Becker muscular dystrophy (BMD) is a debilitating X-linked muscle disease caused by in-frame mutations of the dystrophin gene.^1–3 BMD-causing mutations result in production of a truncated isoform of dystrophin protein that is partially functional and expressed at reduced amounts. Patients have a variable presentation; some individuals show severe muscle weakness in early childhood with loss of ambulation by late teens to early 20s, whereas others remain largely asymptomatic.^4–8 Ultimately, heart problems develop in most patients, with up to 50% of BMD patients eventually dying from cardiomyopathy.^9,10 As a rare disease with variable pathology and no current animal model, BMD represents an understudied and underserved group with no approved therapy and very few clinical trials (two interventions in active clinical trials for BMD vs. 30 for DMD). Development of clinically pertinent BMD mouse models will facilitate an improved understanding of disease pathology and functionality of dystrophin isoform domains while also providing a preclinical platform for development of the first BMD therapeutics.

BMD patients show variability in dystrophin protein levels that partially correlate with disease severity, though even ‘mild’ patients exhibit muscle pathology.^2,11–15 Inter-patient and intra-patient variability is observed with respect to dystrophin protein amount. Specifically, variable and reduced dystrophin protein levels are observed in muscle biopsies from different patients, from different muscles and even within different regions of a single muscle biopsy. Elevated serum CK levels are present at birth, and up to 95% of patients can be detected by screening for serum CK levels. Muscle biopsies show increases in fibre size variability, centralized nuclei, fibre degeneration and fibre branching.^4,6,7 Muscle atrophy and pseudohypertrophy are also seen, with fibrosis or fatty replacement of muscle.¹⁶

BMD provides hope to the Duchenne muscular dystrophy (DMD) community because it provides evidence that expressing a truncated dystrophin isoform can result in a milder disease. DMD is caused by a complete loss of functional dystrophin and is more severe with an earlier onset. A promising area of therapeutics seeks to restore expression of ‘Becker-like’ isoforms of dystrophin through mRNA-splice modulating antisense oligos (AOs). Preclinical dystrophinopathy research has focused primarily on DMD because there are several available mouse models that recreate dystrophin-null mutations. These include mdx23, mdx52 and several CRISPR mouse and rat models.^17–21 Importantly, studies in mdx mice have led to development and accelerated approval of four exon-skipping AO drugs for DMD (eteplirsen, golodirsen, viltolarsen and casimersen). Although these dystrophin restoration therapies are promising, they are not curative. In the best-case scenario, these therapeutics would convert a DMD genotype into a milder BMD phenotype. BMD therefore serves as a model for efficient dystrophin restoration therapies, and as these therapies enter widespread clinical use, there will be a further need for development of BMD therapeutics⁹ and disease models.

Here we introduce a large (approximately 40 000 bp) deletion mutation via CRISPR to remove exons 45–47 of the endogenous murine dystrophin (Dmd) gene, recreating the most common BMD-causing deletion in humans. The resulting bmx mouse model (for Becker muscular dystrophy, X-linked) has molecular, histopathological and functional deficits consistent with BMD patients while displaying phenotypes that are intermediate to control wild-type (WT) and DMD model (mdx52) mice. These studies establish the bmx mouse as a novel model of BMD. Moving forward, the bmx mouse can be used to gain new insights into BMD disease pathology, to model dystrophin restoration therapies in DMD and to facilitate the development of BMD therapeutics as well as DMD co-therapeutics.

All animal studies were conducted according to the NIH Guide for the Care and Use of Laboratory Animals, all national laws and 1964 Declaration of Helsinki standards and amendments and approval of the Institutional Animal Care and Use Committee of Children's National Hospital (CNH). C57/BL6-mdx∆52 mice (mdx52) contain a deletion of exon 52 of the Dmd gene, resulting in absence of full-length dystrophin,²¹ and were originally provided as a gift from Dr Shin'ichi Takeda. Wild-type C57/BL6 (WT) mice were purchased from Jackson Laboratory (Bar Harbor, ME). All strains are currently maintained in-house at CNH.

bmd∆45-47 (bmx) mice were generated on a C57/BL6 background via CRISPR using guide RNAs (gRNAs) to delete exons 45–47 of the murine dystrophin (Dmd) gene. gRNAs were designed to target protospacer adjacent motif (PAM) sequences upstream of Dmd exon 45 and downstream of Dmd exon 47. Subsequent DNA sequencing of pups was performed to verify germline transmission.

Serum creatine kinase, muscle-type (CKM) was assayed via ELISA according to manufacturer's instructions (Novus Biologicals #NBP2-75306). Blood collection and serum isolation details can be found in the Supporting Information.

Muscles were flash frozen in liquid-nitrogen. Eight-micrometre sections were lysed in High SDS buffer containing 0.02% EDTA (pH 8.0), 0.075% Tris–HCL (pH 6.8) and protease inhibitors. Capillary Western immunoassay (Wes) was performed according to manufacturer's instructions using 66–440 kDa Separation Modules (ProteinSimple). Details can be found in the Supporting Information.

