Martin D W, Weber P C
Infectious Diseases Section, Parke-Davis Pharmaceutical Research Division, Warner-Lambert Company, Ann Arbor, Michigan 48105, USA.
J Virol. 1996 Dec;70(12):8801-12. doi: 10.1128/JVI.70.12.8801-8812.1996.
The herpes simplex virus type 1 (HSV-1) genome consists of two components, L (long) and S (short), that invert relative to each other during productive infection to generate four equimolar isomeric forms of viral DNA. Recent studies have indicated that this genome isomerization is the result of DNA replication-mediated homologous recombination between the large inverted repeat sequences that exist in the genome, rather than site-specific recombination through the terminal repeat a sequences present at the L-S junctions. However, there has never been an unequivocal demonstration of the dispensability of the latter element for this process using a recombinant virus whose genome lacks a sequences at its L-S junctions. This is because the genetic manipulations required to generate such a viral mutant are not possible using simple marker transfer, since the cleavage and encapsidation signals of the a sequence represent essential cis-acting elements which cannot be deleted outright from the viral DNA. To circumvent this problem, a simple two-step strategy was devised by which essential cis-acting sites like the a sequence can be readily deleted from their natural loci in large viral DNA genomes. This method involved initial duplication of the element at a neutral site in the viral DNA and subsequent deletion of the element from its native site. By using this approach, the a sequence at the L-S junction was rendered dispensable for virus replication through the insertion of a second copy into the thymidine kinase (TK) gene of the viral DNA; the original copies at the L-S junctions were then successfully deleted from this virus by conventional marker transfer. The final recombinant virus, HSV-1::L-S(delta)a, was found to be capable of undergoing normal levels of genome isomerization on the basis of the presence of equimolar concentrations of restriction fragments unique to each of the four isomeric forms of the viral DNA. Interestingly, only two of these genomic isomers could be packaged into virions. This restriction was the result of inversion of the L component during isomerization, which prevented two of the four isomers from having the cleavage and encapsidation signals of the a sequence in the TK gene in a packageable orientation. This phenomenon was exploited as a means of directly measuring the kinetics of HSV-1::L-S(delta)a genome isomerization. Following infection with virions containing just the two packaged genomic isomers, all four isomers were readily detected at a stage in infection coincident with the onset of DNA replication, indicating that the loss of the a sequence at the L-S junction had no adverse effect on the frequency of isomerization events in this virus. These results therefore validate the homologous recombination model of HSV-1 genome isomerization by directly demonstrating that the a sequence at the L-S junction is dispensable for this process. The strategy used to remove the a sequence from the HSV-1 genome in this work should be broadly applicable to studies of essential cis-acting elements in other large viral DNA molecules.
单纯疱疹病毒1型(HSV-1)基因组由两个部分组成,即长片段(L)和短片段(S),在增殖性感染期间它们会相对彼此发生倒位,从而产生四种等摩尔的病毒DNA异构形式。最近的研究表明,这种基因组异构化是基因组中存在的大反向重复序列之间DNA复制介导的同源重组的结果,而不是通过L-S连接处存在的末端重复a序列进行的位点特异性重组。然而,从未使用基因组在L-S连接处缺少a序列的重组病毒明确证明后者对于此过程是可有可无的。这是因为使用简单的标记转移不可能进行产生这种病毒突变体所需的基因操作,因为a序列的切割和包装信号代表必需的顺式作用元件,不能从病毒DNA中直接删除。为了解决这个问题,设计了一种简单的两步策略,通过该策略可以轻松地从大型病毒DNA基因组中的天然位点删除像a序列这样的必需顺式作用位点。该方法包括首先在病毒DNA的中性位点复制该元件,然后从其天然位点删除该元件。通过使用这种方法,通过将第二个拷贝插入病毒DNA的胸苷激酶(TK)基因,使得L-S连接处的a序列对于病毒复制变得可有可无;然后通过常规的标记转移成功地从该病毒中删除了L-S连接处的原始拷贝。最终的重组病毒HSV-1::L-S(δ)a,基于病毒DNA四种异构形式各自特有的等摩尔浓度的限制性片段的存在,被发现能够进行正常水平的基因组异构化。有趣的是,这些基因组异构体中只有两种可以包装到病毒粒子中。这种限制是异构化过程中L组分倒位的结果,这使得四种异构体中的两种无法以可包装的方向在TK基因中具有a序列的切割和包装信号。这种现象被用作直接测量HSV-1::L-S(δ)a基因组异构化动力学的一种手段。在用仅含有两种包装好的基因组异构体的病毒粒子感染后,在与DNA复制开始同时的感染阶段很容易检测到所有四种异构体,这表明L-S连接处a序列的缺失对该病毒中异构化事件的频率没有不利影响。因此,这些结果通过直接证明L-S连接处的a序列对于此过程是可有可无的,验证了HSV-1基因组异构化的同源重组模型。在这项工作中用于从HSV-1基因组中去除a序列的策略应该广泛适用于其他大型病毒DNA分子中必需顺式作用元件的研究。
