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Allen Herbst, Jeong W. Pak, Debbie McKenzie, Entela Bua, Marwa Bassiouni, Judd M. Aiken, Accumulation of Mitochondrial DNA Deletion Mutations in Aged Muscle Fibers: Evidence for a Causal Role in Muscle Fiber Loss, The Journals of Gerontology: Series A, Volume 62, Issue 3, March 2007, Pages 235–245, https://doi.org/10.1093/gerona/62.3.235
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Abstract
Although mitochondrial mutation abundance has been recognized to increase in an age-dependent manner, the impact of mutation has been more difficult to establish. Using quantitative polymerase chain reaction, we measured the intracellular abundance of mutant and wild-type mitochondrial genomes along the length of individual laser-captured microdissected muscle fibers from aged rat quadriceps. Aged muscle fibers possessed segmental, clonal intracellular expansions of unique somatically derived mitochondrial DNA (mtDNA) deletion mutations. When the mutation abundance surpassed 90% of the total mitochondrial genomes, the fiber lost cytochrome c oxidase activity and exhibited an increase in succinate dehydrogenase activity. In addition to the mitochondrial enzymatic abnormalities, some fibers displayed abnormal morphology such as fiber splitting, atrophy, and breakage. Deletion mutation accumulation was linked to these aberrant morphologies with more severe cellular pathologies resulting from higher deletion mutation abundance. In summary, our measurements indicate that age-induced mtDNA deletion mutations expand within individual muscle fibers, eliciting fiber dysfunction and breakage.
DUE to a multifactorial etiology, the specific series of molecular events that contribute to the aging process has not been elucidated. Dissecting and deciphering specific physiological mechanisms responsible for age-associated phenotypes is critical for advancing our understanding of the aging process. In accordance with the mitochondrial theory of aging (1,2), the accumulation of defective mitochondrial genomes has contributed to the physiological decline associated with aging (3–5). Sarcopenia, the age-associated loss of skeletal muscle mass and function (6), is a prime nonpathological contributor to the frailty associated with aging. Of the proposed mechanisms for sarcopenia (loss of muscle stem cell activity, denervation and/or renervation, endocrine changes, oxidative stress, or mitochondrial genome instability), the cumulative loss of individual muscle fibers represents a primary and permanent deficit.
In humans, 40% of muscle mass is lost between the ages of 20 and 80 (7). This muscle mass loss is due to decreased muscle cross-sectional area, loss of muscle fibers, and fiber atrophy (8,9). In the rat quadriceps muscles, rectus femoris and vastus lateralis, muscle mass decreased by 33% and 60% and fiber number decreased 30% and 58% between 18 and 36 months of age (10,11).
Concurrent with the age-dependent loss of muscle fibers, multiple mitochondrial DNA (mtDNA) deletion mutations accumulate over time in many tissues and species (12–16). MtDNA deletion mutations were initially considered to be at low abundance (<0.1%) when calculated against the total mitochondria pool in tissue homogenates (17,18). When, however, discrete numbers of muscle fibers were analyzed, the abundance of mtDNA deletion mutations was found to be inversely proportional to the number of cells analyzed (19). In situ hybridization studies demonstrated that mtDNA deletion mutations were not distributed homogeneously throughout a tissue, but amplified focally within a subset of individual cells, appearing as a segmental pattern along the length of muscle fibers and as a mosaic distribution between cells (20–26).