Grip strength: Forelimb and hindlimb grip strength was assessed using a grip strength meter (Columbus Instruments) daily for 2 consecutive days according to Treat NMD protocols (DMD_M.2.2.001), with data interpreted as averaged maximum daily values. Wire and box hang: Two-limb wire hang and four-limb grid hang tests were performed in accordance with Treat NMD protocols (DMD_M.2.1.005). Details can be found in the Supporting Information.

To measure in vivo torque production of the anterior crural muscles [TA, extensor digitorum longus (EDL), peroneus tertius and extensor hallucis longus], mice were anesthetized with 1.5% isoflurane-mixed O₂ and hair removed from lower hindlimbs, whereas the foot was attached to the dual-mode lever and maintained at 90° for isometric torque assessment (Aurora Scientific). See Supporting Information for full details.

An eccentric injury protocol was performed in male bmx, mdx52 and WT mice based on previously reported protocols. Details and citations can be found in the Supporting Information.

See Supporting Information for full details and citations.

Muscles were mounted, frozen in liquid-nitrogen cooled isopentane and sectioned (8 μm) onto slides. For most immunofluorescence, muscle sections were fixed in ice-cold acetone for 10 min. For anti-IgM immunofluorescence, muscle sections were fixed with 4% paraformaldehyde for 10 min at room temperature. Slides were washed, blocked for 1 h (1X PBST with 0.1% Triton X-100, 1% BSA, 10% goat serum and 10% horse serum), washed three times, then exposed to primary antibodies overnight at 4°C and secondary antibodies for 1 h at RT. Coverslips were mounted using Prolong Gold Mounting Medium with DAPI. Slides were imaged using an Olympus VS-120 scanning microscope at 20×. Antibody dilutions can be found in the Supporting Information.

Mice aged 8–10 weeks were administered water containing 0.8 mg/mL BrdU for 1 week followed by normal water for 1 week. Muscle was then stained for BrdU. Full details can be found in the Supporting Information.

qRT-PCR of miRNAs and mRNAs was performed. Details and assay IDs are provided in the Supporting Information.

To create bmx mice (for Becker muscular dystrophy, X-linked) that model the most common BMD patient mutation,¹⁴ we used CRISPR/Cas9 to introduce a ~40 000 bp genomic deletion into the endogenous murine dystrophin (Dmd) gene, excising exons 45–47. Guide RNAs (gRNAs) were designed to target protospacer adjacent motif (PAM) sequences upstream of Dmd exon 45 and downstream of Dmd exon 47 (Figure 1A). DNA sequencing confirmed genomic deletion of dystrophin exons 45–47 (Figure 1B), which is predicted to disrupt spectrin-type repeats (STRs) and neuronal nitric oxide synthase (nNOS) binding (Figure 1C). qRT-PCR was used to validate deletion of exons 45–47 and to quantify overall Dmd transcript levels. We observed similar expression of Dmd between WT and bmx mice using probes at the 5′ and 3′ ends of the Dmd transcript (exon 2–3 or 76–77) while using a probe for exons Dmd 45–46 confirmed bmx quadriceps (Figure 1D), TA, heart and diaphragm (Figure S1) lack this region. We observed progressively reduced amounts of Dmd mRNA in the 5′–3′ direction in mdx52 consistent with 3′ destabilization as previously reported (Figure 1D).²²

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Figure 1. Generation of the bmx mouse model of BMD by deletion of dystrophin exons 45–47. (A) Schematic of the dystrophin gene showing CRISPR/Cas9-targeted deletion of exons 45–47. (B) DNA sequencing showing genomic deletion of dystrophin exons 45–47. (C) Protein structure of dystrophin Δ45–47 shows disruption of the nNOS binding domain and a disruption of the rod domain that results in an out-of-phase spectrin-type repeat (STR) pattern. (D) mRNA levels of dystrophin exons 2–3 and exons 76–77 are unchanged in Becker muscular dystrophy (bmx) mice, whereas dystrophin exons 45–46 are deleted in quadriceps muscle. NT = amino-terminus, H = Hinge, R = STR, CR = cysteine-rich, CT = carboxy-terminus. ANOVA; n = 7–8; ***P [less than] 0.001, ****P ≤ 0.0001.

