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使用简并寡核苷酸分析与DNA结合的核因子I

Analysis of nuclear factor I binding to DNA using degenerate oligonucleotides.

作者信息

Gronostajski R M

出版信息

Nucleic Acids Res. 1986 Nov 25;14(22):9117-32. doi: 10.1093/nar/14.22.9117.

Abstract

Nuclear factor I (NFI) binds tightly to DNA containing the consensus sequence TGG(N)6-7GCCAA. To study the role of the spacing between the TGG and GCCAA motifs, oligonucleotides homologous to the NFI binding site FIB-2 were synthesized and used for binding assays in vitro. The wild-type site (FIB-2.6) has a 6bp spacer region and binds tightly to NFI. When the size of this spacer was altered by +/- 1 or 2bp the binding to NFI was abolished. To further assess the role of the spacer and bases flanking the motifs, two oligonucleotide libraries were synthesized. Each member of these libraries had intact TGG and GCCAA motifs, but the sequence of the spacer and the 3bp next to each motif was degenerate. The library with a 6bp spacer bound to NFI to 40-50% the level of FIB-2.6. The library with a 7bp spacer bound to NFI to only 4% the level of FIB-2.6 and some of this binding was weaker than that of FIB-2.6 DNA. This novel use of degenerate DNA libraries has shown that: 1) the structural requirements for FIB sites with a 7bp spacer are more stringent than for sites with a 6bp spacer and 2) a limited number of DNA structural features can prevent the binding of NFI to sites with intact motifs and a 6bp spacer region.

摘要

核因子I(NFI)与含有共有序列TGG(N)6-7GCCAA的DNA紧密结合。为了研究TGG和GCCAA基序之间间隔的作用,合成了与NFI结合位点FIB-2同源的寡核苷酸,并用于体外结合试验。野生型位点(FIB-2.6)有一个6bp的间隔区,能与NFI紧密结合。当这个间隔区的大小改变±1或2bp时,与NFI的结合就会被消除。为了进一步评估间隔区和基序侧翼碱基的作用,合成了两个寡核苷酸文库。这些文库的每个成员都有完整的TGG和GCCAA基序,但间隔区和每个基序旁边3bp的序列是简并的。有6bp间隔区的文库与NFI的结合水平为FIB-2.6的40%-50%。有7bp间隔区的文库与NFI的结合水平仅为FIB-2.6的4%,且其中一些结合比FIB-2.6 DNA的结合更弱。这种对简并DNA文库的新应用表明:1)有7bp间隔区的FIB位点的结构要求比有6bp间隔区的位点更严格;2)有限数量的DNA结构特征可以阻止NFI与有完整基序和6bp间隔区的位点结合。

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