Johnson P H, Miller M J, Wild E, Kelly S V, Grossman L I
J Virol. 1979 Nov;32(2):629-39. doi: 10.1128/JVI.32.2.629-639.1979.
The replication cycle of bacteriophage phi X174 DNA has been analyzed by agarose gel electrophoresis. The electrophoretic behavior of the predominant species of parental and progeny DNA molecules formed between 5 and40 min after infection was deduced and quantitated. Migration through 1.4% agarose at 5 and 10 V/cm resolved all known viral DNA species as well as fragments of host chromosomal DNA. Among parental replicative form(RF) molecules synthesized, 1 to 3% were full length linear duplexes (RFIII) and approximately 65% were closed circular duplexes (RFI). Most of the input viral strands remained in a duplex structure throughout the period of infection studied here. Among progeny molecules, RFIII was not readily detected unless viral DNA synthesis was inhibited by chloramphenicol. Late in infection, 20% of the progeny RF were found to exist as form I dna. in addition, approximately 1% of the viral DNA was found as unit length linear single strands. Electrophoretic analysis of RF DNA after controlled denaturation suggests the existence of four populations of closed circular RF: (i) molecules of native superhelix density (RFI); (ii) a population of molecules of altered topological linking number, alpha, differing in increments of one superhelical turn (tau) between tau values of 0 and approximately -31; (iii) a superimposed population of topological isomers which under electrophoresis conditions have mean tau value (tau) equal to +5; and (iv) a population of "complexed" molecules with a reduced number of superhelical turns due to their association with single-stranded DNA and RNA. Complexed parental molecules isolated from cells infected at high multiplicity released FRI and homologous single-stranded DNA upon denaturation and are postulated to be intermediates in genetic recombination. Complexed RF DNA isolated from cells infected at low multiplicity release native supercoils upon reaction with RNase H and are observed by electron microscopy to contain displacement loops. Such molecules are likely intermediates in transcription. Our results are consistent with a structure of complexed RFI involving a partially triple-stranded helix in which a covalently closed circular duplex molecule contains a reduced number of superhelical turns due to the unwinding produced by base pairing between one strand of the supercoil and an associated homologous single strand of DNA or RNA.
通过琼脂糖凝胶电泳分析了噬菌体φX174 DNA的复制周期。推导并定量了感染后5至40分钟内形成的亲本和子代DNA分子主要种类的电泳行为。在5和10 V/cm电压下通过1.4%琼脂糖凝胶的迁移分离出了所有已知的病毒DNA种类以及宿主染色体DNA片段。在合成的亲本复制型(RF)分子中,1%至3%是全长线性双链体(RFIII),约65%是闭环双链体(RFI)。在此研究的感染期间,大多数输入的病毒链始终保持双链结构。在子代分子中,除非用氯霉素抑制病毒DNA合成,否则不易检测到RFIII。感染后期,发现20%的子代RF以I型DNA形式存在。此外,约1%的病毒DNA以单位长度线性单链形式存在。对经控制变性后的RF DNA进行电泳分析表明,存在四种闭环RF群体:(i)天然超螺旋密度的分子(RFI);(ii)拓扑连接数α改变的分子群体,在0至约-31的τ值之间,超螺旋圈数(τ)以一个超螺旋圈的增量变化;(iii)拓扑异构体的叠加群体,在电泳条件下其平均τ值(τ)等于+5;(iv)由于与单链DNA和RNA结合而超螺旋圈数减少的“复合”分子群体。从高感染复数感染的细胞中分离出的复合亲本分子在变性时释放出FRI和同源单链DNA,推测它们是基因重组的中间体。从低感染复数感染的细胞中分离出的复合RF DNA与RNase H反应后释放出天然超螺旋,通过电子显微镜观察发现其含有置换环。这类分子可能是转录的中间体。我们的结果与复合RFI的结构一致,该结构涉及部分三链螺旋,其中共价闭环双链分子由于超螺旋的一条链与相关同源单链DNA或RNA之间的碱基配对导致解旋,从而超螺旋圈数减少。
