Skeletal Muscle Contractions Induce Acute Changes in Cytosolic Superoxide, but Slower Responses in Mitochondrial Superoxide and Cellular Hydrogen Peroxide

Skeletal muscle generation of reactive oxygen species (ROS) is increased following contractile activity and these species interact with multiple signaling pathways to mediate adaptations to contractions. The sources and time course of the increase in ROS during contractions remain undefined. Confocal microscopy with specific fluorescent probes was used to compare the activities of superoxide in mitochondria and cytosol and the hydrogen peroxide content of the cytosol in isolated single mature skeletal muscle (flexor digitorum brevis) fibers prior to, during, and after electrically stimulated contractions. Superoxide in mitochondria and cytoplasm were assessed using MitoSox red and dihydroethidium (DHE) respectively. The product of superoxide with DHE, 2-hydroxyethidium (2-HE) was acutely increased in the fiber cytosol by contractions, whereas hydroxy-MitoSox showed a slow cumulative increase. Inhibition of nitric oxide synthases increased the contraction-induced formation of hydroxy-MitoSox only with no effect on 2-HE formation. These data indicate that the acute increases in cytosolic superoxide induced by contractions are not derived from mitochondria. Data also indicate that, in muscle mitochondria, nitric oxide (NO) reduces the availability of superoxide, but no effect of NO on cytosolic superoxide availability was detected. To determine the relationship of changes in superoxide to hydrogen peroxide, an alternative specific approach was used where fibers were transduced using an adeno-associated viral vector to express the hydrogen peroxide probe, HyPer within the cytoplasmic compartment. HyPer fluorescence was significantly increased in fibers following contractions, but surprisingly followed a relatively slow time course that did not appear directly related to cytosolic superoxide. These data demonstrate for the first time temporal and site specific differences in specific ROS that occur in skeletal muscle fibers during and after contractile activity.


Introduction
Reactive oxygen species (ROS) are generated continuously by skeletal muscle cells and this process is widely recognised to be increased with contractile activity [1]. The primary reactive oxygen and nitrogen species generated by skeletal muscle are superoxide and nitric oxide [1,2], but there is an on-going discussion about the specific sub-cellular sites that contribute to superoxide generation in muscle during contractions. ROS interact with multiple signalling processes including pathways that mediate adaptive and potentially protective processes in skeletal muscle, such as the transcription factors AP-1 and NF-kB [3]. An increase in superoxide and NO can also lead to oxidative damage, through the formation of highly reactive secondary species such as peroxynitrite and hydroxyl radical [4][5][6][7].
The lack of any definitive conclusion concerning the sub-cellular sources of ROS that are active during contractions has been in part due to a lack of definitive analytical approaches to study the processes in situ. There are multiple potential approaches to monitoring ROS including electron paramagnetic resonance [8], monitoring of secondary products of ROS reaction with proteins, lipids and DNA [4] and fluorescence microscopy utilising ROS sensitive probes [9][10][11]. Fluorescence microscopy offers the potential to obtain real-time measurements from living cells, but has been severely hampered by the lack of specificity of the probes that are widely available. MitoSox Red and dihydroethidium (DHE) which localise predominantly to the mitochondrial and cytoplasmic compartments of cells respectively [12][13][14] are commonly used probes to detect intracellular superoxide. DHE accumulates in the cell cytoplasm by diffusion and following oxidation the product binds with negatively charged DNA that results in enhanced fluorescence and facilitates indirect superoxide detection. MitoSox is DHE with a triphenylphoshonium cation that facilitates its preferential accumulation (100-1000-fold) and retention within mitochondria [15]. Following oxidation the product also interacts with mitochondrial DNA and RNA with enhanced fluorescence. Many previous studies have monitored non-specific ethidium fluorescence as an index of superoxide activity following loading of cells with DHE or MitoSox, but recent studies have identified 2-hydroxyethidium (2-HE) and the equivalent hydroxylated product of MitoSox (hydroxy-MitoSox) as specific products of the reaction of DHE or MitoSox with superoxide [16,17]. Analysis of the fluorescence spectra of DHE, MitoSox and their oxidation products has identified a specific excitation wavelength for monitoring hydroxy-MitoSox and 2-HE. The fluorescent detection of the superoxide specific products for both MitoSox and DHE has been reported to require excitation at 396 nm whereas non-specific oxidation products are detected using an excitation of 510 nm with emissions at either excitation monitored at wavelengths .560 nm [12,15].
Previous approaches to assess hydrogen peroxide within muscle fibers and other cells have primarily used DCFH (29, 79 dichlorodihydrofluorescein), but despite its extensive use the lack of specificity of this probe is widely recognised and it has been shown to be sensitive to a number of ROS and reactive nitrogen species (RNS) including superoxide, nitric oxide and peroxynitrite in addition to hydrogen peroxide [18,19]. The genetically encoded probe, HyPer is a circularly permuted yellow fluorescent protein (cpYFP) inserted into the regulatory domain of the specific prokaryotic hydrogen peroxide-sensing protein, OxyR [20] that has been developed to provide a specific probe for hydrogen peroxide, but cells must be transfected with this probe. In the current study isolated muscle fibers were transduced using an adeno-associated virus to express HyPer within the cytoplasmic compartment.
Although older data indicated that mitochondria are important in generation of ROS in skeletal muscle following contractions [1,2], more recent studies have identified a potential role for NADPH oxidases (Noxs) in this process [21][22][23]. Skeletal muscle has been shown to express Nox2 [21] and Nox4 [24] and the Nox4 isoform appears to be present in muscle mitochondria [22], hence these studies also do not define the key sub-cellular sites for ROS generation during contractions. The aims of this study were therefore to use specific approaches to monitor the activities of superoxide in mitochondria and cytosol of isolated mature skeletal muscle fibers prior to, during, and after periods of contractile activity compared with fibers at rest. The relationship of superoxide activity to hydrogen peroxide content of fibers was also examined following transfection of fibers with the hydrogen peroxide-specific probe, HyPer.

