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血鞭毛虫路氏锥虫的动质体脱氧核糖核酸。

Kinetoplast deoxyribonucleic acid of the hemoflagellate Trypanosoma lewisi.

作者信息

Renger H C, Wolstenholme D R

出版信息

J Cell Biol. 1970 Dec;47(3):689-702. doi: 10.1083/jcb.47.3.689.

Abstract

Cesium chloride centrifugation of DNA extracted from cells of blood strain Trypanosoma lewisi revealed a main band, rho = 1.707, a light satellite, rho = 1.699, and a heavy satellite, rho = 1.721. Culture strain T. lewisi DNA comprised only a main band, rho = 1.711, and a light satellite, rho = 1.699. DNA isolated from DNase-treated kinetoplast fractions of both the blood and culture strains consisted of only the light satellite DNA. Electron microscope examination of rotary shadowed preparations of lysates revealed that DNA from kinetoplast fractions was mainly in the form of single 0.4 micro circular molecules and large masses of 0.4 micro interlocked circles with which longer, often noncircular molecules were associated. The 0.4 micro circular molecules were mainly in the covalently closed form: they showed a high degree of resistance to thermal denaturation which was lost following sonication; and they banded at a greater density than linear DNA in cesium chloride-ethidium bromide gradients. Interpretation of the large masses of DNA as comprising interlocked covalently closed 0.4 micro circles was supported by the findings that they banded with single circular molecules in cesium chloride-ethidium bromide gradients, and following breakage of some circles by mild sonication, they disappeared and were replaced by molecules made up of low numbers of apparently interlocked 0.4 micro circles. When culture strain cells were grown in the presence of either ethidium bromide or acriflavin, there was a loss of stainable kinetoplast DNA in cytological preparations. There was a parallel loss of light satellite and of circular molecules from DNA extracted from these cells.

摘要

对从血液株路氏锥虫细胞中提取的DNA进行氯化铯离心,结果显示有一条主带,ρ = 1.707,一条轻卫星带,ρ = 1.699,以及一条重卫星带,ρ = 1.721。培养株路氏锥虫DNA仅包含一条主带,ρ = 1.711,以及一条轻卫星带,ρ = 1.699。从血液株和培养株的经脱氧核糖核酸酶处理的动质体组分中分离出的DNA仅由轻卫星DNA组成。对裂解物的旋转阴影制备物进行电子显微镜检查发现,来自动质体组分的DNA主要呈单个0.4微米环状分子以及大量0.4微米互锁环形式,还有较长的、通常为非环状的分子与之相关联。0.4微米环状分子主要呈共价闭合形式:它们对热变性表现出高度抗性,超声处理后这种抗性丧失;并且在氯化铯-溴化乙锭梯度中,它们的条带密度比线性DNA更高。大量DNA由互锁的共价闭合0.4微米环组成这一解释得到以下发现的支持:在氯化铯-溴化乙锭梯度中,它们与单个环状分子一起条带化,并且在轻度超声处理使一些环断裂后,它们消失并被由少量明显互锁的0.4微米环组成的分子所取代。当培养株细胞在溴化乙锭或吖啶黄素存在的情况下生长时,细胞学制备物中可染色的动质体DNA会丢失。从这些细胞中提取的DNA中,轻卫星和环状分子也会相应丢失。

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