DNA-binding factors assemble in a sequence-specific manner on the maize mitochondrial atpA promoter

被引:0
|
作者
Ching-Chun Chang
D. B. Stern
机构
[1] Boyce Thompson Institute for Plant Research,
[2] Cornell University,undefined
[3] Tower Road,undefined
[4] Ithaca,undefined
[5] NY 14853-1801,undefined
[6] USA e-mail: ds28@cornell.edu Tel.: +1-607-254 1306; Fax: +1-607-255 6695,undefined
来源
Current Genetics | 1999年 / 35卷
关键词
Key words Toeprinting; Maize; Mitochondria; Transcription;
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摘要
The maize mitochondrial atpA promoter has been well-characterized using in vitro transcription. The functional elements of this promoter comprise a central domain extending from –7 to +5 relative to the transcription start site, and an upstream domain of 1–3 bp that is purine-rich and centered around positions –11 to –12. As a first step in characterizing the transcriptional machinery, exonuclease-III mapping (toeprinting) was used to map the borders of DNA-protein interactions using either a 107-bp wild-type template or transcriptionally-inactive templates containing linker-scanning mutations. These experiments revealed that, with a wild-type promoter, protein factors occupy as much as 36 bp, from positions –20 to +16 relative to the transcription initiation site. Protein-binding patterns were altered when the linker-scanning mutants were used, suggesting that either the number or conformation of DNA-binding proteins could account for their inability to promote transcription initiation.
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页码:506 / 511
页数:5
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