1. Introduction
Mitochondrial diseases (mtD) in people are a heterogeneous group of genetically, biochemically, and clinically diverse disorders caused by defects in the metabolic pathways of oxidation phosphorylation (OXPHOS) and ATP production [1,2]. Both the nuclear and mitochondrial genomes encode components of the enzyme complexes of the OXPHOS system, resulting in the genetic bases of mtD being transmitted in a Mendelian fashion, maternally, or as sporadic diseases. The pathogenicity is further complicated by heteroplasmy, in which several different mitochondrial genomes exist within a given cell [3]. A major challenge in the diagnosis of mtD is the clinical heterogeneity of these disorders, with most patients having a multi-system disease with three or more organs affected, characteristically affecting tissues with high energy demands such as the central nervous system, skeletal muscle, eye and heart [4]. Novel clinical syndromes have been reported in association with mitochondrial dysfunction and many patients can be misdiagnosed. The advent of next-generation sequencing has resulted in the discovery of new pathogenetic variants and has become the standard for the diagnosis of mtDs [5].
Mitochondrial diseases can arise from mutations in both nuclear and mitochondrial genomes as most proteins involved in mitochondrial metabolism, and all those involved in mtDNA maintenance, are encoded in the nuclear DNA (nDNA) [6,7,8]. Mutations in more than 350 genes, both nuclear and mitochondrial, are currently known to cause primary mitochondrial disorders in people [5]. Those disorders caused by a large-scale mutation in the mtDNA include Kearns–Sayre syndrome [9,10], chronic progressive external ophthalmoplegia (CPEO) [9,11], myopathy, encephalopathy, lactic acidosis and stroke-like episodes (MELAS) [12,13,14], and myoclonic episodes with ragged-red fibers (MERRF) [15], among others. Cases with multiple mtDNA deletions (i.e., deletions of various sizes in the mtDNA) are usually associated with a nuclear gene defect involved in mtDNA maintenance which can provide guidance for analysis of variants detected by next-generation sequencing [3].
In dogs, variants in both nuclear and mitochondrial DNA have also been associated with four forms of encephalopathies and five forms of myopathies in various breeds. Encephalopathies include two different SLC19A3 gene variants associated with subacute necrotizing encephalopathy or Leigh syndrome (OMIA#001097-9615), one in Alaskan Huskies [16] and the other in Yorkshire terriers [17]; a cytochrome b variant (OMIA#002684-9615) causing canine spongiform leukoencephalomyelopathy in Australian blue heelers and Shetland sheepdogs [18]; and a NDUFS7 variant (OMIA#002840-9615) in a Jack Russell–Chihuahua mixed-breed dog, the most common gene associated with Leigh syndrome in people [19]. Nuclear gene variants associated with canine mitochondrial myopathies include a mutation in the PDP1 gene (OMIA#001406-9615), encoding the phosphatase enzyme that activates the pyruvate dehydrogenase complex, in Clumber and Sussex spaniels [20]; a variant in the mitochondrial aspartate/glutamate carrier gene SLC25A12 (OMIA#002294-9615) that causes an inflammatory myopathy in Dutch shepherd dogs [21]; and a variant in the ACADVL gene (OMIA# 002140-9615) encoding the very-long-chain acryl-CoA dehydrogenase associated with exercise-induced myopathy in German Hunting terriers [22]. A mitochondrial myopathy in Old English Sheepdogs associated with reduced mitochondrial mRNA and decreased cytochrome c oxidase activities in fibroblasts and skeletal muscle has been reported although a specific gene variant has not been identified [23]. Several other case reports have described mitochondrial myopathies in dogs based on histopathological and morphological changes, and biochemical activities, but these have also not yet been subjected to genetic evaluation [24]. A sensory ataxic neuropathy associated with a deletion in the mitochondrial tRNATyr gene has been described in golden retriever dogs [25], and cardiomyopathy and arrhythmia have been described in a family of Rhodesian ridgeback dogs with a missense variant in the nuclear gene QIl1 (also called MICOS13; OMIA# 001040-9615) [26]. To the author’s knowledge, mitochondrial deletion diseases are rare in canine encephalopathies and not yet reported in canine myopathies.
Here, we describe an adult standard poodle with chronic weakness and exercise intolerance, diagnose a mitochondrial myopathy based on light and electron microscopy of muscle biopsies, and identify multiple deletions in its mtDNA via whole-genome sequencing (WGS) of DNA extracted from muscle biopsies. Insertion of a DYNLT1 retrogene into the nuclear genome, and downstream alteration of expression of the mitochondrial voltage-dependent anion channel (VDAC), is suspected of being the underlying cause. While not typically evaluated in WGS analyses, this study demonstrates that the evaluation of mtDNA sequences obtained from WGS data can be highly useful in the diagnosis of mitochondrial myopathy.
2. Materials and Methods
2.1. Clinical Case
An approximately 7-year-old male neutered rescue standard poodle was presented to a board-certified veterinary neurologist at the VCA Animal Care Center of Sonoma County in Rohnert Park, California, USA for evaluation of a 2–3-year history of progressive weakness and exercise intolerance. A neuromuscular disease was suspected and further evaluations including electromyography and muscle biopsies were performed. All studies were performed for diagnostic purposes and with the owner’s consent.
