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USER fusion: a rapid and efficient method for simultaneous fusion and cloning of multiple PCR products

机译:USER Fusion:一种快速有效的方法,可同时融合和克隆多种PCR产物

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摘要

We present a method that allows simultaneous fusion and cloning of multiple PCR products in a rapid and efficient manner. The procedure is based on the use of PCR primers that contain a single deoxyuridine residue near their 5′ end. Treatment of the PCR products with a commercial deoxyuridine-excision reagent generates long 3′ overhangs designed to specifically complement each other. The combination of this principle with the improved USER cloning technique provides a simple, fast and very efficient method to simultaneously fuse and clone multiple PCR fragments into a vector of interest. Around 90% positive clones were obtained when three different PCR products were fused and cloned into a USER-compatible vector in a simple procedure that, apart from the single PCR amplification step and the bacterial transformation, took approximately one hour. We expect this method to replace overlapping PCR and the use of type IIS restriction enzymes in many of their applications.
机译:我们提出了一种方法,该方法允许以快速有效的方式同时融合和克隆多个PCR产物。该程序基于使用在其5'末端附近包含单个脱氧尿苷残基的PCR引物。用市售的脱氧尿苷切除试剂处理PCR产物会产生较长的3'突出端,这些突出端设计为可以特异性互补。该原理与改进的USER克隆技术的结合提供了一种简单,快速且非常有效的方法,可将多个PCR片段同时融合并克隆到目标载体中。当将三个不同的PCR产物融合并以简单的程序克隆到USER兼容的载体中时,获得了大约90%的阳性克隆,该过程除了单个PCR扩增步骤和细菌转化外,大约需要一个小时。我们希望这种方法能够代替重叠PCR并在其许多应用中使用IIS型限制酶。

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