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Bacteriophage lambda DNA packaging: scanning for the terminal cohesive end site during packaging.

机译:噬菌体λDNA包装:在包装过程中扫描末端粘性末端。

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摘要

Bacteriophage lambda packages the DNA of the related phage 21 poorly [Hohn, B. (1975) J. Mol. Biol. 98, 93--106]. To understand the nature of the packaging defect, the interaction of the cohesive end site (cos) specific for phage 21 (cos phi 21) with phage lambda terminase has been investigated. The ability of lambda terminase to cleave cos phi 21 was studied in vitro; lambda terminase cleaved cos phi 21 only 1% as well as it cleaved the phage lambda cohesive end site (cos lambda). In vitro packaging experiments showed that the lambda and 21 packaging specificities observed in vivo are also found in vitro. The cos cleavage reaction was modified so that competition experiments could be performed; these experiments showed that cos phi 21 was unable to bind lambda terminase, thus identifying the nature of the defect. Previous work [Feiss, M., Fisher, R. A., Siegele, D. A., Nichols, B. P. & Donelson, J. E. (1979) Virology 92, 56--67] has shown that the base pairs giving lambda or 21 packaging specificity are at the left end of the chromosome, outside the 22-base-pair symmetry region that includes the annealed cohesive ends. Therefore, terminase binding to cos requires interactions with base pairs to the Nu1 side of the cohesive end symmetry segment. The evidence supports the proposition that cos consists of adjacent sites for binding of terminase and for nicking by terminase. Because cos phi 21 can be cut by lambda terminase to terminate DNA packaging, it is proposed that the terminase that binds and nicks at the initial cos site is brought into contact with the terminal cos site by the packaging process. Terminase recognizes and nicks the cohesive end sequence of the terminal cos without requiring the binding site.
机译:噬菌体λ包装相关噬菌体21的DNA很差[Hohn,B。(1975)J.Mol.Biol.215:403-10。生物学98,93--106]。为了了解包装缺陷的性质,已经研究了噬菌体21(cos phi 21)特有的内聚末端位点(cos)与噬菌体λ末端酶的相互作用。体外研究了λ末端酶切割cos phi 21的能力; Lambda末端酶仅切割cos phi 21 1%,也切割了噬菌体Lambda内聚末端位点(cos lambda)。体外包装实验表明,在体外观察到的lambda和21种包装特异性也在体外发现。修改了cos裂解反应,从而可以进行竞争实验;这些实验表明,cos phi 21无法结合λ末端酶,从而确定了缺陷的性质。以前的工作[Feiss,M.,Fisher,RA,Siegele,DA,Nichols,BP&Donelson,JE(1979)Virology 92,56--67]已显示给出lambda或21包装特异性的碱基对在左侧。染色体末端,位于包含退火内聚末端的22个碱基对的对称区域之外。因此,末端酶与cos的结合需要与内聚末端对称段的Nu1侧的碱基对相互作用。证据支持这样一个命题,即cos由末端位点组成,用于结合末端酶和通过末端酶形成切口。因为cos phi 21可以被lambda末端酶切割而终止DNA包装,所以建议通过包装过程使在初始cos位点结合并形成切口的末端酶与末端cos位点接触。终止酶无需结合位点即可识别并刻痕末端cos的内聚末端序列。

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