The overall aim of this study was to (1) evaluate the adaptive value of mitochondrial DNA by comparing mitochondrial performance in populations possessing different haplotypes and distribution, and to (2) evaluate the sensitivity of different enzymes of the electron transport system (ETS) during temperature-induced changes. We measured the impact of temperature of mitochondrial respiration and several key enzymes of mitochondrial metabolism in two mitotypes (siII and siIII) of Drosophila simulans. The temperature dependencies of oxygen consumption for mitochondria isolated from flight muscle was assessed with complex I substrates (pyruvate + malate + proline) and with sn glycerol-3-phosphate (to reduce complex III via glycerophosphate dehydrogenase) in both coupled and uncoupled states. Activities of citrate synthase, cytochrome c oxidase (COX), catalase and aconitase, and the excess capacity of COX at high convergent pathway flux were also measured as a function of temperature. Overall, our results showed that functional differences between the two mitotypes are few. Results suggest that differences between the two mitotypes could hardly explain the temperature-specific differences measured in mitochondria performances. It suggests that some other factor(s) may be driving the maintenance of mitotypes. We also show that the different enzymes of the ETS have different thermal sensitivities. The catalytic capacities of these enzymes vary with temperature changes, and the corresponding involvement of the different steps on mitochondrial regulation probably varies with temperature. For example, the excess COX capacity is low, even non-existent, at high and intermediate temperatures (18°C, 24°C and 28°C) whereas it is quite high at a lower temperature (12°C), suggesting release of respiration control by COX at low temperature.

Mitochondrial DNA (mtDNA) encodes 13 key peptides of the mitochondrial electron transport system (ETS), and it is therefore suspected to partly evolve to adjust oxidative phosphorylation (OXPHOS) to environmental conditions of the organism (Das, 2006). For example, mtDNA has been suggested to influence the ability to acclimate to different thermal environments (Blier et al., 2001; Fontanillas et al., 2005), and the thermal sensitivity of mitochondrial complexes could therefore be of major significance in the impairment of the functional properties of mitochondria during temperature changes in ectotherms (Blier and Lemieux, 2001). A good strategy to assess the adaptive value of mtDNA is therefore to compare performances of mitochondria from populations characterised by different haplotypes and contrasting ecology or distribution.

Drosophila simulans, an ectothermic and eurythermic species, was recently proposed as a new model to study the adaptive value of mtDNA; it harbours three geographically distinct, subdivided haplogroups (siI, siII, siIII) with nearly 3% interhaplogroup divergence but less than 0.06% intrahaplogroup diversity (Ballard, 2000a; Ballard, 2005). Differences in the functional properties of mitochondrial ETS have been detected between these three lines of Drosophila with distinct mtDNAs, and one of these (siII) has been proposed to have a selective advantage (Ballard, 2005; Katewa et al., 2007). These differences have been considered as strong support of mitochondrial genome adaptation.

In ectothermic species, acclimation or acclimatization to low temperature usually increases the activity of enzymes in the oxidative pathway and the mitochondrial volume density (Guderley, 2004). A metabolic limitation at the level of mitochondrial catalytic capacity is thought to be the cause of these responses (for reviews, see Pörtner, 2002; Guderley, 2004; Blier et al., 2006). Moreover, metabolic rates of Drosophila melanogaster and D. simulans coming from populations evolving in low-temperature environments are higher than those from populations evolving at higher temperatures (Watada et al., 1986; Berrigan, 1997; Berrigan and Partridge, 1997). This suggests qualitative or quantitative mitochondrial adaptations in these populations, probably resulting from catalytic or regulatory limitations at low temperatures. Chamberlin, in a study on tobacco hornworm (Manduca sexta) midgut mitochondria, tried to identify the steps of the OXPHOS process that drive the changes in mitochondrial respiration during temperature variation (Chamberlin, 2004). These results showed that the ‘substrate oxidation system’ (including tricarboxylic acid cycle, electron transport chain and metabolite transporters), which produces the proton-motive force, confers most of the control over mitochondrial respiration during temperature declines. However, Chamberlin's study was not able to determine what individual reaction within the subsystems exerts this control (Chamberlin, 2004). According to Blier and Lemieux, cytochrome c oxidase (COX, complex IV) in trout has a thermal response that is similar to that of mitochondrial respiration (Blier and Lemieux, 2001). COX was, however, generally found in excess in mitochondria and this excess compared with the aerobic mitochondrial capacity is a basis for the high oxygen affinity of the respiration chain (Gnaiger et al., 1998). In this context, thermally induced changes in COX activity would have little effect on the maximal respiration rate while still acting on regulation of respiration mainly through impact upon the redox state of ETS (Blier and Lemieux, 2001).

However, the control of OXPHOS and regulation of mitochondrial respiration is highly complex and other parameters of the system may be influenced by temperature. The oxygen property to diffuse, its availability and its capacity to act as the terminal electron acceptor in the mitochondrial chain for energy production are also affected by temperature; at low temperatures, the aerobic capacity of mitochondria may impose a limit to metabolic capacity whereas at high temperatures, excessive oxygen demand would cause an uncompensated decrease in oxygen levels in body fluids (Pörtner, 2002). At lower temperature, mitochondria probably require a greater availability for ADP to reach a given relative activity than they do at higher temperature because reduced temperatures appeared to decrease mitochondrial sensitivity to control by ADP availability (Blier and Guderley, 1993).

