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矮牵牛Cab基因启动子中的新型顺式作用元件。

Novel cis-acting elements in Petunia Cab gene promoters.

作者信息

Gidoni D, Brosio P, Bond-Nutter D, Bedbrook J, Dunsmuir P

机构信息

Advanced Genetic Sciences, Inc., Oakland, CA 94611.

出版信息

Mol Gen Genet. 1989 Jan;215(2):337-44. doi: 10.1007/BF00339739.

Abstract

In order to identify specific cis-acting elements which regulate the expression of the divergent Cab22R and Cab22L genes of Petunia, we conducted systematic mutational studies of the 1 kb intergenic promoter region. Sequence analysis revealed three GATA box sequence repeats positioned between the TATA and CAAT box elements. These GATA elements are conserved in corresponding promoter regions of all LHCII Type I Cab genes in Petunia and other dicotyledonous plants we have examined. Site-specific mutations in the CAAT box and the GATA box elements of the Cab22R promoter resulted in 8-fold and 5-fold reductions in Cab22R transcript levels respectively. A deletion of 52 bp, adjacent and upstream from the CAAT box (-92 to -145) in the Cab22R promoter reduced transcript levels 20-fold. This deletion contains a region of 13 bp which is conserved between many Petunia Cab genes. These results indicate that the quantitative expression of the Cab22 promoters is regulated by multiple cis-acting elements including CAAT and GATA box elements as well as sequences located between -92 and -145. The deletion of the region between -92 and -145 is partially compensated by homologous sequences present in the adjacent divergent promoter Cab22L.

摘要

为了鉴定调控矮牵牛中反向排列的Cab22R和Cab22L基因表达的特定顺式作用元件,我们对1 kb的基因间启动子区域进行了系统的突变研究。序列分析揭示了位于TATA盒和CAAT盒元件之间的三个GATA盒序列重复。这些GATA元件在矮牵牛以及我们研究过的其他双子叶植物中所有LHCII I型Cab基因的相应启动子区域中都是保守的。Cab22R启动子的CAAT盒和GATA盒元件中的位点特异性突变分别导致Cab22R转录水平降低8倍和5倍。Cab22R启动子中CAAT盒(-92至-145)相邻且上游52 bp的缺失使转录水平降低了20倍。该缺失包含一个13 bp的区域,该区域在许多矮牵牛Cab基因之间是保守的。这些结果表明,Cab22启动子的定量表达受多种顺式作用元件调控,包括CAAT盒和GATA盒元件以及位于-92至-145之间的序列。-92至-145之间区域的缺失部分由相邻反向启动子Cab22L中存在的同源序列补偿。

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