ISP. (iii) Starting from partially reduced QCR the oxidation of b-type hemes occurs immediately without a lag.
In the sections that follow we try through simulations to explain these observations based on the Q cycle mechanism that we propose in a mechanistic model. It is expected that the redox behavior of heme bL, heme bH, and heme c1 as observed in the present study are reproduced well semiquantitatively, and the behavior of other components would be described too. This model also helps to test the validity of some ideas about the function of QCR and allows predictions.
Reaction ModelFig. 5 illustrates the reaction
scheme for simulating the reaction profiles of hemes b and
heme c1 in a single turnover. Monomeric QCR is
assumed to be a functional unit and to behave independently of each
other, although the structural studies indicate that QCR is dimeric and
suggest some interactions between the monomers (4, 23). The maximum
number of different redox states of QCR during the oxidation amounts to
144 if calculated by a simple combination. Out of them 56 states were
selected according to the rule that follows and are shown in the model
with ID numbers. Each state will be referred to as S1 (State 1), S2,
etc. and each reaction step as RS1 (Reaction Step 1), RS2, etc. This
selection rule is based on the Q cycle mechanism in principle that
assumes an essential role of ubiquinone in mediating the electron flow from reduced heme b moieties to ISP. Furthermore, we assume
some constraints as follows. (i) QCR during the reaction is a closed system that interacts with cytochrome c of the oxidizing
system only through heme c1. Exchange of
ubiquinone with the Q pool is not assumed explicitly. (ii) Either
ubiquinol or ubiquinone shuttles (or flip-flops) between center
o and center i, and ubisemiquinone generated in
either site stays there. (iii) While heme bL
remains in the reduced state ubiquinol gives two electrons
consecutively to oxidized ISP that is regenerated by the action of the
oxidizing system. (iv) When both heme bL and ISP
are in the oxidized state ubisemiquinone preferentially reduces ISP
because this reaction is more favorable thermodynamically. (v)
Ubisemiquinone generated in center o reduces oxidized heme
bL, if any, as long as ISP is in the reduced
state. (vi) Ubiquinone generated in center o moves to center
i without oxidizing reduced heme
bL.
In this reaction scheme (Fig. 5) the fully reduced QCR is at C1R1 if we regard this arrangement as a (sparse) matrix and if the location is represented by a combination of the column (C) and the row (R). The oxidation proceeds toward right and downward. Except for the fully reduced (S1) and fully oxidized (S40) forms, the reaction intermediates having reducing equivalents between 5 and 1 are grouped into two columns for each number of equivalent as shown by a roman numeral at the top of the column. In the left column in each pair every species has oxidized heme c1 whereas that in the right has reduced heme c1 ready to be oxidized. Forty members in 10 rows from R1 to R10 are grouped into the upper block and the others into the lower block, and these two blocks are connected by the reaction of electron exchange between ubisemiquinone and oxidized heme bL in center o. In the upper block S40 is in the fully oxidized state, whereas the most oxidized states in the lower block from S53 to S56 still retain one reducing equivalent either on heme b or SQ, although actually this will be lost during a long standing time by a mechanism that cannot be specified.
Simulations of QCR OxidationRate constants used for
simulating the oxidation of fully reduced QCR are shown in Table
I. (i) The apparent rate constant for the oxidation of
heme c1, 40 s1, was estimated from
three exponential analyses of the absorbance change at 554-540 nm in
Fig. 1A. (ii) Rate constants for intramolecular electron
transfer (ET) among redox centers in QCR were assumed to be in the
order of 105 s
1 that belongs to the uppermost
estimate in the previous studies (3, 24, 45-48). Simulations indicate,
as will be discussed later, that the rate constants for ET can be in
the orders lower than 105 s
1 because
intramolecular ET is rarely rate-limiting. (iii) The potential
differences for a redox pair exchanging an electron were derived from
the values in Table I and used to estimate the relative rate constants
for intramolecular ET. It is to be noted that no free energy change is
assumed for the oxidation of ubiquinol by oxidized ISP
(
Em =
Em, SQ/QH
Em, ISP = 0) (where
Em indicates midpoint redox potential). (iv) A
decrease in an apparent rate constant for the oxidation of heme
c1 in later stages of the reaction was assumed
appropriately to explain both a transient accumulation of reduced heme
c1 following the initial rapid oxidation and a slow oxidation that follows (Fig. 1). (v) Translocation of ubiquinone from center o to center i was equated with an
appearance of a species with ubiquinone in center i and vice
versa. Usually the rate constants for translocation of ubiquinone and
ubiquinol, kot and krt,
were changed to give the satisfactory result.
|
Fractional changes of ubiquinol, ubisemiquinone, ubiquinone, reduced ISP, reduced heme c1, reduced heme bH, and reduced heme bL were obtained by summing up every intermediate that contains either of these components (Table II).
|
Fig. 6 illustrates semiquantitative simulations of three
cases, the oxidation of fully reduced QCR in the absence (Fig.