Temperature alterations can also lead to the formation of reactive oxygen species (ROS) such as superoxide (O2·−) and hydrogen peroxide (H2O2) (Abele et al., 1998). These reactive molecules can oxidise DNA, proteins and lipids (Barja and Herrero, 2000; Das et al., 2001; Bokov et al., 2004), and lead to an oxidative stress when antioxidant enzymes [catalase (CAT), glutathione peroxidase and superoxide dismutase] and other non-enzymatic antioxidant compounds are overwhelmed (Beckman and Ames, 1998). These species arise largely, but not exclusively, from the mitochondria (Abele et al., 2002; Keller et al., 2004), which are known as the major ROS producers (Sastre et al., 2000). Unlike the nuclear DNA, histone proteins do not protect mtDNA and there is evidence that mtDNA exhibits more oxidative damage than nuclear DNA (Wei et al., 1998; Barja and Herrero, 2000) because of its closer proximity to ROS production sites and its limited repair mechanisms (Bogenhagen, 1999).

In Drosophila, ROS are mostly generated by complex I (NADH dehydrogenase), complex III (cytochrome bc) (both encoded by mtDNA and nuclear DNA) and by glycerol-3-phosphate dehydrogenase (Chen et al., 2003; Miwa et al., 2003; Andreyev et al., 2005). Katewa et al. showed that there were significant differences between two mitotypes of D. simulans (siII and siIII) for mitochondrial H2O2 production but also for oxygen consumption, COX activity and ATPase activity (Katewa et al., 2007).

Our study is aimed at identifying differences in mitochondrial performance and thermal sensitivity associated with haplotype divergences in the siII and siIII mitotypes of D. simulans. Different parameters of the mitochondrial metabolism were estimated at 12°C, 18°C, 24°C [24°C is considered as an optimal temperature for Drosophila species (David, 1988)] and 28°C. The thermal sensitivity of mitochondrial respiration was measured with pyruvate, malate and l-proline as substrates to reduce complex I and with sn glycerol-3-phosphate to reduce complex III via glycerol-3-phosphate dehydrogenase. We also determined the thermal sensitivity of an enzyme of the tricarboxylic acid cycle (citrate synthase, CS), as well as that of COX activity. Thermal sensitivity of uncoupled respiration [with carbonyl cyanide 4-(trifluoromethoxy)phenylhydrazone, FCCP] and of OXPHOS (ADP/O ratios) as well as that of the excess capacity of COX at high convergent pathway flux (with pyruvate + malate + proline + sn glycerol-3-phosphate) using inhibitor titration experiments were determined in order to compare overall mitochondrial performances at different temperatures of both mitotypes. Finally, enzyme activities of CAT (antioxidant enzyme), aconitase (ACO, tricarboxylic acid cycle) and levels of thiobarbituric reactive substances (TBARS, markers of lipid oxidative damages) were measured to evaluate the antioxidant capacity.

Fly lines

Two mitotypes of Drosophila simulans (Sturtevant 1919) were used during experiments: siII and siIII mitotypes, both from Kenya. In each mitotype, four isofemale lines (namely 2KY0412, 2KY0415, 2KY0418 and 2KY0421 for siII; 3KY0410, 3KY0412, 3KY0414 and 3KY0420 for siIII) were reared from flies collected in Nairobi (Kenya) during November 2004 as described previously (Ballard et al., 2007). Within the haplotype groups (four siII and four siIII fly lines) there was low amino acid variation within a 4.5 kb region spanning from position 1450 to position 5983 of the mtDNA genome while significant divergences were noticed (2.04×10−2% nucleotide divergences, 1.21×10−2% amino acid divergences) between the haplotypes (see supplementary material Table S1) (Ballard, 2000b). This region contains three protein-coding loci of complex IV (COI, COII and COIII) and the two of complex V (ATP6 and ATP8) (Katewa et al., 2007). Moreover, many studies have not been able to detect significant nuclear divergences between the two haplotypes (Ballard, 2000a; Ballard et al., 2002; Dean et al., 2003).

Flies were fed with standard cornmeal medium, containing a mixture of 10 g of agar–agar, 12 g of sugar, 54 g of dried yeast and 106 g of cornmeal flour dissolved in 2 l of tap water. Propionic acid (8 ml) and methyl-4-hydroxybenzoate 10% (w/v) in ethanol (32 ml) were added to the mixture to avoid mite and mould contamination. All Drosophila lines were maintained at constant density (100 flies for approximately 25 ml of standard cornmeal medium), temperature (24.0±0.1°C), humidity (50% RH) and diurnal cycle (12 h:12 h light:dark). For all experiments, only males were selected because females have a large number of mitochondria in abdominal oocytes, which could bias experiment measurements. After being allowed to spawn in sterile recipients for two days, parents were removed and experimental flies were then sexed on ice two days after hatching and transferred to new recipients for an additional eight days prior to study. To avoid fitness problems due to aging, all chosen parents were less than 14 days old and all experimental male flies were 10 days old. Flies were reared in two incubators (A and B) at the same time to have replicates of experimental lines and avoid the ‘incubator’ effect. For each recipient of 100 male flies, 40 were used for mitochondrial isolation and others were immediately stored at −80°C for further enzymatic analysis within one month.

mtDNA was determined using allele-specific PCR as described previously in each isofemale line (Dean, 2003), and Wolbachia infection was verified using conserved 16S rDNA primers (James and Ballard, 2000). According to Ballard et al. there is only one nonsynonymous change within siII lines and one nonsynonymous change within siIII lines over 5500 bp analysed (Ballard et al., 2007). PCR assays showed that all isofemale lines belonged to the corresponding mtDNA haplotype and were not infected by Wolbachia.

