Pedro Veliça1, Chris M Bunce. 1. School of Biosciences, University of Birmingham, Edgbaston, Birmingham B15 2TT, UK. velica@gmail.com
Abstract
INTRODUCTION: C2C12 myoblasts undergo in vitro myogenesis to form protein-rich multinucleated myotubes. Determining the fraction of total nuclei incorporated into myotubes is a commonly used method to quantify the extent of differentiation, but it is labor-intensive and susceptible to operator bias. METHODS: We have developed a simple method to quantify myotube formation using micrographs of Jenner-Giemsa-stained C2C12 cultures. Because myotubes are darkly stained by Jenner-Giemsa dyes, the extent of myotube formation correlates with an increase in pixels attributed to the darkest tones. Thus, image histograms were obtained from photographs using ImageJ software, and the sum of the darkest tones was used as a measure of myotube density. RESULTS: Measurements of myotube density mirrored those of fusion index during C2C12 differentiation and after treatment with prostaglandin D(2) , an inhibitor of C2C12 myogenesis. CONCLUSIONS: We propose this inexpensive, quick, and unbiased method to quantify C2C12 differentiation as a complement of the fusion index analysis.
INTRODUCTION: C2C12 myoblasts undergo in vitro myogenesis to form protein-rich multinucleated myotubes. Determining the fraction of total nuclei incorporated into myotubes is a commonly used method to quantify the extent of differentiation, but it is labor-intensive and susceptible to operator bias. METHODS: We have developed a simple method to quantify myotube formation using micrographs of Jenner-Giemsa-stained C2C12 cultures. Because myotubes are darkly stained by Jenner-Giemsa dyes, the extent of myotube formation correlates with an increase in pixels attributed to the darkest tones. Thus, image histograms were obtained from photographs using ImageJ software, and the sum of the darkest tones was used as a measure of myotube density. RESULTS: Measurements of myotube density mirrored those of fusion index during C2C12 differentiation and after treatment with prostaglandin D(2) , an inhibitor of C2C12 myogenesis. CONCLUSIONS: We propose this inexpensive, quick, and unbiased method to quantify C2C12 differentiation as a complement of the fusion index analysis.
Authors: L Simon; S M Ford; K Song; P Berner; C Vande Stouwe; S Nelson; G J Bagby; P E Molina Journal: Am J Physiol Regul Integr Comp Physiol Date: 2017-06-21 Impact factor: 3.619
Authors: Liz Simon; Nicole LeCapitaine; Paul Berner; Curtis Vande Stouwe; Jason C Mussell; Timothy Allerton; Stefany D Primeaux; Jason Dufour; Steve Nelson; Gregory J Bagby; William Cefalu; Patricia E Molina Journal: Am J Physiol Regul Integr Comp Physiol Date: 2014-03-26 Impact factor: 3.619