Muscle-specific RING finger-1 interacts with titin to regulate sarcomeric M-line and thick filament structure and may have nuclear functions via its interaction with glucocorticoid modulatory element binding protein-1

McElhinny, Abigail S.; Kakinuma, Kazumi; Sorimachi, Hiroyuki; Labeit, Siegfried; Gregorio, Carol C.

doi:10.1083/jcb.200108089

Cited by 227 publications

(209 citation statements)

References 56 publications

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“…Interaction of titin with MuRF1 in sarcomeres has previously been reported (13,18). Our data and that of other groups indicate that MuRF1 exists in multiple locations within the cell, including the cytosol, along the sarcomere, and within the nucleus.…”

Section: Discussionsupporting

confidence: 80%

“…Previous studies have shown that MuRF1 is found in several niches within myocytes: the cytosol, nucleus, and along myofibrils (13,18). We also observed similar localization of MuRF1 in cardiomyocytes treated with or without PE (Fig.…”

Section: Murf1supporting

confidence: 86%

“…These observations may be relevant to the role played by MuRF1 in the sarcomere. MuRF1 binds to titin and disrupts its interactions with the M-line without inducing the degradation of titin, thus partially disrupting sarcomere assembly (18). We hypothesize that MuRF1 may destabilize sarcomeres by binding to titin, which would in turn provide MuRF1 with access to its substrate troponin I. Troponin I could then be targeted for ubiquitylation and proteasome-dependent degradation by MuRF1.…”

Section: Discussionmentioning

confidence: 98%

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Muscle-specific RING finger 1 is a bona fide ubiquitin ligase that degrades cardiac troponin I

Kedar

McDonough

Arya

et al. 2004

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

293

245

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Muscle-specific RING finger protein 1 (MuRF1) is a sarcomereassociated protein that is restricted to cardiac and skeletal muscle. In skeletal muscle, MuRF1 is up-regulated by conditions that provoke atrophy, but its function in the heart is not known. The presence of a RING finger in MuRF1 raises the possibility that it is a component of the ubiquitin-proteasome system of protein degradation. We performed a yeast two-hybrid screen to search for interaction partners of MuRF1 in the heart that might be targets of its putative ubiquitin ligase activity. This screen identified troponin I as a MuRF1 partner protein. MuRF1 and troponin I were found to associate both in vitro and in vivo in cultured cardiomyocytes. MuRF1 reduced steady-state troponin I levels when coexpressed in COS-7 cells and increased degradation of endogenous troponin I protein in cardiomyocytes. The degradation of troponin I in cardiomyocytes was associated with the accumulation of ubiquitylated intermediates of troponin I and was proteasome-dependent. In vitro, MuRF1 functioned as a ubiquitin ligase to catalyze ubiquitylation of troponin I through a RING finger-dependent mechanism. In isolated cardiomyocytes, MuRF1 reduced indices of contractility. In cardiomyocytes, these processes may determine the balance between hypertrophic and antihypertrophic signals and the regulation of myocyte contractile responses in the setting of heart failure.

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Section: Discussionsupporting

confidence: 80%

Section: Murf1supporting

confidence: 86%

Section: Discussionmentioning

confidence: 98%

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Muscle-specific RING finger 1 is a bona fide ubiquitin ligase that degrades cardiac troponin I

Kedar

McDonough

Arya

et al. 2004

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

293

245

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“…46 MuRF-1 binds the giant sarcomeric protein titin, suggesting that MuRF-1 regulates the stability of the large structural protein. 47 In addition, Cohen et al 48 reported that MuRF-1 ubiquitinates MyBP-C, MyLC1, and MyLC2, including in myofibrils. Because these proteins stabilize the thick filament, their selective ubiquitination may facilitate thick filament disassembly.…”