Mammalian mitochondria encode 22 transfer RNAs (tRNAs), 2 ribosomal RNAs (rRNAs), and 13 polypeptides from a 16.5-kilobase circular genome. Mitochondrial genomes exist as a cellular multiplicity and, as a result, mtDNA molecules complement each other, protecting against deleterious mutations. When mutations do occur, a state of heteroplasmy exists within individual mitochondria and cells. The cellular and systemic impact of mtDNA mutation is illustrated by a group of genetic diseases known as the mitochondrial myopathies and encephalomyopathies (27–29). Mitochondrial diseases are caused by the intracellular accumulation of mutated mtDNA to levels that eventually disrupt the synthesis of mitochondrially encoded components of the electron transport system (ETS). The abundance at which specific mutations cause ETS dysfunction is termed the phenotypic threshold effect (reviewed in 30,31). A characteristic cellular phenotype exhibited by patients with mitochondrial myopathies is the histological absence of cytochrome c oxidase (COX) activity and an upregulation of succinate dehydrogenase (SDH) activity (24). In situ hybridization studies on COX− fibers measured mitochondrial transcript abundance and/or mtDNA concentrations and found that wild-type and deletion-specific transcript levels were proportional to genotype abundance (20–23). Some studies found that wild-type genomes were reduced, whereas others suggested that wild type was maintained in COX− regions [reviewed by Shoubridge (32)].
Whereas the same mtDNA mutation is distributed among multiple tissues in the mitochondrial myopathies and encephalomyopathies, mitochondrial mutations also originate as a result of spontaneous somatic mutation events within individual cells. These age-associated mtDNA deletion mutations also induce COX−/SDH++ fibers, and are distributed mosaically intercellularly and segmentally intracellularly (26). Thus, accurate quantitation of the abundance of these enzymatic abnormalities requires the analysis of numerous sections of tissue along the length of the muscle. Based on histological analysis of aged muscles, the calculated tissue burden of ETS abnormalities was found to be 15% of all remaining muscle fibers in 36-month old rat rectus femoris (10), and 60% in 34-year-old rhesus monkey vastus lateralis (26). Additionally, muscles that display a large age-dependent loss of skeletal muscle fibers contain high levels of ETS abnormalities (33). Concomitant with observed ETS enzymatic abnormalities are often morphological changes in muscle fiber structure including fiber splitting, atrophy, and breakage.
The association of ETS abnormalities, mtDNA deletion mutations, fiber loss, and muscle mass loss suggest that these age-dependant events might share a common etiology. In this study, we tested the hypothesis that mtDNA mutation accumulation underlies the fiber splitting, atrophy, and breakage associated with ETS abnormalities. By taking a longitudinal single fiber approach to understanding the relationship between mitochondrial genotype and cellular phenotype, we link mtDNA deletion mutation accumulation with these dysfunctional cellular phenotypes and, ultimately, with muscle fiber loss.
Methods
Animals and Tissue Preparation
The rectus femoris and the vastus lateralis muscles were dissected from 36-month-old male Fischer 344 × Brown Norway F1 hybrid rats purchased from the National Institute on Aging colony maintained by Harlan Sprague Dawley (Indianapolis, IN). Rats were housed and killed in accordance with the Guide for the Care and Use of Laboratory Animals. The muscles were bisected at the midbelly, embedded in optimal cutting temperature medium (Miles Inc., Elkhart, IN), and flash frozen in liquid nitrogen. Samples were stored at −80°C until analyzed. Using a cryostat, we cut 100 or 200 10-μm-thick serial transverse cryosections and placed them on Probe-on Plus slides. At 60 μm intervals, cross-sections were stained for COX and SDH as previously described (10), and ETS abnormal fibers were identified. Fibers were also stained for cell morphology and nuclei with hematoxylin and eosin.
Laser Capture Microdissection
Histological sections were dehydrated through a series of graded ethanol and xylene (10). ETS abnormal fibers were subsequently microdissected using a PixCell II laser capture microscope (Arcturus, Mountain View, CA). Finally, captured fibers were further dissected from the capture film to eliminate all potential contamination.