2.2. Histopathology, Histochemistry, Immunohistochemistry and Electron Microscopy
Unfixed chilled and formalin-fixed diagnostic muscle and peripheral nerve biopsies were collected from the cranial tibial and triceps muscles, and the common peroneal nerve under general inhalational anesthesia. All biopsies were shipped by an express service under refrigeration to the Comparative Neuromuscular Laboratory, University of California San Diego. Upon receipt, the unfixed muscle biopsies were snap-frozen in isopentane pre-cooled in liquid nitrogen and stored at −80 °C until further processed. Cryosections were evaluated using a standard panel of histochemical stains and reactions including the mitochondrial-specific reactions succinic dehydrogenase (SDH) and cytochrome c oxidase (COX) [27]. Immunofluorescence staining using a monoclonal antibody against mitochondrial voltage-dependent anion channels (1:100, VDAC, Abcam, Boston, MA, USA) was used on case and control cryosections and co-stained with a polyclonal rabbit anti-laminin antibody (1:100, Abcam, Boston, MA; ab11575). Secondary antibodies were goat anti-mouse or goat-anti-rabbit FITC-labeled antibodies from Jackson Immunoresearch, Westgrove, PA, USA. The fixed nerve biopsy was araldite embedded and evaluated in 1 µm resin sections. Formalin-fixed muscle was processed into paraffin by standard procedures, further post-fixed in osmium tetroxide, and dehydrated in serial alcohol solutions and propylene oxide prior to embedding in araldite resin. Sections (1 μm) were stained with toluidine blue for light microscopy and ultrathin sections were stained with uranyl acetate and lead citrate for electron microscopy.
2.3. Whole Genome Sequencing and Variant Analysis
DNA was isolated from archived frozen diagnostic muscle biopsy specimens using the Qiagen DNEasy kit according to package instructions. A PCR-free library was prepared from this case and 150 bp paired-end reads were generated on an Illumina HiSeq 4000 sequencer by Azenta Life Sciences (South Plainfield, NJ 07080, USA). For this case, 1.2 billion paired-end reads were generated, corresponding to a mean 70.9-fold genome-wide coverage. Reads were mapped against the dog reference genome assembly (UU Cfam GSD_1.0/canFam4) [28,29] and processed using the OnlyWAG pipeline as described [30]. Raw sequence reads are available in NCBI’s Short Read Archive (submitted on 28 March 2024; SRR28501896) (
WGS variants from this case were compared to those of control genomes from an internal WGS database developed at the University of Minnesota which contained a total of 671 dogs of 63 diverse breeds including 38 standard poodles. The WGS data from these 671 dogs were processed using the same bioinformatics pipelines referenced above. Variants unique to the affected dog that were within or in close proximity to coding exons were prioritized as high (frame shift, loss or gain of stop or start codon, affecting a splice junction), moderate (missense), or low (synonymous, near splice junction) for further evaluation. A list of the unique coding variants is provided in Table S1. Visual inspection of the entire length of the mtDNA was performed within the integrative genomics viewer (IGV) and compared to a control archived frozen muscle biopsy specimen. Additionally, visual inspection for the presence of the DYNLT1 retrogene and mtDNA deletions was performed within IGV and compared to an internal collection of 38 standard poodle WGSs. Analysis of retrogene sequence for the presence of promoter and regulatory sites was performed with Promoter 2.0 [31] and TSSG Promoter prediction [32].
3. Results
3.1. Clinical Case
A neurological examination showed difficulty rising and a stiff, slow gait, worse in the pelvic limbs without ataxia. The dog could only walk 60–80 feet before becoming progressively stiffer and lying down. Cranial nerve examination and postural reactions were normal. Patellar reflexes were absent bilaterally and withdrawal reflexes were reduced in strength in all four limbs. No apparent discomfort was elicited with vertebral column palpation. A neuromuscular disease was suspected and a chronic myopathy was considered most likely. Prior spinal pain could not be ruled out based on the history. The dog was re-evaluated shortly after the initial exam due to becoming acutely unable to stand after a second trip to the groomer. At that time, the dog could only walk about five steps before sitting down and remained weaker in the pelvic limbs; the exam was otherwise unchanged.
Prior to presentation, creatine kinase (CK) activity was elevated (16,585 U/L; reference range 10–200). A recheck of CK activity one week later was 205 U/L and serial CK evaluations remained normal at 305 U/L and 605 U/L, with the latter performed following the trip to the groomer when the dog’s condition had acutely declined. Additional diagnostic testing included vertebral column radiographs showing mild L7-S1 ventral spondylosis, unremarkable routine laboratory evaluations including a CBC and biochemistry panel, normal total T4 (1.9 ug/dL, reference range 1–4), negative Toxoplasma serum titers for IgG/IgM, Neospora serology, and Leptospirosis PCR, negative tick serology panel with Lyme Quant C6, negative Rocky Mountain Spotted Fever serology, unremarkable abdominal ultrasound and thoracic radiographs with no obvious megaesophagus. The acetylcholine receptor antibody titer was 0.12 nmol/L (reference range < 0.6 nmol/L).
Lumbar MRI showed mild to moderate L7-S1 intervertebral disc herniation and mild contrast enhancement of the caudal L7 endplate consistent with discospondylitis. Lumbar cerebrospinal fluid analysis revealed protein cytologic dissociation (nucleated cell count 2/uL, protein 67.2 mg/dL) and cytology showed a mild increase in the proportion of neutrophils, consistent with possible mild inflammation. Electromyography (EMG) demonstrated prolonged insertional activity in all muscles evaluated and frequent positive sharp waves and fibrillation potentials in the gastrocnemius, quadriceps, triceps, supraspinatus, infraspinatus and cervical paraspinal muscle groups. Biopsies of the peroneal nerve, cranial tibial muscle and triceps muscle were collected in a standard manner under general inhalational anesthesia [33] and submitted to the UCSD Comparative Neuromuscular Laboratory. Pending biopsy results, the dog was treated with oral amoxicillin clavulanate at 16.6 mg/kg PO q12h for suspected discospondylitis. Tramadol was continued at 4 mg/kg PO q8-12 h for pain and meloxicam was discontinued. The dog showed slight improvement and seemed more comfortable. Prednisone was initiated at 0.8 mg/kg/day 1 week later with no notable improvement and was subsequently tapered without clinical decline.
