Abstract
Friedreich ataxia, a neurodegenerative disorder resulting from frataxin deficiency, is thought to involve progressive cellular damage from oxidative stress. In Drosophila larvae with reduced frataxin expression (DfhIR), we evaluated possible mechanisms of cellular neuropathology by quantifying mitochondrial axonal transport, membrane potential (MMP), and reactive oxygen species (ROS) production in the DfhIR versus wild-type nervous system throughout development. Although dying-back neuropathy in DfhIR larvae did not occur until late third instar, reduced MMP was already apparent at second instar in the cell bodies, axons and neuromuscular junctions (NMJs) of segmental nerves. Defects in axonal transport of mitochondria appeared late in development in distal nerve of DfhIR larvae, with retrograde movement preferentially affected. As a result, by late third instar the neuromuscular junctions (NMJs) of DfhIR larvae accumulated a higher density of mitochondria, many of which were depolarized. Notably, increased ROS production was not detected in any neuronal region or developmental stage in DfhIR larvae. However, when challenged with antimycin A, neurons did respond with a larger increase in ROS. We propose that pathology in the frataxin-deficient nervous system involves decreased MMP and ATP production followed by failures of mitochondrial transport and NMJ function.
Introduction
The health of neurons depends critically on the movement, distribution and function of their mitochondria (Hollenbeck and Saxton, 2005). This is nowhere more evident than in a range of mitochondrial dysfunctions that are manifested prominently or exclusively as diseases of the nervous system (McKenzie et al., 2004; Schapira, 2006; McFarland et al., 2007). Mitochondria supply ATP, buffer cytosolic calcium and control apoptosis, but in addition to these activities—indeed, as their consequence—mitochondria produce reactive oxygen species (ROS). Oxidative damage has been suggested as the major source of pathology for many mitochondrial diseases (Wallace, 2005), and for neurodegenerative diseases in general (Fukui and Moraes, 2008). However, neuropathology can result from other changes in mitochondrial functions, such as the disruption of mitochondrial axonal transport (Zhao et al., 2001; Baloh et al., 2007; De Vos et al., 2007), fission/fusion (Alexander et al., 2000; Delettre et al., 2000; Kijima et al., 2005; Verhoeven et al., 2006), protein import (Bauer and Neupert, 2001), and DNA replication (Schapira, 2006). To understand the mechanisms by which mitochondrial disorders cause neuronal dysfunction and death, it will be necessary to evaluate many elements of mitochondrial biology.
Friedreich ataxia (FRDA) is an autosomal recessive neurodegenerative disease caused by a GAA repeat expansion in intron 1 of the frataxin gene. The resulting deficiency in expression is associated with a dying-back neuropathy affecting sensory neurons and spinocerebellar and corticospinal motor tracts (Gibson et al., 1996; Delatycki et al., 2000; Patel and Isaya, 2001; Puccio and Koenig, 2002). Frataxin is thought to be an iron chaperone responsible for formation of iron-sulfur (Fe-S) clusters, but its deficiency is associated not only with diminished activity of Fe-S-containing enzymes, but also with altered defense against oxidative stress (Calabrese et al., 2005; Bencze et al., 2006). Evidence that FRDA pathology involves increased ROS levels or susceptibility to oxidative stress comes from studies of sera, tissues and isolated cells of patients (Delatycki et al., 1999; Wong et al., 1999; Emond et al., 2000; Schulz et al., 2000; Chantrel-Groussard et al., 2001; Jiralerspong et al., 2001; Piemonte et al., 2001) and from transgenic mice (Chantrel-Groussard et al., 2001; for review, see Puccio and Koenig, 2002). However, recent data from transgenic mouse models show that FRDA pathology can occur, associated with deficient activities of the electron transport chain (ETC) and other Fe-S enzymes, but without evidence of increased oxidative stress (Seznec et al., 2004, 2005).
It is difficult to predict whether a particular defect in mitochondrial function will cause ROS production to increase, decrease, or remain unchanged (Pitkanen and Robinson, 1996; Smeitink et al., 2004; for review, see Balaban et al., 2005; Fukui and Moraes, 2008). Because frataxin affects the activity of many Fe-S enzymes (Rotig et al., 1997; Lodi et al., 1999; Bradley et al., 2000), its deficiency should produce broader, more diffuse metabolic insufficiency than mutations in specific ETC components (Taylor and Turnbull, 2005; Schapira, 2006). However, mitochondrial functions such as membrane potential or axonal transport and distribution in axons and synapses have gone largely unexamined in the disease and its models. We have examined quantitatively the cellular neuropathology of frataxin deficiency using the frataxin knock-down Drosophila strain of Anderson (Anderson et al., 2005, 2008). We find that in the frataxin-deficient nervous system, mitochondria show universally diminished membrane potential early in development, followed by temporally and geographically specific axonal transport deficits and abnormal synaptic distribution.
Materials and Methods
Genetics.