Fly sampling

Due to the low intrahaplogroup variation (Katewa et al., 2007), we have been able to pool flies of each line from the two groups (siII and siIII). The pooling strategy minimises individual differences caused by the nuclear genome of a particular fly line and enables us to detect more general differences that are due to the mtDNA in itself and/or of fixed nuclear differences that interact with each mtDNA haplogroup (Ballard, 2000a; Dean and Ballard, 2003; Katewa et al., 2007). Flies used for mitochondrial isolations were weighed as a pool of the four isofemale lines and from each mitotype while those used for enzymatic analyses were weighed individually with an electrobalance (Mettler-Toledo Inc., Columbus, OH, USA) with a resolution of 0.1 μg. All flies used for this study were reared in the same conditions, and males were weighed at 10 days of age. No mass differences were observed between the different pools of 40 flies (0.754±0.054 mg for siII incubator A; 0.751±0.052 mg for siII incubator B; 0.748±0.052 mg for siIII incubator A; 0.751±0.052 mg for siIII incubator B) or between flies of the two mitotypes weighed individually (0.670–0.831 mg for siII both A and B incubators; 0.674–0.839 mg for siIII both A and B incubators).

Isolation of intact mitochondria

Intact mitochondria were isolated as previously described by Katewa et al. (Katewa et al., 2007). Briefly, flight muscle mitochondria were isolated from 160 thoraxes (40 of each line of each mtDNA type) of 10-day-old male D. simulans. All steps were done at 4°C. Thoraxes were separated from abdomens and heads and placed in 400 μl of isolation buffer containing 250 mmol l−1 sucrose, 5 mmol l−1 Tris, 2 mmol l−1 EGTA, 0.1% bovine serum albumin (BSA) (w/v), pH 7.4. Thoraxes were then homogenised with a Kontes polypropylene pellet pestle (Kimbal Kontes, Vineland, NJ, USA). The pestle was pressed firmly to the bottom avoiding any grinding action. Thoraxes were pressed 120 times to produce a smooth, grey homogenate. Homogenates were filtered through gauze pad and the volume was raised to 2.1 ml with isolation buffer. After a first 3 min centrifugation at 300 g, the supernatant was refiltered through gauze (approximately 1.8 ml final volume) and recentrifuged for 10 min at 9000 g. The supernatant was then discarded and the pellet was washed two times in 400 μl of isolation buffer before being resuspended in 120 μl of the same buffer. The mitochondrial preparations were stored on ice and used within 2 h of isolation for mitochondrial oxygen measurements, inhibitor titration experiments and ACO activity. Integrity of mitochondrial preparations was verified in preliminary experiments with cytochrome c injection during the respiration state 2 (state 2c). The ratio between state 2 and state 2c measured at 24°C with seven different mitochondrial preparations gave 0.971±0.061, which confirms high quality of preparation.

Mitochondrial respiration

Mitochondrial oxygen consumption was measured at four different temperatures (12°C, 18°C, 24°C and 28°C) using an oxygraph Oxyg 32 (Hansatech Instruments Ltd, Pentney, Norfolk, UK) connected to a circulating water bath. Measurements were done in a final volume of 500 μl at each temperature with 15 μl of mitochondrial preparation incubated in 485 μl of mitochondrial respiration medium containing 120 mmol l−1 KCl, 5 mmol l−1 KH2PO4, 3 mmol l−1 Hepes, 1 mmol l−1 EGTA, 1 mmol l−1 MgCl2 and 0.2% BSA (w/v), pH 7.2. The polarographic system was calibrated with nanopure water saturated with oxygen at the incubation temperature.

Complex I and III

Pyruvate (10 mmol l−1), l-proline (10 mmol l−1, pH 7.2) and malate (10 mmol l−1, pH 7.2) were added to the chambers to provide substrates for complex I reduction and to achieve state 2 respiration. Sn glycerol-3-phosphate (20 mmol l−1, pH 7.2) was used as a substrate to supply electrons to the ubiquinone pool via glycerol-3-phosphate dehydrogenase in order to reduce complex III.

ADP (100 μmol l−1, pH 7.2) supplemented with MgCl2 (0.6 mol mol−1 ADP to keep [Mg2+] constant during respiration measurement) was added to reach state 3 respiration and state 4 was obtained after exhaustion of ADP. These states were used to calculate ADP/O ratios of complex I and complex III (as an index of mitochondrial efficiency). After first exhaustion, ADP (400 μmol l−1, pH 7.2) was introduced again to achieve maximum active state 3 (state 3m) and state 4o was measured after the addition of oligomycin (2 μg ml−1), which inhibits mitochondrial ATPase and phosphoryl group transfer. According to our preliminary tests, this concentration is higher than required to fully inhibit ATPase in mitochondria that have already reached state 4. Respiratory control ratios (RCRs) were calculated as state 3m/state 4o (as an index of functional integrity of mitochondria). FCCP was then added by steps of 0.1 μmol l−1 and uncoupled control ratio (UCR) was measured as state U/state 3m, with state U representing the maximum uncoupled respiration rate (reached between 0.2 μmol l−1 and 0.5 μmol l−1 of FCCP) to evaluate metabolic flux control by the phosphorylation system over the electron transport capacity.