Following receipt of the biopsy results and a diagnosis of mitochondrial myopathy, the dog was again examined approximately 2- weeks later and showed slightly less stiffness in the pelvic limbs, improved ability to rise from recumbency, no signs of discomfort and mild improvement in walking strength, although the dog still tired quickly. Additional diagnostics included resting and post exercise (defined as walking as far as it could and then laying down) serum lactate concentrations which were 8.65 mmol/L and 9.56 mmol/L, respectively (reference range 0.4–2.8). As mitochondrial myopathy was suspected, supplementation with L-carnitine 50 mg/kg PO q12h, Coenzyme Q10 q24h, and vitamin B12 (Cobalequin) q24h was initiated.
At the time of manuscript preparation, approximately 4 months after the initial examination, the dog remains on amoxicillin/clavulanate and the supplements. No signs of discomfort were reported by the owners at home (moaning, kyphosis). Strength is static; the dog is able to walk around the house and outside to urinate and defecate but spends a lot of time lying down and remains reluctant to jump out of the car.
3.2. Light and Electron Microscopy
A moderate variability in myofiber size was present in cryosections of the triceps muscle with the H&E stain and several myofibers contained internal dark blue deposits with the SDH mitochondrial-specific reaction. Approximately 36% of the myofibers were COX-negative and stained blue with the combined COX/SDH reaction (Figure 1). Similar changes were present in cryosections from the cranial tibial muscle biopsy (not shown). Ultra-structurally, abnormal mitochondria containing concentrically arrayed tubular cristae and crystalloid inclusions were identified (Figure 2). No abnormalities were identified in the nerve biopsy.
3.3. Whole Genome, Mitochondrial DNA Sequencing, and Variant Analysis
Genomic DNA extracted from the triceps muscle of the case was submitted for WGS where excellent coverage of both the nDNA and mtDNA was obtained (70.9 fold genome-wide coverage; mtDNA read depth > 18,000). Visual analysis of the mtDNA sequence reads from the case compared to a control French bulldog whose DNA was also derived from skeletal muscle identified numerous deletions that varied in size and were concentrated from approximately chrM:1000–11,000 (Figure 3A) resulting in the full or partial deletion of up to eight mitochondrial genes. Resorting the data alignments according to insert size demonstrated that approximately 25–30% of the mitochondrial genome reads were indicative of a large-scale deletion (Figure 3B).
The phenomenon of multiple mtDNA deletions is often associated with mutations in nuclear-encoded genes involved with mitochondrial maintenance [3]. Analysis of the WGS from the case identified several variants that meet the prioritization criteria for high impact on the encoded gene and were unique to the case (Table S1). All 17 high-impact variants were visually inspected within IGV, and 14 were found to be mapping errors. The three remaining variants included a heterozygous stop codon in TRANK1, a heterozygous stop gain point mutation in POLR2B, and a retrogene intergenic copy in DYNLT1 (which was identified as a splice site variant in the VCF due to the cDNA copy). After further investigation, the TRANK1 gene appeared to have no clear mitochondrial connection. The POLR2B gene encodes an RNA polymerase II subunit B component of the cytoplasmic transcriptional machinery that produces both cytoplasmic and most mitochondrial proteins. This stop gained variant results in the truncation of greater than 50% of the POLR2B protein. However, there is no evidence that any other aspect of cellular structure or function is altered as would be expected if the transcriptional apparatus was diminished.
The third variant is a heterozygous intergenic retrogene insertion (chr8: 54,073,620; Figure 4A–C) of DYNLT1, a regulator of the voltage-dependent anion channel (VDAC), that plays an important role in mitochondrial function. This retrogene is derived from the insertion of processed DYNLT1 cDNA from the parent DYNLT1 gene on chromosome 1 and is indicated by WGS read mate pairs in the case aligning to both chromosomes 1 and 8. Detailed analysis of the DYNLT1 retrogenic sequence identified the target-site duplication (TSD) sequences necessary for insertion, as well as sequences enabling the potential for serving as a template for transcription and expression, including a TATA box, promoter, and CpG island (Figure 5).
3.4. Immunohistochemical Staining
We considered it possible that the retrogenic insertion of a DYNLT1 cDNA in the case could potentially be transcribed and in turn alter the level of expression of this regulator of the mitochondrial voltage-dependent anion channel (VDAC, porin). To test this hypothesis immunostaining of case and control muscle cryosections was performed using a monoclonal VDAC antibody (anti-VDAC1, 1:100, ab14734, Abcam). Compared to the control muscle, the staining of muscle from the clinical case was increased (Figure 6).
4. Discussion
Mitochondria are present in all nucleated cell types; thus, mitochondrial diseases can affect any organ or tissue in the body. Clinical presentation may be as an organ-specific disease, such as myopathy, cardiomyopathy, or optic neuropathy, or a systemic disease. Mitochondrial myopathies are an important group of progressive muscle diseases, caused primarily by the impairment of oxidative phosphorylation (OXPHOS). In fact, myopathy is one of the most common manifestations of adult-onset mtD due to the high cellular energy demand of skeletal muscle [3]. Here, we describe an adult dog with clinical signs of chronic exercise intolerance and resting and post-exercise lactic acidemia without evidence of behavioral changes or cardiomyopathy. It is difficult to reach a diagnosis of a specific myopathy based on clinical presentation alone as many congenital myopathies in dogs can present with signs of exercise intolerance, weakness, stiffness and gait abnormalities [34]. The diagnosis of mitochondrial myopathies therefore should include a multidisciplinary approach including histological, immunohistochemical assays, electron microscopic studies, enzymatic analysis of OXPHOS complexes, and genetic analysis using WGS.
