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在超螺旋 DNA 和超螺旋重组中间体的特定位置上进行碱基取代的化学计量掺入。

Stoichiometric incorporation of base substitutions at specific sites in supercoiled DNA and supercoiled recombination intermediates.

机构信息

Division of Molecular Medicine, Laboratory of Molecular Virology and Bacteriology, Rudjer Boskovic Institute, Zagreb, Croatia.

出版信息

Nucleic Acids Res. 2010 Oct;38(18):e175. doi: 10.1093/nar/gkq674. Epub 2010 Aug 6.

Abstract

Supercoiled DNA is the relevant substrate for a large number of DNA transactions and has additionally been found to be a favorable form for delivering DNA and protein-DNA complexes to cells. We report here a facile method for stoichiometrically incorporating several different modifications at multiple, specific, and widely spaced sites in supercoiled DNA. The method is based upon generating an appropriately gapped circular DNA, starting from single-strand circular DNA from two phagemids with oppositely oriented origins of replication. The gapped circular DNA is annealed with labeled and unlabeled synthetic oligonucleotides to make a multiply nicked circle, which is covalently sealed and supercoiled. The method is efficient, robust and can be readily scaled up to produce large quantities of labeled supercoiled DNA for biochemical and structural studies. We have applied this method to generate dye-labeled supercoiled DNA with heteroduplex bubbles for a Förster resonance energy transfer (FRET) analysis of supercoiled Holliday junction intermediates in the λ integrative recombination reaction. We found that a higher-order structure revealed by FRET in the supercoiled Holliday junction intermediate is preserved in the linear recombination product. We suggest that in addition to studies on recombination complexes, these methods will be generally useful in other reactions and systems involving supercoiled DNA.

摘要

超螺旋 DNA 是许多 DNA 转化的相关底物,并且已被发现是向细胞递送 DNA 和蛋白-DNA 复合物的有利形式。我们在此报告了一种简便的方法,可以在超螺旋 DNA 中多个特定且间隔较远的位置进行化学计量地掺入几种不同的修饰。该方法基于从具有相反复制起点的两个噬菌粒的单链环状 DNA 起始,生成适当缺口的环状 DNA。缺口的环状 DNA 与标记和未标记的合成寡核苷酸退火,形成多个缺口的环,该环被共价封闭并超螺旋化。该方法效率高、稳健,可轻松扩展规模,以生产大量用于生化和结构研究的标记超螺旋 DNA。我们已将该方法应用于生成带有异源双链泡的染料标记的超螺旋 DNA,以进行 λ 整合重组反应中超螺旋 Holliday 连接中间体的Förster 共振能量转移(FRET)分析。我们发现,FRET 在超螺旋 Holliday 连接中间体中揭示的高级结构在线性重组产物中得以保留。我们认为,除了在重组复合物的研究外,这些方法在涉及超螺旋 DNA 的其他反应和系统中也将具有普遍的应用价值。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/38ad/2952878/1c168ec4f5d9/gkq674f1.jpg

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