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紫外线照射对5-溴脱氧尿苷取代的噬菌体T4 DNA命运的影响。

Effects of UV irradiation on the fate of 5-bromodeoxyuridine-substituted bacteriophage T4 DNA.

作者信息

Restifo L L, Vogelbacker H H, Madara T, Ling S K, Kozinski A W

出版信息

J Virol. 1983 Jul;47(1):151-70. doi: 10.1128/JVI.47.1.151-170.1983.

DOI:10.1128/JVI.47.1.151-170.1983
PMID:6345803
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC255218/
Abstract

We have carried out a series of experiments designed to characterize the impact of UV irradiation (260 nm) on 5-bromodeoxyuridine-labeled (heavy) T4 bacteriophage, both before and after infection of Escherichia coli. In many respects, these effects differ greatly from those previously described for non-density-labeled (light) phage. Moreover, our results have led us to propose a model for a novel mechanism of host-mediated repair synthesis, in which excision of UV-damaged areas is followed by initiation of replication, strand displacement, and a considerable amount of DNA replication. UV irradiation of 5-bromodeoxyuridine-labeled phage results in single-stranded breaks in a linear, dose-dependent manner (1.3 to 1.5 breaks per genomic strand per lethal hit). This damage does not interfere with injection of the phage genome, but some of the UV-irradiated heavy phage DNA undergoes additional intracellular breakdown (also dose dependent). However, a minority (25%) of the injected parental DNA is protected, maintaining its preinjection size. This protected moiety is associated with a replicative complex of DNA and proteins, and is more efficiently replicated than is the parental DNA not so associated. Most of the progeny DNA is also found with the replicative complex. The 5-bromodeoxyuridine of heavy phage DNA is debrominated by UV irradiation, resulting in uracil which is removed by host uracil glycosylase. Unlike the simple gap-filling repair synthesis after infection with UV-irradiated light phage, the repair replication of UV-irradiated heavy phage is extensive as determined by density shift of the parental label in CsC1 gradients. The newly synthesized segments are covalently attached to the parental fragments. The repair replication takes place even in the presence of chloramphenicol, a protein synthesis inhibitor, suggesting it is host mediated. Furthermore, the extent of the repair replication is greater at higher doses of UV irradiation applied to the heavy phage. This abundant synthesis results ultimately in dispersion of the parental sequences as short stretches in the midst of long segments of newly synthesized progeny DNA. Together, the extensive replication and the resulting distribution pattern of parental sequences, without significant solubilization of parental label, are most consistent with a model of repair synthesis in which the leading strand displaces, rather than ligates to, the encountered 5' end.

摘要

我们进行了一系列实验,旨在表征紫外线照射(260纳米)对5-溴脱氧尿苷标记的(重)T4噬菌体在感染大肠杆菌之前和之后的影响。在许多方面,这些影响与先前描述的非密度标记的(轻)噬菌体的影响有很大不同。此外,我们的结果使我们提出了一种宿主介导的修复合成新机制的模型,其中紫外线损伤区域的切除之后是复制的起始、链置换和大量的DNA复制。对5-溴脱氧尿苷标记的噬菌体进行紫外线照射会以线性、剂量依赖性方式导致单链断裂(每基因组链每致死剂量1.3至1.5个断裂)。这种损伤不会干扰噬菌体基因组的注入,但一些紫外线照射的重噬菌体DNA会发生额外的细胞内降解(也是剂量依赖性的)。然而,少数(25%)注入的亲本DNA受到保护,保持其注入前的大小。这种受保护的部分与DNA和蛋白质的复制复合体相关,并且比未与之相关的亲本DNA更有效地复制。大多数子代DNA也与复制复合体一起被发现。重噬菌体DNA的5-溴脱氧尿苷被紫外线照射脱溴,产生尿嘧啶,然后被宿主尿嘧啶糖基化酶去除。与紫外线照射的轻噬菌体感染后的简单缺口填充修复合成不同,紫外线照射的重噬菌体的修复复制如通过CsC1梯度中亲本标记的密度转移所确定的那样广泛。新合成的片段与亲本片段共价连接。即使在存在蛋白质合成抑制剂氯霉素的情况下,修复复制也会发生,这表明它是由宿主介导的。此外,对重噬菌体施加更高剂量的紫外线照射时,修复复制的程度更大。这种大量的合成最终导致亲本序列分散为新合成的子代DNA长片段中间的短片段。总之,广泛的复制以及由此产生的亲本序列分布模式,而亲本标记没有明显溶解,与一种修复合成模型最为一致,在该模型中,前导链取代而不是连接到遇到的5'末端。

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本文引用的文献

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