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A molecular chaperone for mitochondrial complex I assembly is mutated in a progressive encephalopathy
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     1Montreal Neurological Institute, McGill University, Montreal, Quebec, Canada.

    2Department of Molecular and Medical Genetics, Oregon Health & Science University, Portland, Oregon, USA.

    3Department of Human Genetics, McGill University, Montreal, Quebec, Canada.

    Abstract

    NADH:ubiquinone oxidoreductase (complex I) deficiency is a common cause of mitochondrial oxidative phosphorylation disease. It is associated with a wide range of clinical phenotypes in infants, including Leigh syndrome, cardiomyopathy, and encephalomyopathy. In at least half of patients, enzyme deficiency results from a failure to assemble the holoenzyme complex; however, the molecular chaperones required for assembly of the mammalian enzyme remain unknown. Using whole genome subtraction of yeasts with and without a complex I to generate candidate assembly factors, we identified a paralogue (B17.2L) of the B17.2 structural subunit. We found a null mutation in B17.2L in a patient with a progressive encephalopathy and showed that the associated complex I assembly defect could be completely rescued by retroviral expression of B17.2L in patient fibroblasts. An anti-B17.2L antibody did not associate with the holoenzyme complex but specifically recognized an 830-kDa subassembly in several patients with complex I assembly defects and coimmunoprecipitated a subset of complex I structural subunits from normal human heart mitochondria. These results demonstrate that B17.2L is a bona fide molecular chaperone that is essential for the assembly of complex I and for the normal function of the nervous system.

    See the related Commentary beginning on page 2689

    Introduction

    NADH:ubiquinone oxidoreductase (complex I) catalyzes the first step in the mitochondrial respiratory chain, in which transfer of electrons from NADH to ubiquinone (coenzyme Q) is accompanied by the translocation of protons across the inner mitochondrial membrane. This contributes to the proton electrochemical gradient used to synthesize ATP by complex V, the ATP synthetase. In prokaryotes, complex I is composed of a basic core of 14 structural subunits thought to have evolved from the fusion of separate modules for electron transfer and proton transport (1). Over the course of evolution, a number of so-called supernumerary subunits have been added to the complex, which now comprises 37–40 subunits in aerobic fungi and at least 46 in mammals, 7 of which are encoded in mtDNA (2-4). The complex forms an L-shaped structure, with a hydrophobic arm containing the mtDNA-encoded subunits that is embedded in the inner mitochondrial membrane and a hydrophilic peripheral arm containing the NADH binding site and redox active centers that extends into the mitochondrial matrix (5, 6).

    Disease-causing mutations have now been described in 9 of the nuclear-encoded structural subunits of complex I (NDUFS1, NDUFS2, NDUFS3, NDUFS4, NDUFS7, NDUFS8, NDUFV1, NDUFS6, and NDUFV2) (7-15). These are associated with a variety of autosomal recessive, early onset, fatal clinical phenotypes including Leigh syndrome, cardiomyopathy, and encephalomyopathy. A survey of nearly all of the genes coding for structural subunits in 1 cohort of autosomal recessive complex I patients failed to identify mutations in about 60% of the cases (16), suggesting that factors involved with assembly or maintenance of complex I are an important cause of disease; however, little is known about the regulation of these processes in mammals.

    The model organism most extensively used for the study of complex I biogenesis is the aerobic fungus Neurospora crassa. The enzyme in N. crassa assembles the matrix and membrane arms as independent modules, which are then joined together in a stepwise fashion to form the holoenzyme (17). Mutations in structural subunits that prevent assembly of one or the other arms result in the accumulation of the unaffected arm. The membrane arm is itself formed from the association of a small and a large subcomplex, and 2 assembly proteins, CIA30 and CIA84, play a role in this process by transiently associating with the large membrane arm subcomplex (18). CIA30 has a mammalian homologue, but its function in mammalian cells has not yet been demonstrated, and mutations in this gene have not been identified in patients with complex I assembly defects (19).

    It has been argued that assembly of the human complex I occurs by a mechanism similar to that in Neurospora (20); however, the presence of independent subcomplexes of the membrane and peripheral arms has not been convincingly demonstrated, while subcomplexes containing components of both arms have been identified in the skeletal muscle of some patients with complex I assembly defects (21). Additionally, mutations in structural subunits of the membrane arm (22) that prevent assembly of the holoenzyme do so without the apparent accumulation of subcomplexes.

