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兔β1珠蛋白基因在细胞核及超螺旋质粒中的脱氧核糖核酸酶I和核酸酶S1敏感性

DNase I and nuclease S1 sensitivity of the rabbit beta 1 globin gene in nuclei and in supercoiled plasmids.

作者信息

Margot J B, Hardison R C

出版信息

J Mol Biol. 1985 Jul 20;184(2):195-210. doi: 10.1016/0022-2836(85)90373-0.

DOI:10.1016/0022-2836(85)90373-0
PMID:2993630
Abstract

We have examined the nuclease sensitivity of the 5' flanking region of the rabbit beta 1 globin gene in bone marrow nuclei and in supercoiled plasmids. A DNase I hypersensitive site was found about 100 base-pairs 5' to the cap site in bone marrow nuclei. S1 nuclease can introduce a specific double-strand cut in the DNA in the same region. The presence of the nuclease-hypersensitive region correlates with the active transcription of gene beta 1 in bone marrow. Treatment with nuclease S1 of a supercoiled plasmid containing 1400 base-pairs of 5' flanking sequences as well as part of the beta 1 gene reveals a major double-strand cut 400 base-pairs 5' to the cap site. This cut maps within a stretch of repeating dinucleotides (C-T)12 and does not correspond to the in vivo site. Introduction of an RsaI fragment containing the nuclease S1-hypersensitive site into plasmid pBR322 shows that this fragment alone is sufficient to generate the hypersensitive site. Deletion of that RsaI fragment from the beta 1 plasmid reveals another site 1300 base-pairs upstream. Further deletion of this secondary site uncovers numerous other sites, none of which corresponds to the site in nuclei. Chromatin reconstitution with plasmids carrying the 5' flanking region of beta 1 and histones is capable of suppressing the in vitro nuclease-S1-hypersensitive site at --400 but is incapable of generating the in vivo site at --100. Fine analysis at the nucleotide level of the early events in the digestion with nuclease S1 shows that the enzyme attacks preferentially the sequence (G-A)12 on the message complementary strand. The region of DNA containing the supercoil-dependent S1 site adopts at least three different conformations that can be resolved electrophoretically. These different conformations are detected in linear restriction fragments and may represent non-B DNA or unusual B-form DNA.

摘要

我们已经检测了兔β1珠蛋白基因5'侧翼区在骨髓细胞核和超螺旋质粒中的核酸酶敏感性。在骨髓细胞核中,发现了一个位于帽位点5'端约100个碱基对处的DNase I超敏感位点。S1核酸酶可在同一区域的DNA中引入特异性双链切口。核酸酶超敏感区域的存在与β1基因在骨髓中的活跃转录相关。用S1核酸酶处理含有1400个碱基对的5'侧翼序列以及部分β1基因的超螺旋质粒,发现在帽位点5'端400个碱基对处有一个主要的双链切口。该切口位于一段重复二核苷酸(C-T)12内,与体内位点不对应。将包含S1核酸酶超敏感位点的RsaI片段导入质粒pBR322表明,仅该片段就足以产生超敏感位点。从β1质粒中缺失该RsaI片段后,在其上游1300个碱基对处发现了另一个位点。进一步缺失这个次要位点后,又发现了许多其他位点,但没有一个与细胞核中的位点对应。用携带β1基因5'侧翼区的质粒和组蛋白进行染色质重建,能够抑制体外-400处的S1核酸酶超敏感位点,但无法产生体内-100处的位点。对S1核酸酶消化早期事件进行核苷酸水平的精细分析表明,该酶优先攻击信使互补链上的(G-A)12序列。含有超螺旋依赖性S1位点的DNA区域至少采用三种不同的构象,这些构象可通过电泳分辨。这些不同的构象在线性限制片段中被检测到,可能代表非B型DNA或异常的B型DNA。

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