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Evaluation of the efficiency and utility of recombinant enzyme-free seamless DNA cloning methods

机译:重组无酶无缝DNA克隆方法的效率和实用性评估

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Simple and low-cost recombinant enzyme-free seamless DNA cloning methods have recently become available. In vivo Escherichia coli cloning (iVEC) can directly transform a mixture of insert and vector DNA fragments into E. coli, which are ligated by endogenous homologous recombination activity in the cells. Seamless ligation cloning extract (SLiCE) cloning uses the endogenous recombination activity of E. coli cellular extracts in vitro to ligate insert and vector DNA fragments. An evaluation of the efficiency and utility of these methods is important in deciding the adoption of a seamless cloning method as a useful tool. In this study, both seamless cloning methods incorporated inserting DNA fragments into linearized DNA vectors through short (15–39 bp) end homology regions. However, colony formation was 30–60-fold higher with SLiCE cloning in end homology regions between 15 and 29 bp than with the iVEC method using DH5α competent cells. E. coli AQ3625 strains, which harbor a sbcA gene mutation that activates the RecE homologous recombination pathway, can be used to efficiently ligate insert and vector DNA fragments with short-end homology regions in vivo. Using AQ3625 competent cells in the iVEC method improved the rate of colony formation, but the efficiency and accuracy of SLiCE cloning were still higher. In addition, the efficiency of seamless cloning methods depends on the intrinsic competency of E. coli cells. The competency of chemically competent AQ3625 cells was lower than that of competent DH5α cells, in all cases of chemically competent cell preparations using the three different methods. Moreover, SLiCE cloning permits the use of both homemade and commercially available competent cells because it can use general E. coli recA strains such as DH5α as host cells for transformation. Therefore, between the two methods, SLiCE cloning provides both higher efficiency and better utility than the iVEC method for seamless DNA plasmid engineering.
机译:简单和低成本的无重组酶的无缝DNA克隆方法最近已经可用。体内大肠杆菌克隆(iVEC)可以将插入片段和载体DNA片段的混合物直接转化为大肠杆菌,并通过细胞中的内源同源重组活性进行连接。无缝连接克隆提取物(SLiCE)克隆利用体外大肠杆菌细胞提取物的内源重组活性来连接插入片段和载体DNA片段。在决定采用无缝克隆方法作为有用工具时,评估这些方法的效率和实用性很重要。在这项研究中,这两种无缝克隆方法都将DNA片段通过短(15-39 bp)末端同源区域插入线性化DNA载体中。然而,与使用DH5α感受态细胞的iVEC方法相比,SLiCE克隆在15至29bp之间的末端同源区域克隆的形成要高30-60倍。带有激活RecE同源重组途径的sbcA基因突变的大肠杆菌AQ3625菌株可用于有效连接体内具有短端同源区域的插入片段和载体DNA片段。在iVEC方法中使用AQ3625感受态细胞可以提高集落形成的速率,但是SLiCE克隆的效率和准确性仍然更高。另外,无缝克隆方法的效率取决于大肠杆菌细胞的固有能力。在所有使用三种不同方法制备化学感受态细胞的情况下,化学感受态AQ3625细胞的能力均低于感受态DH5α细胞的能力。此外,SLiCE克隆允许同时使用自制的和市售的感受态细胞,因为它可以使用一般的大肠杆菌recA -菌株(例如DH5α)作为宿主细胞进行转化。因此,在两种方法之间,SLiCE克隆比用于无缝DNA质粒工程的iVEC方法提供更高的效率和更好的实用性。

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