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An expanded CRISPRi toolbox for tunable control of gene expression in Pseudomonas putida

机译:一个扩展的CRIPRI工具箱,用于PSEUDOUNAS PITIDA中基因表达的可调控制

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Owing to its wide metabolic versatility and physiological robustness, together with amenability to genetic manipulations and high resistance to stressful conditions, Pseudomonas putida is increasingly becoming the organism of choice for a range of applications in both industrial and environmental applications. However, a range of applied synthetic biology and metabolic engineering approaches are still limited by the lack of specific genetic tools to effectively and efficiently regulate the expression of target genes. Here, we present a single-plasmid CRISPR-interference (CRISPRi) system expressing a nuclease-deficient cas9 gene under the control of the inducible XylS/P-m expression system, along with the option of adopting constitutively expressed guide RNAs (either sgRNA or crRNA and tracrRNA). We showed that the system enables tunable, tightly controlled gene repression (up to 90%) of chromosomally expressed genes encoding fluorescent proteins, either individually or simultaneously. In addition, we demonstrate that this method allows for suppressing the expression of the essential genes pyrF and ftsZ, resulting in significantly low growth rates or morphological changes respectively. This versatile system expands the capabilities of the current CRISPRi toolbox for efficient, targeted and controllable manipulation of gene expression in P. putida.
机译:由于其广泛的代谢多功能性和生理稳健性,与遗传操作和高抗压力条件的敏感性,Pseudomonas普韦达越来越多地成为工业和环境应用中一系列应用的选择。然而,一系列应用的合成生物学和代谢工程方法仍然受到缺乏特异性遗传工具的限制,以有效和有效地调节靶基因的表达。在这里,我们在诱导型Xyls / PM表达系统的控制下,在诱导Xyls / PM表达系统的控制下表达表达核酸酶缺陷Cas9基因的单质粒Crisprup(Crispri)系统,以及采用组成思考的指导RNA(SGRNA或CRRNA和tracrrna)。我们表明该系统能够通过单独或同时进行可调谐,紧密控制的基因抑制(高达90%)的染色体表达基因编码荧光蛋白。此外,我们证明该方法允许抑制必需基因PyrF和FTSZ的表达,从而分别产生明显低的生长率或形态变化。这种多功能系统扩展了当前CRISPRI工具箱的能力,以便在P. Pivida中的基因表达的有效,有针对性和可控操作。

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