DNA Isolation, Breakpoint Analysis, and Quantitative Real-Time Polymerase Chain Reaction
DNA isolation and mtDNA breakpoint analysis were performed as previously described (34). Oligonucleotide primers (Table 1) specific for either full-length or deleted genomes were designed for use in quantitative polymerase chain reaction (PCR) assays based on the unique sequence of each mtDNA deletion obtained from the breakpoint analysis. The full-length primer set is designed to amplify a region of the genome within the confines of the deleted mtDNA, ensuring the s specific amplification of full-length wild-type genomes. Deletion primer sets flank the breakpoint such that amplification of the deleted genomes yields an amplicon of ∼200 base pairs. The deletion primer sets cannot amplify full-length mtDNA due to the short extension time in the elongation phase of the PCR. Total DNA concentration is determined every cycle by the fluorescence emission generated by the binding of SYBR Green to the minor groove of DNA. Microdissected samples are amplified in parallel with known standards generated by cloning the deletion-specific as well as full-length sequences into the pGEM T-easy vector (Promega, Madison, WI). Standards were quantified by spectrophotometry at A260, and dilutions were prepared using National Institute of Standards and Technology (NIST)–calibrated volumetric pipets. Linearity of dilutions was confirmed by quantitative PCR and regression analysis. Samples and standards for both wild-type and deletion-specific primer sets were amplified in triplicate using iQ SYBR Green supermix (BIO-RAD Laboratories, Hercules, CA). Standard curves were generated for the primer sets (Figures 1B and 2), and the starting quantities of wild-type and deleted mitochondrial genomes were calculated. Specificity of amplification reactions was confirmed by melting point analysis (Figure 1C) and gel electrophoresis.
Results
Serial longitudinal cross-sections of aged muscle tissue were stained histochemically at 60 μm intervals to identify muscle fibers containing ETS abnormal regions (Figures 3–6A). Four fibers containing COX−/SDH++ regions were selected based on their morphology and the contiguity of the ETS abnormal region within the series of sections. Fibers 1 and 2 contain a 440 μm and 460 μm nonatrophic ETS abnormal phenotype (Figures 3 and 4). Fiber 3 contains an ETS abnormal region that colocalizes with a region undergoing fiber splitting. The fiber splits along its length first into two and, subsequently, three fibers before returning to a single unified fiber (Figure 5). Fiber 4 atrophies, eventually becoming undetectable for 250 μm, and then reappears as an ETS abnormal fiber (Figure 6).
Multiple sections of each of these fibers were individually microdissected, DNA-isolated and, through the use of mtDNA-specific primers, amplified and subsequently sequenced. A single smaller-than-wild-type genome (an mtDNA deletion mutation) was identified in each fiber's ETS abnormal region. The size of these deletion-containing genomes varied between fibers and ranged from 8148 to 11,268 base pairs. All deletion mutations removed portions of the wild-type mitochondrial genome along the major arc and disrupted or abrogated genes coding for COX, ATP synthase, NADH dehydrogenase, as well as the interspersed mitochondrial tRNAs. The specific deletion mutation in fiber one removed nucleotides 6013–14,165, fiber two nucleotides 7455–14,731, fiber three nucleotides 6710–12,542 and fiber four nucleotides 7389–14,485.
The absolute quantity of deleted and wild-type mitochondrial genomes was determined by breakpoint-specific quantitative PCR assays on laser-captured cell sections collected along the length of individual muscle fibers. The intracellular abundance of mtDNA deletion mutations within each fiber's ETS abnormal region was greater than 90%. In every fiber, the COX−/SDH++ phenotype was flanked by adjacent ETS normal regions that contained detectable levels of deletion mutations, albeit at lower levels (Figures 3–6). Fiber 1, for example, contained a 440-μm ETS abnormal region within a 770-μm region that contained an accumulation of mtDNA deletion mutations. As the abundance of mtDNA mutation decreased, there was an intermediate ETS abnormal transitional phenotype characterized by slightly reduced COX activity, and slightly increased SDH activity (Figures 3A [slides 44/45] and 4A [slides 16/17]). In fiber regions distant from the ETS abnormality, only wild-type genomes were detected, and mtDNA deletion mutations were undetectable. The COX-negative, SDH hyper phenotype occurred in regions that contained greater than 90% mutant mtDNA (Figures 3–6). Wild-type genomes were consistently detected in both ETS normal and abnormal regions (Figure 7).
