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Methylation and expression of the Myo D1 determination gene.

作者信息

Jones P A, Wolkowicz M J, Harrington M A, Gonzales F

机构信息

Kenneth Norris Jr Comprehensive Cancer Center, University of Southern California, Los Angeles 90033.

出版信息

Philos Trans R Soc Lond B Biol Sci. 1990 Jan 30;326(1235):277-84. doi: 10.1098/rstb.1990.0011.

Abstract

Mouse embryo cells induced to differentiate with the demethylating agent 5-azacytidine represent an excellent model system to investigate the molecular control of development. Clonal derivatives of 10T1/2 cells that have become determined to the myogenic or adipogenic lineages can be isolated from the multipotential parental line after drug treatment. These determined derivatives can be cultured indefinitely and will differentiate into end-stage phenotypes on appropriate stimulation. A gene called Myo D1, recently isolated from such a myoblast line, will confer myogenesis when expressed in 10T1/2 or other cell types (Davis et al. 1987). The cDNA for Myo D1 contains a large number of CpG sequences and the gene is relatively methylated in 10T1/2 cells and an adipocyte derivative, but is demethylated in myogenic derivatives. Myo D1 may therefore be subject to methylation control in vitro. On the other hand, preliminary observations suggest that Myo D1 is not methylated at CCGG sites in vivo so that a de novo methylation event may have occurred in vitro. These observations may have significance in the establishment of immortal cell lines and tumours.

摘要

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