    In this study, we sought to identify complex I assembly factors using a bioinformatics approach. We show that B17.2L, a paralogue of a gene encoding a small structural subunit in the matrix arm, serves as a complex I assembly factor and, when mutated, causes an early onset, progressive encephalopathy.

    Results

    Identification of candidate complex I assembly genes.

    The fermentative yeast Saccharomyces cerevisiae is the model organism most extensively used to study mitochondrial oxidative phosphorylation; however, it lacks a complex I, and this has hampered research on complex I biogenesis. Recently, the genomes of several other yeast species have been sequenced in their entirety, and 2 of these, Yarrowia lipolytica and Debaryomyces hansenii, are aerobic yeasts that express a complex I. We reasoned that it should be possible to find complex I assembly genes by using whole genome subtraction to identify mitochondrial proteins common to aerobic yeasts but missing in fermentative yeasts. To test this idea, we first evaluated all predicted proteins in gene families common to Y. lipolytica and D. hansenii but absent in S. cerevisiae, Kluyveromyces lactis, and Candida glabrata (1080 sequences in 472 families, classified on the Genolevures website) for mitochondrial targeting using the MITOPRED program. This produced 141 families in which 1 or more members were predicted to be mitochondrial. We then used PSI-Blast searches to identify mammalian homologues of these proteins. These were retested using MITOPRED and MitoProt II for mitochondrial targeting. This strategy would be expected to pick up the majority of nuclear-encoded complex I structural subunits, and indeed, we were able to identify 16 of the 27 predicted nuclear encoded subunits in Y. lipolytica with human homologues (2). In addition, we identified the orthologues of the only known complex I assembly factors, CIA30 and CIA84, which have been characterized in the fungus N. crassa. After exclusion of these complex I structural subunits and assembly factors, we were left with 36 gene families. Manual curation removed a further 22 families where the function of the protein was already well characterized or the targeting prediction was obviously wrong.

    Among the genes revealed by this search, 1, which we called B17.2L (for B17.2-Like), seemed like a particularly good candidate as a complex I assembly factor. B17.2L is a paralogue of B17.2, a gene that codes for a small structural subunit in the matrix arm of complex I. While not present in the nuo operon, which contains the core 14 structural subunits of complex I in prokaryotes, the B17.2 structural subunit is present in the genome of -proteobacteria (COG 3761), the direct ancestors of mitochondria. It is absent in other bacteria, including Escherichia coli.

    Alignment of the B17.2 and B17.2L predicted proteins showed that they are 17% identical and 31% similar, with no large blocks of sequence conservation (Figure 1A). The B17.2L gene appears to be an ancient duplication of the gene for the structural subunit, as it is present in all eukaryotes whose genomes have been sequenced, except those fungi that lack complex I, but it is absent in prokaryotes (4). A multiple sequence alignment of B17.2L in the vertebrates and Y. lipolytica showed a relatively high degree of sequence homology in the N terminal part of the protein and the loss of a long C terminal tail in the vertebrates (Figure 1B). Overall the yeast protein is 20% identical and 34% similar to the human protein.

    B17.2L maps to human chromosome 5q, and there is a pseudogene on human chromosome 2. It is likely to be a soluble protein, as it is not predicted to have a transmembrane domain (TMpred or TMHMM).

    Mitochondrial targeting and expression of B17.2L in human tissues.

    The B17.2L protein product is predicted to be mitochondrially targeted by MITOPRED (100%) and MitoProt II (97%). To test this, we transiently expressed a B17.2L-GFP fusion protein in HEK293 cells and compared its distribution with that of MitoTracker red, a mitochondrial marker. Superposition of the 2 images showed complete overlap of the red and green fluorescent signals (Figure 2A), confirming the mitochondrial targeting of B17.2L. Immunoblot analysis showed that B17.2L is ubiquitously expressed, although there is some variation in the steady-state level of the protein among tissues when compared to other mitochondrial markers (Figure 2B). In particular, there is less B17.2L in skeletal muscle relative to either porin or the 49-kDa complex I subunit as compared with heart, liver, or fibroblasts.

    Mutation in B17.2L in a patient with a deficiency in complex I assembly and a progressive encephalopathy.

