Mouse models of two missense mutations in actin-binding domain 1 of dystrophin associated with Duchenne or Becker muscular dystrophy

McCourt, Jackie L; Talsness, Dana M; Lindsay, Angus; Arpke, Robert W.; Chatterton, Paul D; Nelson, D'anna M.; Chamberlain, Christopher M.; Olthoff, John; Belanto, Joseph J.; McCourt, Preston M.; Kyba, Michael; Lowe, Dawn A.; Ervasti, James M.

doi:10.1093/hmg/ddx414

Cited by 15 publications

(28 citation statements)

References 47 publications

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“…The simultaneous induction of ZFAND5 by enhancing the proteasomes' degradative activity should promote the clearance of these ubiquitinated proteins, presumably to promote the efficient clearance of ubiquitinated proteins. Moreover, some forms of Duchenne and Becker muscular dystrophy are due to missense mutations in dystrophin that lead to its rapid degradation by the UPS, and recently down-regulation of ZFAND5 was shown to raise the levels of this critical protein (11). Because down-regulation of ZFAND5 reduced muscle wasting and proteolysis by the UPS, pharmacological antagonists of ZFAND5 might represent a therapy to ameliorate the debilitating loss of muscle protein in various cachectic conditions, as well as in these muscular dystrophies.…”

Section: Discussionmentioning

confidence: 99%

“…These findings strongly suggest ZFAND5's involvement in protein breakdown (9), especially in the accelerated proteolysis responsible for skeletal muscle wasting. Accordingly, downregulation of ZFAND5 (and several other components of the ubiquitin proteasome system) in mouse muscle was recently found to raise the levels of a mutant form of dystrophin found in Duchenne muscular dystrophy (11). In addition, in the macrophage line, RAW264.7, ZFAND5 expression is induced by RANKL, TNFα, and IL-1β, and its expression inhibits their differentiation into octeoclasts (12).…”

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confidence: 99%

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ZFAND5/ZNF216 is an activator of the 26S proteasome that stimulates overall protein degradation

Lee

Takayama

Goldberg

2018

Proc. Natl. Acad. Sci. U.S.A.

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ZFAND5/ZNF216, a member of the zinc finger AN1-type domain family, is abundant in heart and brain, but is induced in skeletal muscle during atrophy (although not in proteotoxic stress). Because mice lacking ZFAND5 exhibit decreased atrophy, a role in stimulating protein breakdown seemed likely. Addition of recombinant ZFAND5 to purified 26S proteasomes stimulated hydrolysis of ubiquitinated proteins, short peptides, and ATP. Mutating its C-terminal AN1 domain abolished the stimulation of proteasomal peptidase activity. Mutating its N-terminal zinc finger A20 domain, which binds ubiquitin chains, prevented the enhanced degradation of ubiquitinated proteins without affecting peptidase activity. Mouse embryonic fibroblast (MEF) cells lacking ZFAND5 had lower rates of protein degradation and proteasomal activity than WT MEFs. ZFAND5 addition to cell lysates stimulated proteasomal activity and protein degradation. Unlike other proteasome regulators, ZFAND5 enhances multiple 26S activities and overall cellular protein breakdown.

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Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 99%

ZFAND5/ZNF216 is an activator of the 26S proteasome that stimulates overall protein degradation

Lee

Takayama

Goldberg

2018

Proc. Natl. Acad. Sci. U.S.A.

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“…Each ECC was separated by 3 min of rest to prevent fatigue. The corresponding force drop associated with this protocol for mdx EDL muscle is 85–90% but variations in mechanical parameters across other laboratories can cause force drop from 39% to 90% . The force measured at each ECC was expressed as a percentage of the force produced during the first (“initial”) contraction.…”