Azide titration experiment

Following the first experiment, mitochondrial isolations were used to measure oxygen consumption in the presence of pyruvate (10 mmol l−1), l-proline (10 mmol l−1, pH 7.2), malate (10 mmol l−1, pH 7.2) and sn glycerol-3-phosphate (20 mmol l−1, pH 7.2) ensuring high metabolic flux through the ETS. After addition of ADP (800 μmol l−1, pH 7.2, this concentration ensured excess ADP during the entire experimental period and the state 3m reached was not different than with 400 μmol l−1), the following steps of azide concentrations were introduced at appropriate intervals to progressively inhibit complex IV (1, 2, 7, 12, 32, 52, 102, 202, 702, 1202, 1702 and 2202 μmol l−1) or until maximum inhibition was achieved. The inhibition constant (Ki) was calculated from transformed data using the Dickson linearisation (Kuznetsov et al., 1996). As azide is a non-competitive inhibitor, the flux control coefficient (Ci) was calculated using the following equation:
(1)
where J is the respiration flux, dJ is the decrement of respiration flux caused by increment of inhibitor addition dI (between 0 μmol l−1 and 80 μmol l−1) and Ki is the inhibition constant for sodium azide (Kuznetsov et al., 1996).

These steps were repeated for each mitochondrial preparation. Extraction and mitochondrial preparations were performed on five different pools of flies for each incubator, at each temperature and for each mitotype (total of 80 mitochondrial isolations). Measurements were averaged and respiration rates are expressed in nmol of oxygen consumed per minute per mg of mitochondrial protein.

Enzymatic analyses and oxidative stress markers

ACO, CS, CAT activities and protein content were measured using a UV/VIS spectrophotometer (Perkin Elmer, Lambda 11, Foster City, CA, USA), and TBARS levels were measured using a fluorescence spectrophotometer (F-2500 from Hitachi High Technologies America, Shaumburg, IL, USA), both equipped with a thermostated cell holder and a circulating refrigerated water bath. COX activity was measured polarographically with the same oxygraph as for mitochondrial oxygen consumption. Each measurement was done in duplicate, and for each incubator, at each temperature and for each mitotype, five different analyses were averaged.

ACO was measured on fresh mitochondria. The remaining mitochondria were then frozen at −80°C for further CS analysis and protein content measurement.

For CAT and protein analysis, 12 flies (three from each isofemale line of each mitotype) were homogenised in 600 μl of ice-cold buffer [100 mmol l−1 KH2PO4, 1 mmol l−1 EDTA, 0.1% (v/v) Triton X-100, pH 7.5]. In separate preparations, 16 flies (four from each isofemale line of each mitotype) were homogenised in 400 μl of the same ice-cold buffer for malondialdehyde (MDA) assessment and in 400 μl of imidazole buffer [50 mmol l−1 imidazole, 2 mmol l−1 MgCl2, 5 mmol l−1 EDTA, 0.09% (v/v) Triton X-100, pH 7.4] for COX activity measurement.

CS

Mitochondria (1 μl) were transferred in 100 mmol l−1 imidazole-HCl (pH 8), 0.1 mmol l−1 5,5′-dithiobis(2-nitrobenzoic acid) (DTNB), 0.1 mmol l−1 acetyl CoA and 0.15 mmol l−1 oxaloacetate. Activities were measured at the four different temperatures by following the increase in absorbance due to the reduction of DTNB at 412 nm (ε412=13.6 ml cm−1 μmol−1) (Thibeault et al., 1997).

ACO

Mitochondria (1 μl) were transferred in 50 mmol l−1 Tris-HCl, 0.1% Triton X-100 (v/v), 0.6 mmol l−1 MnCl2, 5 mmol l−1 sodium citrate, 0.2 mmol l−1 NADP, 0.4 U ml−1 isocitrate dehydrogenase, pH 7.4. Activity was measured at the four temperatures by following the appearance of NADPH at 340 nm (ε340=6.22 ml cm−1 μmol−1) (Miwa and Brand, 2005).

ACO activity was normalised with CS activity and results are expressed in U (units) of ACO activity per U of CS activity in order to express the activity of ACO according to a marker of mitochondria quantity.

COX

The reaction medium for COX activity contained 130 mmol l−1 KCl, 30 mmol l−1 Hepes, 10 mmol l−1 KH2PO4, 11 mmol l−1 MgCl2 hexahydrate, 20 mmol l−1 glucose, 10 mmol l−1 ascorbic acid and 5% (w/v) BSA (Blier and Lemieux, 2001). After homogenates were centrifuged at 750 g for 5 min, 5 μl of the supernatant were incubated in respiration chambers with 995 μl of reactive medium. After addition of cytochrome c (150 μmol l−1), azide was introduced step-by-step at concentrations described previously (see Azide titration experiment). This method was compared with the classic method of complex IV titration by azide using the same protein concentration in the chambers (Letellier et al., 1994; Villani and Attardi, 1997) with N,N,N′,N′-tetramethyl-p-phenylenediamine (TMPD, 1 mmol l−1) and ascorbate (5 mmol l−1) as substrates after inhibition of complex I and III with rotenone (0.5 μmol l−1) and antimycin A (2.5 μmol l−1), respectively, and activation by ADP (800 μmol l−1) and cytochrome c (150 μmol l−1) addition. Oxidation rates due to autoxidation of TMPD, ascorbate and cytochrome c were subtracted from the activity (Gnaiger and Kuznetsov, 2002). Results showed that there were no significant differences for Ki, for metabolic flux control Ci (Table 1), as well as for maximum velocity (Vmax) (12.14±4.14 nmol min−1 ml−1 and 14.16±2.73 nmol min−1 ml−1 for siII and siIII, respectively, for our method; 14.50±5.94 and 14.48±4.00 for siII and siIII, respectively, for the TMPD/ascorbate method) between the two methods at 24°C when using the same protein concentration of homogenates or isolations, which allowed us to validate our protocol (N=5 in duplicate for both methods, Fig. 1A,B). We chose the first method because there were no differences between mitotypes in the weights of flies, it did not need any mitochondrial isolation, it required a lower number of flies and it allowed us to freeze the remaining flies. There were no significant differences between the two methods, and consequently we can consider that the membrane solubilisation using Triton X-100 for homogenates preparations was not different from using TMPD. COX activity was measured for the four temperatures and expressed as nmol of oxygen consumed per minute per mg protein.