Histological examination of skeletal muscle biopsies by a neuromuscular pathologist using specific histologic and histochemical stains and reactions is important for ruling out other congenital, dystrophic and acquired myopathies and obtaining a correct diagnosis. Staining of muscle cryosections with the modified Gomori trichrome stain can identify the presence of ragged-red fibers. Ragged-blue fibers can be detected using the SDH reaction (SDH, complex II). Both reactions detect mitochondrial aggregates in the subsarcolemmal region of the muscle fiber due to mitochondrial proliferation that occurs with mitochondrial OXPHOS dysfunction [27]. Another important diagnostic finding is the presence of cytochrome c oxidase (COX, complex IV) negative fibers detected by sequential COX/SDH histochemistry (Figure 1). A mosaic pattern is commonly observed with COX-negative fibers appearing blue, while the normal COX-positive fibers appear brown. The mosaic pattern is due to different levels of heteroplasmy with a high mutation load leading to respiratory chain deficiency. As aging individuals can accumulate a low frequency of COX-negative fibers, a diagnosis of mitochondrial myopathy is only made when individuals harbor COX-negative fibers at a frequency of >5% [35,36]. In our case, 36% of muscle fibers were COX-negative supporting a clear diagnosis of mitochondrial myopathy. Ultrastructural evaluation of muscle confirmed the presence of abnormal appearing mitochondria and paracrystalline inclusions. The determination of serum lactate concentrations at rest and following exercise with documentation of lactic acidemia has also become a diagnostic tool for mitochondrial myopathy [37].
WGS was performed to analyze both the nuclear and mitochondrial DNA genomes for the presence of candidate functional variants consistent with the diagnosis of mitochondrial myopathy. In addition to the identification of potentially causative variants in nuclear genes, WGS also allows the detection of alterations in the mitochondrial genome including low levels of heteroplasmy, point mutations, and breakpoints of single, large-scale and multiple mtDNA deletions [3]. This enabled the identification of multiple mtDNA deletions in this clinical case compared to a control genome (Figure 3A,B). The presence of multiple mtDNA deletions in muscle is often a hallmark of mitochondrial myopathy, particularly those caused by mutations in nuclear genes encoding proteins required for mtDNA homeostasis, replication and maintenance such as POLG, POLG2 and TWNK, the mitochondrial polymerase and helicase [38]. No unique coding or structural POLG or TWNK variants were identified in our case. Three other variants were considered to have a high negative impact using protein predictors and were not identified in a large canine control population in the University of Minnesota database including 38 standard poodles. These included a heterozygous stop codon in TRANK1, a heterozygous stop gain point mutation in POLR2B, and a retrogene intergenic copy in DYNLT1. After further investigation, the TRANK1 gene appeared to have no clear mitochondrial connection. Although POLR2B is an RNA polymerase II, alterations in RNA translational proteins are thought to result in decreased quantities of cellular mRNA and protein expression but do not affect mtDNA replication or repair. POLR2B is also not reported in OMIM (180661,
While not thought to be relevant to mtDNA maintenance or repair, the DYNLT1 gene encodes an important regulator of the voltage-dependent anion channel VDAC, a gated porin that permits the transport of peptides, metabolites and ions [39,40,41,42]. We considered the hypothesis that an alteration in DYNLT1, with subsequent effects on increasing VDAC expression, could be an important event underlying the pathogenesis of this mtD. VDAC plays an important role in mitochondrial processes such as signaling, apoptosis, and calcium homeostasis and all three isoforms reported in humans are present at high levels in the heart, kidney, skeletal muscle and brain [43]. VDACs form pores in the outer mitochondrial membrane capable of metabolite transport. The gating of VDAC includes open, closed, multimeric, and blockage of the pore by specific proteins and metabolites. When these interactions are disrupted, they lead to disease states including Fredreich’s ataxia and Parkinson’s disease [44]. VDAC channels are permeable to calcium from the cytosol and an increase in flux of calcium into the mitochondria is known to lead to apoptosis [44].
Increased VDAC expression in the case was demonstrated by immunostaining of muscle cryosections. This is consistent with a DYNLT1-mediated process and could potentially be a result of overexpression or atypical of DYNLT1 through the retrogene insertion of its cDNA into a transcriptionally active form. Although we have no direct evidence to show that the DYNLT1 retrogene is expressed, its cDNA sequence is identical to that derived from the nuclear gene, so if transcribed it could presumably be translated into a functional protein. Work by others suggests such retrogenes can be active by borrowing contextual regulatory elements such as upstream promoter sequences, or enhanced by a CpG island, to promote expression of the retrogene with control provided by the 3” UTR [45]. In addition to the lack of additional frozen tissue to assess DYNLT1 gene expression, other limitations to this study include the absence of DNA from parents of the case or other family members as the dog was obtained as a rescue. Thus, we are unable to tell if this was an inherited condition or a spontaneous mutation.
5. Conclusions
A mitochondrial myopathy based on a histological and histochemical phenotype was determined to be the cause of exercise intolerance and lactic acidemia in our adult dog. WGS established the presence of multiple mtDNA deletions suggesting an underlying nuclear DNA variant affecting mitochondrial replication, repair or metabolism. The significance of the DYNLT1 retrogene as a functional candidate is not entirely clear but presents an intriguing possibility through its links to the VDAC and overall mitochondrial function. Although beyond the scope of this case report, functional studies in cell lines (fibroblast culture) to investigate protein and RNA analyses, protein transport and import, and transcription and mtDNA maintenance, and model systems (yeast, drosophila, zebrafish or mouse) are necessary to prove causality.
Conceptualization, G.D.S.; methodology, G.D.S., L.T.G., S.G.F., J.N.C. and K.M.M. software, S.G.F. and J.N.C.; validation, S.G.F., J.N.C. and K.M.M.; formal analysis, G.D.S., S.G.F., K.M.M., L.T.G. and J.N.C.; clinical investigation, J.M.M.; resources, G.D.S. and S.G.F.; data curation, S.G.F., J.N.C. and K.M.M.; writing—original draft preparation, G.D.S.; writing—review and editing, G.D.S., J.R.M. and K.M.M.; visualization, G.D.S. All authors have read and agreed to the published version of the manuscript.
