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骨骼肌细胞分化过程中的糖鞘脂:正常成肌细胞与融合缺陷型成肌细胞的比较

Glycosphingolipids during skeletal muscle cell differentiation: comparison of normal and fusion-defective myoblasts.

作者信息

Cambron L D, Leskawa K C

机构信息

Department of Anatomical Sciences and Neurobiology, School of Medicine, University of Louisville, KY 40292.

出版信息

Mol Cell Biochem. 1994 Jan 26;130(2):173-85. doi: 10.1007/BF01457398.

Abstract

The regulation of glycosphingolipid (GSL) synthesis in culture by fusion-competent (E63) myoblasts and fusion-defective (fu-1) cells was examined. Upon reaching confluency E63 cells fused to form multinucleated myotubes and demonstrated many characteristics of developing skeletal muscle including induction of creatine kinase activity and a shift in creatine kinase isozymes to the MM isoform. The fu-1 cells displayed none of these characteristics, despite the fact that both cells were cloned from the same parental myoblast line (rat L8). There was a transient increase in the synthesis of total neutral GSLs by E63 cells at the time of membrane fusion. In contrast, neutral GSL synthesis by fu-1 cells gradually decreased with time in culture. The major GSLs synthesized by both cell types were lactosylceramide and ganglioside GM3, with more complex structures being observed with prolonged time in culture. Several glycosyltransferase activities were assayed at varying times in culture. Generally, the changes in activities fell into three groups. One group was maximally activated at the end of the culture period (GalT-3, GalNAcT-1 and GalT-6). Another group was maximally activated during the time of active membrane fusion (GlcT and SAT-1). A third group was maximally activated at the time of cell contact and the beginning of membrane fusion (GlcNAcT-1 and GalT-2). In terms of the times of maximal activation there were few differences between E63 and fu-1 cells, with one notable exception. The activity of GalT-2 (lactosylceramide synthase) in E63 cells increased dramatically upon contact and the beginning of membrane fusion, whereas there were no changes in GalT-2 activity in fu-1 cells during time in culture. These results support our hypothesis that membrane glycosphingolipids play an important role in the differentiation of skeletal muscle cells.

摘要

研究了具有融合能力的(E63)成肌细胞和融合缺陷型(fu-1)细胞对培养中糖鞘脂(GSL)合成的调节作用。达到汇合状态时,E63细胞融合形成多核肌管,并表现出许多发育中骨骼肌的特征,包括肌酸激酶活性的诱导以及肌酸激酶同工酶向MM同工型的转变。尽管这两种细胞都克隆自同一亲本成肌细胞系(大鼠L8),但fu-1细胞却没有表现出这些特征。在膜融合时,E63细胞合成的总中性GSL有短暂增加。相比之下,fu-1细胞中性GSL的合成在培养过程中随时间逐渐减少。两种细胞类型合成的主要GSL是乳糖基神经酰胺和神经节苷脂GM3,随着培养时间延长,可观察到更复杂的结构。在培养的不同时间测定了几种糖基转移酶活性。一般来说,活性变化分为三组。一组在培养期结束时被最大程度激活(GalT-3、GalNAcT-1和GalT-6)。另一组在活跃膜融合时被最大程度激活(GlcT和SAT-1)。第三组在细胞接触和膜融合开始时被最大程度激活(GlcNAcT-1和GalT-2)。就最大激活时间而言,E63细胞和fu-1细胞之间几乎没有差异,但有一个明显例外。E63细胞中GalT-2(乳糖基神经酰胺合酶)的活性在接触和膜融合开始时急剧增加,而在培养期间fu-1细胞中GalT-2活性没有变化。这些结果支持了我们的假设,即膜糖鞘脂在骨骼肌细胞分化中起重要作用。

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