CAT

After homogenates were centrifuged at 13,000 g for 3 min at 4°C, the supernatant was incubated with 100 mmol l−1 of sodium phosphate and 60 mmol l−1 of H2O2. Decrease in absorbance, corresponding to the decomposition rate of H2O2, was measured at the four temperatures and at a wavelength of 240 nm for 1 min (ε240=43.6 ml cm−1 μmol−1) (Orr and Sohal., 1992).

MDA

MDA, the product of the peroxidation of fatty acids, was measured with a TBARS assay kit from Zeptometrix (Buffalo, NY, USA). This method relies on the fluorometric measurement of pink chromophor produced during the reaction of thiobarbituric acid with MDA. MDA contents were measured with light excitation set at 530 nm, emission set at 550 nm and width of 5 nm, and estimated following the manufacturer's protocol.

Protein content

Total protein content was determined both for mitochondria and homogenates in duplicate by the bicinchoninic acid method (Smith et al., 1985). As isolation buffer contained BSA, the protein due to the buffer was subtracted from the mitochondrial preparations.

Temperature coefficient values (Q10)

Q10 values for mitochondrial functions (state 3 and state 4 for both complexes I and III, COX activity and ACO/CS ratios) were calculated using the following formula:
(2)
where Rate 1 is for the rate of the parameter measured at the temperature t1, and Rate 2 is the rate of the parameter measured at the temperature t2.

Chemicals

All chemicals were purchased from Sigma-Aldrich (Mississauga, ON, Canada) except for the TBARS determination assay kit from Zeptometrix.

Construction of biochemical threshold plots

An azide titration experiment of elevated pathway flux (with pyruvate, l-proline, malate, sn glycerol-3-phosphate and ADP), as well as azide titration experiment of COX activity allowed us to construct plots of relative respiration rate against the percentage of inhibition of COX activity at the same azide concentration (Letellier et al., 1994; Villani and Attardi, 1997). Measurements were done at the four temperatures and COX excess capacity was determined for each temperature as previously described.

Statistical analyses

All statistical analyses were performed with SAS software (9.1.3, SAS Institute, Cary, IN, USA). O'Brien's tests for homogeneity and analysis of variance (ANOVA) with three independent variables (incubator, temperature and mitotype) were performed using a general linear model (GLM) procedure with the least square means method for multiple comparisons tests. This allowed us to determine any interactions between the variables, and the effect of each variable on the different parameters measured. Significance was defined at P<0.05. Data are expressed as means of five different samples from each incubator, at each temperature, and for each mitotype measured in duplicate.

No differences between incubators were detected for all the parameters measured, consequently data from incubators A and B were pooled.

Mitochondrial respiration

State 3m

For both complexes, state 3m exhibited the same pattern between the mitotypes for 12°C, 18°C and 24°C (Fig. 2A,B) as well as among the temperatures for the two mitotypes. There were significant differences between the two mitotypes at 18°C (P=0.0168 for pyruvate + malate + proline and P<0.0001 for sn glycerol-3-phopshate), siII being higher than siIII.

siII showed a slight increase from 12°C to 24°C, with significant differences between 12°C and 18°C (P-values ≤0.0201 for both complexes), and between 18°C and 24°C (P<0.0001 for both complexes). We detected a significant decrease when comparing 28°C with 24°C (P<0.0001 for both mitotypes). The state 3m of complex III markedly increased from 18°C to 24°C (P<0.0001) while staying similar at 24°C and 28°C (siII) or slightly increasing for siIII (P=0.0426).

State 4o

siII had a significantly higher state 4o than siIII at 18°C (P≤0.0021 for both complexes) and 24°C (P-values ≤0.0123 for both complexes), while at 12°C and 28°C, it was significantly higher for siIII (P-values ≤0.0497) but only when substrates are provided to complex I (Fig. 2C,D).

We also observed significant differences between 12°C and 18°C (complex I, P<0.0001), 12°C and 24°C (P<0.0001 for both complexes), and between 18°C and 24°C (P-values ≤0.0011 for both complexes) in siII. At 28°C, a significant decrease was observed comparatively with 24°C for complex I in siII (P=0.0002).

In siIII state 4o of complex I significantly increased from 12°C to 28°C while in complex III it decreased between 12°C and 18°C (P=0.0106) and increased between 18°C, 24°C and 28°C (Fig. 2C,D).

ADP/O ratios

When using substrates for complex I (Fig. 2E), there was a statistical difference between the two lines at 12°C, with a higher ADP/O ratio for the siII mitotype (P=0.0003). Among the temperatures, siII and siIII exhibited significant differences, with a higher ADP/O ratio at 24°C compared with 12°C, 18°C and 28°C (all P-values ≤0.0002).

