Fu Changlin, Wehr Daniel R, Edwards Janice, Hauge Brian
Monsanto Company, 800 N. Lindbergh Blvd., St Louis, MO 63167, USA.
Nucleic Acids Res. 2008 May;36(9):e54. doi: 10.1093/nar/gkn167. Epub 2008 Apr 19.
As an increasing number of genes and open reading frames of unknown function are discovered, expression of the encoded proteins is critical toward establishing function. Accordingly, there is an increased need for highly efficient, high-fidelity methods for directional cloning. Among the available methods, site-specific recombination-based cloning techniques, which eliminate the use of restriction endonucleases and ligase, have been widely used for high-throughput (HTP) procedures. We have developed a recombination cloning method, which uses truncated recombination sites to clone PCR products directly into destination/expression vectors, thereby bypassing the requirement for first producing an entry clone. Cloning efficiencies in excess of 80% are obtained providing a highly efficient method for directional HTP cloning.
随着越来越多功能未知的基因和开放阅读框被发现,编码蛋白质的表达对于确定其功能至关重要。因此,对高效、高保真的定向克隆方法的需求日益增加。在现有的方法中,基于位点特异性重组的克隆技术无需使用限制性内切酶和连接酶,已被广泛应用于高通量(HTP)操作。我们开发了一种重组克隆方法,该方法利用截短的重组位点将PCR产物直接克隆到目的/表达载体中,从而无需先构建入门克隆。克隆效率超过80%,为定向HTP克隆提供了一种高效方法。
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