A DfhIR Drosophila strain (“DfhIR1,” or “UDIR1”) produced by Anderson et al. (2005) expressing an inhibitory RNA that specifically inhibits frataxin expression was generously provided to us and its properties have been described in detail (Anderson et al., 2005, 2008). To observe and quantify mitochondrial location and transport in frataxin-deficient larvae, we crossed the DfhIR second chromosome into the mito-GFP strain produced and described by Pilling et al. (2006) to obtain the genotype: w; P{UAS-DfIR}w+/SM2; D42-GAL4 P{UAS-mitoGFP} e/TM3. These were crossed together to obtain mito-GFP, homozygous UAS-DfIR larvae for experiments. The control genotype was w; +; D42-GAL4 P{UAS-mitoGFP} e/TM6B, Tb Hu e. To obtain a strain in which we could observe synaptic (synaptobrevin-containing) vesicles under frataxin-deficient conditions, a similar strategy was used to cross the DfhIR chromosome into the D42-GAL4-syb-GFP background (Estes et al., 2000) to obtain the genotype: w; daG32-GAL4 P{UAS-DfIR}w+/CyO; P{D42-GAL4-syb} e/TM3. The control genotype was as follows: w; +; P{D42-GAL4-syb} e/TM3.
Immunoblotting and immunostaining.
Whole larvae were homogenized in standard denaturing SDS-PAGE buffer and protein from 10 larvae was loaded per lane of an 8% polyacrylamide gel, electrophoresed, and transferred to PDVF. Blots were probed with mouse monoclonal anti-frataxin (Millipore Bioscience Research Reagents) or rabbit anti-GFP (Clontech) and secondary IRDye-800CW goat anti-mouse or anti-rabbit (Rockland), visualized using a Gel Doc EQ epi-illumination system (Bio-Rad), and staining intensity of individual bands was quantified using MetaMorph software (Molecular Devices). For immunostaining of NMJs, partially dissected larvae were fixed with 4% paraformaldehyde, rinsed with PBS, washed with PBS containing 0.1% Triton X-100 and 10 mg/ml BSA (PBSTx), then stained with mouse anti-HRP, washed with PBSTx, stained with Alexa 568 goat anti-mouse (Invitrogen), mounted and observed by laser scanning confocal microscopy (LSCM) (Bio-Rad) with a 568 nm laser line.
Larval preparation for observing neuronal mitochondria.
To observe, track and stain mitochondria in live segmental nerves, larvae were prepared by a variation on previously described methods (Hurd and Saxton, 1996; Pilling et al., 2006). Larvae at second to late third instar were pinned down and opened with an incision through the cuticle on the dorsal side, and the cuticle was peeled back slightly with forceps. Then the fat bodies were pushed gently aside, exposing the ventral ganglion and segmental nerves but leaving the axons connected to their cell bodies in the ventral ganglion and to their peripheral muscle targets. A chamber was formed around the dissected larvae by sandwiching them dorsal-side-up between a glass coverslip and a slide using dental wax as a spacer, and the chamber was filled with Schneider's insect medium (Invitrogen). Mitochondria in cell bodies, axons, and NMJs of motor neurons were observed by LSCM of mito-GFP with a 488 nm laser line.
Quantification of mitochondrial transmembrane potential and ROS levels.
Tetrmethylrhodamine methyl ester (TMRM) (Invitrogen) was added to the dissected larval preparation at 20 nm in Schneider's medium for 20 min, then replaced with 5 nm TMRM. Quantitative fluorescence values were obtained for individual mitochondria and the adjacent cytoplasm, and the ratio of mitochondrial to cytoplasmic fluorescence was calculated as a measure of mitochondrial membrane potential (Verburg and Hollenbeck, 2008). The superoxide indicating dye MitoSOX Red (Invitrogen) was applied at 5 μm in Schneider's medium for 20 min, then washed out with plain medium. Fluorescence values for mitochondria and adjacent cytoplasm were obtained and ratioed as just described. The superoxide indicating dye dihydroethidium (hydroethidine; Sigma) was applied at 5 μm in Schneider's medium for 20 min and washed out before observation. As a positive control for ROS detection, the complex III inhibitor antimycin A was added to larvae at 50 or 100 μm for 10 min.
Measuring mitochondrial axonal transport.
Segmental nerves were observed by LSCM in their proximal (segment A2), middle (segment A4) and distal (segment A7) regions. To track GFP-mitochondria in motor axons, a small region was bleached with the confocal laser as previously described (Pilling et al., 2006) and mitochondria moving into the bleached zone in both directions were observed. Images of mitochondria were obtained every 1 s for 200–250 s and stored as PICT files. Transport was quantified by tracking individual mitochondria using ImageJ software. The transport parameters calculated were as follows: velocity, duty cycle and flux, for both anterograde and retrograde movement. In addition, anterograde, retrograde, and pause duty cycles were calculated for both net anterograde and net retrograde moving mitochondria. Mitochondrial lengths were measured and compared in wild-type and DfhIR axons using MetaMorph software.
Determination of mitochondrial density.
