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A new recombineering system for Photorhabdus and Xenorhabdus

机译:Photorhabdus和Xenorhabdus的新重组系统

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摘要

Precise and fluent genetic manipulation is still limited to only a few prokaryotes. Ideally the highly advanced technologies available in Escherichia coli could be broadly applied. Our efforts to apply lambda Red technology, widely termed ‘recombineering’, in Photorhabdus and Xenorhabdus yielded only limited success. Consequently we explored the properties of an endogenous Photorhabdus luminescens lambda Red-like operon, Plu2934/Plu2935/Plu2936. Bioinformatic and functional tests indicate that Plu2936 is a 5’-3’ exonuclease equivalent to Redα and Plu2935 is a single strand annealing protein equivalent to Redβ. Plu2934 dramatically enhanced recombineering efficiency. Results from bioinformatic analysis and recombineering assays suggest that Plu2934 may be functionally equivalent to Redγ, which inhibits the major endogenous E. coli nuclease, RecBCD. The recombineering utility of Plu2934/Plu2935/Plu2936 was demonstrated by engineering Photorhabdus and Xenorhabdus genomes, including the activation of the 49-kb non-ribosomal peptide synthase (NRPS) gene cluster plu2670 by insertion of a tetracycline inducible promoter. After tetracycline induction, novel secondary metabolites were identified. Our work unlocks the potential for bioprospecting and functional genomics in the Photorhabdus, Xenorhabdus and related genomes.
机译:精确而流畅的遗传操作仍然仅限于少数原核生物。理想地,大肠杆菌中可用的高度先进的技术可以广泛应用。我们在Photorhabdus和Xenorhabdus中应用被广泛称为“重组”的lambda Red技术的努力仅取得了有限的成功。因此,我们探索了内源性光子菌(Photorhabdus luminescens lambda Red)操纵子Plu2934 / Plu2935 / Plu2936的性质。生物信息学和功能测试表明,Plu2936是等同于Redα的5'-3'核酸外切酶,Plu2935是等同于Redβ的单链退火蛋白。 Plu2934大大提高了重组效率。生物信息学分析和重组分析的结果表明,Plu2934在功能上可能与Redγ相同,后者可抑制主要的内源性大肠杆菌核酸酶RecBCD。 Plu2934 / Plu2935 / Plu2936的重组效用已通过工程化的Photorhabdus和Xenorhabdus基因组得到证明,包括通过插入四环素诱导型启动子激活49kb非核糖体肽合酶(NRPS)基因簇plu2670。四环素诱导后,鉴定出新的次级代谢产物。我们的工作释放了Photorhabdus,Xenorhabdus和相关基因组中生物勘探和功能基因组学的潜力。

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