Mice
All experiments were performed in accordance with UK Home Office guidelines and under the UK Animals (Scientific Procedures) Act 1986. The protocol was approved by the University of Liverpool animal ethics committee. Male adult (10-16 months old) C57Bl/6 mice were used for all experiments. Mice were humanely killed and the flexor digitorum brevis (FDB) muscles were rapidly removed for isolation of single fibers.

Isolation of single mature skeletal muscle fibers
Single fibers were isolated from the FDB muscles of mice using the method of Shefer & Yablonka-Reuveni [25] as modified by Palomero et al., [9]. FDB muscles were incubated for 1.5 hr at 37uC in 0.4% (w/v) Type I collagenase (EC 3.4.24.3, Sigma Chemical Co., Poole, Dorset, UK) in minimum essential medium eagle (MEM) media containing 2 mM glutamine, 50 i.u. penicillin, 50 mg ml 21 streptomycin and 10% foetal bovine serum (FBS, Sigma Chemical Co.). The muscles were agitated every 30 minutes during the digestion period. Single myofibers were released by gentle trituration with a wide-bore pipette and fibers were washed three times in MEM media containing 10% FBS. Fibers were plated onto pre-cooled 35 mm glass bottomed cell culture dishes (MatTek, Massachusetts, USA) pre-coated with Matrigel (BD Biosciences, Oxford, UK) in 2.5 ml MEM media containing 10% FBS. Fibers were incubated for 20 hrs at 37uC in a 5% CO 2 tissue culture incubator. Fibers prepared and cultured in this manner are viable for up to 6 days in culture [9] although in practise all fibers were studied within 30 hours. Experiments were performed on fibers that retained good morphology and exhibited prominent cross-striations (see Figure 1).

Use of MitoSox red to monitor mitochondrial superoxide in isolated fibers
Fibers were loaded in 2 ml Dulbecco's phosphate-buffered saline (D-PBS) containing 125 nM MitoSox red for 10 minutes at 37uC in a tissue culture incubator. Fibers were then washed twice with D-PBS and two further washes with MEM solution. Fibers were maintained in 2 ml MEM solution during the experimental protocol. Where L-NAME was used to inhibit nitric oxide synthases [26], this was added 30 minutes prior to the commencement of the experiment and maintained throughout the experiment.

