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在通过添加Ca2+刺激融合的成肌细胞中磷脂酰肌醇的分解。

The breakdown of phosphatidylinositol in myoblasts stimulated to fuse by the addition of Ca2+.

作者信息

Wakelam M J, Pette D

出版信息

Biochem J. 1982 Mar 15;202(3):723-9. doi: 10.1042/bj2020723.

Abstract
  1. The fusion of chick-embryo myoblasts to produce myotubes was studied. The myoblasts were grown for 50 h in medium containing 10--20 microM-Ca2+; during this period they achieve fusion competence. 2. A rapid breakdown of phosphatidylinositol is also observed on addition of 1.4 mM-Ca2+ to these cells. This Ca2+ concentration also stimulates rapid myoblast fusion. 3. The breakdown is complete within 15 min and shows the same dependence on Ca2+ concentration as the fusion process. 4. Fusion-incompetence myoblasts and cells where fusion is inhibited by sodium butyrate exhibit no phosphatidylinositol breakdown on Ca2+ addition. 5. The Ca2+ ionophore A23187 inhibits the Ca2+-stimulated breakdown by about 50%, but has no effect on fusion. 6. A concomitant increase in 1,2-diacylglycerol labelled and fall in phosphatidylinositol labelling was observed when the lipids were labelling with [14C]glycerol on increasing the Ca2+ concentration in the medium to 1.4 mM. 7. We propose that the breakdown of phosphatidylinositol with a resultant increase in 1,2-diacylglycerol content of the cell membrane promotes myoblast fusion.
摘要
  1. 对鸡胚成肌细胞融合形成肌管的过程进行了研究。将成肌细胞在含有10 - 20微摩尔/升钙离子的培养基中培养50小时;在此期间,它们获得融合能力。2. 向这些细胞中添加1.4毫摩尔/升钙离子时,还观察到磷脂酰肌醇的快速分解。该钙离子浓度也刺激成肌细胞快速融合。3. 分解在15分钟内完成,并且与融合过程一样显示出对钙离子浓度的相同依赖性。4. 融合无能的成肌细胞以及融合被丁酸钠抑制的细胞在添加钙离子时不表现出磷脂酰肌醇分解。5. 钙离子载体A23187抑制钙离子刺激的分解约50%,但对融合没有影响。6. 当用[14C]甘油标记脂质,将培养基中的钙离子浓度提高到1.4毫摩尔/升时,观察到1,2 - 二酰基甘油标记物增加,磷脂酰肌醇标记物减少。7. 我们提出,磷脂酰肌醇的分解导致细胞膜中1,2 - 二酰基甘油含量增加,从而促进成肌细胞融合。

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