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Mutations of the phage lambda attachment site alter the directionality of resolution of Holliday structures.

机译:噬菌体λ附着位点的突变改变了霍利迪结构解析的方向性。

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摘要

Integrative recombination of bacteriophage lambda occurs by two sequential, reciprocal strand exchanges at specific positions within the attachment sites. Both exchanges are promoted by the lambda Int protein; the first forms a Holliday structure, and the second resolves it to recombinant products. Recombination requires sequence homology within the 7 bp 'overlap' region that separates the two points of strand exchange. To see if homology promotes the second strand exchange, we constructed attachment site Holliday structures by annealing DNA strands and then assayed Int-promoted resolution. Holliday structures corresponding to strand exchange between sites with homologous overlap regions were efficiently resolved to give mixtures of recombinants and parents. Holliday structures corresponding to exchanges between heterologous sites fell into two classes. Members of the first class, in which heterology limited but did not completely prevent migration of the branchpoint within the overlap region, were resolved efficiently and preferentially to parental molecules. We propose that resolution to recombinants occurs only if homology allows branch migration from the first to the second exchange site. Members of the second class, in which heterology constrained the branchpoint within an Int binding site, were resolved poorly. We suggest that Holliday structures that have a branchpoint within an Int binding site are poor substrates for Int.
机译:噬菌体λ的整合重组发生在附着位点的特定位置,发生了两个顺序的,相互的链交换。 λInt蛋白可促进两种交换。第一个形成霍利迪结构,第二个将其解析为重组产物。重组需要在7 bp的“重叠”区域内将序列交换的两个点分开的序列同源性。为了查看同源性是否能促进第二条链交换,我们通过退火DNA链构建了附着位点的霍利迪结构,然后测定了Int促进的分辨率。有效地解析对应于具有同源重叠区域的位点之间的链交换的Holliday结构,以提供重组体和亲本的混合物。对应于异源位点之间交换的霍利迪结构分为两类。杂种有限但不能完全阻止分支点在重叠区域内迁移的第一类成员可以有效地解决,优先解决亲本分子问题。我们建议只有在同源性允许分支从第一个交换位点迁移到第二个交换位点的情况下,才能发生重组重组体的分离。第二类成员,其中异质性限制了Int结合位点内的分支点,解决起来很差。我们建议在Int结合位点内具有分支点的Holliday结构是Int的较差底物。

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