Use of dihydroethidium to monitor cytoplasmic superoxide in isolated fibers
Fibers were loaded by incubation in 2 ml D-PBS containing 5 mM DHE for 20 minutes at 37uC in a tissue culture incubator. Fibers were then washed twice with D-PBS and two further washes with MEM solution. Fibers were maintained in 2 ml MEM solution during the experimental protocol.

Use of HyPer to specifically monitor hydrogen peroxide in isolated fibers
Cyto-HyPer obtained from Evrogen (Moscow, Russia) was cloned into a recombinant adeno-associated viral vector (pseudotype 6; rAAV6) to generate vector particles that were used for transduction of isolated muscle fibers prior to experimentation. Preparation of rAAV6 vectors was performed essentially as described previously [27]. Fibers were exposed to 7.5610 9 adeno-associated viral particles containing the cyto-HyPer immediately after isolation and maintained in the presence of the particles for 72 hours in a tissue culture incubator. Fibers then washed three times and maintained in 2 ml MEM-solution during the experimental protocol.

Confocal microscopy
A Nikon E-Ti inverted microscope with an Okolab heated stage insert to a motorised stage (TI-S-EJOY, Nikon) for a 35 mm petri dish equipped with a C1 confocal (Nikon Instruments Europe BV, Surrey, UK) was used. The confocal had 3 lasers, a diode (UV) with 405 nm excitation, argon with 488 nm excitation and a helium-neon with 543 nm excitation. Acquisition software was EZC1 V.3.9 (12 bit). For assessment of 2-HE and hydroxy-MitoSox, excitation was at 405 nm with the emission collected through a 605/15 filter. For the non-specific (ethidium) products of DHE and MitoSox oxidation, excitation was at 488 nm with the emission collected through a 605/15 filter. To examine cytoplasmic DHE, an additional scan was undertaken (at 405 nm excitation) and the emission was collected through a 450/35 filter. Cyto-HYPER was sequentially excited at 405 and 488 nm with emission collected between 515/30 nm, with the ratio of 488/ 405 nm excitation being presented. Bright field images were acquired using the 543 nm laser. The objective was a PlanApo VC 660A/1.2NA/0.27 mm working distance water immersion. Pinhole size was 150 mm with a 1.86 msec pixel dwell time in all cases. Regions of interest for determination of fluorescence/area were selected as previously reported [10]. All experiments were performed at 25uC.

Electrical stimulation of muscle contraction in isolated fibers
Single muscle fibers were subjected to electrical field stimulation (Harvard Apparatus, Kent, UK) in 35 mm petri dishes using platinum electrodes (Advent, Oxford, UK) as previously described [28]. The total incubation time for the fibers was for 60 minutes with confocal images captured every ten minutes. Following an initial 10 minutes at rest, fibers were stimulated to contract for 10 minutes with trains of bipolar square wave pulses of 2 ms in duration for 0.5 sec repeated every 5 sec at 50 Hz and 30 V/well. Fibers then remained at rest for 20 minutes followed by a second identical stimulation protocol and a final 10 minute recovery period at rest.

Statistical Analysis
Data are presented as means 6 SE for each experiment, where n represents number of mice. Data were analysed using SPSS V.17. Data distribution was checked using KS-test and were normal throughout, variance was checked using Levene's test. Data were then examined by General linear models repeated measures examining treatments (i.e. exposure to drug and/or exposure to contraction), followed by one way ANOVA or Student's t test. Data were considered significant at P,0.05.