    We initially sequenced the cDNA for B17.2L in 8 patients in whom we had previously characterized complex I assembly defects. We found an apparently homozygous C182T mutation in exon 2 of B17.2L, predicting a premature stop at amino acid 45 (R45X) in the protein in a patient with a progressive encephalopathy (Figure 3, A and B). Sequencing of exon 2 in genomic DNA showed the same apparently homozygous mutation, which was confirmed by RFLP analysis of a PCR product containing the mutated site (Figure 3C). A restriction enzyme-based analysis of a PCR product from genomic DNA encompassing exon 2 from both parents showed that the mother was heterozygous for the mutation; however, the father appeared homozygous for the wild-type sequence. This suggested to us that the patient may have inherited 2 alleles from her mother (isodisomy) or that the patient was in fact hemizygous for the mutant allele, having inherited a deleted allele from her father. Using microsatellite markers covering chromosome 5, we found that 16/18 markers were heterozygous in the patient (data not shown), making maternal isodisomy unlikely and suggesting that the father transmitted a deleted allele to his daughter and that both are hemizygous for B17.2L. Sequencing of a further 20 patients with complex I deficiency failed to identify additional mutations in B17.2L.

    Functional complementation of the complex I defect in patient fibroblasts.

    To test whether the R45X mutation was in fact the disease-causing mutation, we transduced patient fibroblasts with a retroviral vector expressing the wild-type B17.2L cDNA and looked for rescue of the complex I assembly defect by blue native PAGE (BN-PAGE) and restoration of complex I catalytic activity using an in-gel assay. In 2 independent experiments, both the amount of fully assembled complex I and its activity were restored to control levels in cells transduced with the vector expressing B17.2L (Figure 4A). The amount and activity of the complex I–III supercomplex were also restored to control levels.

    We raised an antibody against a C terminal peptide in B17.2L and used immmunoblot analysis to examine the effect of the mutation on the protein and its expression in cells transduced with B17.2L. There was no detectable immunoreactivity for the full-length protein in the patient cells, but expression of the wild-type cDNA from the retroviral vector restored it to about twice the level observed in controls (Figure 4B).

    B17.2L is an assembly protein that associates with subassembly of complex I.

    To investigate the function of B17.2L, we used BN-PAGE to analyze the composition of complex I subassemblies in muscle mitochondria from 2 siblings with a complex I assembly defect in whom we had previously identified mutations in NDUFV1, which codes for the 51-kDa complex I structural subunit (unpublished results). These patients fail to assemble normal amounts of the holoenzyme, and accumulate complex I subassemblies (Figure 5A). The first dimension BN gel showed anti-B17.2L immunoreactivity in a subcomplex of about 830 kDa in both patients (Figure 5B). No immunoreactivity was detectable in the control, or, as expected, in the B17.2L patient who is null for the B17.2L protein (Figure 5B). This result suggests that B17.2L associates with a specific subassembly of complex I but not with the mature holoenzyme. To ensure that this represented real immunoreactivity for B17.2L, we analyzed samples from 1 of the above patients and from 2 other patients with complex I assembly defects on a second-dimension denaturing gel (Figure 5C). One of the additional patients (Bo) has a mutation in NDUFS4 (18-kDa subunit, our unpublished results) and accumulates the 830-kDa subcomplex (and a supercomplex that contains this subcomplex and complex III) but does not assemble any of the mature holoenzyme (Figure 5D). The molecular defect in the other patient (F) remains unknown. Immunoreactivity for B17.2L is clearly present in the 830-kDa subcomplex from the 2 patients with the known structural subunit defects (Figure 5C). It appears as a short smear at its approximate monomeric molecular weight in the control and in patient F.

    To test the generality of these results we examined fibroblast cell lines from 2 other patients who accumulate the 830-kDa subcomplex and 2 additional patients with assembly defects who do not accumulate this subcomplex at detectable levels (Figure 6A). This analysis clearly showed B17.2L immunoreactivity associated with the 830-kDa complex (patients Be, Br, Bo, Ly, and O) but not in lower molecular weight (380 and 480 kDa) subassemblies (visible in patients F and M) (Figure 6B). B17.2L immunoreactivity was also observed in a higher molecular-weight complex of greater then 1 MDa (labeled in Figure 6A). This likely represents a supercomplex (23), in which the 830-kDa subassembly associates with complex III.

    Immunoprecipitation of a complex I subassembly with anti-B17.2L.