For complex III (Fig. 2F), the only significant difference between mitotypes occurred at 28°C, with siIII being lower (P=0.0093). Among the temperatures, no significant differences were detected for siII while siIII exhibited significant increases at 18°C and 24°C compared with 12°C (P-values ≤0.0054) and with 28°C (P-values ≤0.0026).

RCRs and UCRs

Results of RCRs are presented in Fig. 3. Comparisons between mitotypes showed that there were significantly higher RCRs for siII at 12°C at the complex I level (P=0.0231), as well as at 28°C at the complex III level (P=0.0143). Surprisingly, the RCR of siII was significantly lower than siIII at 24°C (P=0.0292) when the substrates were provided to complex I.

In both mitotypes, RCRs of complex I were not different between 18°C and 28°C but both were significantly higher at 12°C (P-values ≤0.0309 for both mitotypes) and 24°C (P-values ≤0.0139 for both mitotypes). Moreover, RCR at 12°C was higher than at 24°C for siII (P=0.0238), while we observed the opposite trend for siIII (P=0.0043). We observed slight but significant increases from 12°C to 28°C at the complex III level. Results of UCRs are shown in Table 2. No significant differences were detected in UCRs between strains or between temperatures.

Enzymatic measurements

No significant differences were detected between mitotypes (Fig. 4A) in ACO activity at any temperature, suggesting no differences in the oxidative stress supported by each of these lines, at least in mitochondria. This is reflected by absences of significant differences between both mitotypes in MDA levels (data not shown).

COX activity was significantly higher for siIII only at 12°C (P<0.0001; Fig. 4B). Moreover, we observed a slight increase from 12°C to 28°C for both mitotypes with significant differences between 12°C, 18°C, 24°C and 28°C.

At 18°C CAT activity was higher in siII compared wih siIII (P=0.0116) whereas at 28°C it was lower (P=0.0005) (Fig. 4C).

COX excess capacity and flux metabolic control

Complex IV activity and mitochondrial respiration with pyruvate, malate, l-proline and sn glycerol-3-phosphate were inhibited by sodium azide. We examined the apparent excess capacity of COX at high flux through the ETS using a combination of substrates that maximally reduce complexes I and III. Azide titration resulted in hyperbolic inhibition of COX. The threshold plots display pathway flux as a function of COX activity; the threshold for inhibition of COX is defined as the intercept of the initial slope with the linear fit of the final slope (Fig. 5). The apparent excess capacity of COX is the intercept of the extrapolation of the linear regression for the final slope with the axis at zero COX inhibition. We detected a threshold, and consequently, a COX excess capacity at 12°C with no distinctions between the two mitotypes (604%, R2=0.9139 for siII and 613%, R2=0.9301 for siIII).

Surprisingly, with increasing temperatures the COX excess capacity vanished and comparisons were made between the different Ki and Ci. We observed increasing Ki with increasing temperatures but no differences between mitotypes were detected (Table 1).

For Ci comparisons, there were no significant differences between mitotypes but significant increases were detected from 12°C to 28°C (Table 1). All temperature comparisons were significantly different (all P-values ≤0.0005).

Q10 values for ACO/CS and state 3m are presented in Table 3.

Comprehension of the physiological and biochemical bases of temperature sensitivity of mitochondrial function appears essential to determine the capacity of organisms to cope with changing environmental conditions and constraints they may face under these conditions. In our study, we compared two mitotypes of D. simulans in order to (1) evaluate the plasticity of different enzymes of the ETS, and to (2) link mtDNA divergences with mitochondrial bioenergetics at several steps of the ETS. To our knowledge, this study is the first to deal with impact of temperature variations on mitochondrial functions in different mitotypes of the same species.

The two Krebs' cycle enzymes that are fully encoded by the nuclear genome, CS and ACO, showed no differences between mitotypes. This result suggests a weak impact of the nuclear genes on divergences of mitochondrial functions between these two populations. ACO is an enzyme selectively carbonylated and functionally altered in the housefly mitochondrial matrix by ROS (Yan et al., 1997; Yan and Sohal, 1998; Yarian and Sohal, 2005), and can be used as a proxy of the steady-state concentration of O2·− in the matrix (Gardner, 2002; Miwa and Brand, 2005). CAT activity of siII mitotype was higher at 18°C than siIII. The latter mitotype showed more elevated CAT activity at 28°C. As MDA levels and ACO activities remain constant between mitotypes at all temperatures, we suggest that these different CAT thermal sensitivities may result from expression of different allozymes in both populations, and consequently of different antioxidant activity.

The maximal rates of mitochondrial respiration were reached at 24°C for both mitotypes and when mitochondria were provided via glycerophosphate dehydrogenase to reduce complex III these rates were similar to those found at 25°C by Katewa et al. (Katewa et al., 2007). However, when mitochondria were supplied in electrons by pyruvate + malate + proline to reduce the complex I, we obtained higher respiration rates than these authors, which are likely to be due to the addition of malate as substrate in the present study. Katewa et al. found significant differences between mitotypes at 25°C whereas we did not detect any differences between mitotypes except at 18°C where siII showed higher catalytic capacity (Katewa et al., 2007). Interestingly, this higher capacity came with higher CAT activity. Maximal state 3m with pyruvate + malate + proline was found at 24°C whereas with sn glycerol-3-phosphate it was at 24°C and 28°C.