Mitochondrial density was calculated from LSCM images using MetaMorph software. In motor cell bodies of the ventral ganglion, the area of mito-GFP fluorescence in each cell body was divided by the area of the cell body. In NMJs, paraformaldehyde-fixed larvae were immunostained with anti-HRP to reveal the full outline of the NMJs, and the area of mito-GFP staining in each NMJ was divided by the total NMJ area. Synaptic vesicle density in NMJs was observed and quantified in identical fashion using larvae of the DfhIR; D42-syb-GFP strain.
Preparation and staining of larval sections.
Larvae were fixed with paraformaldehyde, paraffin embedded, and cross sectioned at a thickness of 10 μm. Sections were subjected to Bodian stain, counterstained with hematoxylin and eosin, and observed and recorded using a Nikon E800 microscope with a SPOT Flex color-mosaic camera (Diagnostic Instruments). Quantitative morphometry was performed using MetaMorph software with sections from second, early third and late third instar larvae. The cortical area and number of motor cell bodies were determined at all stages, and the cross sectional area of the segmental nerve was quantified in the proximal (A2), middle (A4) and distal (A6 and A8) regions of the nerve.
Results
DfhIR motor neurons show distal axonal degeneration and cell body loss in the ventral ganglion by late third instar
To check that the DfhIR; mito-GFP strain retained the decreased frataxin expression of the original DfhIR line (Anderson et al., 2005), we performed anti-frataxin immunoblots using extracts of whole DfhIR; mito-GFP larvae at second, early third and late third instar (Fig. 1A). At all three stages, the DfhIR; mito-GFP larvae showed decreased frataxin expression compared with the wild-type mito-GFP larvae. To assess the overall neuropathology of DfhIR larvae, we examined segmental nerves (Fig. 1B,C) and motor cell bodies in the ventral ganglion (Fig. 1D–F) in sections of larvae using Bodian and hematoxylin and eosin (H&E) staining. The DfhIR segmental nerves showed no morphological difference from wild type in any region from second to early third instar, but pathology become apparent in the distal nerve late in development. At late third instar the cross sectional area of the distal nerve had declined to 72% of wild type at segment A6 and further to 61% at A8 (Fig. 1B,C). The structure of the ventral ganglion of DfhIR larvae was also indistinguishable from wild type until late third instar, when the cortical area declined to 62% of that in wild type, and the number of motor cell bodies per section was reduced to 61%, from a mean of just above 80 to just under 50 (Fig. 1D–F). Thus, DfhIR larvae showed dying-back neuropathy, but not until late in larval development.
Axonal degeneration from the distal end and neuronal cell death in the ventral ganglion are apparent at third instar in DfhIR larvae. A, Anti-frataxin immunoblots were performed with extracts of whole larvae, at second, early third and late third instar (2, E3 and L3, respectively) quantified, and normalized for GFP content using anti-GFP. DfhIR crossed into the mito-GFP background resulted in a 30–40% reduction in whole-larval frataxin expression relative to wild type at the same stage. Bodian- and H&E-stained paraffin sections of larvae were used to quantitate changes during development: B shows wild-type and DfhIR segmental nerve cross sections at L3 in the distal axon; D shows wild-type and DfhIR ventral ganglia at L3. C, Quantitive morphometry showed that in wild-type larvae, the cross sectional area of the segmental nerve did not change during development, or along the proximodistal axis at any point during development. In DfhIR larvae, the cross sectional area was significantly decreased in the distal region of the nerve (at segments A6 and A8) at L3. E, F, Morphometry of cell bodies in the ventral ganglion showed that in DfhIR larvae, both the area of the cortical region of the ganglion (E) and the number of cell bodies (F) were significantly decreased at L3 in DfhIR relative to wild type. All error bars represent the SD, and significant differences between DfhIR and wild-type values for specific stages or regions are indicated (*p < 0.05, n = 40 for all experiments).
To search for the underlying cellular basis of this pathology, we went on to quantify three essential features of mitochondrial activity in neurons within intact segmental nerves of these larvae: mitochondrial transport, mitochondrial transmembrane potential, and ROS production. Each of these was assessed across time and space: at three stages of larval development (second, early third and late third instar) and, where applicable, in five regions of the neurons: cell bodies in the ventral ganglion; axons in the proximal (A2), middle (A4) and distal (A7) region of the nerve, and neuromuscular junctions (NMJs).