To determine whether bmx mice exhibit functional impairments, we performed phenotyping at 10 weeks (forelimb/hindlimb grip strength), 14 weeks (two-limb wire hang), and 15 weeks (four-limb grid hang). bmx mice showed reduced grip strength versus WT for forelimb (14.90% decrease, P = 0.0465) and hindlimb (36.81% decrease, P < 0.0001) (Figure 2A). Reduced suspension times for bmx were also found in wire hang (−54.25%, P = 0.0087) and box hang (−39.85%, P = 0.0489) (Figure 2B). Assaying in vivo isometric torque produced in the tibialis anterior (TA), bmx mice showed significantly reduced maximum isometric torque vs. WT mice (1.465 vs. 1.650 mN*m, P = 0.0110), though there was no significant improvement in bmx versus mdx52 (Figure 2C, left). Additionally, the deficit in isometric torque was observed at all frequencies for bmx (Figure 2C, right). In vivo specific isometric torque showed modest reductions in maximal values for bmx versus WT (48.74 vs. 53.63 mN*m/kg, P = 0.1235) and were significantly elevated versus mdx52 (P = 0.0295) (Figure S2A).

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Figure 2. The bmx mouse has reduced motor function, muscle force and heart function. (A) Grip strength of bmx mice was reduced in both the forelimb (P = 0.0465) and hindlimb (P = 0.0002) grip strength tests. n = 8. (B) Suspension time of bmx mice was reduced in the wire hang test (P = 0.0087) and in the box hang test (P = 0.0489). n = 8. (C) In vivo maximum isometric torque and torque-frequency curve for anterior crural muscles of WT, bmx, and mdx52 mice. Maximum isometric torque was reduced in bmx mice (P = 0.0110). n = 6–7. (D) Left; ex vivo eccentric contraction-induced lengthening force drop in EDL, bmx shows increased injury (force drop) versus WT. (P = 0.0249); right; force drop, expressed as a percent of initial eccentric contraction force, is shown across 10 eccentric contractions. (E) Echocardiography of aged (18-month-old) bmx mice shows a deficit in heart function through a decrease in fractional shortening (P = 0.0036) and ejection fraction (P = 0.0131). n = 5–7. (F) Representative M-mode images of the parasternal short axis are provided. (G) Serum CKM levels in aged (1-year-old) mice assayed via ELISA. n = 6–7. ANOVA, *P ≤ 0.05, **P ≤ 0.01, ***P ≤ 0.001, ****P ≤ 0.0001.

We next sought to examine contractile performance and resistance to eccentric injury in bmx mice. Ten eccentric contractions of WT EDL muscle resulted in a 15.53% drop in ex vivo peak force. In contrast, this protocol reduced peak force by 20.16% in bmx EDL muscles (P = 0.0239 bmx vs. WT) and 20.86% in mdx EDL (Figure 2D). This injury protocol also resulted in a 42.49% drop in isometric force in bmx EDL (P = 0.0307) vs. 33% isometric force drop in WT and a 38% drop in mdx EDL (Figure S2B).

Heart function was assessed via echocardiography in 18-month-old WT, bmx and mdx52 mice. We chose this age because reduced heart function is observed in mdx52 mice starting around 12 months of age and reasoned that comparable heart function declines in bmx should therefore be present by 12–18 months of age. bmx mice showed significant declines in heart function measures (Figure 2E,F) including fractional shortening and ejection fraction (−25.07%, P < 0.0036, −27.67% P < 0.0131 vs. WT). We also assayed serum creatine kinase levels in aged mice; bmx mice showed an ~62-fold (P < 0.0001) increase in serum creatine kinase, muscle-type (CKM) over WT (Figure 2G). bmx serum CKM levels (28 447 ng/ml) were intermediate to WT (457 ng/ml) and mdx (40 514 ng/ml), and bmx CKM was significantly lower than mdx (P = 0.0217). These data indicate aged bmx mice have reduced heart function and increased serum CK, consistent with human disease.

In mdx mice, limb muscles undergo dramatic necrosis, which is followed by regeneration, increased hypertrophy and increased muscle mass.²³ Loss of muscle mass then occurs in older mdx mice (12–18 months).^23,24 BMD patients also have both muscle pseudohypertrophy and true hypertrophy.^6,25 Examining body and muscle mass at 5 months, bmx showed a 9.57% increase (P = 0.0633) in body weight compared with WT mice (Figure 3A). Increased muscle mass was present in every skeletal muscle examined: TA (18.16% increase, P = 0.0096), quadriceps (9.75% increase, P = 0.0456), gastrocnemius (9.135% increase, P = 0.0143), and triceps (17.95% increase, P = 0.0583) (Figures 3B,C and S3). No significant difference was seen in heart mass (P = 0.4288) versus WT and bmx mice (Figure 3D). As mdx52 spleens are enlarged due to increased systemic inflammation, we also examined spleen mass. We observed a moderate increase in bmx spleen mass, which did not reach significance (12.45% increase, P = 0.1048) (Figure 3E), but may suggest increased circulating inflammation in bmx.

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Figure 3. bmx mice have increased muscle mass. Body and tissue weights of age-matched WT, bmx and mdx52 mice were assayed at 5 months of age. (A) bmx mice show moderate increases in body mass at 5 months (P = 0.0633; n = 8). (B,C) The weight of the tibialis anterior (TA; P = 0.0096) and (C) quadriceps (P = 0.0456; n = 12) is significantly increased in bmx mice. (D) Heart weight in bmx mice is similar to that of WT mice (P = 0.4288; n = 8). (E) Spleen weight was elevated in bmx mice but was not significant (P = 0.1048; n = 6–8). ANOVA, *P ≤ 0.05, **P ≤ 0.01, ****P [less than] 0.0001.

