In ovo L‐arginine supplementation stimulates myoblast differentiation but negatively affects muscle development of broiler chicken after hatching

Summary In this study, we tested the hypothesis that in ovo feeding (IOF) of L‐arginine (L‐Arg) enhances nitric oxide ( NO ) production, stimulates the process of myogenesis, and regulates post‐hatching muscle growth. Different doses of L‐Arg were injected into the amnion of chicken embryos at embryonic day ( ED ) 16. After hatching, the body weight of individual male chickens was recorded weekly for 3 weeks. During in vitro experiments, myoblasts of the pectoralis major ( PM ) were extracted at ED 16 and were incubated in medium containing 0.01 m m L‐Arg, 0.05 m m L‐Arg, and (or) 0.05 m m L‐nitro‐arginine‐methyl‐ester (L‐ NAME ), an inhibitor of nitric oxide synthase ( NOS ). When 25 mg/kg L‐Arg/initial egg weight was injected, no difference was observed in body weight at hatch, but a significant decrease was found during the following 3 weeks compared to that of the non‐injected and saline‐injected control, and this also affected the growth of muscle mass. L‐ NAME inhibited gene expression of myogenic differentiation antigen (MyoD), myogenin, NOS , and follistatin, decreased the cell viability, and increased myostatin ( MSTN ) gene expression. 0.05 m m L‐Arg stimulated myogenin gene expression but also depressed muscle cell viability. L‐ NAME blocked the effect of 0.05 m m L‐Arg on myogenin mRNA levels when co‐incubated with 0.05 m m L‐Arg. L‐Arg treatments had no significant influence on NOS mRNA gene expression, but had inhibiting effect on follistatin gene expression, while L‐ NAME treatments had effects on both. These results suggested that L‐Arg stimulated myoblast differentiation, but the limited number of myoblasts would form less myotubes and then less myofibers, while the latter limited the growth of muscle mass.