The first and most pervasive defect in DfhIR neurons is loss of mitochondrial transmembrane potential
To compare the activity of mitochondria between wild-type and DfhIR neurons, we stained live larval preparations with a subquenching concentration of the mitochondrial dye TMRM (Farkas et al., 1989; Scaduto and Grotyohann, 1999; Verburg and Hollenbeck, 2008). The partitioning of TMRM between the cytoplasm and mitochondrial matrix is driven by the inner mitochondrial membrane potential (MMP); thus we used the ratio of mitochondrial to cytoplasmic TMRM fluorescence (Fm/Fc) as the most sensitive and accurate available indicator of MMP. We found that in all regions of the neuron and from the earliest stage we observed, neurons in DfhIR nerves showed a significantly lower MMP than wild type (Fig. 2). In cell bodies of the ventral ganglion, Fm/Fc was 25% lower in DfhIR neurons at second instar and declined further by late third instar (Fig. 2A,B). Mitochondria throughout the length of DfhIR axons also showed lower MMP than wild type, a difference that became more pronounced with both larval age and position along the nerve. The Fm/Fc in the distal region of DfhIR axons was already <70% of controls at second instar and declined further to <50% by late third instar (p < 0;05 for 2 vs L3, Fig. 2D). The most extreme MMP phenotype was seen in NMJs (Fig. 2E), where the TMRM signal in DfhIR neurons declined to a mean of only 30% that of controls by late third instar (Fig. 2G). More important, DfhIR NMJs contained significant numbers of mitochondria that had no greater TMRM fluorescence than the surrounding cytoplasm and were thus completely depolarized (Fig. 2E, apparent as GFP-positive mitochondria with no yellow TMRM signal in the merged DfhIR image). Such mitochondria are virtually never seen in wild-type NMJs.
Mitochondrial transmembrane potential is diminished throughout the neurons of DfhIR larvae compared with wild-type. A, B, In individual cell bodies in the ventral ganglion, mito-GFP fluorescence was used to identify mitochondria (A, green) and TMRM fluorescence was used to measure membrane potential (red, overlap is yellow in merged image). Note that the TMRM signal includes mitochondria in sensory axons that do not express mito-GFP and were not included in any measurements. B, The ratio of mitochondrial to cytoplasmic TMRM fluorescence values (FM/FC) was determined at second, early third, and late third instar (2, E3, L3, respectively), divided by the wild-type second instar mean value to normalize and plotted, showing that DfhIR cell bodies had diminished MMP throughout development relative to wild-type mito-GFP cell bodies. C, D, In segmental nerve axons, mitochondria were observed throughout development in all three regions—here, images of mitochondrial GFP fluorescence and TMRM in the distal axon at L3 show the diminished MMP in DfhIR axons. D, The mitochondrial FM/FC was determined in segmental nerves at each stage and axonal region and divided by the wild-type proximal second instar value to normalize. Plots of these values show that in wild-type larvae MMP did not vary with age or distance from the ventral ganglion (D, left); however, DfhIR larvae not only showed diminished MMP at all stages and axonal positions, but also showed an increasing effect with age and distance from the ventral ganglion (D, right). E–G, In neuromuscular junctions, mitochondrial TMRM fluorescence intensity per area of the NMJ had already declined relative to controls by second instar, and dropped to <70% of control levels by late third instar (F); the TMRM fluorescence per mitochondrial area declined to less than half wild type (G). Merged images of TMRM (red) and mito-GFP fluorescence at right show that at late third instar, many mitochondria in DfhIR NMJs show complete depolarization (E). Scale bars: A, C, E, 10 μm. *p < 0.05, **p < 0.01; error bars denote SD; n = 30 for all TMRM measurements.
DfhIR larvae show specific defects in axonal transport of mitochondria in the distal axon, late in larval development
We observed and quantified mitochondrial transport by a modification of the method of Pilling et al. (2006), photobleaching the mito-GFP in a region of segmental nerve and then following mitochondria entering that region from the proximal and distal sides. We tracked individual organelles from 250-frame sequences acquired in the proximal, middle and distal segmental nerves at second, early third and late third instar (Fig. 3A,D). From these data we calculated mitochondrial flux, duty cycle, run length, run time, and pause time for the anterograde and retrograde directions of movement in each region at each developmental stage (supplemental Table 1, available at www.jneurosci.org as supplemental material).
In segmental nerve axons of DfhIR larvae, mitochondrial flux, transport duty cycle and velocity are diminished compared with wild type at late third instar. Mitochondrial movements were tracked in segmental nerves of second, early third and late third instar larvae, in the proximal, middle and distal region of the nerves. All images are oriented with the cell bodies (ventral ganglion) to the left, so that anterograde transport is from left to right. A shows images of mitochondria in a wild-type late third instar larva moving into a bleached region in both directions in all three regions of the nerve. B, C, Both the flux of mitochondria (B) and their duty cycle (C) decline from the proximal to distal axons. D shows mitochondria moving into a bleached region of the distal nerve of normal larvae in both directions, at three stages of development. E, F, In axons of the distal nerve, both the flux of mitochondria (E) and their duty cycle (F) increase during development from second to late third instar. G compares mitochondrial movements between wild-type and DfhIR larvae at late third instar in the distal region. H–K, In DfhIR larvae, mitochondrial flux (H), duty cycle (I) and velocity (J) are significantly reduced in both directions, but retrograde flux and duty cycle are more strongly affected than anterograde (K). Scale bars, 10 μm. *p < 0.05, n ≥ 30 for each experiment; error bars represent the SD.