Detection of superoxide in mitochondria of skeletal muscle fibers using MitoSox red
MitoSox red was used to detect superoxide within mitochondria of single muscle fibers. In initial experiments, fibers were loaded with both MitoSox red and mitotracker green (20 nM) to determine whether MitoSox co-localised with mitotracker ( Figure 1A) The ability of MitoSox red in fibers to detect superoxide within mitochondria was confirmed by use of antimycin A, an inhibitor of the electron transport chain that induces generation of superoxide from complex III [29]. Figure 1B shows changes in fluorescence from MitoSox-loaded muscle fibers monitored using two excitation wavelengths, 405 and 488 nm (n = 3). Fibers were exposed to antimycin A (10 mM) at 0 minutes, and throughout the rest of the experiment. After 90 minutes exposure to antimycin A the MitoSox fluorescence had increased by 44628% when monitored at 405 nm excitation and 143617% at 488 nm excitation. Best fit slopes of linear lines fitted to the MitoSox fluorescence at the 2 wavelengths between 0 to 95 minutes were significantly different with the slope from fluorescence with 488 nm excitation being approximately 36 steeper than that obtained with 405 nm excitation (slopes of 1.44 versus 0.44 arbitrary units respectively, t-test, P = 0.04). Thus exposure to antimycin A induced oxidation of MitoSox that was detectable using the non-specific excitation wavelength and by analysis of hydroxy-MItoSox albeit at a lower sensitivity. For all subsequent experiments, results using 405 nm excitation (i.e. 2-HE or hydroxy-MitoSox) are presented. Changes in mitochondrial superoxide were investigated using MitoSox red in resting, non-stimulated single FDB fibers and fibers that were electrically stimulated to contract ( Figure 2). Fiber contraction was stimulated by two protocols separated by twenty minutes at rest. The timing of contraction periods are shown by bars on the Figure. Data are presented as the relative fluorescence normalised to the initial fluorescence value (Figures 2B and D) and as the change in fluorescence compared with non-stimulated fibers over each 10 minute period ( Figures 2C and E). Figure 2B shows the hydroxy-MitoSox fluorescence changes over time from fibers that were not stimulated to contract and fibers exposed to the two contraction protocols (n = 6 for both groups). Non-stimulated fibers showed no significant increase in hydroxy-MitoSox fluoresecence over time. Stimulated fibers showed a small increase in hydroxy-MitoSox fluorescence over the course of the experiment and by the end a 1565% increase in fluorescence from these fibers was seen. This change in fluorescence only achieved statistical significance at the final time point compared with values from non-stimulated fibers (one way ANOVA, P = 0.04). Repeated measures analysis over the whole time course showed no significant effect of stimulation between the two groups (F = 4.2, P = 0.069, General linear model). The net change in hydroxy-MitoSox fluorescence did not differ significantly between stimulated and non-stimulated fibers at any time point ( Figure 2C).
Since superoxide can rapidly react with NO to form peroxynitrite and hence excess NO might limit superoxide availability for reaction with MitoSox, the effect of the NOS inhibitor, L-NAME, on MitoSox fluorescence was examined ( Figures 2D and E). In the presence of L-NAME, the hydroxy-MitoSox fluorescence from non-stimulated fibers was unchanged, but there was an overall increase in the MitoSox fluorescence from stimulated fibers that reached statistical significance after the second contraction protocol and showed a 37616% increase above non-stimulated values (P = 0.028, one way ANOVA). Analysis over the whole time course showed a significant effect of stimulation (F = 5.3, P = 0.04, General linear model repeated measures) between the stimulated and non-stimulated groups in the presence of L-NAME. Analysis of the rate of change in hydroxy-MitoSox fluorescence in the presence of L-NAME showed increases during the first and second periods of muscle contraction and during the resting period30-40 minutes compared with non-stimulated fibers at the same time points.
Detection of superoxide in the cytoplasm of resting and contracted skeletal muscle fibers using DHE DHE was used to detect superoxide within the cytoplasm of non-stimulated and stimulated muscle fibers in the presence and absence of L-NAME (Figure 3). Fluorescence was monitored from nuclei and showed a significant effect of stimulation with respect to time (repeated measures F = 6.6, P = 0.016). No significant effect of L-NAME on fluorescence from non-stimulated or stimulated fibers was seen. The fluorescence from 2-HE increased acutely and significantly in response to each of the two periods of muscle contraction, exhibiting a 2066% and 1764% increase above baseline in the first and second contraction periods in the absence of L-NAME when compared with non-stimulated fibers at the same time points ( Figure 3B, one way ANOVA P,0.02 for first and second contractions). Very similar data were obtained in the presence of L-NAME ( Figure 3D).
The net change in 2-HE fluorescence ( Figure 3C) from the nuclei of non-stimulated fibers showed a significant increase with each period of stimulation (1 st stimulation P = 0.01, 2 nd stimulation P = 0.01, Student's t-test) compared with non-stimulated fibers. In the 10 minute time period following each stimulation there was significant reversal in the rate of change of fluorescence in the stimulated fibers, leading to a net decline in fluorescence values (after 1 st stimulation P = 0.02; after 2 nd stimulation P = 0.006, Student's t-test). An identical pattern of changes was observed in the presence of L-NAME ( Figure 3E).