Owner approval for all clinical diagnostic evaluations was obtained (JMM). IACUC approval was not required for evaluating diagnostic tissue specimens. Muscle or venous blood samples for DNA isolation from dogs were obtained under the University of Minnesota IACUC protocol 1903–36865A.
No human participants were involved in this study. The dog in the case described was evaluated in a specialty clinical practice and informed consent was provided by the owner to the clinician (JMM) for the diagnostic studies performed.
Raw sequence reads are available in NCBI’s Short Read Archive (SRR28501896) under BioProject PRJNA937381. Permanent link provided following publication.
The authors thank Richard Haas and Robert Naviaux for helpful discussions of mitochondrial diseases.
The authors declare no conflicts of interest.
Footnotes
Disclaimer/Publisher’s Note: The statements, opinions and data contained in all publications are solely those of the individual author(s) and contributor(s) and not of MDPI and/or the editor(s). MDPI and/or the editor(s) disclaim responsibility for any injury to people or property resulting from any ideas, methods, instructions or products referred to in the content.
Supplementary Materials
The following supporting information can be downloaded at:
References
1. Taylor, R.W.; Turnbull, D.M. Mitochondrial DNA mutations in human disease. Nat. Rev. Genet.; 2005; 6, pp. 389-402. [DOI: https://dx.doi.org/10.1038/nrg1606] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/15861210]
2. DiMauro, S.; Schon, E.A.; Carelli, V.; Hirano, M. The clinical maze of mitochondrial neurology. Nat. Rev. Neurol.; 2013; 9, pp. 429-444. [DOI: https://dx.doi.org/10.1038/nrneurol.2013.126] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/23835535]
3. Ahmed, S.T.; Craven, L.; Russell, O.M.; Turnbull, D.M.; Vincent, A.E. Diagnosis and treatment of mitochondrial myopathies. Neurotherapeutics; 2018; 15, pp. 943-953. [DOI: https://dx.doi.org/10.1007/s13311-018-00674-4] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/30406383]
4. Parikh, S.; Goldstein, A.; Karaa, A.; Koenig, M.K.; Anselm, I.; Brunel-Guitton, C.; Christodoulou, J.; Cohen, B.H.; Dimmock, D.; Enns, G.M. et al. Patient care standards for primary mitochondrial disease: A consensus statement from the Mitochondrial Medicine Society. Genet. Med.; 2017; 19, 107. [DOI: https://dx.doi.org/10.1038/gim.2017.107] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/28749475]
5. Emmanuele, V.; Ganesh, J.; Vladutiu, G.; Haas, R.; Kerr, D.; Saneto, R.P.; Cohen, B.H.; Van Hove, J.L.K.; Scaglia, F.; Hoppel, C. et al. North American Mitochondrial Disease Consortium (NAMDC). Time to harmonize mitochondrial syndrome nomenclature and classification: A consensus from the North American Mitochondrial Disease Consortium (NAMDC). Mol. Genet. Metab.; 2022; 136, pp. 125-131. [DOI: https://dx.doi.org/10.1016/j.ymgme.2022.05.001] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/35606253]
6. Shoubridge, E.A. Nuclear genetic defects of oxidative phosphorylation. Hum. Mol. Genet.; 2001; 10, pp. 2277-2284. [DOI: https://dx.doi.org/10.1093/hmg/10.20.2277] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/11673411]
7. DiMauro, S.; Schon, E.A. Mitochondrial respiratory-chain diseases. N. Engl. J. Med.; 2003; 348, pp. 2656-2668. [DOI: https://dx.doi.org/10.1056/NEJMra022567] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/12826641]
8. Zeviani, M.; Di Donato, S. Mitochondrial disorders. Brain; 2004; 127, pp. 2153-2172. [DOI: https://dx.doi.org/10.1093/brain/awh259] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/15358637]
9. Holt, I.J.; Harding, A.E.; Morgan-Hughes, J.A. Deletions of muscle mitochondrial DNA in patients with mitochondrial myopathies. Nature; 1988; 331, pp. 717-719. [DOI: https://dx.doi.org/10.1038/331717a0]
10. Zeviani, M.; Moraes, C.T.; DiMauro, S.; Nakase, H.; Bonilla, E.; Schon, E.A.; Rowland, L.P. Deletions of mitochondrial DNA in Kearns-Sayre syndrome. Neurology; 1988; 38, pp. 1339-1346. [DOI: https://dx.doi.org/10.1212/WNL.38.8.1339]
11. Moraes, C.T.; DiMauro, S.; Zeviani, M.; Lombes, A.; Shanske, S.; Miranda, A.F.; Nakase, H.; Bonilla, E.; Werneck, L.C.; Servidei, S. et al. Mitochondrial DNA deletions in progressive external ophthalmoplegia and Kearns-Sayre syndrome. N. Engl. J. Med.; 1989; 320, pp. 1293-1299. [DOI: https://dx.doi.org/10.1056/NEJM198905183202001] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/2541333]
12. Goto, Y.; Nonaka, I.; Horai, S. A mutation in the tRNA(Leu)(UUR) gene associated with the MELAS subgroup of mitochondrial encephalomyopathies. Nature; 1990; 348, pp. 651-653. [DOI: https://dx.doi.org/10.1038/348651a0] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/2102678]
13. Santorelli, F.M.; Tanji, K.; Kulikova, R.; Shanske, S.; Vilarinho, L.; Hays, A.P.; DiMauro, S. Identification of a novel mutation in the mtDNA ND5 gene associated with MELAS. Biochem. Biophys. Res. Commun.; 1997; 238, pp. 326-328. [DOI: https://dx.doi.org/10.1006/bbrc.1997.7167]