Discussion
Age-associated mtDNA deletion mutations form as the result of somatic mutation of wild-type genomes. The cellular impact, however, is the result of the clonal accumulation of mutant genomes to sufficiently high levels to affect mitochondrial and cellular function. The presence of mutant mtDNA genomes outside the ETS abnormal phenotype (Figures 3–6) indicates that the ETS abnormal phenotype results from the intracellular accumulation of mtDNA deletion mutations, not vice versa. The maintenance of wild-type genomes throughout the abnormal region (Figure 7) at levels that are similar to ETS normal regions and the coordinated decrease in mutation abundance in the ETS normal region indicate that the accumulation of deleted genomes, and not the selective depletion of wild type, is responsible for phenotypic threshold effect. The loss of COX activity in the presence of wild-type genomes suggests that incompetent genomes and their derived transcripts may compete with wild-type genomes for binding of transcriptional and translational machinery leading to a breakdown in the amount of functional polypeptides and loss of enzymatic activity.
We measured the absolute quantity of mitochondrial genomes, full-length and deletion-containing, to determine the threshold for the loss of COX activity. A 90% threshold for age-induced mtDNA mutations is consistent with previous measurements that determined the threshold for loss of COX activity to be between 60% (35) and 90% (20,21,36), depending upon tissue type (HeLa cells, or multinucleated muscle fibers from patients with mitochondrial myopathies, respectively). The maintenance of full-length wild-type genomes in ETS abnormal segments is consistent with in situ hybridization studies from patients with mitochondrial myopathies (20,21) as well as aged muscle fibers (25,26).
Muscle fiber splitting is a characteristic phenotype of many primary muscle diseases including dystrophies. In the split muscle fiber (Figure 5), the same molecular mutation was detected in each of the daughter fibers, indicating that the mutation was present before the split occurred and, consequently, that the fiber is undergoing splitting and not fusion. Muscle fiber splitting has been observed to be associated with 35% of ETS abnormal muscle fibers; however, the split region rarely colocalized with the abnormal enzymatic phenotype (10). Our data suggest that, whereas there is no overlap between the ETS abnormal region and the split fiber regions, there is a colocalization of fiber splitting and the accumulation of mtDNA deletion mutations (Figure 5C), albeit at levels below the threshold for the expression of the ETS abnormal phenotype. Splitting may represent a precursor phenotype to fiber atrophy via the independent breakage of daughter fibers or a protective mechanism that allows segregation of mutant and wild-type genomes altering the level of heteroplasmy in each branch.
We have previously reported, in aged rat quadriceps muscle, that 25% of ETS abnormal fibers are associated with fiber atrophy and 7% with fiber breakage (10). Similar observations have been made in rhesus macaques (25,26). The proliferation of an mtDNA deletion mutation across a broken fiber segment (Figure 6) and the subsequent ETS abnormality directly supports the hypothesis that accumulation of mtDNA deletions can result in fiber breakage. The broken ends of the fiber (Figure 6C) contain exceedingly high levels of the same unique mtDNA deletion mutation suggesting that the fiber was once continuous, subsequently atrophied, and ruptured. The broken ends of the fiber contain the highest level of mtDNA mutations measured, 3 × 105 mutant genomes, demonstrating a profound ETS abnormal phenotype.