The decrease of catalytic capacities of mitochondrial state 3m respiration between 24°C and 28°C (Table 3) follow the same pattern as in other ectothermic species as reported in rainbow trout red muscle (Blier and Guderley, 1993; Guderley et al., 1997) and in Arctic char (Blier and Lemieux, 2001), which show a decrease at high temperature. There is however no decrease in the catalytic capacities when electrons are supplied to the ubiquinone pool via glycerophosphate dehydrogenase (Table 3). This clearly suggests that the decline in respiration rates at higher temperature when electrons are supplied at the level of complex I is induced by decreasing activities of enzymes upstream complex III.

Interestingly, state 4o follows the same pattern as state 3m with more pronounced differences between mitotypes (for all temperatures using complex I substrates, and for 18°C and 24°C using sn glycerol-3-phosphate). At 18°C and 24°C, siII exhibits a higher state 4o than siIII for both complexes whereas at extreme temperatures (12°C and 28°C) the higher state 4o is measured in siIII but only with complex I substrates and this difference is not maintained for sn glycerol-3-phosphate. During state 4, O2·− and H2O2 production are believed to be the highest (Forman and Boveris, 1982). Our results on state 4o are consistent with a previous study by Katewa et al. (Katewa et al., 2007), which showed higher H2O2 production in siII at 25°C. Our results could also suggest that flies with siII mtDNA are better adapted to a large temperature range and specifically to extreme temperatures whereas siIII has a smaller thermal range. This would be in line with the lower impact of lower temperature on ADP/O ratio as well as with the geographical distribution of both mitotypes. Flies from the two mitotypes were collected in Kenya where they live in sympatry; however, siII has a worldwide distribution whereas siIII is endemic to continental east Africa, Madagascar and Reunion Island (see supplementary material Fig. S1) (Ballard, 2004). This spatial niche differentiation hypothesis does not however exclude the possible temporal niche differentiation (diurnal or seasonal differences in haplotype performance/abundance). Obviously, at this stage of experimentation we cannot determine if the differences in mtDNA per se have any adaptive significance. Indeed, while there are isolated temperature-specific differences between mitotypes, these differences are not consistent across the various functional attributes measured. Consequently, there is little support for a conclusion that one mitotype has a broader temperature range for mitochondrial performance than the other.

The ratio of OXPHOS capacity to leak respiration is used as a coupling index of isolated mitochondria and of the functional integrity of mitochondria (RCR) (Chance and Williams, 1956). RCRs obtained using substrates for complex I and the substrate sn glycerol-3-phosphate indicate a well-coupled respiration. siII showed more coupled respiration, as well as a higher ADP/O ratio at 12°C when mitochondria were supplied in electrons at complex I level. This result shows that siII exhibits a higher efficiency of substrate oxidation and OXPHOS capacity at 12°C. Moreover, low RCRs at 18°C (5.78±1.2 for siII and 5.79±1.1 for siIII) and 28°C (5.67±0.7 for siII and 5.27±0.8 for siIII) suggest that the mixture pyruvate + malate + proline is associated with a lower efficiency of OXPHOS at these temperatures, which is supported by ADP/O ratios calculated at the same temperature. The ADP/O ratios for complex I also show optimal temperature at 24°C. The decrease in ADP/O ratios are probably induced by higher thermal sensitivity (and decrease) in state 3m respiration compared with state 4o as illustrated by RCRs. Surprisingly, high RCR values for both mitotypes at 12°C do not correspond to high ADP/O ratios, even if differences in RCRs between mitotypes were paralleled by differences in ADP/O ratios for this temperature. This result can only be explained by loss of OXPHOS capacity during state 3m at low temperature.

When mitochondria are supplied at the complex III level via glycerophosphate dehydrogenase, we observe a slight increase of RCRs from 12°C to 28°C. The only difference between mitotypes for this complex occurs at 28°C where, once again, siII exhibits higher RCR. At all temperatures, RCRs as well as ADP/O ratios are more elevated in complex I, showing higher OXPHOS capacity with pyruvate + malate + proline induced by activation of complex I proton pump. The only exception is at 28°C, where the higher RCR with sn glycerol-3-phosphate reflects a lower thermal sensitivity of state 3 respiration when ETS is supplied with sn glycerol-3-phosphate. However, at this temperature, we do not observe a concomitant increase in the ADP/O ratios, which suggest that OXPHOS capacity is partly dissipated downstream of the ETS during state 3m respiration (at complex IV, or by higher rate of proton leakage). When comparing state 3m respiration of mitochondria supplied either with pyruvate + malate + proline or sn glycerol-3-phosphate, the state 3m is higher with electrons provided to complex I, illustrating that complex IV (cytochrome c oxidase) can support much higher rate of oxidation than the one provided when supplying electrons only via glycerol-3-phosphate dehydrogenase to reduce complex III (sn glycerol-3-phosphate), at least at three temperatures we tested. The important decrease of complex I state 3m respiration between 24°C and 28°C, despite the absence of thermal sensitivity of complex III state 3m respiration at these same temperatures, suggests that the likely limitation of respiration comes upstream of complex III. This is also supported by the low UCR values (below but not significantly different from 1.0, Table 2) at any temperature, suggesting that ATP synthesis capacity (ATP synthase) can support the maximum respiration rates.

