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噬菌体T7包装的双链DNA基因组的构象与相互作用。

Conformation and interactions of the packaged double-stranded DNA genome of bacteriophage T7.

作者信息

Overman S A, Aubrey K L, Reilly K E, Osman O, Hayes S J, Serwer P, Thomas G J

机构信息

Division of Cell Biology and Biophysics, School of Biological Sciences, University of Missouri-Kansas City 64110-2499, USA.

出版信息

Biospectroscopy. 1998;4(5 Suppl):S47-56. doi: 10.1002/(SICI)1520-6343(1998)4:5+<S47::AID-BSPY6>3.0.CO;2-7.

DOI:10.1002/(SICI)1520-6343(1998)4:5+<S47::AID-BSPY6>3.0.CO;2-7
PMID:9787914
Abstract

The structure of the packaged double-stranded DNA genome of bacteriophage T7 was compared to that of unpackaged T7 DNA using digital difference Raman spectroscopy. Spectral data were obtained at 25 degrees C from native T7 virus (100 mg/mL), empty T7 capsids (50 mg/mL), and purified T7 DNA (40 mg/mL) in buffer containing 200 mM NaCl, 10 mM MgCl2, and 10 mM Tris at pH 7.5. At these conditions, the local conformation of T7 DNA was not affected by packaging. Specifically, the local B-form secondary structure of unpackaged T7 DNA, including furanose C2'-endo pucker, anti glycosyl torsion, Watson-Crick base pairing, and base stacking, were essentially fully (> 98%) retained when the genome was condensed within the viral capsid. However, the average electrostatic environment of T7 DNA phosphates was altered dramatically by packaging as revealed by large perturbations in the Raman bands associated with localized vibrations of the DNA phosphate groups. The change in the phosphate environment was attributed to Mg2+ ions that were packaged with the genomic DNA, and the observed Raman perturbations of genomic DNA were equivalent to those generated by a 50-100-fold increase in Mg2+ concentration in aqueous phosphodiester model compounds. The T7 data were qualitatively and quantitatively similar to those observed previously for packaged DNA of bacteriophage P22 and imply that genomic DNAs of T7 and P22 are both organized in a similar fashion within their respective capsids. The results show that the condensed genome does not contain kinks or folds that would disrupt the local B conformation by more than 2%. The present findings are discussed in relation to previously proposed models for condensation and organization of double-stranded and single-stranded viral DNA.

摘要

利用数字差分拉曼光谱法,将噬菌体T7包装后的双链DNA基因组结构与未包装的T7 DNA结构进行了比较。在25摄氏度下,于含有200 mM氯化钠、10 mM氯化镁和10 mM Tris(pH 7.5)的缓冲液中,获取了天然T7病毒(100 mg/mL)、空T7衣壳(50 mg/mL)和纯化的T7 DNA(40 mg/mL)的光谱数据。在这些条件下,T7 DNA的局部构象不受包装影响。具体而言,当基因组在病毒衣壳内浓缩时,未包装的T7 DNA的局部B型二级结构,包括呋喃糖C2'-内式褶皱、反式糖基扭转、沃森-克里克碱基配对和碱基堆积,基本完全(> 98%)得以保留。然而,如与DNA磷酸基团局部振动相关的拉曼谱带中的大幅扰动所示,包装显著改变了T7 DNA磷酸基团的平均静电环境。磷酸环境的变化归因于与基因组DNA一起包装的镁离子,并且观察到的基因组DNA的拉曼扰动等同于在水性磷酸二酯模型化合物中镁离子浓度增加50至100倍所产生的扰动。T7的数据在定性和定量上与先前观察到的噬菌体P22包装DNA的数据相似,这意味着T7和P22的基因组DNA在各自的衣壳内均以相似的方式组织。结果表明,浓缩的基因组不包含会使局部B构象破坏超过2%的扭结或折叠。结合先前提出的双链和单链病毒DNA浓缩与组织模型,对本研究结果进行了讨论。

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