6A) and presence (Fig. 6B) of antimycin A and the
oxidation of partially reduced QCR (Fig. 6C). Fig.
6A reproduces the triphasic oxidation of heme
c1, the oxidation of heme b with a
lag (Fig. 1B), and the oxidation of heme
bL prior to heme bH (Fig.
1C) in the absence of antimycin A. The reaction model
predicts that the oxidation of heme b always accompanies a
lag because either ubisemiquinone (SQo) or ubiquinone
(Qo) that acts as a direct oxidant of reduced heme
bL appears for the first time in the
intermediates in R4 (SQo) or in R5 (Qo).
In addition to the redox behavior of heme bH, heme bL, and heme c1, Fig. 6A also simulates a rapid oxidation of ubiquinol with an apparent half-time of 100 ms. This is comparable to the oxidation of fully reduced QCR from yeast by ferricyanide (12). The oxidation profiles of ISP and heme c1 are similar although heme c1 is oxidized faster than ISP. The oxidation of heme bL starts with a lag and almost parallels that of ubiquinol. The oxidation of heme bH lags behind heme bL. This order of oxidation is reverse to the initial oxidation of heme bH followed by heme bL that is assumed in the reaction scheme of Fig. 5. It is highly possible that the immediate filling of the oxidized heme bH with an electron from heme bL by rapid intramolecular ET gives a feature as if heme bL were oxidized first. The reduction level of heme bH stays around 20% for the rest of the reaction. In line with this, the SQ/Q ratio at 3 s after initiation of the reaction is about 4.
The effect of antimycin A on the oxidation of fully reduced QCR is simulated by assuming that the rate constant for the oxidation of reduced heme bH by ubiquinone in center i is zero (Fig. 6B). Although the oxidation of heme c1 is simulated as a multiphasic change, it becomes apparently biphasic if the initial rapid changes, which proceed during the dead time of the stopped-flow apparatus, are neglected. The simulation satisfactorily reproduces the non-oxidizability of heme b, also. It is reported that inhibition of submitochondrial particles oxidizing succinate by antimycin A induces superoxide anion generation, and the reaction of SQo with molecular oxygen is supposed to be the cause (49). This will occur competitively with the consecutive oxidation of SQo through the high potential (ISP and heme c1) pathway.
The reaction model also explains the oxidation of partially reduced QCR
(Fig. 6C), which is equated to a mixture of S11 and S12. A
model for this reaction consists of the intermediates at and below R6
in the scheme shown in Fig. 5 and was derived by assuming
k11 = k24 =
k35 = k48 = 0 and
k11b = k24b = k35b = k48b = 0. For
simulation, the initial condition of S11 = 0.8 and S12 = 0.2 was assumed based on a redox potential of 0.025 V poised by the
succinate/SCR system. The rate constant for electron exchange between
heme bH and SQi and that for the
oxidation of heme c1 were reduced to
khs = 2 s1 and
kox = 10 s
1 from the values of
1 × 105 s
1 and 40 s
1
(listed in Table I), respectively, to comply with slower changes than
those in Fig. 1. The simulation shows clearly an immediate oxidation of
heme b and a triphasic oxidation of heme
c1, suggesting that the succinate-fumarate plus
SCR system is inhibitory to such processes because of its redox
buffering capacity. The successful simulations of the three different
experimental results based on the common reaction model encourage us to
explore the molecular characteristics of the Q cycle mechanism in more
detail as follows.
The
simulation shown by Fig. 6A can be resolved
into the rise and decay of each intermediate in the reaction scheme
(Fig. 5), and all the reaction intermediates are classified tentatively into six classes according to the maximal fraction that they attain in
the time course (class 5 0.05 > class 4
0.02 > class 3
0.01 > class 2
0.005 > class
1
0.001 > class 0). Among 56 species, 46 intermediates
belong to the lower five classes. The most significant 10 intermediates
are S1, S2, S3, S4, S11, S18, S43, S44, S55, and S56 and cumulatively
can explain most of the simulation result. Their fractional changes as
a function of time are shown in Fig. 7A. Reaction
intermediates on the upper block (Fig. 7A, top
and middle) contribute to the change in the early stage of
the oxidation, and those on the lower block (Fig. 7A, bottom) explain most of the later change. In addition to
these intermediates, contributions to the reaction by the others are illustrated in Fig. 7B that will be called the reaction map
hereafter. The intermediates on the upper block in the reaction scheme
are funneled into the lower block through RS59 and RS67. A transient accumulation of S44 is most prominent approaching 0.64 in fraction, and
this as well as S43 decays with time being replaced by a growth of S55
and S56 (Fig. 7A, bottom). An accumulation of SQ
is mostly represented by S56, suggesting that SQ is stabilized in
center i while heme bH remains in the
oxidized state. On the contrary, S55 contains reduced heme
bH. Contributions from more oxidized intermediates on the upper block (S39 and S40) to the spectral change
are almost negligible, and the reduction of oxidized heme bL by SQ in center o that leads to
RS59 (S27
S41) and RS67 (S34
S45) must play a crucial role in
establishing the reaction pathways.
