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Improved genetic transformation of Synechococcus elongatus PCC 7942 using linear DNA fragments in association with a DNase inhibitor

机译:使用线性DNA片段与DNase抑制剂联用,改进了伸长Synechococcus longusus PCC 7942的遗传转化

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The genetic manipulation in many cyanobacterial strains is challenging yet. Thus, the development of new transformation protocols is desirable to facilitate the genetic engineering in cyanobacteria. Transformations using linear fragments yielded by PCR have advantages such as: less laborious methodology, faster procedure, low cost and unnecessary cloning steps. However, some strains presence extracellular nucleases, which reduce the efficiency in obtaining transformants. In this study, we demonstrate an improved protocol for genetic transformation in Synechococcus elongatus PCC 7942 using linear fragments employing EDTA-mediated inhibition of DNases. To conduct the transformation, linear PCR products containing the spectinomycin antibiotic resistance gene were employed. As result, 40 mM EDTA treatment increased the number of transformants obtained by eightfold in comparison to the conventional protocol using plasmid DNA. Thus, the application of exonuclease inhibitors can be considered a relevant improvement to manipulate cyanobacteria in a more efficient, faster way and as a low-cost alternative. This protocol must be helpful for other strains of cyanobacteria.
机译:许多蓝细菌菌株的遗传操作仍具有挑战性。因此,期望开发新的转化方案以促进蓝细菌中的基因工程。使用通过PCR产生的线性片段进行转化具有以下优点:省力的方法,更快的过程,低成本和不必要的克隆步骤。但是,一些菌株存在细胞外核酸酶,这降低了获得转化子的效率。在这项研究中,我们证明了使用线性片段采用EDTA介导的DNases抑制作用的改良的延长球藻PCC 7942遗传转化方案。为了进行转化,使用了包含壮观霉素抗生素抗性基因的线性PCR产物。结果,与使用质粒DNA的常规方案相比,40mM EDTA处理使获得的转化体数目增加了八倍。因此,外切核酸酶抑制剂的应用可以被视为以更有效,更快的方式并且作为低成本替代品操纵蓝细菌的相关改进。该协议必须对其他蓝细菌菌株有所帮助。

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