In wild-type segmental nerves, mitochondrial flux was greater in the anterograde than retrograde direction, and increased with larval age (Fig. 3E) while declining with distance from the cell body (Fig. 3B). Wild-type mitochondrial movement also became less directionally persistent with increased distance from the ventral ganglion: for anterograde-moving organelles, the anterograde duty cycle declined in the distal nerve while their retrograde and pausing duty cycles increased; the converse was true for retrograde-moving mitochondria. (Fig. 3C). However, the direction of movement was more persistent in all regions of older nerves than younger nerves (Fig. 3F).
In DfhIR segmental nerves, mitochondrial transport was similar to wild type in all parameters at second instar, but began to show small defects in the distal axons at early third instar that rose to significance at late third instar (Fig. 3G). Specifically, anterograde and retrograde flux, duty cycle, and velocity all declined significantly in distal DfhIR axons (Fig. 3H–J). The velocities of anterograde- and retrograde-moving mitochondria were almost equally affected, dropping to 77% and 73% of wild type, respectively. However, flux and duty cycle were more profoundly affected in the retrograde direction: anterograde flux dropped to 81% of wild type while retrograde flux dropped to 70%, and anterograde duty cycle dropped to 83% of wild type while retrograde duty cycle dropped to 70%. These diminutions of the flux and duty cycle, but not velocity, were significantly greater for retrograde movement than for anterograde movement (Fig. 3K). Thus, frataxin deficiency causes an inhibition of mitochondrial transport that is manifested in the distal axon late in larval development, and preferentially affects retrograde movement. The magnitude of these effects on mitochondrial transport is similar to that seen for hypomorphic mutant alleles of the motor proteins kinesin and dynein (Pilling et al., 2006) (our supplemental Fig. 2, supplemental Table 2, available at www.jneurosci.org as supplemental material). Finally, measurements of mitochondrial length at late third instar detected no difference between wild-type axons (mean ± SEM = 1.23 ± 0.05 μm; n = 71) and DfhIR axons (1.37 ± 0.14 μm, n = 73).
DfhIR larvae accumulate excess depolarized mitochondria in their NMJs
Preferential diminution of retrograde transport in the distal region would be expected to result in an abnormal accumulation of mitochondria in the NMJs of DfhIR larvae. To test this, we measured the density of mitochondria in NMJs of second, early third, and late third instar larvae using mito-GFP and anti-HRP immunofluorescence signals (Fig. 4). As a baseline, we first established the developmental pattern for mitochondrial density in the cell bodies of these neurons in the ventral ganglion of live wild-type and DfhIR larvae. The projected area of mitochondria per cell body in LSCM cross sections did not vary through development for either genotype, nor between wild-type and DfhIR larvae (Fig. 4A). In NMJs of fixed wild-type larvae, we found that the mitochondrial content and total area of NMJs both increased modestly through development, yielding no increase in mitochondrial density (Fig. 4D–F). However, in DfhIR NMJs, the total NMJ area increased during development identically to wild type, but the NMJ mitochondrial content increased significantly more than did wild type at late third instar, resulting in a 1.3-fold higher mitochondrial density in DfhIR NMJs (Fig. 4F). Thus, by late third instar, frataxin deficiency leads an accumulation of excess mitochondria in NMJs, many of which are partially or completely depolarized, as shown in Figure 2E–G.
DfhIR larvae show an abnormal accumulation of mitochondria in the NMJs by late third instar. A, The density of mitochondria in motor cell bodies of the ventral ganglion, determined as the ratio of mito-GFP area to neuronal cell body area, remains nearly constant during development and is the same in wild-type and DfhIR larvae. B, A merged image of HRP immunostaining (red) and mito-GFP (green, yellow in overlap with HRP) shows wild-type NMJs of second, early third, and late third instar larvae. C, A merged image of mito-GFP and HRP immunostaining shows that in late third instar larvae, NMJs of DfhIR larvae have a higher mitochondrial density than those of wild type. D–F, Quantitation of the area of mito-GFP signal per NMJ (D), total NMJ area (E), and the fraction of the NMJ occupied by mitochondria (F) for wild-type and DfhIR larval NMJs from second through late third instar shows the increases in both mitochondrial and total NMJ area with development, and confirms the excessive mitochondrial density of late third instar DfhIR NMJs. Scale bar, 5 μm. *p < 0.05, n = 40 for all experiments; error bars represent the SD.
To ascertain whether the accumulation of organelles in the NMJs was specific to mitochondria or more general, we also quantified the density of synaptic (synaptobrevin-containing) vesicles using an n-syb-GFP; DfhIR strain (Estes et al., 2000). Using n-syb-GFP fluorescence and anti-HRP immunostaining in fixed larvae (Fig. 5A), we found that the synaptic vesicle density of NMJs rose similarly through development in both wild-type and DfhIR larvae, but that by late third instar the DfhIR NMJs accumulated synaptic vesicles to a 1.3-fold excess over wild type (Fig. 5B), very similar to that seen for mitochondria.