Changes in the muscle fiber content of cytoplasmic DHE during contractions
The data in Figure 3 show increased nuclei fluorescence resulting from the contractions that was rapidly followed by a decrease in fluorescence to near baseline values. To find a potential explanation for these changes we repeated the experiments with additional measurements of non-oxidised cytoplasmic DHE (see Figure 4Aiii) in parallel with the changes in nuclear 2-HE fluorescence (Figure 4Ai). A potential explanation for the decline in fluorescence signal was that oxidised DHE, which exhibits a 20-40 fold increase in fluorescent intensity upon binding to DNA, might be displaced from DNA resulting in a decline in fluorescence. Because of the proportional increase in fluorescence that occurs on binding to DNA, a decline in signal might result from a modest amount of oxidised DHE being displaced from DNA. Figure 4B shows the pattern of changes in 2-HE measured from the nuclei of contracted fibers in comparison with the total content of DHE from the cytoplasm of the same cells (open symbols) The apparent rates of loss of DHE from fibers were generally similar between stimulated and non-stimulated fibers, but there were small increases in the rate of loss of non-oxidised DHE during the stimulation periods (potentially due to additional loss of DHE to an oxidised form which binds to DNA) followed by small but significant declines in the rate of loss of DHE in the periods immediately following the stimulations ( Figure 4C) which we speculate reflects an effect due to DHE being displaced from DNA.

Detection of hydrogen peroxide in the cytoplasm of resting and contracted skeletal muscle fibers using HyPer
Transduction of fibers with a rAAV6 vector [27] expressing cyto-HyPer (Evrogen, Moscow) led to the expression of HyPer within the cytoplasm of all fibers. Figure 5A shows the distribution of HyPer in a single fiber at 72 hours post-transduction and demonstrates the predominant localisation to the cytoplasmic compartment. Figure 5B shows the non-specific fluorescence from control fibers that were not transfected with HyPer, but exposed to the contraction protocols. In HyPer transfected fibers fluorescence was generally increased in the contracted fibers ( Figure 5C), but the rate of change in fluorescence was only significantly increased in the contracted fibers during the time periods immediately after cessation of contractions ( Figure 5D).

