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杜兴氏肌营养不良基因一种新的主要转录本的特征及细胞类型分布

Characterization and cell type distribution of a novel, major transcript of the Duchenne muscular dystrophy gene.

作者信息

Rapaport D, Lederfein D, den Dunnen J T, Grootscholten P M, Van Ommen G J, Fuchs O, Nudel U, Yaffe D

机构信息

Department of Cell Biology, Weizmann Institute of Science, Rehovot, Israel.

出版信息

Differentiation. 1992 Apr;49(3):187-93. doi: 10.1111/j.1432-0436.1992.tb00666.x.

Abstract

Previously we identified a novel 6.5 kb mRNA transcribed from the Duchenne muscular dystrophy (DMD) gene. This mRNA differs in coding content and tissue distribution from the known muscle type and brain type 14 kb DMD mRNAs which code for dystrophin. The novel transcript shares with dystrophin most of the sequence coding for the cysteine-rich and C-terminal domains. Here we used cDNA cloning to identify the divergence point between the common region and the sequence unique to the novel mRNA at the 5' end of the sequence encoding the cysteine-rich domain of dystrophin. This unique sequence containing the translation initiation site is located in a new exon in the intron between exons 62 and 63 of the dystrophin gene. Using probes containing RNA sequences specific to the novel mRNA, we investigated the expression of this mRNA in various tissues and cell types. The study reveals that this mRNA is the main DMD gene product detectable in a variety of nonmuscle tissues including brain cells. The amount of this mRNA in some tissues is comparable to the amount of dystrophin mRNA in the muscle. The expression of the 6.5 kb mRNA is down-regulated during differentiation of myogenic cells; it is present in small amounts in proliferating myoblasts but is undetected in differentiated muscle cultures depleted of mononucleated cells.

摘要

此前我们鉴定出一种由杜兴氏肌营养不良症(DMD)基因转录而来的新型6.5 kb mRNA。该mRNA在编码内容和组织分布上与已知的编码抗肌萎缩蛋白的肌肉型和脑型14 kb DMD mRNA不同。这种新型转录本与抗肌萎缩蛋白在富含半胱氨酸和C末端结构域的大部分编码序列上相同。在此,我们利用cDNA克隆来确定在抗肌萎缩蛋白富含半胱氨酸结构域编码序列5'端的共同区域与新型mRNA特有序列之间的分歧点。这个包含翻译起始位点的独特序列位于抗肌萎缩蛋白基因第62和63外显子之间内含子中的一个新外显子内。我们使用含有新型mRNA特异性RNA序列的探针,研究了该mRNA在各种组织和细胞类型中的表达情况。研究表明,这种mRNA是在包括脑细胞在内的多种非肌肉组织中可检测到的主要DMD基因产物。在某些组织中,这种mRNA的量与肌肉中抗肌萎缩蛋白mRNA的量相当。6.5 kb mRNA的表达在成肌细胞分化过程中下调;它在增殖的成肌细胞中少量存在,但在耗尽单核细胞的分化肌肉培养物中未检测到。

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