The simulation results are insensitive to the rate of an elementary ET
step as long as the rate constant is between 105 and
103 s1, and the ratio between the forward and
backward rate constants is kept constant. The simulations are more
sensitive to the reaction steps with rate constants around 100 s
1 or below that correspond to the oxidation of reduced
heme c1 and translocation of ubiquinone and
ubiquinol between center o and center i. The rate
of oxidation of heme c1 was intentionally reduced in the present experiments by decreasing the amount of cytochrome c, an electron mediator between QCR and CCO, and
by lowering the temperature to 10 °C. Under this specified
condition, the translocation rates of ubiquinone and ubiquinol
seemingly are most important in controlling the reaction.
The simulation shown in Fig. 6A and Fig. 7
was done successfully by assuming no thermodynamic barrier for the
initial oxidation of ubiquinol in center o by oxidized ISP.
Here a positive thermodynamic barrier is supposed for an endergonic
reaction, whereas the negative reaction is for an exergonic process.
Ding et al. (24), however, assumed that a thermodynamic
barrier imposed by the SQo formation (Em = Em, SQ/QH
Em, ISP = 0.23 V) was essential for the
bifurcation (24). Thus, the effects of imposing either the positive or
negative thermodynamic barrier on the oxidation kinetics were examined
based on the present reaction model. When the thermodynamic barrier was
Em = 0.1 V, the oxidation of heme
bL and heme bH slowed
down slightly, and re-reduction of ISP and heme
c1 was also suppressed slightly (Fig.
8A). The others are almost the same as in the
case of
Em = 0 (Fig. 6A).
When the imposed barrier was Em = 0.25 V, which
was close to 0.23 V as suggested by Ding et al. (24), the
oxidation of all redox components was suppressed appreciably (Fig.
8B). Remarkably the oxidation of ubiquinol itself lagged
behind that of heme bL and heme
bH. This is caused mainly by suppression of ET
from ubiquinol to ISP, due to a high thermodynamic barrier, even when
both ISP and heme c1 are in the oxidized state.
Such a high barrier cannot exist because the simulation deviates
appreciably from the experimental result (compare Fig. 8B
with Fig. 1).
When the negative thermodynamic barrier was imposed
(Em =
0.1 V), the oxidation of heme
bL and heme bH were
accelerated appreciably. In accordance with this, the re-reduction of
ISP and heme c1 was also promoted (Fig.
8C). Fig. 9 depicts how ubisemiquinone is
generated depending on the thermodynamic barrier imposed. SQo is generated only once in the initial stage of the reaction, and this
is shown by the time course of S4 because contributions from S6, S7,
and S14 containing SQo are negligible. On the other hand,
SQi is generated twice as shown by transient formation of S11,
S18, S24, and S31 and by S44, S48, S52, and S56, although the extents
of contribution are variable. Thus, generation of SQo in the
initial stage of the reaction is appreciable with
Em =
0.1 V as expected (Fig. 9A). Even when
Em = 0, SQo is generated
transiently to a maximal fraction of above 0.1 (Fig. 9B).
Only with the positive barrier the level of SQo becomes
negligibly low (Fig. 9C). In this case only SQi is
detected. Therefore, if the non-occurrence of SQo is proved by
the ESR measurement (17, 29), it is a sure sign for the existence of
the positive thermodynamic barrier although its advantage in
controlling the reaction is not clear.
Thermodynamic Barrier Versus Kinetic Control
We have shown that starting from fully reduced QCR, ubiquinol in center o participates in two kinds of reactions (Reactions 1 and 2).
