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14型鼻病毒接种的KB细胞中的细胞质DNA合成。

Cytoplasmic DNA synthesis in rhinovirus type 14-inoculated KB cells.

作者信息

Griffith M M, Kelley L, Upson R, Carlson E, Dinowitz M, Gauntt C J

出版信息

Biochim Biophys Acta. 1978 Jul 24;519(2):331-47. doi: 10.1016/0005-2787(78)90086-2.

DOI:10.1016/0005-2787(78)90086-2
PMID:208615
Abstract

Rhinovirus type 14 (RV14) incuced a transient statistically significant stimulation in synthesis of DNA which appeared between 0 and 3 h post-inoculation in the cytoplasm of high density monolayer cultures of KB cells. Newly synthesized DNA was measured by incorporation of [3H] thymidine into acid-insoluble DNAase-sensitive material and the cytoplasmic location established by cell fractionation and electron microscope radioautographic methods. A minimum of 10 plaque-forming units per cell of RV14 was required to stimulate DNA synthesis which did not occur above 34.5 degrees C, a temperature optimal for virus replication. Cytoplasmic DNA taken from RV14-infected or control cells could be differentiated from the bulk of cell (nuclear) DNA by several criteria, including: (1) RV14 induction of synthesis; (2) lower buoyant density and greater heterogeneity in CsCl and ethidium bromide/CsCl gradients; and (3) a different kinetic complexity upon reannealing. The Cot 1/2 value of cytoplasmic DNA, calclated as 50--100 from reassociation profiles, was about 10-fold less complex than the Cot 1/2 value of nuclear DNA (800-1000). These data rule out the possibility that cytoplasmic DNA arises by random breakage of nuclear DNA during cell disruption and extraction and are compatible with the hypothesis that inoculation of KB cells with RV14 results in stimulation of synthesis of a specific class of cell DNA which is detected in the cytoplasm.

摘要

14型鼻病毒(RV14)在接种后0至3小时之间,在KB细胞高密度单层培养物的细胞质中诱导了DNA合成的短暂统计学显著刺激。通过将[3H]胸苷掺入酸不溶性对DNA酶敏感的物质中来测量新合成的DNA,并通过细胞分级分离和电子显微镜放射自显影方法确定细胞质位置。刺激DNA合成需要每个细胞至少10个RV14噬斑形成单位,在34.5摄氏度以上不会发生DNA合成,34.5摄氏度是病毒复制的最佳温度。从RV14感染的或对照细胞中提取的细胞质DNA可以通过几个标准与大部分细胞(核)DNA区分开来,包括:(1)RV14诱导的合成;(2)在CsCl和溴化乙锭/CsCl梯度中较低的浮力密度和更大的异质性;(3)重新退火时不同的动力学复杂性。根据重新结合图谱计算,细胞质DNA的Cot 1/2值为50-100,其复杂性比核DNA的Cot 1/2值(800-1000)低约10倍。这些数据排除了细胞质DNA是在细胞破碎和提取过程中由核DNA随机断裂产生的可能性,并且与用RV14接种KB细胞导致在细胞质中检测到的一类特定细胞DNA合成受到刺激的假设相一致。

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