来自噬菌体感染细菌的脱氧核糖核酸的分级分离。

Fractionation of deoxyribonucleic acid from phage-infected bacteria.

作者信息

Smith M G, Burton K

出版信息

Biochem J. 1966 Jan;98(1):229-41. doi: 10.1042/bj0980229.

DOI:10.1042/bj0980229

PMID:5938647

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1264819/

Abstract

DNA has been isolated in 90% yield from T5-infected cultures of Escherichia coli ;pulse'-labelled with [(3)H]thymidine. It had a buoyant density in caesium chloride solution identical with the DNA of mature T5 phage, and no components of unusual buoyant density were detected. 2. The DNA preparation was resolved into two major components of differing specific activity on a column of kieselguhr coated with methylated serum albumin. The DNA of high specific activity could be eluted from the column only with 2n-ammonia, and the firm binding did not appear to be due to an artifact of preparation. 3. A similar fractionation into two DNA components of differing specific activity was observed when the ;pulse'-labelled culture was lysed with sodium dodecyl sulphate and the lysate rocked with phenol. The DNA of high specific activity was found in the interface precipitate between the phenol and aqueous layers. 4. The amounts of DNA in the two fractions were measured at different times after infection and the radioactivity content of each was determined at various times after a short ;pulse' of [(3)H]thymidine. The interface fraction contained the replicating phage DNA, and the DNA from mature phage particles appeared in the aqueous fraction. 5. Analogous results were obtained with T2-infected E. coli. In the presence of chloramphenicol the DNA in the interface fraction was not converted into DNA extractable into the aqueous layer. Since chloramphenicol prevents the condensation of DNA into phage heads, it is suggested that any DNA in extended configuration is trapped inside the rigid-layer framework of the cell wall. 6. Treatment with lysozyme released much of the DNA from the interface precipitate. This DNA was firmly bound by the chromatographic column and had the same buoyant density in caesium chloride solution as normal T5-phage DNA. Sucrose-gradient sedimentation studies showed that it was heterogeneous and that as much as 60% sedimented faster than T5-phage DNA.

摘要

已从用[³H]胸腺嘧啶脉冲标记的T5感染的大肠杆菌培养物中以90%的产率分离出DNA。它在氯化铯溶液中的浮力密度与成熟T5噬菌体的DNA相同，未检测到具有异常浮力密度的成分。2. 在涂有甲基化血清白蛋白的硅藻土柱上，该DNA制剂被分离成两个具有不同比活性的主要成分。高比活性的DNA只能用2n氨水从柱上洗脱下来，这种牢固结合似乎不是制备过程中的人为产物。3. 当用十二烷基硫酸钠裂解“脉冲”标记的培养物并用苯酚振荡裂解物时，观察到类似的分离成两个具有不同比活性的DNA成分的情况。高比活性的DNA存在于苯酚层和水层之间的界面沉淀物中。4. 在感染后的不同时间测量两个部分中的DNA量，并在[³H]胸腺嘧啶短“脉冲”后的不同时间测定每个部分的放射性含量。界面部分含有正在复制的噬菌体DNA，来自成熟噬菌体颗粒的DNA出现在水相部分。5. 用T2感染的大肠杆菌也得到了类似的结果。在氯霉素存在下，界面部分的DNA没有转化为可提取到水相层中的DNA。由于氯霉素阻止DNA凝聚成噬菌体头部，有人提出任何呈伸展构型的DNA都被困在细胞壁的刚性层框架内。6. 用溶菌酶处理从界面沉淀物中释放出了许多DNA。这种DNA被色谱柱牢固结合，在氯化铯溶液中的浮力密度与正常T5噬菌体DNA相同。蔗糖梯度沉降研究表明它是异质的，多达60%的沉降速度比T5噬菌体DNA快。