    To investigate which components of complex I associate with B17.2L in normal cells, we tested whether we could coimmunoprecipitate complex I subunits from normal human heart mitochondria using the anti-B17.2L antibody (Figure 7A). We tested for the presence of 9 different complex I subunits using specific antibodies and for subunits of complexes II and IV to control for nonspecific interactions. Quantitative analysis (Figure 7B) showed that the immunoprecipitate was relatively enriched for ND1 and the 49-, 75-, 18-, 51-, and 30-kDa subunits whereas GRIM19 was recovered at levels only slightly greater than COX-1, and 2 complex I subunits, B14 and the 39-kDa subunit, were not detectable in the immunoprecipitate.

    Discussion

    Several lines of evidence implicate B17.2L as a molecular chaperone that is essential for the efficient assembly of complex I. First, a complex I assembly defect in the patient with a progressive encephalopathy described here is associated with a premature stop mutation in B17.2L that results in the absence of full-length B17.2L protein. When the wild-type B17.2L cDNA is expressed in patient fibroblasts, B17.2L protein accumulates, and the biochemical defect is completely rescued. Second, B17.2L specifically associates with an 830-kDa subassembly of complex I in several patients with assembly defects, but it is not present in the mature holoenzyme. Third, an anti-B17.2L antibody specifically coimmunoprecipitates a subset of complex I structural subunits from mitochondria isolated from normal human heart. Finally, B17.2L is present in all sequenced eukaryotes that contain a complex I but absent in those that do not.

    Although the B17.2L protein does not share a high degree of sequence identity with the B17.2 structural subunit, the genes coding for both are clearly paralogues. This study and a recent phylogenetic analysis of complex I (4) indicated that B17.2L arose as an ancient duplication of the gene coding for the structural subunit in the eukaryotic lineage. Interestingly, B17.2L was also very recently identified as a mitochondrial protein of unknown function in a screen for transcriptional targets of c-myc (24). Knockdown of the protein, which the authors called mimitin (for myc-induced mitochondrial protein), by RNAi was shown to inhibit the growth of some tumor lines. In light of the data we present here, it seems likely that this effect was mediated by a decrease in the content and activity of complex I.

    We do not know exactly when B17.2L is recruited to facilitate the assembly of the nascent complex I; however, the observation that B17.2L specifically associates with a large subassembly of 830 kDa indicates that it is required until the late stages of assembly, as the holoenzyme has an estimated molecular mass of 980 kDa (25). The fact that we have not been able to detect B17.2L associated with smaller subcomplexes in cells from patients with a variety of assembly defects and the observation that it coimmunoprecipitates with components of both the matrix and membrane arms also support the idea that it plays a role in late assembly. Further, the patient who is null for B17.2L protein accumulated subassemblies of 380 and 480 kDa (subassemblies V and VI in ref. 21) but did not have detectable amounts of the 830-kDa subcomplex. The evidence from the patients with mutations in NDUFV1 (51 kDa) and NDUFS4 (18 kDa) indicates that the 830-kDa subcomplex is minimally missing these 2 subunits in both cases (our unpublished results). An approximately 800-kDa subcomplex has previously been reported in patients with NDUFS4 mutations who also fail to assemble the holoenzyme complex (26-28), and it almost certainly represents the same subcomplex we identify here. A recent paper reporting a patient with a homozygous nonsense mutation in NDUFS6 (13-kDa subunit) described the accumulation of a 750-kDa subcomplex in patient fibroblasts, but the estimated size of the subcomplex was based on a holoenzyme molecular weight of 900 kDa. This suggests that it may be the same as the 830-kDa subcomplex and that the 13-kDa subunit is also missing from this subcomplex.

    The above observations indicate that the assembly of human complex I is not likely to be as simple as the stepwise addition of the matrix arm with the membrane arm because the 830-kDa subcomplex is too large to represent either of the independent arms. Further, we clearly detected subunits from both arms of the enzyme in the 830-kDa subcomplex by immunoblot analysis and in the subcomplex immunoprecipitated with the anti-B17.2L antibody. Interestingly, 2 of the complex I subunits that did not coimmunoprecipate with B17.2L (B14 and the 39-kDa subunit) have been placed in one model of complex I (4) near the junction of the matrix and membrane arms. Thus we could speculate that B17.2L is somehow involved in stabilizing a large complex I subassembly containing elements of both arms of the enzyme, in which this junction has not fully matured. Although our previous studies (21) established that both the B14 and B39 subunits are present in the 830-kDa complex, it is possible that they are added at this stage in wild-type cells and that the subcomplex we identified in patient cells represents an intermediate that remains stalled after their addition because key structural subunits are missing in the patients.