BMD muscle biopsies show increased myofibre size variability and centrally nucleated fibres, indicative of increased and asynchronous muscle regeneration.^6,26 To examine bmx muscle architecture, gastrocnemius muscle sections were immunostained for laminin-α2. Visually, we observed fibre size variability and some centrally localized nuclei in bmx muscles, indicating pathology (Figure 4A). Muscle fibre measurements including minimal Feret's diameter and myofibre cross-sectional area (CSA) were then determined.²⁷ Whereas mdx52 showed a shift towards smaller, regenerating fibres, with some intermittent large fibres, bmx mice showed a greater number of both smaller and larger myofibres versus WT, as indicated by histograms plotting minimal Feret's diameter and CSA measurements (Figure 4B,C). Differences in fibre size variation were additionally determined by calculating variance coefficients (VCs). VCs showed significant differences between fibre size variability for bmx versus WT, for minimal Feret's diameter (+18.91%, P = 0.0017) and CSA (+14.96%, P = 0.0182) (Figure 4B,C). bmx also had significantly more centrally nucleated fibres versus WT (4.573% vs. 0.5594%, P = 0.0002) (Figure 4D).

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Figure 4. Muscles from bmx mice show centrally localized nuclei and increased variation in fibre size. (A) Laminin immunofluorescence of WT, bmx and mdx52 gastrocnemius muscle. DAPI was used as counterstain to visualize myonuclei. Bar = 100 μM. (B) Histogram of minimal Feret's diameter and the variance coefficient (VC) of minimal Feret's diameter. Bmx myofibres have increased variation of minimal Feret's diameter (P = 0.0017; n = 4). (C) Histogram of myofibre cross sectional area (CSA) and VC of myofibre CSA. bmx myofibres have increased variation of CSA (P = 0.0182; n = 4). (D) The percentage of centrally nucleated myofibres was increased in bmx mice (P [less than] 0.0001; n = 4). (e) % of BrdU+ fibres in the tibialis anterior (P = 0.0058; n = 6). (F) BrdU immunofluorescence, Bar = 50 μM. ANOVA, *P ≤ 0.05, **P ≤ 0.01, ***P ≤ 0.001.

We next used the thymidine analogue bromodeoxyuridine (BrdU) to label recently generated myofibres, as BrdU incorporates into newly synthesized DNA and therefore labels newly ‘born’ myofibres. Mice were given BrdU for 7 days at 19 weeks of age; BrdU+ centralized nuclei-containing myofibres were counted as an indicator of myoblasts that had proliferated and fused into myofibres during labelling. Approximately five per cent of mdx52 myofibres were BrdU+ after 1 week of labelling (Figure 4E,F). Although there were very few BrdU+ fibres in WT TAs, bmx showed a significant increase in the percentage of actively regenerating muscle fibres, which was intermediate to WT and mdx52 (0.1%, P = 0.0058; Figure 4E,F). These data show that bmx mice have increased regeneration and myofibre hypertrophy versus WT muscles while also having significantly less severe pathology versus mdx52.

We previously reported BMD patients with deletion of DMD exons 45–47 have decreased and variable dystrophin protein levels, whereas mRNA levels are unchanged.¹⁵ To determine if bmx mice recapitulate this phenotype, we first performed qRT-PCR using a probe against the Dmd 76–77 exon junction. We chose this junction as previous work shows that a 3–5′ destabilization of Dmd mRNA occurs in mdx52 and DMD muscle, so we reasoned a 3′-specific probe was more likely to show apparent differences in transcript abundance and stability.²² In all muscles measured (diaphragm, quad, TA, gastroc, triceps, heart), Dmd transcript levels were not decreased in bmx, whereas expectedly, Dmd was reduced in mdx52 muscles (Figure 5A). Additionally, in both TA and gastrocnemius muscles, bmx showed higher levels of Dmd mRNA than WT (TA + 28.85%, P = 0.0005, gastroc +57.54%, P = 0.0061). This shows that there is not a Dmd gene expression deficit in bmx, and conversely, in some muscles, Dmd transcript levels are more abundant than in WT.

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Figure 5. Dystrophin protein levels, but not RNA, are reduced in bmx mice. (A) qRT-PCR showing levels of Dmd mRNA as measured by a probe specific to the exon 76–77 junction in the diaphragm, quadriceps, tibialis anterior, gastrocnemius, triceps and heart of WT, bmx and mdx52 mice. n = 7–8. (B) Dystrophin (red) and laminin (green) immunofluorescence staining shows reduction of dystrophin in skeletal and cardiac muscles in bmx mice. DAPI was used as a counterstain to visualize myonuclei. Bar = 50 μM. ANOVA, *P ≤ 0.05, ****P 0.0001.

