Role of insulin-like growth factor binding protein-3 (IGFBP-3) in the differentiation of primary human adult skeletal myoblasts

Abstract

Although muscle satellite cells were identified almost 40 years ago, little is known about the induction of their proliferation and differentiation in response to physiological/pathological stimuli or to growth factors/cytokines. In order to investigate the role of the insulin‐like growth factor (IGF)/IGF binding protein (IGFBP) system in adult human myoblast differentiation we have developed a primary human skeletal muscle cell model. We show that under low serum media (LSM) differentiating conditions, the cells secrete IGF binding proteins‐2, ‐3, ‐4 and ‐5. Intact IGFBP‐5 was detected at days 1 and 2 but by day 7 in LSM it was removed by proteolysis. IGFBP‐4 levels were also decreased at day 7 in the presence of IGF‐I, potentially by proteolysis. In contrast, we observed that IGFBP‐3 initially decreased on transfer of cells into LSM but then increased with myotube formation. Treatment with 20 ng/ml tumour necrosis factor‐alpha (TNFα), which inhibits myoblast differentiation, blocked IGFBP‐3 production and secretion whereas 30 ng/ml IGF‐I, which stimulates myoblast differentiation, increased IGFBP‐3 secretion. The TNFα‐induced decrease in IGFBP‐3 production and inhibition of differentiation could not be rescued by addition of IGF‐I. LongR~3~IGF‐I, which does not bind to the IGFBPs, had a similar effect on differentiation and IGFBP‐3 secretion as IGF‐I, both with and without TNFα, confirming that increased IGFBP‐3 is not purely due to increased stability conferred by binding to IGF‐I. Furthermore reduction of IGFBP‐3 secretion using antisense oligonucleotides led to an inhibition of differentiation. Taken together these data indicate that IGFBP‐3 supports myoblast differentiation. © 2003 Wiley‐Liss, Inc.