14. Kirby, D.M.; McFarland, R.; Ohtake, A.; Dunning, C.; Ryan, M.T.; Wilson, C.; Ketteridge, D.; Turnbull, D.M.; Thorburn, D.R.; Taylor, R.W. Mutations of the mitochondrial ND1 gene as a cause of MELAS. J. Med. Genet.; 2004; 41, pp. 784-789. [DOI: https://dx.doi.org/10.1136/jmg.2004.020537]
15. Shoffner, J.M.; Lott, M.T.; Lezza, A.M.; Seibel, P.; Ballinger, S.W.; Wallace, D.C. Myoclonic epilepsy and ragged-red fiber disease (MERRF) is associated with a mitochondrial DNA tRNA(Lys) mutation. Cell; 1990; 61, pp. 931-937. [DOI: https://dx.doi.org/10.1016/0092-8674(90)90059-N] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/2112427]
16. Vernau, K.M.; Runstadler, J.A.; Brown, E.A.; Cameron, J.M.; Huson, H.J.; Higgins, R.J.; Ackerley, C.; Sturges, B.K.; Dickinson, P.J.; Puschner, B. et al. Genome-wide association analysis identifies a mutation in the thiamine transporter 2 (SLC19A3) gene associated with Alaskan Husky encephalopathy. PLoS ONE; 2013; 8, e57195. [DOI: https://dx.doi.org/10.1371/journal.pone.0057195]
17. Drögemüller, M.; Letko, A.; Matiasek, K.; Jagannathan, V.; Corlazzoli, D.; Rosati, M.; Jurina, K.; Medl, S.; Gödde, T.; Rupp, S. et al. SLC19A3 Loss-of-Function Variant in Yorkshire Terriers with Leigh-Like Subacute Necrotizing Encephalopathy. Genes; 2020; 11, 1215. [DOI: https://dx.doi.org/10.3390/genes11101215]
18. Li, F.Y.; Cuddon, P.A.; Song, J.; Wood, S.L.; Patterson, J.S.; Shelton, G.D.; Duncan, I.D. Canine spongiform leukoencephalomyelopathy is associated with a missense mutation in cytochrome b. Neurobiol. Dis.; 2006; 21, pp. 35-42. [DOI: https://dx.doi.org/10.1016/j.nbd.2005.06.009]
19. Christen, M.; Gregor, A.; Gutierrez-Quintana, R.; Bongers, J.; Rupp, A.; Penderis, J.; Shelton, G.D.; Jagannathan, V.; Zweier, C.; Leeb, T. NDUFS7 variant in dogs with Leigh syndrome and its functional validation in a Drosophila melanogaster model. Sci. Rep.; 2024; 14, 2975. [DOI: https://dx.doi.org/10.1038/s41598-024-53314-7]
20. Cameron, J.M.; Maj, M.C.; Levandovskiy, V.; MacKay, N.; Shelton, G.D.; Robinson, B.H. Identification of a canine model of pyruvate dehydrogenase phosphatase 1 deficiency. Mol. Genet. Metab.; 2007; 90, pp. 15-23. [DOI: https://dx.doi.org/10.1016/j.ymgme.2006.09.011]
21. Shelton, G.D.; Minor, K.M.; Li, K.; Naviaux, J.C.; Monk, J.; Wang, L.; Guzik, E.; Guo, L.T.; Porcelli, V.; Gorgoglione, R. et al. A Mutation in the Mitochondrial Aspartate/Glutamate Carrier Leads to a More Oxidizing Intramitochondrial Environment and an Inflammatory Myopathy in Dutch Shepherd Dogs. J. Neuromuscul. Dis.; 2019; 6, pp. 485-501. [DOI: https://dx.doi.org/10.3233/JND-190421] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/31594244]
22. Lepori, V.; Mühlhause, F.; Sewell, A.C.; Jagannathan, V.; Janzen, N.; Rosati, M.; Alves de Sousa, F.M.M.; Tschopp, A.; Schüpbach, G.; Matiasek, K. et al. A Nonsense Variant in the ACADVL Gene in German Hunting Terriers with Exercise Induced Metabolic Myopathy. G3; 2018; 8, pp. 1545-1554. [DOI: https://dx.doi.org/10.1534/g3.118.200084] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/29491033]
23. Vijayasarathy, C.; Giger, U.; Prociuk, U.; Patterson, D.F.; Breitschwerdt, E.B.; Avadhani, N.G. Canine mitochondrial myopathy associated with reduced mitochondrial mRNA and altered cytochrome c oxidase activities in fibroblasts and skeletal muscle. Comp. Biochem. Physiol. A Physiol.; 1994; 109, pp. 887-894. [DOI: https://dx.doi.org/10.1016/0300-9629(94)90236-4] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/7530157]
24. Tkaczyk-Wlizło, A.; Kowal, K.; Ślaska, B. Mitochondrial DNA alterations in the domestic dog (Canis lupus familiaris) and their association with development of diseases: A review. Mitochondrion; 2022; 63, pp. 72-84. [DOI: https://dx.doi.org/10.1016/j.mito.2022.02.001] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/35134592]
25. Baranowska, I.; Jäderlund, K.H.; Nennesmo, I.; Holmqvist, E.; Heidrich, N.; Larsson, N.G.; Andersson, G.; Wagner, E.G.; Hedhammar, A.; Wibom, R. et al. Sensory ataxic neuropathy in golden retriever dogs is caused by a deletion in the mitochondrial tRNATyr gene. PLoS Genet.; 2009; 5, e1000499. [DOI: https://dx.doi.org/10.1371/journal.pgen.1000499] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/19492087]
26. Meurs, K.M.; Friedenberg, S.G.; Olby, N.J.; Condit, J.; Weidman, J.; Rosenthal, S.; Shelton, G.D. A QIL1 Variant Associated with Ventricular Arrhythmias and Sudden Cardiac Death in the Juvenile Rhodesian Ridgeback Dog. Genes; 2019; 10, 168. [DOI: https://dx.doi.org/10.3390/genes10020168] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/30795627]
27. Dubowitz, V.; Sewry, C.A.; Oldfors, A. Histological and histochemical stains and reactions. Muscle Biopsy: A Practical Approach, 5th ed; Elsevier: Amsterdam, The Netherlands, 2021.
