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Development of a genetic toolset for the highly engineerable and metabolically versatile Acinetobacter baylyi ADP1

机译:开发遗传工具集,用于高易懂和代谢通甲贝利ADP1

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One primary objective of synthetic biology is to improve the sustainability of chemical manufacturing. Naturally occurring biological systems can utilize a variety of carbon sources, including waste streams that pose challenges to traditional chemical processing, such as lignin biomass, providing opportunity for remediation and valorization of these materials. Success, however, depends on identifying micro-organisms that are both metabolically versatile and engineerable. Identifying organisms with this combination of traits has been a historic hindrance. Here, we leverage the facile genetics of the metabolically versatile bacterium Acinetobacter baylyi ADP1 to create easy and rapid molecular cloning workflows, including a Cas9-based single-step marker-less and scar-less genomic integration method. In addition, we create a promoter library, ribosomal binding site (RBS) variants and test an unprecedented number of rationally integrated bacterial chromosomal protein expression sites and variants. At last, we demonstrate the utility of these tools by examining ADP1's catabolic repression regulation, creating a strain with improved potential for lignin bioprocessing. Taken together, this work highlights ADP1 as an ideal host for a variety of sustainability and synthetic biology applications.
机译:合成生物学的一个主要目标是提高化学制造的可持续性。天然存在的生物系统可以利用各种碳源,包括对传统化学加工的废物流,例如木质素生物量,为这些材料提供修复和算的机会。然而,成功取决于鉴定代谢通用和可造成的微生物。用这种特征的组合鉴定生物是历史性的障碍。在这里,我们利用代谢通用的细菌百叶菌ADP1的细胞遗传学,以创造容易快速的分子克隆工作流程,包括基于Cas9的单步标记和疤痕的基因组积分法。此外,我们制造促进剂库,核糖体结合位点(RBS)变体,并测试前所未有的合理综合细菌染色体蛋白表达位点和变体。最后,我们通过检查ADP1的分解代谢镇压调控来展示这些工具的效用,从而产生一种改善木质素生物处理的潜力的菌株。在一起,这项工作突出了ADP1作为各种可持续性和合成生物应用的理想主持人。

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