Discussion
The potential for skeletal muscle to generate reactive oxygen and nitrogen species in response to contractile activity has been widely examined, but despite extensive descriptive studies there remains considerable debate about the nature and time-course of changes in different cellular compartments [1,2]. Inhibitor and other studies have recently indicated that non-mitochondrial sources may be important [21][22][23], but recent developments in approaches to localise ROS-sensitive probes within sub-cellular compartments of cells and to improve the specificity of probes provide the opportunity to directly address these questions. The  current study has demonstrated that cytosolic superoxide activity increases acutely in response to contractions, but this was not accompanied by a similar acute change in mitochondrial superoxide availability and that modification of NO availability only influenced mitochondrial superoxide with no effect on cytosolic superoxide. Surprisingly, changes in cytosolic hydrogen peroxide monitored using the HyPer probe were found to follow a considerably slower time course than the rapid changes in cytosolic superoxide observed following contractions.
Loading of cells with DHE and monitoring of its oxidation through measurement of ethidium fluorescence has been used for a considerable time as an index of superoxide activity [14,30,31], but more recent studies have identified 2-hydroxyethidium (2-HE) as a specific product of the reaction of DHE with superoxide [12,15,16]. Monitoring of 2-HE has been described through analysis by HPLC techniques [11,13,16,32] or through selective excitation of the 2-HE product in fluorescence microscopy [12,15]. DHE and MitoSox are structurally similar, the triphenyl-phosphonium cation being incorporated into MitoSox to facilitate its charge dependant accumulation in mitochondria. The superoxide specific product of MitoSox oxidation has also been reported to be detected by selective excitation of the hydroxy-MitoSox product in fluorescence microscopy in an analogous manner to 2-HE [12,15]. The data shown in Figure 1 confirms the localisation of MitoSox to the mitochondria of isolated mature muscle fibers. MitoSox red fluorescence was found to co-localise with mitotracker green ( Figure 1A(v)) confirming the mitochondrial selectivity and no MitoSox fluorescence was seen from nuclei ( Figure 1A(ii-iii) respectively). In contrast, the distribution of DHE-oxidation products in DHE loaded fibers was predominantly nuclear ( Figure 3A(i-ii)). Although DHE is able to enter mitochondria, it does not accumulate and predominantly remains cytosolic. Following oxidation of DHE, the products intercalate into nuclear DNA and fluorescence is measured from nuclei. The data in Figure 1 also show the relative insensitivity of monitoring of 2-HE (with excitation at 405 nm) compared with the monitoring of non-specific oxidation products with 488 nm excitation. Nevertheless changes in the specific product were detectable following treatment with antimycin A and this approach was used for all further studies.
A comparison of the pattern of formation of 2-HE in the cytosol of DHE loaded fibers (Figure 3) with hydroxy-MitoSox in the mitochondria of MitoSox-loaded fibers (Figure 2) showed that cytosolic superoxide increased acutely in response to contractile activity but there was no similar acute increase in hydroxy-MitoSox in response to contractions. In addition treatment of fibers with the NOS inhibitor, L-NAME significantly increased the formation of hydroxy-MitoSox, but had no effect on 2-HE formation. Taken together, these data do not support the possibility that contractile activity induces an increase in mitochondrial superoxide generation that results in a subsequent increase in cytosolic superoxide. Skeletal muscle is reported to contain both the type I (neuronal) and type III (endothelial) NOS isoforms with eNOS localised to mitochondria [33]. Contraction increases the production of NO by muscle fibers [2,10,34] that is reported to occur primarily through activation of nNOS [10]. The data presented here indicate that non-specific inhibition of NOS using L-NAME had a significant effect on superoxide availability in mitochondria, but no effect on the cytosolic superoxide implying that the effect is likely to be due to an effect on mitochondrial eNOS [33], but this cannot be confirmed by the current data.
The rapid decline in 2-hydroxyethidium fluorescence that occurred following the end of the contraction protocols is difficult to explain since the fluorescent oxidised products of DHE should not degrade rapidly. Data in Figure 4 suggest that this may be due to some dislocation of the oxidised DHE from nuclei and since the fluorescence from DHE oxidation products is increased markedly by binding to DNA, a relatively small dislocation of these products from DNA might produce the effect observed in the period following the end of contractions.