28. Wang, C.; Wallerman, O.; Arendt, M.L.; Sundström, E.; Karlsson, Å.; Nordin, J.; Mäkeläinen, S.; Pielberg, G.R.; Hanson, J.; Ohlsson, Å. et al. A novel canine reference genome resolves genomic architecture and uncovers transcript complexity. Commun. Biol.; 2021; 4, 185. [DOI: https://dx.doi.org/10.1038/s42003-021-01698-x] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/33568770]
29. Meadows, J.R.S.; Kidd, J.M.; Wang, G.D.; Parker, H.G.; Schall, P.Z.; Bianchi, M.; Christmas, M.J.; Bougiouri, K.; Buckley, R.M.; Hitte, C. et al. Genome sequencing of 2000, canids by the Dog10K consortium advances the understanding of demography, genome function and architecture. Genome Biol.; 2023; 24, 187. [DOI: https://dx.doi.org/10.1186/s13059-023-03023-7]
30. Cullen, J.N.; Friedenberg, S.G. Whole Animal Genome Sequencing: User-friendly, rapid, containerized pipelines for processing, variant discovery, and annotation of short-read whole genome sequencing data. G3; 2023; 13, jkad117. [DOI: https://dx.doi.org/10.1093/g3journal/jkad117]
31. Knudsen, S. Promoter2.0: For the recognition of PolII promoter sequences. Bioinformatics; 1999; 15, pp. 356-361. [DOI: https://dx.doi.org/10.1093/bioinformatics/15.5.356]
32. Solovyev, V.V.; Shahmuradov, I.A.; Salamov, A.A. Identification of promoter regions and regulatory sites. Methods Mol. Biol.; 2010; 674, pp. 57-83. [DOI: https://dx.doi.org/10.1007/978-1-60761-854-6_5] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/20827586]
33. Dickinson, P.J.; LeCouteur, R.A. Muscle and nerve biopsy. Vet. Clin. N. Am. Small Anim. Pract.; 2002; 32, pp. 63-102. [DOI: https://dx.doi.org/10.1016/S0195-5616(03)00080-9] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/11785735]
34. Glass, E.N.; Kent, M. The clinical examination for neuromuscular disease. Vet. Clin. N. Am. Small Anim. Pract.; 2002; 32, pp. 1-29. [DOI: https://dx.doi.org/10.1016/S0195-5616(03)00078-0] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/11785724]
35. Bua, E.; Johnson, J.; Herbst, A.; Delong, B.; McKenzie, D.; Salamat, S.; Aiken, J.M. Mitochondrial DNA-deletion mutations accumulate intracellularly to detrimental levels in aged human skeletal muscle fibers. Am. J. Hum. Genet.; 2006; 79, pp. 469-480. [DOI: https://dx.doi.org/10.1086/507132] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/16909385]
36. Rygiel, K.A.; Picard, M.; Turnbull, D.M. The ageing neuromuscular system and sarcopenia: A mitochondrial perspective. J. Physiol.; 2016; 594, pp. 4499-4512. [DOI: https://dx.doi.org/10.1113/JP271212] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/26921061]
37. Volpi, L.; Ricci, G.; Orsucci, D.; Alessi, R.; Bertolucci, F.; Piazza, S.; Simoncini, C.; Mancuso, M.; Siciliano, G. Metabolic myopathies: Functional evaluation by different exercise testing approaches. Musculoskelet. Surg.; 2011; 95, pp. 59-67. [DOI: https://dx.doi.org/10.1007/s12306-011-0096-9] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/21373907]
38. El-Hattab, A.W.; Craigen, W.J.; Scaglia, F. Mitochondrial DNA maintenance defects. Biochim. Biophys. Acta Mol. Basis Dis.; 2017; 1863, pp. 1539-1555. [DOI: https://dx.doi.org/10.1016/j.bbadis.2017.02.017] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/28215579]
39. Varughese, J.T.; Buchanan, S.K.; Pitt, A.S. The Role of Voltage-Dependent Anion Channel in Mitochondrial Dysfunction and Human Disease. Cells; 2021; 10, 1737. [DOI: https://dx.doi.org/10.3390/cells10071737] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/34359907]
40. Fang, Y.d.; Xu, X.; Dang, Y.m.; Zhang, Y.m.; Zhang, J.p.; Hu, J.-Y.; Zhang, Q.; Dai, X.; Teng, M.; Zhang, D.-X. et al. MAP4 Mechanism that Stabilizes Mitochondrial Permeability Transition in Hypoxia: Microtubule Enhancement and DYNLT1 Interaction with VDAC1. PLoS ONE; 2011; 6, e28052. [DOI: https://dx.doi.org/10.1371/journal.pone.0028052]
41. Huang, L.; Wei, B.; Zhao, Y.; Gong, X.; Chen, L. DYNLT1 promotes mitochondrial metabolism to fuel breast cancer development by inhibiting ubiquitination degradation of VDAC1. Mol. Med.; 2023; 29, 72. [DOI: https://dx.doi.org/10.1186/s10020-023-00663-0]
42. Schwarzer, C.; Barnikol-Watanabe, S.; Thinnes, F.P.; Hilschmann, N. Voltage-dependent anion-selective channel (VDAC) interacts with the dynein light chain Tctex1 and the heat-shock protein PBP74. Int. J. Biochem. Cell Biol.; 2002; 34, pp. 1059-1070. [DOI: https://dx.doi.org/10.1016/S1357-2725(02)00026-2] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/12009301]
43. Naghdi, S.; Hajnóczky, G. VDAC2-specific cellular functions and the underlying structure. Biochim. Biophys. Acta; 2016; 1863, pp. 2503-2514. [DOI: https://dx.doi.org/10.1016/j.bbamcr.2016.04.020] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/27116927]
44. Pinton, P.; Giorgi, C.; Siviero, R.; Zecchini, E.; Rizzuto, R. Calcium and apoptosis: ER-mitochondria Ca2+ transfer in the control of apoptosis. Oncogene; 2008; 27, pp. 6407-6418. [DOI: https://dx.doi.org/10.1038/onc.2008.308]
45. Parker, H.G.; VonHoldt, B.M.; Quignon, P.; Margulies, E.H.; Shao, S.; Mosher, D.S.; Spady, T.C.; Elkahloun, A.; Cargill, M.; Jones, P.G. et al. An expressed fgf4 retrogene is associated with breed-defining chondrodysplasia in domestic dogs. Science; 2009; 325, pp. 995-998. [DOI: https://dx.doi.org/10.1126/science.1173275] [PubMed: https://www.ncbi.nlm.nih.gov/pubmed/19608863]
