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Method for induction of mutations in physically defined regions of the herpes simplex virus genome.

机译:在单纯疱疹病毒基因组的物理定义区域中诱导突变的方法。

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摘要

A procedure was developed for inducing mutations in isolated restriction enzyme fragments of herpes simplex virus type 1 (HSV-1) DNA with nitrous acid. The mutations were then transferred to the viral genome by genetic recombination during cotransfection of rabbit kidney cells with the mutagenized fragments and intact HSV-1 DNA. The HpaI restriction enzyme fragments LD, B, LG, I, and J were mutagenized. Temperature-sensitive mutants were found at frequencies of 1 to 5% among the progeny of the transfections. Syncytial mutants also were found at high frequency when fragment B or LD was used for mutagenesis. Fifteen of these mutants, 11 temperature sensitive and 4 syncytial, were used for further studies, including complementation analysis, DNA synthesis, and marker rescue. Marker rescue data presented here and in the accompanying publication (A. L. Goldin, R. M. Sandri-Goldin, M. Levine, and J. C. Glorioso, J. Virol. 38: 50-58, 1981) confirm the map position of some of the newly isolated mutants.
机译:开发了一种用亚硝酸在单纯疱疹病毒1型(HSV-1)DNA的限制性酶切片段中诱导突变的方法。然后,在用诱变的片段和完整的HSV-1 DNA共转染兔肾细胞的过程中,通过基因重组将突变转移到病毒基因组中。将HpaI限制酶片段LD,B,LG,I和J诱变。在转染的子代中发现温度敏感突变体的频率为1%至5%。当使用片段B或LD诱变时,合胞体突变体的频率也很高。这些突变体中的15个,即11个对温度敏感和4个合胞体突变,被用于进一步研究,包括互补分析,DNA合成和标志物拯救。此处和随附出版物中发表的标志物拯救数据(AL Goldin,RM Sandri-Goldin,M。Levine和JC Glorioso,J. Virol。38:50-58,1981)证实了一些新近分离的突变体的定位。

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