Construction of two pGEM-7Zf(+) phagemid T-tail vectors using AhdI-restriction endonuclease sites for direct cloning of PCR products.

Jeung J; Cho S; Shim K; Ok S; Lim D; Shin J

首页> 外文期刊>Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems >Construction of two pGEM-7Zf(+) phagemid T-tail vectors using AhdI-restriction endonuclease sites for direct cloning of PCR products.

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Construction of two pGEM-7Zf(+) phagemid T-tail vectors using AhdI-restriction endonuclease sites for direct cloning of PCR products.

机译：使用AhdI限制性内切核酸酶位点构建两个pGEM-7Zf（+）噬菌粒T尾载体，用于PCR产物的直接克隆。

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For applications such as sequencing, transfection, and in vitro transcription, PCR products have to be subcloned into plasmids. Many strategies are used for cloning, blunt-end ligation or the incorporation of restriction endonuclease sites into PCR primers for appropriate vectors. However, the most convenient and direct method is T/A cloning. In this study, we developed two of the pGEM-7Zf(+) phagemid T-tail vectors using AhdI-restriction endonuclease sites, and these T vectors have all the features of pGEM-7Zf(+): f1 ori, T7, and SP6 RNA polymerase promoters, the alpha-peptide coding region of beta-galactosidase for X-gal blue/white color selection, the beta-lactamase gene for recombinant colony selection, and binding sites for pUC/M13 forward and reverse sequencing primers. These AhdI-containing phagemid vectors, pGEM-NJ105 and pGEM-NJ107, are useful for the easy and inexpensive preparation of T vectors and direct cloning of PCR products.

机译：对于测序，转染和体外转录等应用，PCR产物必须亚克隆到质粒中。许多策略被用于克隆，平末端连接或将限制性核酸内切酶位点掺入适当载体的PCR引物中。但是，最方便直接的方法是T / A克隆。在这项研究中，我们使用AhdI限制性内切核酸酶位点开发了两个pGEM-7Zf（+）噬菌粒T-tail载体，这些T载体具有pGEM-7Zf（+）的所有功能：f1，ori，T7和SP6 RNA聚合酶启动子，用于X-gal蓝色/白色选择的β-半乳糖苷酶的α-肽编码区，用于重组菌落选择的β-内酰胺酶基因以及pUC / M13正向和反向测序引物的结合位点。这些含AhdI的噬菌粒载体pGEM-NJ105和pGEM-NJ107可用于简便，廉价地制备T载体和直接克隆PCR产物。

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《Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems》 |2002年第2期|共1页
作者
Jeung J; Cho S; Shim K; Ok S; Lim D; Shin J;
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正文语种 eng
中图分类医学遗传学;
关键词
Polymerase Chain Reaction; Cloning; DNA Restriction Enzymes; Construction; 聚合酶链反应; DNA限制酶类;

机译：Polymerase Chain Reaction;Cloning;DNA Restriction Enzymes;Construction;聚合酶链反应;DNA限制酶类;

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1. Construction of two pGEM-7Zf(+) phagemid T-tail vectors using AhdI-restriction endonuclease sites for direct cloning of PCR products. [J] . Jeung J, Cho S, Shim K, Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems . 2002,第2期

机译：使用AhdI限制性内切核酸酶位点构建两个pGEM-7Zf（+）噬菌粒T尾载体，用于PCR产物的直接克隆。
2. Construction of T-Vectors for the Direct, Unidirectional Cloning, and Analysis of PCR-Amplified Promoters [J] . B. L. Wang, X. X. Li, F. Zheng Molecular Biology . 2007,第4期

机译：直接，单向克隆和PCR扩增启动子分析的T载体的构建
3. Construction of T-vectors, a rapid and general system for direct cloning of unmodified PCR products [J] . Nucleic acids research . 1991,第5期

机译：T载体的构建，一种直接克隆未修饰PCR产物的快速通用系统
4. Cloning of barley genomic DNA fragments into the hind ill site of the plasmld pGEM-7Zf(-) [C] . Jubrael Jaladet M.S., Ibrahim Suhaila A., Abed Harb A. Regional Symposium on Integrated Crop-Livestock Systems in the Dry Areas of West Asia and North Africa . 1997

机译：将大麦基因组DNA片段克隆到PGEM-7ZF（ - ）的后病皮病点
5. Collaborative homing directed by site-specific endonucleases in bacteriophages [D] . Zeng, Qinglu 2008

机译：噬菌体中位点特异性核酸内切酶指导的协同归巢
6. Construction of T-vectors a rapid and general system for direct cloning of unmodified PCR products. [O] . D Marchuk, M Drumm, A Saulino, 1991

机译：T载体的构建这是一种直接克隆未修饰PCR产物的快速通用系统。
7. Construction of T-vectors, a rapid and general system for direct cloning of unmodified PCR products. [O] . Marchuk, D, Drumm, M, Saulino, A, 1991

机译：T载体的构建，这是一种直接克隆未修饰PCR产物的快速通用系统。

Construction of two pGEM-7Zf(+) phagemid T-tail vectors using AhdI-restriction endonuclease sites for direct cloning of PCR products.

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