    The complete absence of full-length B17.2L does not entirely prevent assembly of mature complex I as the BN-PAGE in gel and spectrophotometric enzyme assays showed the presence of residual enzyme activity in the patient cells and tissues. This is reminiscent of the situation in patients with loss of function SURF1 mutations (29), the vast majority of whom have no immunodetectable Surf1 protein but can nevertheless make 15–20% of holocomplex IV (30, 31). Thus these molecular chaperones may serve as facilitators to bring some of the components of the enzyme together, perhaps by stabilizing subassemblies of the complex as argued above, thereby increasing the efficiency of the process. In the case of B17.2L, there seems to be some tissue specificity in the severity of the biochemical defect. The deficiency in the patient’s skeletal muscle was rather modest (about 40% of control activity) while the defect in fibroblasts was more striking (less than 20% of control activity). Paradoxically, the expression of B17.2L was lowest in muscle compared with the other tissues we examined, including fibroblasts (Figure 2B). Again, there are some parallels with deficiencies in complex IV due to assembly gene mutations that variously affect the heart, liver, brain, or skeletal muscle depending upon the nature of the gene defect (32-34). The basis for these tissue-specific effects in ubiquitously expressed housekeeping genes remains unknown, but it seems likely to involve differential regulation of assembly to meet tissue-specific metabolic demands.

    The most common clinical phenotype associated with pediatric complex I cases is Leigh syndrome, or subacute necrotizing encephalopathy (35). This neurodegenerative disorder is associated with bilaterally symmetrical spongiform lesions, especially in the thalamus and brainstem (36). The clinical presentation of the B17.2L patient does not resemble that of Leigh syndrome patients, nor is it typical of most other patients with mitochondrial disease (though it must be said that the clinical spectrum of mitochondrial disease is extraordinarily broad). In fact, the patient shares most of the characteristic diagnostic criteria for a disease entity called leukoencephalopathy with vanishing white matter (37), which is caused by mutations in any of 5 different cytosolic translation factors (38). The fact that we have not identified other patients with B17.2L mutations may reflect the fact that this clinical phenotype has not generally been associated with mitochondrial disease.

    Patients with complex I assembly defects have been assigned to several different genetic complementation groups (ref. 15 and our unpublished results), so it is unlikely that we will find a common gene defect in these cases. The genome subtraction strategy we have used to find the B17.2L gene might be useful for finding other complex I assembly genes, but it does have its limitations. The 2 most obvious arise from inaccuracies in the in silico mitochondrial targeting prediction algorithms (about 80% accurate) and the fact that proteins that are part of large gene families with members in many yeast species would not survive the screen. It is interesting that B17.2L, the first characterized mammalian complex I assembly factor gene, is a paralogue of a structural subunit of the complex itself. None of the assembly factors that have been identified for complexes III, IV, or V have any obvious relationship with the structural subunits of these complexes. A recent analysis of the evolution of complex I (4) identified several paralogs of complex I structural genes, and these must now also be considered as candidates for complex I assembly factors.

    Methods

    Case report.

    The patient was a full-term female, born by cesarean section for breech presentation to a mother of Chinese and Portuguese heritage and a Jewish father from the Caucasus. She seemed healthy until 12–14 months of age when horizontal nystagmus and wide-based gait were noted; brain MRI was normal. At 3 years of age, she developed acute ataxia, lethargy, dehydration, and worsening nystagmus following an ear infection. She had right dysconjugate gaze, pale right optic disc, myopathic facies, decreased reflexes, and normal sensory examination. Blood lactate was normal although CSF lactate was slightly increased (4.2 mM; controls 1.4–3.9 mM). Electromyogram (EMG) and nerve conduction velocity (NCV) tests suggested a demyelination, possibly a polyradiculoneuropathy. Brain MRI (Figure 8, A and B) showed symmetric lesions in the mamillothalamic tracts, substantia nigra/medial lemniscus, medial longitudinal fasciculus, and spinothalamic tracts. Confluent areas of hyperintense signal were also seen in the corpus medullare of the cerebellum. After 3 days of steroid therapy for presumed acute disseminated encephalomyelitis, hypertrophic cardiomyopathy was detected and steroid therapy was stopped. She was then given i.v. immunoglobulins and propranolol. She improved clinically and the cardiomyopathy resolved. Pyruvate dehydrogenase deficiency was excluded by activity measurement in peripheral blood lymphocytes.