DfhIR larvae accumulate excess synaptobrevin-containing vesicles in their synaptic NMJs at third instar compared with controls. A, Synaptic (synaptobrevin-containing) vesicles in motor neurons were visualized by D42-syb-GFP (green) and NMJs were counterstained with anti-HRP antibody (red, overlap with green shown as yellow); late third instar is shown here. B, Synaptic vesicle densities were determined as the ratio of the number of syb-GFP pixels to the number of HRP pixels at second, early third and late third instar. Late third instar DfhIR larvae show increased density of synaptic vesicles in their NMJs relative to wild type. All error bars represent the SD and significant differences between DfhIR and wild-type NMJs are indicated (*p < 0.05, n = 40 for all experiments). Scale bar, 2.5 μm.
DfhIR neurons do not produce higher levels of ROS, but are more susceptible to complex III inhibition late in development
The body of work on Friedreich ataxia and frataxin deficiency suggests that a likely component of the pathology is generation of excess ROS (Calabrese et al., 2005; Bencze et al., 2006). We used fluorescent probes for superoxide to quantify the level of ROS in the motor neurons of live larvae. To detect superoxide levels in mitochondria, we treated larval preparations with MitoSOX red, a fluorescent lipophilic cation that, like TMRM, partitions into mitochondria and has a fluorescence intensity that increases with superoxide concentration (Mukhopadhyay et al., 2007). Using the mito-GFP signal to identify mitochondrial pixels in the confocal images, we determined MitoSOX fluorescence in cell bodies, axons and NMJs throughout larval development (Fig. 6). In wild-type larvae, in all regions of the neurons, ROS levels remained relatively constant during development, but they responded sharply to the application of the complex III inhibitor antimycin A (Staniek and Nohl, 2000; Chen et al., 2003), demonstrating the capacity of the probe to detect increases in [ROS] (Fig. 6B,D,F).
DfhIR neurons do not produce intrinsically higher levels of ROS, but are more susceptible to treatment with the complex III inhibitor antimycin. A–F, Fluorescence intensities of mitoGFP (green) and MitoSOX (red) were used to determine relative levels of ROS production in cell bodies in the ventral ganglion (A, B), axons (C, D), and NMJs (E, F) of DfhIR and wild-type neurons, with and without antimycin treatment, and throughout larval development. Neither wild-type nor DfhIR cell bodies showed increased ROS during development, and DfhIR cell bodies (B, top histogram) did not show higher ROS levels than wild type (B, bottom histogram). Both 50 and 100 μm antimycin treatments elicited higher ROS levels in wild-type and DfhIR cell bodies at all developmental stages, but at late third instar, DfhIR cell bodies responded to antimycin with higher ROS levels than did wild type (B). In axons (C), there were also no significant differences between DfhIR and wild-type ROS levels in any region of the nerve or time in development, but DfhIR axons showed higher ROS levels in response to antimycin in the middle region of the axons at late third instar, and in the distal region at early and late third instar (D). There was also no difference between ROS levels in DfhIR and wild-type NMJs through development, but DfhIR NMJs at late third instar responded to antimycin with higher ROS levels than wild type (E, F). For quantification, all error bars represent the SD and significant differences between DfhIR and wild-type values are indicated (*p < 0.05, **p < 0.01, n = 40 for all experiments).
In cell bodies in the ventral ganglion, elevated mitochondrial ROS levels were not detected in DfhIR larvae relative to wild type at any stage in development. However, at late third instar, the DfhIR cell bodies did respond to a 100 μm antimycin A challenge with a 40% greater increase in ROS than did wild type (Fig. 6B). This pattern also occurred in axonal mitochondria: DfhIR axons showed no greater ROS levels than wild type at any region or stage of development, but in response to antimycin A, they showed significantly greater mitochondrial ROS increases in the middle axons at late third instar (125% of wild type), and in distal axons at early and late third instar (145% and 155%, respectively) (Fig. 6C,D). In NMJs, DfhIR larvae also did not show increased ROS compared with wild type until late third instar, when DfhIR NMJs showed a much greater ROS response to antimycin A challenge (160%) than did wild type (Fig. 6G–I). Very similar results were obtained using dihydroethidium to detect total cytoplasmic superoxide: in unperturbed preparations, wild type and DfhIR did not have detectably different ROS levels at any stage of development or region of the neurons, but an antimycin challenge elicited higher ROS levels in cytoplasm of DfhIR cell bodies (170%), distal axons (175%) and NMJs (160%) at late third instar only (supplemental Fig. 3, available at www.jneurosci.org as supplemental material). Thus, in the unperturbed larval nervous system frataxin deficiency did not result in detectably higher ROS levels, but it did produce hypersensitivity to complex III inhibition late in development.
Discussion
Many defects in mitochondrial function are associated with diseases of the nervous system (McKenzie et al., 2004; Wallace, 2005; Schapira, 2006; McFarland et al., 2007), but in most cases we understand neither which of these potential defects underlie the cellular neuropathology, nor their temporal and causal relationships. In this study we chose a model mitochondrial disorder, frataxin deficiency, and dissected the cellular basis of its pathology in the live, intact nervous system of Drosophila larvae. We found evidence for a developmentally ordered, counterintuitive series of defects in mitochondrial function that preceded dying-back neuropathy and did not involve apparent excess ROS production.
