Literature DB >> 26891613

Cell Density and Joint microRNA-133a and microRNA-696 Inhibition Enhance Differentiation and Contractile Function of Engineered Human Skeletal Muscle Tissues.

Cindy S Cheng1, Lydia Ran1, Nenad Bursac1, William E Kraus1,2, George A Truskey1.   

Abstract

To utilize three-dimensional (3D) engineered human skeletal muscle tissue for translational studies and in vitro studies of drug toxicity, there is a need to promote differentiation and functional behavior. In this study, we identified conditions to promote contraction of engineered human skeletal muscle bundles and examined the effects of transient inhibition of microRNAs (miRs) on myogenic differentiation and function of two-dimensional (2D) and 3D cultures of human myotubes. In 2D cultures, simultaneously inhibiting both miR-133a, which promotes myoblast proliferation, and miR-696, which represses oxidative metabolism, resulted in an increase in sarcomeric α-actinin protein and the metabolic coactivator PGC-1α protein compared to transfection with a scrambled miR sequence (negative control). Although PGC-1α was elevated following joint inhibition of miRs 133a and 696, there was no difference in myosin heavy chain (MHC) protein isoforms. 3D engineered human skeletal muscle myobundles seeded with 5 × 10(6) human skeletal myoblasts (HSkM)/mL and cultured for 2 weeks after onset of differentiation consistently did not contract when stimulated electrically, whereas those seeded with myoblasts at 10 × 10(6) HSkM/mL or higher did contract. When HSkM were transfected with both anti-miRs and seeded into fibrin hydrogels and cultured for 2 weeks under static conditions, twitch and tetanic specific forces after electrical stimulation were greater than for myobundles prepared with HSkM transfected with scrambled sequences. Immunofluorescence and Western blots of 3D myobundles indicate that anti-miR-133a or anti-miR-696 treatment led to modest increases in slow MHC, but no consistent increase in fast MHC. Similar to results in 2D, only myobundles prepared with myoblasts treated with anti-miR-133a and anti-miR-696 produced an increase in PGC-1α mRNA. PGC-1α targets were differentially affected by the treatment. HIF-2α mRNA showed an expression pattern similar to that of PGC-1α mRNA, but COXII mRNA levels were not affected by the anti-miRs. Overall, joint inhibition of miR-133a and miR-696 accelerated differentiation, elevated the metabolic coactivator PGC-1α, and increased the contractile force in 3D engineered human skeletal muscle bundles.

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Year:  2016        PMID: 26891613      PMCID: PMC4841083          DOI: 10.1089/ten.TEA.2015.0359

Source DB:  PubMed          Journal:  Tissue Eng Part A        ISSN: 1937-3341            Impact factor:   3.845


  43 in total

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Review 4.  Tissue Elasticity Bridges Cancer Stem Cells to the Tumor Microenvironment Through microRNAs: Implications for a "Watch-and-Wait" Approach to Cancer.

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5.  Human, Tissue-Engineered, Skeletal Muscle Myobundles to Measure Oxygen Uptake and Assess Mitochondrial Toxicity.

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Journal:  Tissue Eng Part C Methods       Date:  2017-03-24       Impact factor: 3.056

Review 6.  Bio-instructive materials for musculoskeletal regeneration.

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7.  Tissue engineered skeletal muscle model of rheumatoid arthritis using human primary skeletal muscle cells.

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8.  Glucose Uptake and Insulin Response in Tissue-engineered Human Skeletal Muscle.

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Review 9.  Development and application of human skeletal muscle microphysiological systems.

Authors:  George A Truskey
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10.  MiR-696 Regulates C2C12 Cell Proliferation and Differentiation by Targeting CNTFRα.

Authors:  Han Wang; Lei Shi; Tingting Liang; BinBin Wang; WangJun Wu; Guosheng Su; Julong Wei; Pinghua Li; Ruihua Huang
Journal:  Int J Biol Sci       Date:  2017-03-11       Impact factor: 6.580

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