![]() |
(Reaction 1) |
![]() |
(Reaction 2) |
The production of superoxide anion from submitochondrial particles that
oxidize succinate in the presence of antimycin A (49) may be taken as a
sign for the incomplete oxidation of ubiquinol and, accordingly, to
indicate that further oxidation of SQo to Q is suppressed. In
fact, the simulation with Em = 0 indicates that
SQo is generated transiently to a maximal fraction of 0.13, and
this may have a chance to react with molecular oxygen to generate
superoxide anion. If SQo escapes the attack by oxygen, it will
be oxidized to ubiquinone through the high potential (ISP and heme
c1) pathway.
Reaction 2 occurs for S26 and S33 in which both ISP and heme bL are oxidized with ubiquinol being in center o. This is the situation that originated from ubiquinol bifurcation of electron flow into ISP and heme bL is expected to occur during turnover of QCR. First, starting from S26, RS38 proceeds because this is favorable thermodynamically. Then RS59, ET from SQo to oxidized heme bL, must follow as this is essential to explain the emergence of S43, S44, S55, and S56 on the lower block. It is to be noted that RS59 (and RS67) proceeds only when ISP is in the reduced state, and it is likely that this situation is brought about under a delicate kinetic control. Brandt et al. (25, 26) have proposed a catalytic switch mechanism as a prerequisite for the bifurcation of the electron pathway at center o and speculated that ISP in the reduced state directs the electron flow into heme bL stressing its important role in the timing of the reaction. Our analyses essentially support this proposal and furthermore suggest that the bifurcation can be purely a kinetic event. Because of this, we would like to propose a "kinetic switch" mechanism. Whether conformational changes are involved in the switching mechanism as assumed by Brandt et al. (25, 26) should be answered by further studies.
A concern of the kinetic control is shown by the following example with
the previous case of Em = 0 as a reference (Figs.
6A and 7B). The rate constant for ET from
SQo to heme bL in S27,
ksl, was changed to 1 s
1 to make
this comparable to k45 = 40/20 s
1
which is the rate constant for oxidation of heme
c1 in S27 (Table I). All the other constants
were kept unchanged. Although the oxidation profiles of heme
bL and heme bH were
almost the same as in the reference, the oxidation of both ISP and heme
c1 slowed down appreciably. Apparently, the
oxidation of heme c1 is almost biphasic (Fig.
10A). At the same time, the oxidation of
ubiquinol was rapid for the initial one-third but stalled temporarily
and was followed by a slower oxidation. During the stall, the extent of
SQ generation approached a maximal level transiently up to 0.3 in
fraction and approached a constant level. Contrary to ubiquinol and SQ,
ubiquinone was generated gradually with an initial lag. At 3 s the
relative fraction of quinone to ubisemiquinone was about 4 contrary to
1/4 observed in the reference. On the other hand, during the
turnover the transient appearance of S20, S26, and S27 became apparent
in the reaction map (Fig. 10B) caused by the kinetic barrier
imposed on RS59 and RS67. Consequently, S40, which is a fully oxidized
species, was formed to an appreciable extent, and accordingly, an
accumulation of S56 became less significant. These clearly indicate the
significance of the kinetic control mechanism.
The simplified reaction scheme based on the Q cycle mechanism and shown in Fig. 5 explains satisfactorily the following experimental observations. (i) Starting from the fully reduced QCR the oxidation of b-type hemes accompanies an initial lag; apparently heme bL is oxidized first, followed by heme bH. Antimycin A inhibits the oxidation. The oxidation of heme c1 is triphasic and becomes biphasic in the presence of antimycin A. (ii) The substoichiometric amount of Q10 is essential for electron transfer from b-type hemes to ISP and heme c1. (iii) Starting from partially reduced QCR the oxidation of b-type hemes occurs immediately without a lag.
Based on the simulation studies the following mechanisms are proposed. When both heme bL and heme bH are in the reduced state ubiquinol in center o is oxidized consecutively by the high potential (ISP and heme c1) pathway, providing ubiquinone in center i. This initiates the delayed oxidation of heme bH followed by heme bL. Even if the consecutive oxidation pathway does function, however, the kinetic control mechanism directs an electron flow preferentially into oxidized heme bL when this becomes available to SQo. The key point of this mechanism is that the fate of SQo is determined by the redox state of ISP; only when ISP is in the reduced state SQo can act as an electron donor to heme bL. Thus, ISP is regarded as a redox-linked switch. No endergonic process is required for the bifurcation to occur.
The current mechanistic Q cycle model has proved its usefulness in allowing the semiquantitative analysis of the redox behavior of the metal centers and intrinsic ubiquinone in QCR, and in predicting the kinetic mechanism that controls the electron flow. This approach will become a powerful tool in studying the molecular mechanism of energy conservation if elaborated for more rigorous and quantitative treatment of the dynamic data.
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