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大肠杆菌中ColE1 DNA共价闭合复制中间体的纯化与特性分析

Purification and characterization of covalently closed replicative intermediates of ColEl DNA from Escherichia coli.

作者信息

Katz L, Williams P H, Sato S, Leavitt R W, Helinski D R

出版信息

Biochemistry. 1977 Apr 19;16(8):1677-83. doi: 10.1021/bi00627a024.

Abstract

Pulse-labeled ColEl DNA molecules, undergoing replication in Escherichia coli cells either in the absence or presence of chloramphenicol, were extracted and purified by neutral sucrose density gradient sedimentation and equilibrium centrifugation in an ethidium bromide-cesium chloride gradient. In the dye-buoyant density gradient, the replicating molecules were found in regions between the supercoiled and open-circular nonreplicating plasmid DNA, as well as in the open-circular region. In a neutral sucrose gradient, peaks of pulse label were found in the region of 26 to 38 S as well as at the 23 and 17 S positions corresponding to the positions of supercoiled and open-circular ColEl DNA. In alkaline sucrose gradient, nascent ColEl DNA was found to sediment as discrete peaks corresponding to 5-6, 7-9, and 14-16 S, indicating that at least one growing strand of the replicating molecule is produced discontinuously. In the electron microscope, many of the molecules appeared as partially supercoiled structures containing two open-circular branches of equal length, of less than 20% to more than 90% replicated. Branched open-circular molecules were not observed to any significant extent without prior treatment to induce single-strand scissions. The parental strands of the replicating molecules were determined to be covalently closed, but the superhelical density of the DNA was shown to be progressively decreased as replication proceeded.

摘要

对在有无氯霉素存在的情况下于大肠杆菌细胞中进行复制的脉冲标记的ColE1 DNA分子,通过中性蔗糖密度梯度沉降以及在溴化乙锭-氯化铯梯度中的平衡离心进行提取和纯化。在染料浮力密度梯度中,复制分子出现在超螺旋和开环非复制质粒DNA之间的区域以及开环区域。在中性蔗糖梯度中,脉冲标记的峰出现在26至38 S区域以及对应于超螺旋和开环ColE1 DNA位置的23和17 S位置处。在碱性蔗糖梯度中,发现新生的ColE1 DNA沉降为对应于5 - 6、7 - 9和14 - 16 S的离散峰,这表明复制分子的至少一条生长链是不连续产生的。在电子显微镜下,许多分子呈现为部分超螺旋结构,包含两条等长的开环分支,复制程度从不到20%到超过90%不等。未经预先处理以诱导单链断裂时,未观察到明显程度的分支开环分子。复制分子的亲代链被确定为共价闭合,但随着复制的进行,DNA的超螺旋密度逐渐降低。

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