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Fos和Jun不会使AP-1识别位点发生弯曲。

Fos and Jun do not bend the AP-1 recognition site.

作者信息

Sitlani A, Crothers D M

机构信息

Department of Chemistry, Yale University, New Haven, CT 06511, USA.

出版信息

Proc Natl Acad Sci U S A. 1996 Apr 16;93(8):3248-52. doi: 10.1073/pnas.93.8.3248.

Abstract

We have used a solution-based DNA cyclization assay and a gel-phasing method to show that contrary to previous reports [Kerppola, T. K. & Curran, T. (1991) Cell 66, 317-326], basic region leucine zipper proteins Fos and Jun do not significantly bend their AP-1 recognition site. We have constructed two sets of DNA constructs that contain the 7-bp 5'-TGACTCA-3' AP-1 binding site, from either the yeast or the human collagenase gene, which is well separated from and phased by 3-4 helical turns against an A tract-directed bend. The cyclization probabilities of DNAs with altered phasings are not significantly affected by Fos-Jun binding. Similarly, Fos-Jun and Jun-Jun bound to differently phased DNA constructs show insignificant variations in gel mobilities. Both these methods independently indicate that Fos and Jun bend their AP-1 target site by <5 degrees, an observation that has important implications in understanding their mechanism of transcriptional regulation.

摘要

我们使用了基于溶液的DNA环化分析和凝胶定相方法,以表明与之前的报道[Kerppola, T. K. & Curran, T. (1991) Cell 66, 317 - 326]相反,碱性区域亮氨酸拉链蛋白Fos和Jun不会使其AP - 1识别位点发生显著弯曲。我们构建了两组DNA构建体,它们包含来自酵母或人胶原酶基因的7碱基对5'-TGACTCA-3' AP - 1结合位点,该位点与A序列导向的弯曲相隔3 - 4个螺旋圈且相位不同。Fos - Jun结合对具有改变相位的DNA的环化概率没有显著影响。同样,与不同相位的DNA构建体结合的Fos - Jun和Jun - Jun在凝胶迁移率上显示出不显著的变化。这两种方法都独立表明Fos和Jun使其AP - 1靶位点弯曲小于5度,这一观察结果对理解它们的转录调控机制具有重要意义。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/12d2/39591/55c96623411d/pnas01515-0100-a.jpg

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