The mechanism driving mtDNA deletion mutation proliferation is not known. MtDNA deletion mutations could accumulate because they possess a replication advantage, because of stochastic events, or because their destruction is disadvantaged. These possibilities have been put forth as biological hypotheses: replicative advantage (21), random drift (37), and survival of the slowest (38), respectively. These mechanisms are not mutually exclusive, however, and the mechanism of mtDNA accumulation may be more complex, especially in multinucleated tissue such as muscle fibers. The strikingly high copy number of deletion-containing genomes (∼100,000 copies) measured within an ETS abnormal section, combined with the relatively stable numbers of wild-type genomes (∼1000 copies), implies that muscle fibers do not maintain a steady state of mtDNA molecules in response to dysfunctional oxidative phosphorylation. That is, mitochondrial deletion mutation replication does not occur at the expense of wild-type replication. Moreover, these measurements suggest that deleted mtDNA molecules are advantaged, replicating to high abundance. One prediction of the advantaged model is the presence of neutral mtDNA deletion mutations that do not accumulate to high levels due to genome size or specific breakpoint location. We compared the specific deletion mutation breakpoints that accumulate in individual ETS abnormal fibers with the breakpoint sequences observed in muscle tissue homogenates (Figure 8). The deletion breakpoints in tissue homogenates were distributed throughout the mitochondrial genome, whereas deletion breakpoints from abnormal fibers were confined to the major arc of the mtDNA indicating specificity for mutations that could accumulate to cause ETS abnormal fibers. The localization of mtDNA deletion mutation breakpoints from ETS abnormal fibers to the major arc was previously attributed to the existence of a “hot spot” for mutation formation (34,39). The difference in deletion mutation patterns between tissue homogenates and single cells, however, suggests an alternative explanation: that the generation of mtDNA deletion mutants is random but that certain mutations, those producing small genomes (large deletions) while retaining both origins of replication, are more likely to accumulate to high intracellular abundance.
Many mechanisms have been proposed to explain the age-associated loss of muscle mass. Our molecular observations of the role of mtDNA deletion mutations in sarcopenia are consistent with the hypothesis that the intracellular accumulation of mtDNA deletion mutations causes mitochondrial dysfunction. The abrogation of mitochondrial and cellular processes induces morphological changes in the fiber such as splitting. The fiber atrophies and eventually ruptures. The somatic generation and subsequent intracellular accumulation of mtDNA deletion mutations contributes to the age-dependent loss of muscle fibers and sarcopenia.
Decision Editor: Huber R. Warner, PhD
Fiber . | Primer Pair . | Wt/del . | Sequence 5′-3′ . |
---|---|---|---|
1,2,4 | RM13645F | Wt | CAACATAACCCCAACATCATCAATCTCATACA |
RM13927R | AATAGTTTTAGGGTTTGGGGGTTCGTTTTT | ||
1 | RM7290F | del | AGGACACCAATGATACTGAAGCTATGAATATACTGACTA |
RM14786R | ATGGAATGGGATTTTGTCTGCGTCG | ||
2 | RM5981F | del | CTTCGACCCCGCTGGAGGTGGAGAC |
RM14347R | GATGAGAATGCTGTTATGGTATCAGACGTGTAGTG | ||
3 | RM7189F | Wt | ATTCTCCCAGCTGTCATTCTTATTCTAATTGCCCTTCC |
RM7332R | TTCATAGTCAGTATATTCATATTCATAGCTTCAGTATCATTGGTGTCCT | ||
3 | RM5360F | del | CCTCTATAGGCTCATTCATCTCACTTACGCC |
RM12683R | GCAAATGTGGAGGAAAGCAAGGTAGGGT | ||
4 | RM7347F | del | CTCCTACATAATCCCAACCAATGACCTAAAACC |
RM14675R | GATGAAGTGGAATGCGAAGAAGCGTGT |
Fiber . | Primer Pair . | Wt/del . | Sequence 5′-3′ . |
---|---|---|---|
1,2,4 | RM13645F | Wt | CAACATAACCCCAACATCATCAATCTCATACA |
RM13927R | AATAGTTTTAGGGTTTGGGGGTTCGTTTTT | ||
1 | RM7290F | del | AGGACACCAATGATACTGAAGCTATGAATATACTGACTA |
RM14786R | ATGGAATGGGATTTTGTCTGCGTCG | ||
2 | RM5981F | del | CTTCGACCCCGCTGGAGGTGGAGAC |
RM14347R | GATGAGAATGCTGTTATGGTATCAGACGTGTAGTG | ||
3 | RM7189F | Wt | ATTCTCCCAGCTGTCATTCTTATTCTAATTGCCCTTCC |
RM7332R | TTCATAGTCAGTATATTCATATTCATAGCTTCAGTATCATTGGTGTCCT | ||
3 | RM5360F | del | CCTCTATAGGCTCATTCATCTCACTTACGCC |
RM12683R | GCAAATGTGGAGGAAAGCAAGGTAGGGT | ||
4 | RM7347F | del | CTCCTACATAATCCCAACCAATGACCTAAAACC |
RM14675R | GATGAAGTGGAATGCGAAGAAGCGTGT |
Note: Wt = Wild-type specific primer; del = deletion specific primers.
