Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates

Farid A. Kadyrov; John W. Drake

首页> 外文期刊>Nucleic Acids Research >Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates

【24h】

Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates

机译：重组在合成圆形基质上的噬菌体T4复制复合物催化的DNA合成的表征

获取原文

获取原文并翻译 | 示例

掌桥外文数据库（机构版） >>

开具论文收录证明 >>

文献代查 >>

页面导航

摘要
著录项
相似文献
相关主题

摘要

Replication complexes were reconstituted using the eight purified bacteriophage T4 replication proteins and synthetic circular 70-, 120- or 240-nt DNA substrates annealed to a leading-strand primer.To differentiate leading strands from lagging strands, the circular parts of the substrates lacked dCMP; thus, no dCTP was required for leading-strand synthesis and no dGTP for lagging-strand synthesis. The size of the substrates was crucial, the longer substrates supporting much more DNA synthesis. Leading and lagging strands were synthesized in a coupled manner. Specifically targeting leading-strand synthesis by decreasing the concentration of dGTP decreased the rate of extension of leading strands. However, blocking lagging-strand synthesis by lowering the dCTP concentration, by omitting dCTP altogether, by adding ddCTP, or with a single abasic site had no immediate effect on the rate of extension of leading strands.

机译：使用八种纯化的噬菌体T4复制蛋白和退火至前导引物的合成环状70、120或240 nt DNA底物重构复制复合物，以区分前导链和滞后链，底物的圆形部分缺少dCMP ;因此，前导链合成不需要dCTP，而落后链合成则不需要dGTP。底物的大小至关重要，较长的底物支持更多的DNA合成。前导链和滞后链以偶联方式合成。通过降低dGTP的浓度专门针对前导链合成可降低前导链的延伸速率。但是，通过降低dCTP浓度，完全省略dCTP，添加ddCTP或具有单个脱碱基位点来阻止滞后链合成，对前导链的延伸速率没有立即的影响。

著录项

来源
《Nucleic Acids Research》 |2002年第20期|共11页
作者
Farid A. Kadyrov; John W. Drake;
展开▼
作者单位

展开▼
收录信息
原文格式 PDF
正文语种 eng
中图分类细胞形态学;
关键词

相似文献

外文文献
中文文献
专利

1. Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates [J] . Farid A. Kadyrov, John W. Drake Nucleic Acids Research . 2002,第20期

机译：重组在合成圆形基质上的噬菌体T4复制复合物催化的DNA合成的表征
2. Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates [J] . Farid A. Kadyrov, John W. Drake Nucleic acids research . 2002,第20期

机译：重组在合成圆形基质上的噬菌体T4复制复合物催化的DNA合成的表征
3. In vitro reconstitution of DNA replication initiated by genetic recombination: a T4 bacteriophage model for a type of DNA synthesis important for all cells [J] . Barry Jack, Wong Mei Lie, Alberts Bruce Molecular biology of the cell . 2019,第1期

机译：通过遗传重组引发的DNA复制的体外重建：一种对所有细胞的DNA合成类型的T4噬菌体模型
4. Studies of viral DNA packaging motors with optical tweezers: a comparison of motor function in bacteriophages φ29, λ, and T4 [C] . Douglas E. Smith, Derek N. Fuller, Dorian M. Raymer, Optical Trapping and Optical Micromanipulation IV; Proceedings of SPIE-The International Society for Optical Engineering; vol.6644 . 2007

机译：带光镊的病毒DNA包装电机的研究：噬菌体φ29，λ和T4中电机功能的比较
5. Rotational-echo double resonance NMR characterization of DNA packaging in bacteriophage T4 and of Saccharomyces cerevisiae lumazine synthase-inhibitor complexes [D] . Yu, Tsyr-Yan 2008

机译：旋转回波双共振NMR表征噬菌体T4中的DNA包装和酿酒酵母鲁嗪合酶-抑制剂复合物
6. Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates [O] . Farid A. Kadyrov, John W. Drake 2002

机译：重组在合成圆形基质上的噬菌体T4复制复合物催化的DNA合成的表征
7. Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates [O] . Kadyrov, Farid A., Drake, John W. 2002

机译：重组在合成圆形基质上的噬菌体T4复制复合物催化的DNA合成的表征
8. Atomic force microscopy images of T4 bacteriophages on silicon substrates [R] . Kolbe, W. F., Ogletree, D. F., Salmeron, M. B. 1991

机译：硅基底上T4噬菌体的原子力显微镜图像

Characterization of DNA synthesis catalyzed by bacteriophage T4 replication complexes reconstituted on synthetic circular substrates

摘要

著录项

相似文献

相关主题

期刊订阅