We assayed dystrophin protein levels via immunofluorescence and saw visual reductions in bmx skeletal and cardiac muscles versus WT (Figure 5B). We next performed capillary Western immunoassays (Wes), as dystrophin quantification using this method has proven to be highly sensitive, reproducible and quantitative over a large dynamic range.²⁸ Indeed, bmx skeletal and heart muscles showed, on average, ~50% less dystrophin than WT (diaphragm, P = 0.0002; triceps, P < 0.0001, heart, P = 0.0001; quadriceps, P = 0.0064; TA, P = 0.0016; gastroc, P = 0.0010) (Figures 6A,B and S4). In the diaphragm, we also detected the shorter, C-terminal, ubiquitously expressed dystrophin isoform Dp71. Consistent with previous reports,²⁹ we observed a ~2.5-fold increase in Dp71 expression in mdx52 diaphragms (P = 0.0445; Figure S5). bmx showed slightly elevated levels of Dp71 (~2-fold); however, this did not reach statistical significance (P = 0.126; Figure S5).

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Figure 6. Quantification of dystrophin protein in bmx mice using capillary Western assay and localization of dystrophin-associated proteins. (A) Dystrophin protein levels were determined by capillary electrophoresis immunoassay. Depicted is a virtual Wes blot. (B) Wes quantification in the diaphragm (P [less than] 0.0001), triceps (P [less than] 0.0001) and heart (P [less than] 0.0001) of bmx mice. ANOVA, n = 7–8. **P ≤ 0.01, ****P ≤ 0.0001. (C) nNOS immunofluorescence (red) was performed in the gastrocnemius muscles and shows an absence of staining for both bmx and mdx. (D) Immunofluorescence for the dystrophin-associated protein α-sarcoglycan (green) was performed in gastrocnemius muscles of WT, bmx and mdx52 muscles. Results show reduced staining and reduced colocalization in bmx and mdx52 at the sarcolemma. Laminin (red) was used to visualize all muscle fibres and DAPI was used as a counterstain to visualize myonuclei. Bar = 50 μM.

We next queried localization of nNOS and of the dystrophin-associated protein (DAP) α-sarcoglycan. Consistent with loss of dystrophin STR R17 (encoded by exon 45), which is necessary for nNOS binding,³⁰ bmx muscles showed complete loss of nNOS localization at the sarcolemma as did dystrophin-null mdx52 muscles (Figure 6C). Examining α-sarcoglycan localization via immunofluorescence we observed both reduced amounts and reduced colocalization at myofibre membranes in both bmx and mdx52 muscle (Figure 6D). Collectively, these data show bmx exhibit reduced association between dystrophin and DAPs at the sarcolemma; this is likely directly linked with the internal dystrophin truncation (nNOS) and reduced dystrophin levels (α-sarcoglycan) in bmx muscle.

We examined levels of inflammation-induced genes using a pre-determined inflammatory panel consisting of Tlr7, Il1b, Ccl2, Tnf and Irf1. Relative levels of inflammatory transcripts for all bmx muscles were determined versus WT and were plotted as a heat map (Figure 7A), which demonstrated that the gastroc muscle has the highest levels of inflammatory transcripts and Ccl2 is the most highly upregulated transcript across all bmx muscles. We also plotted individual transcript levels for WT, bmx and mdx52 gastrocs which demonstrated significant increases in Ccl2 (+375%, P = 0.0012) and Il1b (+80%, P = 0.0140) (Figure 7B). We also analysed miRNA panels that we have previously described—dystrophin-targeting miRNAs (DTMs)¹⁵ and inflammatory miRNAs,³¹ both regulated by the inflammatory transcription factor NF-κB. A heat map showing levels of inflammatory-driven miRNAs in bmx versus WT revealed that the gastroc expresses the highest levels of DTMs and inflammatory miRNAs (Figure 7C). Plotting individual miRNA expression levels in gastroc demonstrated increased DTMs (miR-146a, 72% increase, P = 0.0928; miR-31, 265% increase, P < 0.0001) and inflammatory miRNAs (miR-142-3p, 33.81% increase, P = 0.0183; miR-142-5p, 255.7% increase, P = 0.0583; Figure 7D,E).

