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. 1983 Apr 14;302(5909):591-6.
doi: 10.1038/302591a0.

Specific transcription and RNA splicing defects in five cloned beta-thalassaemia genes

Specific transcription and RNA splicing defects in five cloned beta-thalassaemia genes

R Treisman et al. Nature. .

Abstract

Transcriptional analysis of five different cloned beta-thalassaemia genes introduced into cultured mammalian cells revealed specific defects in transcription and RNA splicing. A single base change 87 base pairs to the 5' side of the mRNA cap site significantly lowers the level of transcription and therefore appears to represent a promoter mutation. Three genes contain different single base changes in the first intervening sequence (IVS) 5' splice site. One mutation, at IVS1 position 1, inactivates the splice site completely; the other two, at IVS1 positions 5 and 6, reduce its activity. Each mutation activates the same three cryptic splice sites. The fifth gene contains a single base change within IVS2 at position 745, which results in the formation of abnormal beta-globin RNA that contains an extra exon.

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