The overall conclusion that mitochondria are not the major source of the acute contraction-induced increase in superoxide is supported by previous studies using MitoSox which assessed the non-specific oxidation products [35] and by measurements of mitochondrial redox potential monitored using mito-roGFP (a mitochondrial targeted redox sensitive GFP) [36]. A number of recent studies have focussed on the potential role of NADPH oxidases as a source of superoxide generation during contractions. This possibility is supported by the presence of Nox2 [21] and Nox4 [24] in skeletal muscle, the demonstration that inhibition of Noxs can reduce contraction-induced generation of ROS [22] and the direct demonstration of activation of Nox2 by electrical stimulation of single FDB fibers [23]. There is also some evidence that Nox4 is found in muscle mitochondria [22], but the data presented here argue against Noxs localised to mitochondria playing a role in the contraction induced generation of superoxide.
A further aspect of the data obtained was the gradual increase in hydroxy-MitoSox fluorescence that was seen to occur with time both in the absence or presence of L-NAME. This increase appeared to be initiated by contractile activity, but unlike the changes in cytosolic 2-hydroxyethidium, the hydroxy-MitoSox fluorescence also increased during some periods when contraction was not occurring. We speculate that these changes in hydroxy-MitoSox reflect a general increase in mitochondrial activity that is stimulated by the contractions, but occurs over a slower and delayed time course. This may be highly relevant to understanding ROS generation during studies of longer term exercise or training programmes and recognition that acute and longer term contraction protocols may activate different sources of superoxide generation could explain several apparent contradictions in the literature [1].
Previous attempts to monitor hydrogen peroxide in muscle fibers have primarily used DCFH or other non-specific probes [19,35]. HyPer is a genetically encoded specific probe for hydrogen peroxide and this was expressed in single isolated muscle fibers using an adeno-associated viral vector [27,37]. The HyPer construct that was used localises the protein to the cytosol and the data in Figure 5 show slow increases in HyPer fluorescence occur over a time course that does not follow those seen from 2hydroxyethidium or hydroxy-MitoSox or reflect the time course seen in previous data obtained with the non-selective probe, DCFH [9]. The HyPer probe is reversible and a decline in fluorescence reflects reduction by endogenous cellular thiols [20,38]. The kinetics of HyPer responses to hydrogen peroxide have been studied by Markincheva et al [38] who reported the half oxidation time of HyPer by hydrogen peroxide to be ,6 seconds. This is slower than DCFH reaction with multiple ROS, but indicates that the rate of oxidation would not be limiting with the experimental design used here (where fluorescence measurements were taken every 10 minutes). Thus the data obtained appear to reflect a true delay in the increase in fiber hydrogen peroxide concentration in response to contractions. The reasons underlying the slower changes are unclear, but may reflect rapid clearance of hydrogen peroxide through intracellular activities of glutathione peroxidise, catalase etc, or may be associated with differences in cellular distribution between DHE and HyPer. An interesting possibility is that since the potential sources for cytosolic superoxide generation, such as NADPH oxidases, are localised to the plasma membrane, the local changes in hydrogen peroxide concentration occur relatively slowly compared with superoxide since hydrogen peroxide can rapidly diffuse across the plasma membrane whereas superoxide cannot.
These data appear to be the first to report specific changes in hydrogen peroxide in muscle fibers resulting from contractile activity and they provide support for the key role that investigators have ascribed to hydrogen peroxide in regulation of multiple cell functions, such as force generation, stress responses and modification of gene expression [1]. An examination of the sensitivity of the HyPer probe in muscle fibers to exogenous hydrogen peroxide is provided as supplementary data ( Figure S1) and shows that changes in HyPer fluorescence from fibers were apparent at ,5 mM external hydrogen peroxide. This sensitivity is approximately equivalent to that of other probes such as DCFH [9] and demonstrates that the likely increase in intracellular hydrogen peroxide in muscle fibers following contractile activity is likely to be less than 1 mM, a figure that is in line with previous estimates [2].
In summary, the current study has demonstrated that cytosolic superoxide activity increased acutely in response to contractions, but this was not accompanied by a similar acute change in mitochondrial superoxide availability and that inhibition of NOS influenced mitochondrial superoxide availability but not cytosolic availability. These data therefore strongly support the hypothesis that the rise in cytosolic superoxide that accompanies contractile activity in skeletal muscle fibers is not derived from mitochondrial sources. Studies with the specific HyPer probe confirm that hydrogen peroxide is generated within muscle fibers, but demonstrate that the acute increase in muscle fiber cytosolic superoxide induced by contractions is not associated with an immediate increase in cytosolic hydrogen peroxide content. Figure S1 Effect of increasing extracellular hydrogen peroxide concentration on the fluorescence monitored at excitations of 488/ 405 nm from fibers transfected with HyPer (n = 4 at each concentration). (TIF)