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肌细胞生成素(MyoD)DNA结合结构域包含肌肉特异性基因激活的识别密码。

The MyoD DNA binding domain contains a recognition code for muscle-specific gene activation.

作者信息

Davis R L, Cheng P F, Lassar A B, Weintraub H

机构信息

Department of Genetics, Hutchinson Cancer Research Center, Seattle, Washington 98104.

出版信息

Cell. 1990 Mar 9;60(5):733-46. doi: 10.1016/0092-8674(90)90088-v.

Abstract

A 60 amino acid domain of the myogenic determination gene MyoD is necessary and sufficient for sequence-specific DNA binding in vitro and myogenic conversion of transfected C3H10T1/2 cells. We show that a highly basic region, immediately upstream of the helix-loop-helix (HLH) oligomerization motif, is required for MyoD DNA binding in vitro. Replacing helix1, helix2, or the loop of MyoD with the analogous sequence of the Drosophila T4 achaete-scute protein (required for peripheral neurogenesis) has no substantial effect on DNA binding in vitro or muscle-specific gene activation in transfected C3H10T1/2 cells. However, replacing the basic region of MyoD with the analogous sequence of other HLH proteins (the immunoglobulin enhancer binding E12 protein or T4 achaete scute protein) allows DNA binding in vitro, yet abolishes muscle-specific gene activation. These findings suggest that a recognition code that determines muscle-specific gene activation lies within the MyoD basic region and that the capacity for specific DNA binding is insufficient to activate the muscle program.

摘要

肌源性决定基因MyoD的一个60个氨基酸的结构域对于体外序列特异性DNA结合以及转染的C3H10T1/2细胞的肌源性转化是必需且充分的。我们发现,在螺旋-环-螺旋(HLH)寡聚化基序上游紧邻的一个高度碱性区域是MyoD体外DNA结合所必需的。用果蝇T4无刚毛-盾片蛋白(外周神经发生所必需的)的类似序列替换MyoD的螺旋1、螺旋2或环,对体外DNA结合或转染的C3H10T1/2细胞中的肌肉特异性基因激活没有实质性影响。然而,用其他HLH蛋白(免疫球蛋白增强子结合E12蛋白或T4无刚毛-盾片蛋白)的类似序列替换MyoD的碱性区域,可允许体外DNA结合,但消除了肌肉特异性基因激活。这些发现表明,决定肌肉特异性基因激活的识别密码存在于MyoD碱性区域内,并且特异性DNA结合能力不足以激活肌肉程序。

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