You have requested "on-the-fly" machine translation of selected content from our databases. This functionality is provided solely for your convenience and is in no way intended to replace human translation. Show full disclaimer
Neither ProQuest nor its licensors make any representations or warranties with respect to the translations. The translations are automatically generated "AS IS" and "AS AVAILABLE" and are not retained in our systems. PROQUEST AND ITS LICENSORS SPECIFICALLY DISCLAIM ANY AND ALL EXPRESS OR IMPLIED WARRANTIES, INCLUDING WITHOUT LIMITATION, ANY WARRANTIES FOR AVAILABILITY, ACCURACY, TIMELINESS, COMPLETENESS, NON-INFRINGMENT, MERCHANTABILITY OR FITNESS FOR A PARTICULAR PURPOSE. Your use of the translations is subject to all use restrictions contained in your Electronic Products License Agreement and by using the translation functionality you agree to forgo any and all claims against ProQuest or its licensors for your use of the translation functionality and any output derived there from. Hide full disclaimer
© 2024 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/). Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.
Abstract
Simple Summary
Mitochondrial diseases in people are a heterogeneous group of genetically, biochemically, and clinically diverse disorders caused by defects in the metabolic pathways of oxidation phosphorylation (OXPHOS) and ATP production. While infrequently described in dogs, mitochondrial diseases may be more common than is currently known. Both the nuclear and mitochondrial genomes encode components of the enzyme complexes of the OXPHOS system, resulting in the genetic bases of mitochondrial diseases being transmitted in a Mendelian fashion, maternally, or as sporadic diseases. The pathogenicity is further complicated by heteroplasmy, with several different mitochondrial genomes existing within a given cell. A major challenge in the diagnosis of mitochondrial diseases is the clinical heterogeneity, with multi-system diseases affecting three or more organs and characteristically affecting tissues with high energy demands such as the central nervous system, skeletal muscle, eye and heart. Novel clinical syndromes have been reported in association with mitochondrial dysfunction and many patients can be misdiagnosed. The advent of next-generation sequencing has resulted in the discovery of new pathogenetic variants and has become the standard for the diagnosis of mitochondrial disease. Here, we describe an adult dog with a chronic myopathy associated with a mitochondrial deletion disorder.
Abstract(1) Background: An adult dog was presented to a board-certified veterinary neurologist for evaluation of chronic weakness, exercise intolerance and lactic acidemia. (2) Methods: A mitochondrial myopathy was diagnosed based on the histological and histochemical phenotype of numerous COX-negative muscle fibers. Whole-genome sequencing established the presence of multiple extended deletions in the mitochondrial DNA (mtDNA), with the highest prevalence between the 1–11 kb positions of the approximately 16 kb mitochondrial chromosome. Such findings are typically suggestive of an underlying nuclear genome variant affecting mitochondrial replication, repair, or metabolism. (3) Results: Numerous variants in the nuclear genome unique to the case were identified in the whole-genome sequence data, and one, the insertion of a DYNLT1 retrogene, whose parent gene is a regulator of the mitochondrial voltage-dependent anion channel (VDAC), was considered a plausible causal variant. (4) Conclusions: Here, we add mitochondrial deletion disorders to the spectrum of myopathies affecting adult dogs.
You have requested "on-the-fly" machine translation of selected content from our databases. This functionality is provided solely for your convenience and is in no way intended to replace human translation. Show full disclaimer
Neither ProQuest nor its licensors make any representations or warranties with respect to the translations. The translations are automatically generated "AS IS" and "AS AVAILABLE" and are not retained in our systems. PROQUEST AND ITS LICENSORS SPECIFICALLY DISCLAIM ANY AND ALL EXPRESS OR IMPLIED WARRANTIES, INCLUDING WITHOUT LIMITATION, ANY WARRANTIES FOR AVAILABILITY, ACCURACY, TIMELINESS, COMPLETENESS, NON-INFRINGMENT, MERCHANTABILITY OR FITNESS FOR A PARTICULAR PURPOSE. Your use of the translations is subject to all use restrictions contained in your Electronic Products License Agreement and by using the translation functionality you agree to forgo any and all claims against ProQuest or its licensors for your use of the translation functionality and any output derived there from. Hide full disclaimer
Details
; Mickelson, James R 2
; Friedenberg, Steven G 3
; Cullen, Jonah N 3 ; Mehra, Jaya M 4 ; Guo, Ling T 1 ; Minor, Katie M 3
1 Department of Pathology, School of Medicine, University of California San Diego, La Jolla, CA 92093-0709, USA;
2 Department of Veterinary and Biomedical Sciences, College of Veterinary Medicine, University of Minnesota, St. Paul, MN 55108, USA;
3 Department of Veterinary Clinical Sciences, College of Veterinary Medicine, University of Minnesota, St. Paul, MN 55108, USA;
4 VCA Animal Care Center of Sonoma County, Rohnert Park, CA 94928, USA;