Fiber . | Primer Pair . | Wt/del . | Sequence 5′-3′ . |
---|---|---|---|
1,2,4 | RM13645F | Wt | CAACATAACCCCAACATCATCAATCTCATACA |
RM13927R | AATAGTTTTAGGGTTTGGGGGTTCGTTTTT | ||
1 | RM7290F | del | AGGACACCAATGATACTGAAGCTATGAATATACTGACTA |
RM14786R | ATGGAATGGGATTTTGTCTGCGTCG | ||
2 | RM5981F | del | CTTCGACCCCGCTGGAGGTGGAGAC |
RM14347R | GATGAGAATGCTGTTATGGTATCAGACGTGTAGTG | ||
3 | RM7189F | Wt | ATTCTCCCAGCTGTCATTCTTATTCTAATTGCCCTTCC |
RM7332R | TTCATAGTCAGTATATTCATATTCATAGCTTCAGTATCATTGGTGTCCT | ||
3 | RM5360F | del | CCTCTATAGGCTCATTCATCTCACTTACGCC |
RM12683R | GCAAATGTGGAGGAAAGCAAGGTAGGGT | ||
4 | RM7347F | del | CTCCTACATAATCCCAACCAATGACCTAAAACC |
RM14675R | GATGAAGTGGAATGCGAAGAAGCGTGT |
Fiber . | Primer Pair . | Wt/del . | Sequence 5′-3′ . |
---|---|---|---|
1,2,4 | RM13645F | Wt | CAACATAACCCCAACATCATCAATCTCATACA |
RM13927R | AATAGTTTTAGGGTTTGGGGGTTCGTTTTT | ||
1 | RM7290F | del | AGGACACCAATGATACTGAAGCTATGAATATACTGACTA |
RM14786R | ATGGAATGGGATTTTGTCTGCGTCG | ||
2 | RM5981F | del | CTTCGACCCCGCTGGAGGTGGAGAC |
RM14347R | GATGAGAATGCTGTTATGGTATCAGACGTGTAGTG | ||
3 | RM7189F | Wt | ATTCTCCCAGCTGTCATTCTTATTCTAATTGCCCTTCC |
RM7332R | TTCATAGTCAGTATATTCATATTCATAGCTTCAGTATCATTGGTGTCCT | ||
3 | RM5360F | del | CCTCTATAGGCTCATTCATCTCACTTACGCC |
RM12683R | GCAAATGTGGAGGAAAGCAAGGTAGGGT | ||
4 | RM7347F | del | CTCCTACATAATCCCAACCAATGACCTAAAACC |
RM14675R | GATGAAGTGGAATGCGAAGAAGCGTGT |
Note: Wt = Wild-type specific primer; del = deletion specific primers.
This work was supported by National Institute on Aging Award R01 AG011604. We thank the National Institute of Environmental Health Sciences (NIEHS) Center for Molecular and Developmental Toxicology (ES 09090) for access to laser capture microdissection.
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