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Figure 7. Muscle inflammation is present in bmx mice. (A) Heat map of inflammatory gene expression depicting fold change in bmx over WT in the diaphragm (Dia), quadriceps (Quad), gastrocnemius (Gas), triceps (Tri) and tibialis anterior (TA). (B) Ccl2 and Il1b are elevated in bmx gastrocnemius muscles n = 8. (C) Heat map of dystrophin-targeting miRNA and inflammatory miRNA expression depicting fold change in bmx over WT. (D) Graphs show elevated levels of dystrophin-targeting miRNAs miR-146a and miR-31 in bmx gastrocnemius muscles n = 8. (E) Graphs show elevated levels of chronic inflammatory miRNAs miR-142-3p and miR-142-5p in bmx gastrocnemius muscles. (F) Haematoxylin and eosin-stained gastrocnemius of WT, bmx and mdx52 mice. Left: representative images, right: quantification of dystrophic foci in muscles showing bmx mice have an increase in inflammation and necrosis n = 5. ANOVA. #P [less than] 0.10; *P [less than] 0.05; **P ≤ 0.01, ****P ≤ 0.0001.

BMD muscle biopsies show immune cell infiltration and myofibre necrosis.³² As bmx gastroc muscles were most affected at the molecular level, we next stained sections with haematoxylin and eosin (H&E) and quantified inflammation and necrosis (dystrophic foci). H&E staining visually demonstrated pathology in bmx, and quantification showed a 29% increase (P = 0.0021) in dystrophic foci as compared with WT (Figure 7F).

DMD muscles show high levels of fibrosis, and BMD patient muscles show variable fibrosis which inversely correlates with functional measures.³³ In mdx52, fibrosis is apparent in the diaphragm by 8–10 months of age and in other skeletal muscles by 20 months.³⁴ Preceding obvious fibrosis, elevated levels of fibrosis-associated genes and increased deposition of perimysial and endomysial collagen are observed.³⁵ We examined a panel of genes indicative of fibrosis signalling including Col1a1, Col3a1, Col6a1, Mmp2 and Tnc^36,37 and plotted relative levels in bmx (vs. WT) as a heat map for all muscles examined (Figure 8A). The bmx gastroc showed the highest upregulation of fibrosis-associated genes (Figure 8A,B). Representative graphs of a few fibrosis-associated transcripts show significant increases in Col1a1 (+188%, P = 0.0288), Col3a1 (+207%, P = 0.0452), and Tnc (+188%, P = 0.0273) in bmx gastroc (Figure 8B), as well as Col3a1 and Tnc in the TA (Figure S6A). Masson's trichrome staining showed increased collagen deposition in bmx versus WT quadriceps (P = 0.0083; Figures 8C and S6B), and Collagen 1a immunofluorescence showed visually increased collagen around the sarcolemma in bmx TA (Figure 8D). qPCR supported this observation (Figure 8D). Additionally, to assess muscle damage, quadriceps muscle sections were immunostained with an anti-IgM antibody. bmx mice had a visual increase in IgM-positive myofibres compared with WT mice (Figures 8E and S6C; P = 0.0878).

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Figure 8. Markers of fibrosis and muscle damage in bmx mice. (A) Heat map showing relative levels of fibrosis-associated genes in all bmx skeletal muscle analysed (vs. WT). (B) qRT-PCR of gastrocnemius muscle from WT, bmx and mdx52 muscles showing elevated Col1a1 (P = 0.0288), Col3a1 (P = 0.0452) and Tnc (P = 0.0273) n = 8. (C) Trichrome staining of quadriceps muscle from WT, bmx and mdx52 mice. Bmx mice show a 41.7% increase in fibrotic staining area (P = 0.0217), ANOVA. (D) left: Col1a1 immunofluorescence was performed in the tibialis anterior (TA) muscles and shows thickening around myofibres in bmx and mdx52 mice; right: qPCR of Col1a1 in TA muscles showed elevated expression in bmx (P = 0.0085) n = 8. (E) WT, bmx and mdx52 quadriceps were immunostained with an antibody against IgM to assess muscle damage. The bmx gastrocnemius muscles showed a 309.2% increase in IgM-positive myofibers (P = 0.0878; n = 3–4). ANOVA, *P ≤ 0.05, **P ≤ 0.01.

Here we describe the characterization of the bmx mouse generated using CRISPR/Cas9 to delete exons 45–47 of the endogenous murine Dmd gene. To our knowledge, this is the first described murine BMD model. These mice recapitulate several features of BMD and harbour a phenotype intermediate to healthy and mdx52 mice. Specifically, bmx mice show deficits in muscle and cardiac function, reduced dystrophin protein in skeletal and cardiac muscle, and histopathology consistent with moderate dystrophy.

A previous report described generation of the first BMD rat model in which exons 3–16 of the rat Dmd gene were deleted using CRISPR/Cas9.³⁸ The BMD rat shows muscle inflammation, muscle fibrosis, heart fibrosis and reduced dystrophin protein, but not mRNA. These molecular and histopathological deficits in the Becker rat, however, do not result in muscle function deficits. We have built upon this important first Becker model by generating and characterizing the first murine BMD model, which we refer to as the bmx mouse; we find histopathological and molecular deficits similar to the BMD rat and additionally observe reduced muscle function. The bmx model described here is thus an important addition to the DMD/BMD field and will enable direct comparisons with mdx studies previously performed.