Section: Methodsmentioning

confidence: 99%

Variable cytoplasmic actin expression impacts the sensitivity of different dystrophin‐deficient mdx skeletal muscles to eccentric contraction

et al. 2019

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Eccentric contractions (ECCs) induce force loss in several skeletal muscles of dystrophin‐deficient mice (mdx), with the exception of the soleus (Sol). The eccentric force : isometric force (ECC : ISO), expression level of utrophin, fiber type distribution, and sarcoendoplasmic reticulum calcium ATPase expression are factors that differ between muscles and may contribute to the sensitivity of mdx skeletal muscle to ECC. Here, we confirm that the Sol of mdx mice loses only 13% force compared to 87% in the extensor digitorum longus (EDL) following 10 ECC of isolated muscles. The Sol has a greater proportion of fibers expressing Type I myosin heavy chain (MHC) and expresses 2.3‐fold more utrophin compared to the EDL. To examine the effect of ECC : ISO, we show that the mdx Sol is insensitive to ECC at ECC : ISO up to 230 ± 15%. We show that the peroneus longus (PL) muscle presents with similar ECC : ISO compared to the EDL, intermediate force loss (68%) following 10 ECC, and intermediate fiber type distribution and utrophin expression relative to EDL and Sol. The combined absence of utrophin and dystrophin in mdx/utrophin−/− mice rendered the Sol only partially susceptible to ECC and exacerbated force loss in the EDL and PL. Most interestingly, the expression levels of cytoplasmic β‐ and γ‐actins correlate inversely with a given muscle's sensitivity to ECC; EDL < PL < Sol. Our data indicate that fiber type, utrophin, and cytoplasmic actin expression all contribute to the differential sensitivities of mdxEDL, PL, and Sol muscles to ECC.

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“…Although it is still under debate, a more than 90% decrease of normal dystrophin levels might have a critical effect on the clinical severity of patients with BMD. Previous studies examined the mechanisms underlying the decrease of tdp427, using in vitro analyses or transgenic mice that overexpress tdp427, and showed that the decreased level of tdp427 was caused by protein degradation following the tertiary instability of the protein ( Henderson et al, 2011 ; McCourt et al, 2015 , 2018 ). However, as patients with BMD exhibit endogenous tdp427 expression under normal promoter activity, such an in vitro or overexpressed tdp427 scenario might not mimic the physiological environment in muscle tissues of patients with BMD.…”

Section: Introductionmentioning

confidence: 99%

Pathological evaluation of rats carrying in-frame mutations in the dystrophin gene: a new model of Becker muscular dystrophy

Teramoto

Sugihara

Yamanouchi

et al. 2020

Disease Models &Amp; Mechanisms

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Dystrophin, encoded by the DMD gene on the X chromosome, stabilizes the sarcolemma by linking the actin cytoskeleton with the dystrophin-glycoprotein complex (DGC). In-frame mutations in DMD cause a milder form of X-linked muscular dystrophy, called Becker muscular dystrophy (BMD), characterized by the reduced expression of truncated dystrophin. So far, no animal model with in-frame mutations in Dmd has been established. As a result, the effect of in-frame mutations on the dystrophin expression profile and disease progression of BMD remains unclear. In this study, we established a novel rat model carrying in-frame Dmd gene mutations (IF rats) and evaluated the pathology. We found that IF rats exhibit reduced expression of truncated dystrophin in a proteasome-independent manner. This abnormal dystrophin expression caused dystrophic changes in muscle tissues, but did not lead to functional deficiency. We also found that the expression of additional dystrophin named dpX, which forms the DGC in the sarcolemma, is associated with the appearance of truncated dystrophin. In conclusion, the outcomes of this study contribute to the further understanding of BMD pathology and help elucidate the efficiency of dystrophin recovery treatments in Duchenne muscular dystrophy, a more severe form of X-linked muscular dystrophy.

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Mouse models of two missense mutations in actin-binding domain 1 of dystrophin associated with Duchenne or Becker muscular dystrophy

Cited by 15 publications

References 47 publications

ZFAND5/ZNF216 is an activator of the 26S proteasome that stimulates overall protein degradation

ZFAND5/ZNF216 is an activator of the 26S proteasome that stimulates overall protein degradation

Variable cytoplasmic actin expression impacts the sensitivity of different dystrophin‐deficient mdx skeletal muscles to eccentric contraction

Pathological evaluation of rats carrying in-frame mutations in the dystrophin gene: a new model of Becker muscular dystrophy

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