    Skeletal muscle and sural nerve biopsies were performed at Oregon Health & Science University at 44 months of age. Muscle and nerve histochemistry and muscle EM were normal. In particular, there were no ragged red fibers or cytochrome c oxidase-negative fibers. Measurement of respiratory chain activities in muscle mitochondria revealed moderate deficiency of complex I (patient, 105 nmol/min/mg protein; controls, 276 ± 84 nmol/min/mg protein). Activities of complexes II, III, IV, and II+III, ATPase, and citrate synthase were all normal. The amount and activity of complex I were less than 20% of control levels in immortalized patient fibroblasts as assessed by BN-PAGE and measurement of in-gel activity (see Figure 4). She was treated with vitamin C, coenzyme Q10, and L-carnitine. Clinically, she had normal intelligence, normal strength, hypotonia, absent deep tendon reflexes, mild ataxia, and optic atrophy. At age 6, she experienced another episode of increased lactic acidosis and worsening ataxia. She remained normal intellectually.

    At 8 years of age, increasing weakness, dysphagia, dysuria, sleep apnea, hypertension, and tachycardia developed, and she suffered respiratory failure associated with an intercurrent respiratory infection. Following these events, she required a tracheostomy for mechanical ventilation, and a gastrostomy for feeding. She remained comatose for several months. She was treated with a vitamin cocktail, coenzyme Q10, carnitine, fish oil, uridine, and creatine. Dichloroacetate was given for 3 months following the respiratory failure. From 8 years, 6 months, until her death at 13 years, 7 months, she was largely immobile, verbally noncommunicative, and had recurrent pneumonias and electrolyte imbalance. She also had muscle wasting, absent deep tendon reflexes, severe optic atrophy, severe osteoporosis, scoliosis, central precocious puberty, temperature instability, and a microcytic anemia. T4 and TSH (thyroid stimulating hormone) were elevated; blood lactate, liver function, and echocardiogram were normal. EMG and NCV tests revealed severe axonal sensorimotor polyneuropathy. Brain MRI (Figure 8, C and D) showed extensive myelomalacia, white matter encephalomalacia, cortical atrophy, and vermian atrophy. She remained ventilator- and gastrostomy-dependent but responsive to music therapy and able to vocalize to indicate discomfort or unhappiness.

    Neuropathological examination of the cerebral hemispheres revealed striking spongiform changes throughout the white matter and deep gray matter with relative sparing of the cortex. There was some preservation of U fibers in the white matter. The corpus callosum was reduced to a very thin lamina, and there was marked atrophy of the striatum and globus pallidum. The thalamus and hypothalamus were very atrophic, but the hippocampal formations were relatively spared. In the midbrain, the aqueduct of Sylvius was enlarged, and there were multicavity lesions involving the periaqueductal region that extended into the tegmentum of the pons. There was marked atrophy of the pons and medulla. There was marked atrophy of the folia throughout the vermis of the cerebellum, and the white matter of the cerebellum was severely involved in the spongiform changes. Microscopic examination of the cerebral cortex, hippocampus, and cerebellum showed extensive and bizarre degeneration of white matter, which was replaced by a glial scar. No oligodendrocytes were present.

    Informed consent was obtained from the parents of the patient, and protocols were approved by the Oregon Health & Science Institutional Review Board and the Research Ethics Board of the Montreal Neurological Hospital and Institute.

    Genome subtraction.

    Files containing the sequences of gene families found in both D. hansenii and Y. lipolytica, but not in C. glabrata or K. lactis, were downloaded from the website of the Genolevures consortium (http://cbi.labri.fr/Genolevures) (39). The web-based program MITOPRED (http://bioinformatics.albany.edu/mitopred/) (40) was then used to predict which of the gene sequences were mitochondrial. Finally PSI Blast (http://helix.nih.gov/docs/gcg/psiblast.html) was used with a Blosum 45 matrix to find human homologues (41), and a second iteration of mitochondrial prediction was done on these homologues using MITOPRED and MitoProt II (http://ihg.gsf.de/ihg/mitoprot.html) (42).

