Florini J R, Ewton D Z, Coolican S A
Biology Department, Syracuse University, New York 13244, USA.
Endocr Rev. 1996 Oct;17(5):481-517. doi: 10.1210/edrv-17-5-481.
It is very clear that the GH-IGF axis plays a major role in controlling the growth and differentiation of skeletal muscles, as it does virtually all of the tissues in the animal body. One aspect of this control is unquestioned: circulating GH acts on the liver to stimulate expression of the IGF-I and IGFBP3 genes, substantially increasing the levels of these proteins in the circulation. It also seems that GH stimulates expression of IGF-I genes in skeletal muscle, although there are a number of cases in which skeletal muscle IGF-I expression is elevated in the absence of GH. It is substantially less clear that GH acts directly on skeletal muscle to stimulate its growth; the presence of GH receptor mRNA in skeletal muscle is well established, but most investigators have been unsuccessful in demonstrating any specific binding of GH to skeletal muscle or to myoblasts in culture. It has been equally difficult to show direct actions of GH on cultured muscle cells; the only positive report concludes that the early insulin-like effects of GH can result from direct interactions between GH and isolated muscle cells. The effects of the IGFs on skeletal muscle are much clearer. It is well established by studies in a number of laboratories on a variety of systems that IGFs stimulate many anabolic responses in myoblasts, as they do in other cell types. IGFs have the unusual property of stimulating both proliferation and differentiation of myoblasts, responses that are generally believed to be mutually exclusive; in myoblasts, they are in fact temporally separated. The stimulation of differentiation by IGF-I is (at least in part) a result of substantially increased levels of the mRNA for myogenin, the member of the MyoD family most directly associated with terminal myogenesis. As levels of myogenin mRNA rise, those of myf-5 mRNA (the only other member of the MyoD family expressed significantly in L6 myoblasts) fall dramatically, although myf-5 expression is required for the initial elevation of myogenin. The effects of IGFs are significantly modulated by IGFBPs secreted by myoblasts in serum-free medium, inhibitory IG-FBPs-4 and -6 are expressed and secreted by L6A1 myoblasts, while expression of IGFBP-5 rises dramatically as differentiation proceeds. Other myoblasts also secrete IGFBP-2. Even if exogenous IGFs are not added to the low-serum "differentiation" medium, myoblasts express sufficient amounts of autocrine IGF-II to stimulate myogenesis after a period of time; some myogenic cell lines, (such as Sol 8) are so active in expressing the IGF-II gene that it is not possible to demonstrate effects of exogenous IGFs. This autocrine expression of IGFs is by no means unique to skeletal muscle cells; indeed, it is so widely seen in cells responding to mitogenic stimuli that we suggest that IGFs can be viewed as extracellular second messengers that mediate most, if not all, such actions of agents that stimulate cell proliferation. The component of serum that suppresses IGF-II gene expression under "growth" conditions appears to be the IGFs themselves, which exhibit a very high potency in the feedback inhibition of IGF-II expression. In addition, IGFs have effects on the expression of other genes related to differentiation. Treatment of L6A1 cell with IGFs suppresses their expression of the myogenesis-inhibiting TGF beta s with a time course consistent with an initial proliferative step followed by differentiation, i.e. expression is first increased and then very substantially decreased. It is not established that this plays a role in control of differentiation, but experiments with FGF antisense constructs suggests that this may well be the case. Until recently, IGFs were the only circulating agents known to stimulate myoblast differentiation, in contrast to the relatively large number of growth factors that inhibit the process. It is now clear that thyroid hormones and RA also stimulate myogenesis, and that IL-15 enhances the stimulatory eff
很明显,生长激素(GH)-胰岛素样生长因子(IGF)轴在控制骨骼肌的生长和分化中起主要作用,就像它在动物体内几乎所有组织中所起的作用一样。这种控制的一个方面是毋庸置疑的:循环中的GH作用于肝脏,刺激IGF-I和IGFBP3基因的表达,从而大幅提高循环中这些蛋白质的水平。似乎GH也刺激骨骼肌中IGF-I基因的表达,尽管在许多情况下,骨骼肌IGF-I表达在没有GH的情况下也会升高。GH是否直接作用于骨骼肌以刺激其生长,这一点尚不清楚;骨骼肌中存在GH受体mRNA这一点已得到充分证实,但大多数研究人员未能证明GH与骨骼肌或培养中的成肌细胞有任何特异性结合。要证明GH对培养的肌肉细胞有直接作用同样困难;唯一的阳性报告得出结论,GH早期类似胰岛素的作用可能源于GH与分离的肌肉细胞之间的直接相互作用。IGF对骨骼肌的作用则要清晰得多。许多实验室在各种系统上进行的研究充分证实,IGF能刺激成肌细胞中的许多合成代谢反应,就像它们在其他细胞类型中所起的作用一样。IGF具有刺激成肌细胞增殖和分化的独特特性,而这两种反应通常被认为是相互排斥的;在成肌细胞中,它们实际上在时间上是分开的。IGF-I对分化的刺激(至少部分)是肌细胞生成素mRNA水平大幅增加的结果,肌细胞生成素是MyoD家族中与终末肌生成最直接相关的成员。随着肌细胞生成素mRNA水平的升高,myf-5 mRNA(MyoD家族中在L6成肌细胞中显著表达的另一个成员)的水平则急剧下降,尽管myf-5的表达是肌细胞生成素最初升高所必需的。血清中由成肌细胞分泌的IGF结合蛋白(IGFBPs)对IGF的作用有显著调节,抑制性IG-FBPs-4和-6由L6A1成肌细胞表达和分泌,而随着分化的进行,IGFBP-5的表达急剧上升。其他成肌细胞也分泌IGFBP-2。即使不向低血清的“分化”培养基中添加外源性IGF,成肌细胞也会在一段时间后表达足够量的自分泌IGF-II来刺激肌生成;一些成肌细胞系(如Sol 8)在表达IGF-II基因方面非常活跃,以至于无法证明外源性IGF的作用。IGF的这种自分泌表达绝非骨骼肌细胞所特有;事实上,在对有丝分裂刺激作出反应的细胞中广泛可见,因此我们认为IGF可被视为细胞外第二信使,介导大多数(如果不是全部)刺激细胞增殖的因子的此类作用。在“生长”条件下抑制IGF-II基因表达的血清成分似乎就是IGF本身,它们在对IGF-II表达的反馈抑制中表现出非常高的效力。此外,IGF对与分化相关的其他基因的表达也有影响。用IGF处理L6A1细胞会抑制它们对抑制肌生成的转化生长因子β(TGFβs)的表达,其时间进程与最初的增殖步骤随后的分化一致,即表达先增加然后大幅下降。目前尚不确定这在分化控制中是否起作用,但用成纤维细胞生长因子(FGF)反义构建体进行的实验表明很可能如此。直到最近,与相对大量抑制该过程的生长因子相比,IGF是已知的唯一能刺激成肌细胞分化的循环因子。现在很清楚,甲状腺激素和视黄酸(RA)也能刺激肌生成,而且白细胞介素-15能增强这种刺激作用。