Dystrophinopathy research has focused almost exclusively on DMD because patients completely lack dystrophin protein, which results in a more severe disease. Indeed, four AO exon skipping therapies, which lead to the production of a BMD-like dystrophin protein, have been approved for DMD. Availability of these drugs, with additional similar drugs in the pipeline, shifts the muscular dystrophy field into a new era where increased numbers of Becker-like patients will need care. Data from the bmx mouse presented here demonstrate that even if dystrophin restoration from exon skipping treatment achieves 100% efficacy, the resultant ‘Becker-like’ dystrophin may be expressed at lower-than-normal levels in muscle due to other factors, and therefore pathology including muscle damage, inflammation, weakness and cardiomyopathy will persist.

Deletion of DMD exons 45–47 (coding for 150 amino acids in the rod domain) is the most common BMD-causing mutation. Previous reports show that this deletion removes STR17, which is necessary for proper nNOS localization.³⁹ Because the exon boundaries do not perfectly correlate with the physical boundaries of individual STRs at the protein level, the 45–47 deletion also leads to a disruption or ‘out-of-phase’ structure of the rod domain's STR pattern.⁴⁰ Several natural history and longitudinal studies show ‘out-of-phase’ mutations lead to more severe disease outcomes. For instance, Bello et al. performed a longitudinal study that categorized BMD patients into groups: deletions beginning at exon 45 ‘del 45’, ending on exon 51 ‘del 51’ or other mutations.^S1 The ‘del 45’ group showed greater severity in almost every measure as compared with other BMD-causing mutations and had lower levels of dystrophin protein. A separate study demonstrated that the exon 45–47 deletion and other STR-disrupting or ‘out-of-phase’ deletions result in earlier onset dilated cardiomyopathy.⁴⁰ The phenotype we have described in the bmx mouse here is consistent with a ‘more severe’ Becker-like phenotype.

To understand the potential implications of DMD exon skipping and Becker-like dystrophin isoforms, much work has focused on natural history data from BMD patients that model the ‘result’ of skipping DMD exons 45, 51 and 53,^41,S2 (Clinical Trial #NCT01539772). Data presented here from bmx mice (model for exon 45 skipping) further contributes to this body of knowledge. bmx mice exhibit significant weakness and cardiac dysfunction despite substantial improvement in pathology over dystrophin-null mice. This supports the idea that exon skipping will slow DMD disease progression, but not completely ameliorate symptoms and pathology. Moving forward, creating additional Becker mouse models for comparison with the bmx mouse will help us to understand which truncated dystrophin isoforms will result in the best outcomes, both for BMD patients and for DMD patients with mutations amenable to exon skipping.

Despite a substantial improvement in pathology over dystrophin-null mice, we show here that bmx mice expressing 100% of a truncated in-frame dystrophin transcript still develop muscle weakness and cardiac dysfunction. In previous murine exon skipping studies, some reports show dystrophin protein levels as low as 30% can improve skeletal muscle degeneration.^S3 Other reports show that ~20% of dystrophin protein expression improves symptoms and that as little as 4% is sufficient to provide some benefit to muscle function and survival.^S4–S7 This brings up the much-debated question: ‘How much dystrophin protein is enough?’ Data presented here suggests that while 20–30% dystrophin protein will significantly improve disease severity, even if 100% of DMD dystrophin transcripts are skipped and therefore in-frame, some muscle damage, inflammation and weakness are still likely because dystrophin levels will be substantially lower than what is seen in healthy muscle.

Interestingly we see reduced dystrophin protein, but not mRNA, in bmx skeletal and cardiac muscle. This is consistent with our previous report showing reduced and variable dystrophin protein, but not mRNA, in BMD patient biopsies that harbour a deletion in DMD exons 45–47.¹⁵ In prior reports, we described dystrophin-targeting miRNAs (DTMs) that reduce dystrophin protein by binding to the dystrophin 3′ UTR.^15,41 Interestingly, in bmx muscles, we observe elevated levels of DTMs, with miR-146a and miR-31 being the most consistently up-regulated. It is likely that these miRNAs function to reduce dystrophin protein levels in bmx muscles. To definitively demonstrate this, however, future experiments in bmx mice will require targeting/inhibiting individual miRNAs, or administering DTM-reducing drugs, followed by a detailed assessment of changes in dystrophin protein levels. bmx muscles also have elevated levels of miRNAs from an ‘inflammatory miRNA’ panel that we previously reported.³¹ These miRNAs can ‘turn on’ NF-κB signalling, activating a positive feedforward loop of inflammation. The collective increase in these pathological miRNAs (DTMs and inflammatory miRNAs) coupled with the reduction in dystrophin protein likely exacerbates inflammation in bmx muscles. We have demonstrated a similar mechanism in myositis where we observe reduced dystrophin and increased pathological miRNAs.⁴¹ In early reports, others also noted abnormal and lower levels of dystrophin in human myositis biopsies.^S8 Further work to determine if this miRNA–dystrophin–inflammation axis is driving disease in other inflammatory muscle disorders will be important, especially given that elevated levels of these miRNAs are found in other muscle disorders.