    Cell lines.

    Primary skin fibroblasts were grown from patient skin biopsy material. To immortalize the cell lines, they were transduced with retroviral vectors expressing the catalytic component of human telomerase and the type 16 human papilloma virus E7 gene (29). The fibroblasts were grown in high glucose DMEM containing 110 mg/l pyruvate and 10% fetal bovine serum.

    Sequencing of cDNA and genomic DNA.

    RNA was isolated from patient and control fibroblasts using the RNeasy Mini Kit (QIAGEN). cDNAs were generated by RT-PCR on total RNA from fibroblasts using the OneStep RT-PCR kit (QIAGEN) and specifically designed primers for the amplification of B17.2L. Exon 2 of B17.2L was amplified from genomic DNA using specific primers. PCR products were sequenced automatically using the same primers.

    B17.2L cDNA constructs.

    Retroviral vectors were created using the Gateway cloning system (Invitrogen Corp.). cDNA from B17.2L was amplified by OneStep RT-PCR (QIAGEN). Specific primers modified for cloning into Gateway vectors were used so that the PCR products could be cloned into a retroviral expression vector, pLXSH (43), modified for use with the Gateway system. The fidelity of the cDNA clones was confirmed by automated DNA sequencing.

    Virus production and transduction of patient fibroblast lines.

    The cDNA containing retroviral vectors were transiently transfected into a Phoenix amphotropic cell line (a kind gift of G.P. Nolan, Stanford University, Stanford, California, USA) using an HBS/CaPO4 method (http://www.stanford.edu/group/nolan/retroviral_ systems/retsys.html). Patient and control fibroblasts were infected 48 hours later by exposure to virus-containing medium with polybrene (4 μg/ml) as previously described (44). Cells expressing the cDNA were selected for in 100 U/ml hygromycin and then harvested for BN-PAGE or SDS-PAGE analysis.

    Preparation of human heart, muscle, liver, and fibroblast mitochondria.

    Mitochondria were prepared from 1 g of frozen control human heart tissue, 100 mg of frozen control human liver, or 5 x 15–cm cell culture plates of fibroblasts from patients and controls. The tissues or cells were homogenized (5%) in 250 mM sucrose, 10 mM Tris-HCl, and 1 mM EDTA (pH 7.4), and Complete protease inhibitors (Roche Diagnostics Corp.) were added to the homogenization buffer at the recommended concentration. To prepare mitochondria from muscle, 100 mg of frozen muscle tissue from patients or controls was homogenized in 150 mM KCl, 20 mM Tris-HCl, and 2 mM EDTA (pH 7.5). All of the above homogenates were centrifuged twice for 10 minutes at 600 g to obtain a postnuclear supernatant. Mitochondria were pelleted by centrifugation for 20 minutes at 14,000 g. Protein concentration was measured by the Micro BCA method (Pierce Biotechnology Inc.).

    BN-PAGE and immunoblot analysis.

    Mitoplasts were prepared from fibroblasts, as described previously (45), by treating the cells with 0.8 mg digitonin/mg of protein. Mitoplasts or mitochondria were solubilized with 1% lauryl maltoside, and 20–30 μg (fibroblasts) or 10–15 μg (tissues) of solubilized protein was used for electrophoresis. BN-PAGE (46) was used to separate the samples in the first dimension on 6–15% polyacrylamide gradients. An in-gel activity assay for complex I was performed as described (47). For analysis of the second dimension, strips of the first-dimension gel were incubated for 45 minutes in 1% SDS and 1% -mercaptoethanol. These strips were then run on a 10% tricine/SDS-PAGE to separate the proteins in the second dimension (46). Subunits of complexes I, II, and IV were detected by Western blot analysis of the above gels using monoclonal and polyclonal antibodies. The following antibodies were purchased from Invitrogen Corp.: complex I, anti-B14 (NDUFA6) subunit, complex II, anti-SD70 (70 kDa) subunit, and complex IV, anti–COX-1. Anti-GRIM19 was purchased from MitoSciences. Other antibodies against complex I subunits were kindly provided as follows: J. Walker (MRC Dunn Human Nutrition Unit, Cambridge, United Kingdom), anti–75-kDa (NDUFS1) and anti–51-kDa (NDUFV1) subunits; B. Robinson (Hospital for Sick Children, Toronto, Ontario, Canada), anti–49-kDa (NDUFS2) subunit; R. Capaldi (University of Oregon, Eugene, Oregon, USA), anti–39-kDa (NDUFA9) subunit; A. Lombes (INSERM U582, Universite Pierre et Marie Curie, Paris, France), anti-ND1; and V. Petruzzella (University of Bari, Bari, Italy), anti–18-kDa (NDUFS4) subunit.