For COX activity, an increase from 12°C to 28°C was observed, as seen in other ectothermic species (Blier and Lemieux, 2001; Lemieux et al., 2009) (H. Lemieux, J.-C. Tardif, J.-D. Dutil and P.U.B., personal communication). We did not detect a loss of activity between 24°C and 28°C (Q1024–28=1.81 for siII and Q1024–28=2.66 for siIII). This result suggests that COX is probably not responsible for the reduction of catalytic capacities at 28°C when mitochondria are supplied in electrons at the complex I level. The decrease of the catalytic capacities of complex I observed at 28°C is therefore likely to be due to upstream ETS (complex I, II or III) or dehydrogenases, which drive the entry of the substrates in the ETS.

COX excess capacity was measured at high pathway flux with both complexes fully fuelled in electrons (pyruvate + malate + proline + glycerol-3-phosphate). An important excess was observed only at 12°C, with an excess of about 604% for siII and 613% for siIII. At this temperature, the COX maximal activity should reach a significantly higher level of inhibition before impairment of mitochondrial respiration (approximately 91.7% for siII and 93.0% for siIII). Excess capacity of COX has been reported in ectotherms (Blier and Lemieux, 2001; Farge et al., 2003) as well as in endotherms (Rossignol et al., 1999). At 12°C, COX catalytic capacities do not exert a strong control over the OXPHOS capacity (Ci=0.12±0.07 for siII and Ci=0.09±0.04 for siIII). From 18°C to 28°C, no excess capacity of COX was detected and Ci increased slightly along with temperature, suggesting important control of OXPHOS capacity by COX. This result also suggests that maximal, uninhibited COX activity could not support higher respiration rates than the maximal rate experimentally measured in the present study, where we used excess concentrations of different substrates. These results may indicate that when the ETS is ‘nearly saturated’ with electrons from carbon substrates, the system is close to its limit and therefore complex IV does not present any excess. Other studies have found high threshold values for the complex IV in Drosophila (Farge et al., 2003), as well as in rat mitochondria (Letellier et al., 1994; Rossignol et al., 1999) but only when the complex I was reduced using glutamate + malate or pyruvate + malate. Particularly, Farge et al. (Farge et al., 2003) found the same type of threshold curve for Drosophila subobscura at 28°C with glutamate + malate that we did at 12°C with pyruvate + malate + proline + glycerol-3-phosphate. This result suggests that at 12°C, when all substrates were used, there is impairment of electron entry into the ETS, and likely at the level of upstream dehydrogenases.

This highlights the fact that the mitochondrial metabolic enzymes have different thermal sensitivities and that temperature changes should necessarily modify the proportions of catalytic capacities of the different enzymes and therefore, the regulation of the whole pathway. At low temperatures (12°C in our study) regulation at the level of COX was relaxed, likely to be due to much higher thermal sensitivity of other mitochondrial enzymes or processes. From 18°C to 28°C, which covers the optimal temperature conditions, mitochondria are more regulated by COX.

In summary, we have shown that differences between the two mitotypes are observed at low temperature (12°C) where siII display higher RCR and ADP/O ratio than siIII as well as lower state 4o. To investigate the significance of state 4o, the experiment must be repeated with an assessment of membrane potential, because proton leak can only be estimated from state 4o when membrane potential is known or controlled. At this stage, we cannot however conclude about the adaptive value of mtDNA partly because the temperature-specific differences detected are not consistent across the various functional parameters measured and they cannot be linked yet to any fitness divergences at the specific ecological niches of the two populations. We have also shown that different ETS enzymes have different thermal sensitivities which can lead to different distribution of control along the ETS and dehydrogenases process at different temperatures leading to quite low level of respiration control by COX at low temperature. However, important properties of mitochondria may differ in vivo and in vitro (Kuznetsov et al., 2008). Further in situ studies (on permeabilised fibres) among mitotypes of D. simulans should reveal characterisation of functional mitochondria in their normal intracellular position and assembly, conserving interactions with other organelles. Moreover, introgressions between mitotypes should highlight the adaptive value of Drosophila mitochondria in co-adapted cellular environments.

Many thanks are due to H. Lemieux, S. Breton and R. Vergilino for their help with experimental protocols. This study was supported by research grants from the Natural Sciences and Engineering Research Council (NSERC) to P.U.B.

     
  • ACO

    aconitase

  •  
  • BSA

    bovine serum albumin

  •  
  • CAT

    catalase

  •  
  • Ci

    flux control coefficient

  •  
  • COX

    cytochrome c oxidase (complex IV)

  •  
  • CS

    citrate synthase

  •  
  • DTNB

    5,5′-dithiobis(2-nitrobenzoic acid)

  •  
  • ETS

    electron transport system

  •  
  • FCCP

    carbonyl cyanide 4-(trifluoromethoxy)phenylhydrazone

  •  
  • H2O2

    hydrogen peroxide

  •  
  • Ki

    inhibition constant

  •  
  • MDA

    malondialdehyde

  •  
  • mtDNA

    mitochondrial DNA

  •  
  • O2·−

    superoxide

  •  
  • OXPHOS

    oxidative phosphorylation

  •  
  • Q10

    temperature coefficient

  •  
  • RCR

    respiratory control ratio

  •  
  • ROS

    reactive oxygen species

  •  
  • TBARS

    thiobarbituric reactive substances

  •  
  • TMPD

    N,N,N′,N′-tetramethyl-p-phenylenediamine

  •  
  • UCR

    uncoupled control ratio

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In the aging housefly aconitase is the only citric acid cycle enzyme to decline significantly
.
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37
,
91
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96
.