The observation of slightly elevated Dp71 expression in the diaphragm is interesting, as a previous study showed increased Dp71 can have a dominant negative effect by displacing full-length dystrophin and further increasing muscle damage.^29,S9 Further, a recent report showed Dp71 overexpression can have detrimental effects on cardiac function.^S10 Though we did not observe a strong signal via Wes in the heart, it should be noted that high molecular weight capillaries that were used to resolve full-length dystrophin may have prevented full resolution of Dp71 signal in cardiac or other tissues. In future studies, it would be interesting to look at cardiac-specific expression over the lifetime of bmx.

Cardiac involvement is present in 70–80% of BMD patients and is a leading cause of mortality for this population.⁴⁰ Specifically, it has been reported that patients can present with arrhythmias, a decline in ejection fraction and dilated cardiomyopathy (DCM) similar to DMD patients.^S11 Interestingly, one study reported a significantly earlier DCM onset in BMD patients with an exon 45–47 deletion (median age of 27 years) versus patients with a 45–48 or 45–49 deletion (median ages of 38 and 41 years, respectively).^S12 Here we utilized echocardiography to measure heart function in aged bmx mice. We find bmx mice develop cardiac dysfunction characterized by a decrease in left ventricular ejection fraction and fractional shortening, consistent with BMD patients. In the clinic, BMD patients are also found to develop regional wall motion abnormalities, late gadolinium enhancement and reduced global strain. In future studies, it will be important to further characterize the life history of bmx hearts, identify preclinical changes, discover useful biomarkers for preclinical drug testing and determine the impact of various stressors on bmx cardiomyopathy.

Glucocorticoid treatment is a proven and FDA-approved intervention for DMD, which is associated with delayed loss of ambulation.^S13 However, glucocorticoid treatment is not commonly used for BMD and has an unclear risk–benefit ratio due to the safety concerns of chronic glucocorticoid treatment over the longer BMD disease course; thus far, the BMD population has avoided widespread glucocorticoid use due to a non-tolerability of glucocorticoid side effects such as weight gain, diabetes, muscle atrophy, bone fragility, adrenal suppression and mood disturbances. However, because we have observed increased NF-κB-driven inflammation, as measured by both expression analysis of genes such as Ccl2 and by quantification of H&E staining, it suggests that BMD patients could benefit from anti-inflammatory drug treatment regimens. Moving forward, the bmx mouse will enable us to look at how efficacy and safety profiles impact Becker-like phenotypes using both traditional glucocorticoids (prednisone and deflazacort) and next-generation drugs with improved safety profiles, such as vamorolone.^36,42 This can inform both current clinical management and future drug development for Becker patients.

There are several promising treatments in clinical trials for BMD. These include EDG-5506 (Edgewise Therapeutics) and vamorolone (ReveraGen BioPharma). Excitingly, EDG-5506 showed improvements in muscle damage biomarkers in a Phase I study of treated BMD patients.^S14 We hope that the generation of the bmx mouse will further advance treatments for BMD patients and enable the elucidation of the mechanism of action of treatments.

In conclusion, our characterization of novel bmx mice here demonstrates the utility of such a model to the DMD/BMD field. Moving forward, this model will be useful for conducting preclinical studies to test novel therapeutic targets or repurposed drugs for BMD and for identifying biomarkers of disease progression. As a follow-up to these studies, there is a need to generate more murine BMD models to better understand BMD disease progression, to test functionality of Becker-like dystrophin isoforms and to test various interventions that would benefit BMD patients and exon skipping-treated DMD patients.

We would like to thank Dr Shin'ichi Takeda for the generous gift of the mdx52 mice and Dr Nick Menhart for discussion of del 45–47 versus 45–48 isoforms. Edgewise would like to thank Dr Ben Robertson for setting up the ex vivo equipment and writing the custom data acquisition and analysis software. Generation and characterization of the bmx mouse was funded by the Recruitment Packages of CRH and AAF, which were provided by Children's National Hospital. CRH receives support from the Foundation to Eradicate Duchenne and the NIH (R01HL153054, R00HL130035, K99HL130035, L40AR068727). AAF receives support from the Foundation to Eradicate Duchenne and the Department of Defense (W81XWH-17-1-0475). The authors of this manuscript certify that they comply with the ethical guidelines for authorship and publishing in the Journal of Cachexia, Sarcopenia and Muscle.⁴³

AJR is co-founder and chief scientific officer of Edgewise Therapeutics. BNS is an employee of Edgewise Therapeutics. Edgewise Therapeutics did not fund the research and did not fund the generation or initial characterization of the bmx mouse model; AJR and BNS performed and analysed ex vivo muscle contraction experiments. CRH and AAF have filed a provisional intellectual property application related to the research in the manuscript.