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KB细胞中的精氨酸剥夺。II. 饥饿期间合成的DNA的特征

Arginine deprivation in KB cells. II. Characterization of the DNA synthesized during starvation.

作者信息

Weissfeld A S, Rouse H

出版信息

J Cell Biol. 1977 Dec;75(3):889-98. doi: 10.1083/jcb.75.3.889.

Abstract

DNA synthesis in cells deprived of arginine was examined. Three lines of evidence indicated that tritiated thymidine ([3H]TdR) incorporation in arginine-starved cells was due to replicative rather than repair DNA synthesis. (a) When made in the presence of bromodeoxyuridine, the [3H]TdR-labeled DNA sedimented at hybrid density in isopycnic gradients. (b) As determined by the diphenylamine reaction, there was a 15% increase in the chemical amount of DNA per culture 30 h after arginine deprivation. (c) [3H]TdR incorporation was hydroxyurea-sensitive. Alkaline velocity sedimentation of the total DNA made during starvation revealed the existence of two distinct size classes: most of the DNA sedimented at a position analogous to that of control DNA, but 40% migrated one-third the distance of the bulk. After arginine restoration, these shorter pieces appeared to be chased into DNA of normal length; thus, one lesion in deprived cultures may cause an arrest in completion of DNA stretches to mature size. These findings, together with results of morphological studies of starved cells, suggest that changes induced by arginine deficiency effect the organization of nucleoproteins. These changes are reversible upon arginine restoration.

摘要

对缺乏精氨酸的细胞中的DNA合成进行了检测。三条证据表明,在精氨酸饥饿细胞中掺入的氚标记胸腺嘧啶核苷([3H]TdR)是由于复制性DNA合成而非修复性DNA合成。(a)当在溴脱氧尿苷存在的情况下进行合成时,[3H]TdR标记的DNA在等密度梯度中以杂交密度沉降。(b)通过二苯胺反应测定,精氨酸剥夺30小时后,每个培养物中DNA的化学量增加了15%。(c)[3H]TdR掺入对羟基脲敏感。饥饿期间合成的总DNA的碱性速度沉降显示存在两种不同的大小类别:大多数DNA沉降在与对照DNA类似的位置,但40%迁移的距离是大部分DNA的三分之一。精氨酸恢复后,这些较短的片段似乎被追踪成长度正常的DNA;因此,饥饿培养物中的一个损伤可能导致DNA延伸至成熟大小的过程停滞。这些发现,连同饥饿细胞形态学研究的结果,表明精氨酸缺乏引起的变化影响核蛋白的组织。精氨酸恢复后,这些变化是可逆的。

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CHROMOSOME CHANGES IN PPLO-INFECTED FL HUMAN AMNION CELLS.感染PPLO的FL人羊膜细胞中的染色体变化
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