Section: Discussionmentioning

confidence: 99%

XIAP Reduces Muscle Proteolysis Induced by CKD

Hu¹,

Zhang

et al. 2010

Journal of the American Society of Nephrology

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X-chromosome-linked inhibitor of apoptosis protein (XIAP) is an endogenous caspase inhibitor. Caspase-3 contributes to the muscle wasting associated with chronic kidney disease (CKD) and other systemic illnesses, but whether XIAP modulates muscle wasting in CKD is unknown. Here, overexpression of XIAP in cultured skeletal muscle cells decreased protein degradation induced by serum deprivation, suggesting that caspase-mediated proteolysis contributes to muscle atrophy. We generated transgenic mice that overexpress human XIAP specifically in skeletal muscle (mXIAP) and evaluated muscle protein degradation induced by CKD. mXIAP mice with normal kidney function exhibited mild skeletal muscle hypertrophy. Muscle weights of mXIAP mice with CKD (mXIAP-CKD) were indistinguishable from wild-type mice, suggesting that overexpression of XIAP in skeletal muscle protects from CKD-induced muscle atrophy. The rate of total protein degradation, proteasome chymotrypsin-like activity, and caspase-3-mediated actin cleavage all were lower in muscle isolated from mXIAP-CKD mice compared with wild-type CKD mice. Concomitant with the reduction in overall proteolysis, mRNA levels of ubiquitin, muscle-specific ring finger 1, and atrogin-1/muscle atrophy F-box were lower in mXIAP-CKD mice, suggesting that decreased expression of the ubiquitin-proteasome pathway components may contribute to the protein-sparing effects of XIAP. In summary, these results demonstrate that XIAP inhibits multiple aspects of protein degradation in skeletal muscle during CKD.

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“…These two genes correspond to ubiquitinprotein ligases expressed solely in skeletal and cardiac muscle that mediate the processes of muscle remodeling and increase proteolysis of disuse atrophy. For instance, MURF1 was firstly identified as the ubiquitin-ligase responsible for the direct binding and degradation of titin, a huge myofibrillar protein, and myosin heavy chain (McElhinny et al 2002;Clarke et al 2007). Further confirm of the functional role of these atrogenes came from the experiments performed on MAFbx-/-and MURF1-/-transgenic mice, refractory to muscle-loss phenomena induced by denervation.…”

Section: Atrophy and Atrogenesmentioning

confidence: 99%

Cellular mechanisms and local progenitor activation to regulate skeletal muscle mass

Cassano

Quattrocelli

Crippa

et al. 2009

J Muscle Res Cell Motil

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Skeletal muscle hypertrophy is a result of increased load, such as functional and stretch-overload. Activation of satellite cells and proliferation, differentiation and fusion are required for hypertrophy of overloaded skeletal muscles. On the contrary, a dramatic loss of skeletal muscle mass determines atrophy settings. The epigenetic changes involved in gene regulation at DNA and chromatin level are critical for the opposing phenomena, muscle growth and atrophy. Physiological properties of skeletal muscle tissue play a fundamental role in health and disease since it is the most abundant tissue in mammals. In fact, protein synthesis and degradation are finely modulated to maintain an appropriate muscle mass. When the molecular signaling is altered muscle wasting and weakness occurred, and this happened in most common inherited and acquired disorders such as muscular dystrophies, cachexia, and age-related wasting. To date, there is no accepted treatment to improve muscle size and strength, and these conditions pose a considerable anxiety to patients as well as to public health. Several molecules, including Magic-F1, myostatin inhibitor, IGF, glucocorticoids and microRNAs are currently investigated to interfere positively in the blueprint of skeletal muscle growth and regeneration.

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Muscle-specific RING finger-1 interacts with titin to regulate sarcomeric M-line and thick filament structure and may have nuclear functions via its interaction with glucocorticoid modulatory element binding protein-1

Cited by 227 publications

References 56 publications

Muscle-specific RING finger 1 is a bona fide ubiquitin ligase that degrades cardiac troponin I

Muscle-specific RING finger 1 is a bona fide ubiquitin ligase that degrades cardiac troponin I

XIAP Reduces Muscle Proteolysis Induced by CKD

Cellular mechanisms and local progenitor activation to regulate skeletal muscle mass

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