HEMA 3 Staining: A Simple Alternative for the Assessment of Myoblast Differentiation

Levitt, Danielle E.; Adler, Katherine; Simon, Liz

doi:10.1002/cpsc.101

Cited by 11 publications

(13 citation statements)

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“…After the 6th day of differentiation, the cells were fixed by methanol. The staining protocol was then performed as previously described [ 21 ]. In brief, the fusion index was calculated by staining the fixed cell and determining the number of nuclei in a myotubule compared to the total number of nuclei in the sample using an inverted Delta Optical IB-100 light microscope.…”

Section: Methodsmentioning

confidence: 99%

Spexin Promotes the Proliferation and Differentiation of C2C12 Cells In Vitro—The Effect of Exercise on SPX and SPX Receptor Expression in Skeletal Muscle In Vivo

Leciejewska

Pruszyńska‐Oszmałek

Mielnik

et al. 2021

Genes

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SPX (spexin) and its receptors GalR2 and GalR3 (galanin receptor subtype 2 and galanin receptor subtype 3) play an important role in the regulation of lipid and carbohydrate metabolism in human and animal fat tissue. However, little is still known about the role of this peptide in the metabolism of muscle. The aim of this study was to determine the impact of SPX on the metabolism, proliferation and differentiation of the skeletal muscle cell line C2C12. Moreover, we determined the effect of exercise on the SPX transduction pathway in mice skeletal muscle. We found that increased SPX, acting via GalR2 and GalR3 receptors, and ERK1/2 phosphorylation stimulated the proliferation of C2C12 cells (p < 0.01). We also noted that SPX stimulated the differentiation of C2C12 by increasing mRNA and protein levels of differentiation markers Myh, myogenin and MyoD (p < 0.01). SPX consequently promoted myoblast fusion into the myotubule (p < 0.01). Moreover, we found that, in the first stage (after 2 days) of myocyte differentiation, GalR2 and GalR3 were involved, whereas in the last stage (day six), the effect of SPX was mediated by the GalR3 isoform. We also noted that exercise stimulated SPX and GalR2 expression in mice skeletal muscle as well as an increase in SPX concentration in blood serum. These new insights may contribute to a better understanding of the role of SPX in the metabolism of skeletal muscle.

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Section: Methodsmentioning

confidence: 99%

Spexin Promotes the Proliferation and Differentiation of C2C12 Cells In Vitro—The Effect of Exercise on SPX and SPX Receptor Expression in Skeletal Muscle In Vivo

Leciejewska

Pruszyńska‐Oszmałek

Mielnik

et al. 2021

Genes

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“…Primary myoblasts were isolated from vastus lateralis muscle samples as previously described (Levitt et al, 2019; Simon et al, 2014, 2017). Samples were washed 3 times in Ham’s F‐12 nutrient mixture (GE Healthcare Life Sciences, Marlborough, MA), minced, and trypsin‐digested (0.25% trypsin EDTA diluted 1:4 in Ham’s F‐12).…”

Section: Methodsmentioning

confidence: 99%

“…Myoblast cell culture was performed according to our previously published detailed methods (Adler et al, 2019; Levitt et al, 2019). Myoblasts were seeded in growth media at a density of 2.8 × 10 3 cells per cm 2 on collagen‐coated 6‐well plates containing either 0 or 50 mM EtOH and maintained in cell culture incubators under standard culture conditions (5% CO 2 , 37°C) until reaching 70 to 80% confluence (3 days).…”

Section: Methodsmentioning

confidence: 99%

“…Fixed cells were stored covered at room temperature until staining. Fixed cells were stained using our previously published HEMA 3 method (Levitt et al, 2019). Cells were treated with HEMA 3 solution I (Fisher HealthCare, Inc., Waltham, MA) for 10 minutes at room temperature.…”

Section: Methodsmentioning

confidence: 99%

“…For each image, total nuclei and nuclei fused into myotubes were counted using ImageJ. Myotubes per field were calculated as the number of cells with 3 or more nuclei and fusion index was calculated as the percentage of all nuclei fused into myotubes (Adler et al, 2019; Levitt et al, 2019; Simon et al, 2014). Final calculations of fusion index, myotubes per field, and total nuclei across the 15 images per well were averaged for analysis.…”

Section: Methodsmentioning

confidence: 99%

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Ethanol‐Impaired Myogenic Differentiation is Associated With Decreased Myoblast Glycolytic Function