Frataxin deficiency depresses MMP early and widely in the larval nervous system
The first abnormality of mitochondrial function was also the most pervasive: DfhIR mitochondria showed significantly reduced MMP from the cell bodies throughout the axons and into the NMJs, and from second instar to late third instar. This is consistent with frataxin's proposed major role of supporting the construction and maintenance of Fe-S cluster-containing enzymes (Puccio and Koenig, 2002). Since the Fe-S components of the ETC complexes are absolutely essential for oxidative phosphorylation, DfhIR neurons are probably manifesting a general deficiency in the ETC activity that generates the MMP. This establishes, at the whole-mitochondrial level, a basis for evidence for reduced metabolic enzyme activity in Friedreich ataxia patient material (Rotig et al., 1997; Bradley et al., 2000), animal models (Puccio et al., 2001; Seznec et al., 2004; Anderson et al., 2005; Lu and Cortopassi, 2007), and yeast or cultured cell studies (Wilson and Roof, 1997; Stehling et al., 2004). However, since the energy of the MMP is harnessed for many functions of mitochondria, its deficiency here raises the possibility that the cellular neuropathology involves additional elements in addition to energy metabolism. Thus, mitochondrial calcium uptake, transport of other ions and metabolites, protein import, fission and fusion, all of which rely on the MMP, are potential targets in frataxin-deficient neurons. It is unclear from first principles which of these functions is most likely to be compromised by partial depolarization of mitochondria, but our data (discussed below) indicate that axonal transport is affected.
MMP in the DfhIR nervous system was not only reduced relative to wild type in all locations and stages of development, but also showed a significant further decline in the middle and distal axons and NMJs late in larval development (Fig. 2), around the time of the dying-back neuropathy. This could reflect the challenge of supporting Fe-S enzyme biosynthesis at the greatest distances from the cell body and nuclear genome, and probably in turn underlies the specific deficits in axonal transport that we observed at the same stage and locations.
Axonal transport deficits and accumulation of depolarized mitochondria are concurrent with axonal neuropathy
The axon relies on the transport of mitochondria (Hollenbeck and Saxton, 2005; Chang and Reynolds, 2006), and mutations in motor proteins can cause neurodegeneration (Saxton et al., 1991; Hurd and Saxton, 1996; Hurd et al., 1996; Gindhart et al., 1998; Yonekawa et al., 1998; Zhao et al., 2001; Hafezparast et al., 2003; Hirokawa and Takemura, 2004; Pilling et al., 2006). But neuropathologies are also associated with transport defects in disorders where motor proteins are not mutated, such as amyotrophic lateral sclerosis (Bruijn et al., 2004; De Vos et al., 2007), Huntington's disease (Gauthier et al., 2004) and Charcot-Marie-Tooth disease type 2A (Baloh et al., 2007). Of particular relevance here, a mouse model of hereditary spastic paraplegia (paraplegin-deficient) showed accumulation of abnormal mitochondria in synaptic terminals well before distal axonopathy or gross symptoms were detected (Ferreirinha et al., 2004). In addition, mutations in proteins such as Milton (Stowers et al., 2002; Glater et al., 2006), Miro (Guo et al., 2005), or Drp1 (Verstreken et al., 2005), whose primary effect is to deny mitochondrial supply to the distal axon, result in cellular and organismal neuropathies.
In frataxin-deficient nerves, we found that mitochondrial transport was reduced in the distal axons at late third instar, the same stage and location as the steepest declines in MMP. However, the nature of the transport deficit was counterintuitive: its net effect was not failure to deliver mitochondria to the NMJs, but failure to retrieve them. Nonetheless, because the excess mitochondria accumulating in the NMJs were profoundly depolarized, the distal axon and synapse were denied adequate mitochondrial function. Since the loss of MMP in DfhIR nerves began well before the transport deficit or dying-back of axons, and because further depolarization in distal axons was matched by transport deficits at the same stage and location, we suggest that the primary failure in the DfhIR neurons was inadequate local production of ATP to support transport. Diminished ATP production has also been reported in FRDA patient tissues (Lodi et al., 1999). The loss of MMP could also affect axonal mitochondrial transport at an indirect, regulatory manner, perhaps through changes in MMP-dependent calcium homeostasis or altered ATP-dependent signaling. In either case, we suggest that the more profound effect of DfhIR physiology on mitochondrial duty cycle than on velocity reflects the fact that velocity of movement is an intrinsic property of motor proteins, which tend to be “on” or “off” without an intermediate, “hobbled” state.
