Höllrigl Alexandra, Hofner Manuela, Stary Martina, Weitzer Georg
Max F. Perutz Laboratories, Department of Medical Biochemistry, Medical University of Vienna, Dr. Bohrgasse 9, A1030 Vienna, Austria.
Differentiation. 2007 Sep;75(7):616-26. doi: 10.1111/j.1432-0436.2007.00163.x. Epub 2007 Mar 23.
Desmin contributes to the stability of the myocardium and its amino-terminal domain influences intermediate filament formation and interacts with a variety of proteins and DNAs. Specific serine residues located in this domain are reversibly phosphorylated in a cell cycle and developmental stage-dependent manner as has been demonstrated also for other cytoplasmic type III intermediate filament proteins. Although absence of desmin apparently does not affect cardiomyogenesis, homozygous deletion of the amino-terminal domain of desmin severely inhibited in vitro cardiomyogenesis. To demonstrate the significance of phosphorylation of this domain in cardiomyogenic commitment and differentiation, we inhibited phosphorylation of serine residues 6, 7, and 8 by mutation to alanine, and investigated early cardiomyogenesis in heterozygous embryoid bodies. As control, serine residues 31 and 32, which are not phosphorylated by kinases mutating serine residues 6, 7, and 8, were mutated to alanine in a second set. Desmin(S6,7,8A) interfered with cardiomyogenesis and myofibrillogenesis in a dominant negative fashion, whereas desmin(S31,32A) produced only a mild phenotype. Desmin(S6,7,8A) led to the down-regulation of the transcription factor genes brachyury, goosecoid, nkx2.5, and mef2C and increased apoptosis of presumptive mesoderm and differentiating cardiomyocytes. Surviving cardiomyocytes which were few in number had no myofibrils. Demonstration that some but not any mutant desmin interfered with the very beginning of cardiomyogenesis suggests an important function of temporarily phosphorylated serine residues 6, 7, and 8 in the amino-terminal domain of desmin in cardiomyogenic commitment and differentiation.
结蛋白有助于心肌的稳定性,其氨基末端结构域影响中间丝的形成,并与多种蛋白质和DNA相互作用。该结构域中的特定丝氨酸残基在细胞周期和发育阶段依赖性的方式下发生可逆磷酸化,其他细胞质III型中间丝蛋白也有类似情况。虽然缺乏结蛋白显然不影响心肌发生,但结蛋白氨基末端结构域的纯合缺失严重抑制了体外心肌发生。为了证明该结构域磷酸化在心肌定向分化和分化中的重要性,我们通过将丝氨酸残基6、7和8突变为丙氨酸来抑制其磷酸化,并研究杂合胚状体中的早期心肌发生。作为对照,在另一组实验中,将不被使丝氨酸残基6、7和8突变的激酶磷酸化的丝氨酸残基31和32突变为丙氨酸。结蛋白(S6,7,8A)以显性负性方式干扰心肌发生和肌原纤维形成,而结蛋白(S31,32A)仅产生轻微表型。结蛋白(S6,7,8A)导致转录因子基因短尾、鹅膏蕈碱、nkx2.5和mef2C的下调,并增加推定中胚层和分化心肌细胞的凋亡。存活的心肌细胞数量很少且没有肌原纤维。一些而非所有突变结蛋白干扰心肌发生起始的结果表明,结蛋白氨基末端结构域中暂时磷酸化的丝氨酸残基6、7和8在心肌定向分化和分化中具有重要功能。