Levitt

Chalapati

Prendergast

et al. 2020

Alcoholism Clin & Exp Res

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Background: Myopathy affects nearly half of individuals with alcohol use disorder (AUD), and impaired skeletal muscle regenerative potential is a probable contributing factor. Previous findings from our laboratory indicate that chronic in vivo and in vitro ethanol (EtOH) treatment decreases myogenic potential of skeletal muscle myoblasts. Myogenesis, a highly coordinated process, requires shifts in cellular metabolic state allowing for myoblasts to proliferate and differentiate into mature myotubes. The objective of this study was to determine whether alcohol interferes with myoblast mitochondrial and glycolytic metabolism and impairs myogenic differentiation. Methods: Myoblasts were isolated from vastus lateralis muscle excised from alcohol-na€ ıve adult male (n = 5) and female (n = 5) rhesus macaques. Myoblasts were proliferated for 3 days (day 0 differentiation; D0) and differentiated for 5 days (D5) with or without 50 mM EtOH. Metabolism was assessed using a mitochondrial stress test to measure oxygen consumption (OCR) and extracellular acidification (ECAR) rates at D0. Differentiation was examined at D5. Expression of mitochondrial and glycolytic genes and mitochondrial DNA (mtDNA) was measured at D0 and D5. Results: Ethanol significantly (p < 0.05) increased myoblast maximal OCR and decreased ECAR at D0, and decreased fusion index, myotubes per field, and total nuclei at D5. The EtOH-induced decrease in ECAR was associated with the EtOH-mediated decreases in fusion index and myotubes per field. EtOH did not alter the decrease in glycolytic gene expression and increase in mtDNA from D0 to D5. Conclusion: During myoblast proliferation, EtOH decreased glycolytic metabolism and increased maximal OCR, suggesting that myoblast metabolic phenotype was dysregulated with EtOH. The EtOH-induced decrease in ECAR was associated with decreased differentiation. These findings suggest that EtOH-mediated shifts in metabolic phenotype may underlie impaired differentiation, which has important clinical implications for myogenesis in those affected by alcoholic myopathy.

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Modulating Myogenesis: An Optimized In Vitro Assay to Pharmacologically Influence Primary Myoblast Differentiation

et al. 2022

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The intentional pharmacological manipulation of myogenesis is an important technique for understanding the underlying mechanisms of muscle differentiation and disease etiology. Using the pharmacological agent metformin as an example molecule, we present a systematic approach to examine the impact of pharmacological agents on the myogenic program. This consists of optimizing the in vitro differentiation of primary myoblast cells followed by the generation of a dose‐response curve for a respective pharmaceutical. To assess myogenic differentiation, we utilized three approaches (incorporating both transcriptional and protein techniques) to assess the effects of biologically active agents on the in vitro differentiation of primary myogenic progenitors. First, the immunofluorescent visualization of myosin heavy chain (MYHC), which is expressed in differentiated myofibers, is used to obtain the fusion index, a quantitative read‐out of differentiation efficiency. Second, quantitative reverse transcription PCR (RT‐qPCR) reveals the expression of myogenic factors (Pax7, Myf5, Myod, Myog, Myh2) at the transcript level. Third, western blotting is used to assess the protein expression levels of the myogenic markers (PAX7, MYF5, MYOD, MYOG, and MYHC). By monitoring the expression of these various myogenic factors during the differentiation process, the relative cellular state and differentiation status between samples can be determined. Combined, these approaches enable the successful assessment of the impact of pharmacological agents on myogenic differentiation. © 2022 The Authors. Current Protocols published by Wiley Periodicals LLC. Basic Protocol: Immunofluorescence assay for qualitative and quantitative assessment of pharmacological agents on in vitro myogenic differentiation Support Protocol 1: Evaluating myogenic gene expression by RT‐qPCR Support Protocol 2: Evaluating myogenic protein expression by western blot

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HEMA 3 Staining: A Simple Alternative for the Assessment of Myoblast Differentiation

Cited by 11 publications

References 13 publications

Spexin Promotes the Proliferation and Differentiation of C2C12 Cells In Vitro—The Effect of Exercise on SPX and SPX Receptor Expression in Skeletal Muscle In Vivo

Spexin Promotes the Proliferation and Differentiation of C2C12 Cells In Vitro—The Effect of Exercise on SPX and SPX Receptor Expression in Skeletal Muscle In Vivo

Ethanol‐Impaired Myogenic Differentiation is Associated With Decreased Myoblast Glycolytic Function

Modulating Myogenesis: An Optimized In Vitro Assay to Pharmacologically Influence Primary Myoblast Differentiation

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