    SDS-PAGE analysis.

    Whole cell extracts were prepared from fibroblasts by solubilization for 30 minutes at 4°C with 1 mg TritonX-100/mg protein. The insoluble cell debris was removed by centrifugation at 750 g for 5 minutes at 4°C. Solubilized protein (10–20 μg) was loaded onto a 10% glycine/SDS-PAGE gel in Laemmli sample buffer. Isolated mitochondria from cells and tissues were solubilized in Laemmli sample buffer prior to loading. Subsequent immunoblotting was done with some of the antibodies described above.

    Anti-B17.2L antibody.

    An antibody against B17.2L was generated by injecting rabbits with a synthetic peptide specific to human B17.2L (CSAPYFGKEEPS), conjugated to keyhole limpet hemocyanin via a reactive sulfhydryl group, and emulsified in Titermax (Pierce Biotechnology Inc.). Testing of the specificity of the B17.2L antisera revealed that affinity purification was not required for immunoblotting, and crude serum was used.

    Immunoprecipitation of B17.2L protein from human heart and human fibroblasts.

    Anti-B17.2L antibody was affinity purified using the SulfoLink kit (Pierce Biotechnology Inc.). Purified antibody (70 μg) was then bound to 20 mg of protein A sepharose 4B fastflow (Sigma-Aldrich) overnight at 4°C. The antibody was cross-linked to the protein A sepharose with 25 mM dimethylpinelimidate in 0.2 M sodium borate, pH 9.0 (30 minutes at room temperature). Cross-linking was terminated with 0.2 M ethanolamine, pH 8.0 (3 hours at room temperature). The beads were equilibrated in 20 mM Tris HCl, pH 7.5, and 1 mM EDTA. Human heart mitochondria (1 mg) were resuspended (10 mg/ml protein) in 20 mM Tris- HCl, pH 7.5, and 1 mM EDTA with Complete protease inhibitors (Roche Diagnostics Corp.). An equal volume of 2% dodecylmaltoside (DDM) in 20 mM Tris HCl, pH 7.5, and 1 mM EDTA was added, and the mitochondria were solubilized for 30 minutes at 4°C. Insoluble material was pelleted by centrifugation at 185,000 g. The supernatant was precleared against naked protein A sepharose beads for 1 hour at room temperature, then incubated with B17.2L protein A sepharose overnight at 4°C. After washing with PBS, pH 8.0, with 0.05% DDM, bound protein was eluted from the beads with 0.1 M glycine, pH 2.5, and 0.05% DDM. Eluent concentration and buffer exchange (PBS, pH 8.0, 0.05% DDM) was done using a Microcon YM-10 (Millipore).

    Acknowledgments

    We are most grateful to the family for their participation in this study. We thank the many physicians who contributed to the care of this patient, particularly Susan Winter, Neil R.M. Buist, Gamal Boutros, Dorit Bar-Din, Rowena Korobkin, Sakkubai Naidu, Andrea Gropman, and Raymond Coleman; we also thank Douglas Kerr for measurement of pyruvate dehydrogenase activity, Beth Lee for measurement of respiratory chain activities, Gregory Ward for help with software for the genome subtraction, and Mary G. Ripple for interpretation of the neuropathology. We also thank Ariel Abramov for her invaluable contributions to this study. This study was supported by a grant from the March of Dimes Birth Defects Association to E.A. Shoubridge. E.A. Shoubridge is a senior scientist of the Canadian Institutes of Health Research and an international scholar of the Howard Hughes Medical Institute.

    Footnotes

    Nonstandard abbreviations used: BN-PAGE, blue native PAGE; complex I, NADH:ubiquinone oxidoreductase; DDM, dodecylmaltoside; EMG, electromyogram; NCV, nerve conduction velocity.

    Conflict of interest: The authors have declared that no conflict of interest exists.

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