The accumulation of not just mitochondria but also vesicles in NMJs (Fig. 5) indicates that the deficit in transport was a broad one, and in each case was retrograde-selective. This is not the first report of a neurodegenerative phenotype associated with selective defects in the retrograde transport machinery (LaMonte et al., 2002; Hafezparast et al., 2003; Puls et al., 2003; Edgar et al., 2004; Horiuchi et al., 2005; Pilling et al., 2006). This selectivity could result from a differential sensitivity of the retrograde transport machinery to ATP concentration, or, again, to calcium- or ATP-dependent signaling effects. It is worth noting that mild mutant alleles of kinesin heavy chain and dynein have effects of similar magnitude to those we observed for DfhIR (supplemental Fig. 2, available at www.jneurosci.org as supplemental material) (Pilling et al., 2006). A failure of retrograde transport might also contribute to cell body loss and dying-back neuropathy by restricting the retrograde flow of trophic support (McCabe et al., 2003; Keshishian and Kim, 2004; Sanyal et al., 2004; Liu and Butow, 2006; Marqués and Zhang, 2006; Ibáñez, 2007). Altogether, our data suggest that the transport deficit is an effect of deficient mitochondrial metabolism that precedes and may contribute to dying-back neuropathy.
ROS production and sensitivity
Contrary to our expectations, in unperturbed DfhIR larvae we were unable to detect any increase in ROS levels in any part of the nervous system at any point in development. The efficiency of the superoxide dismutase, glutathione peroxidase and peroxyredoxin systems, along with small molecule ROS scavengers (Halliwell, 2006), ensures that the net ROS released to the cytoplasm amounts to a very small fraction of the total generated within mitochondria (Balaban et al., 2005)—which is itself probably 1–2 orders of magnitude smaller than often cited (Staniek and Nohl, 2000; St-Pierre et al., 2002). Thus, to ensure that we could detect any increase in ROS production, we measured both cytoplasmic and matrix ROS levels, and both methods were easily able to detect the increase in ROS production that accompanied inhibition of complex III by antimycin A. While studies of yeast, vertebrate cell lines, animal models and patient material indicate that the pathology of FRDA/frataxin deficiency is associated with increased susceptibility to oxidative damage and/or increased ROS production (cited above), animal models have also recapitulated FRDA neuropathology without evidence of increased oxidative damage (Seznec et al., 2004).
In Drosophila, studies of three different frataxin-deficient models have provided some insight. Studies in one frataxin-deficient RNAi-based model showed an organismal phenotype that included reduced life span and climbing activity, and an excessive decline, in response to hyperoxia, of aconitase but not succinate dehydrogenase activity (Llorens et al., 2007). In addition, Runko et al. (2008) have shown that overexpression of frataxin in Drosophila increases both life span and resistance to some oxidative stresses. Using a model expressing one copy of the same DfhIR used in this study, Anderson et al. (2005) showed that overexpression of the ROS-scavenging enzymes superoxide dismutase or catalase did not rescue failed eclosion. However, they subsequently determined that ectopic expression of catalase, but not superoxide dismutase, rescued mitochondrial aconitase activity and life span in DfhIR animals (Anderson et al., 2008). Our studies showed that DfhIR larvae do produce excessive ROS when challenged by complex III inhibition, but only late in development, at a time when loss of distal axons and cell bodies is already occurring.
We propose that the cellular neuropathology of FRDA involves the following series of events: First, long before any gross organismal phenotype is apparent, a loss of Fe-S enzymes leads to deficient activity of the ETC, which is manifested as diminished MMP. This gives rise to diverse possible downstream effects, including reduced ATP production, calcium homeostasis and mitochondrial maintenance, particularly in the distal axon. These in turn result in an abnormal distribution of distal mitochondria, inadequate synaptic function, and neuronal degeneration. An overall inhibition of retrograde retrieval or trophic factors may also contribute to neuronal death. Since low MMP is likely to produce many different downstream effects, we suggest that FRDA be approached at the molecular and cellular level as a multihit phenotype (Brookes et al., 2004). That is, several fundamental defects, in a causative chain or in parallel, exacerbated by an impaired neuronal response during periods of increased environmental and oxidative stress, give rise over time to the neurodegenerative phenotype. Finally, since it is clear that ROS are essential signaling molecules in the nervous system (Floyd, 1999; Maher and Schubert, 2000; Floyd et al., 2002), any consideration of abnormal ROS levels should recognize that their major effects may occur through the subversion of signaling pathways, in addition to nonspecific oxidative damage.
Footnotes
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This work was supported by National Institutes of Health Grant NS027073 from the National Institutes of Neurological Disorders and Stroke to P.J.H. We thank P. R. Anderson and J. P. Phillips (University of Guelph) for the generous gift of the DfhIR fly line. We thank H. C. Chang, N. Perrimon, D. Horiuchi, and A. Pilling for technical advice, W. M. Saxton for the mito-GFP fly line, and J. L. Verburg and D. M. Fekete for critical comments on this manuscript.
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This paper is dedicated to the memory of its first author, Dr. Yujiro Shidara (Jan. 9, 1972–Dec. 9, 2007).
- Correspondence should be addressed to Peter J. Hollenbeck, Department of Biological Sciences, Purdue University, 915 West State Street, West Lafayette, IN 47906. phollenb{at}purdue.edu