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长链特异性醛还原酶的鉴定及其在大肠杆菌中提高脂肪醇产量的应用。

Identification of long chain specific aldehyde reductase and its use in enhanced fatty alcohol production in E. coli.

作者信息

Fatma Zia, Jawed Kamran, Mattam Anu Jose, Yazdani Syed Shams

机构信息

Synthetic Biology and Biofuels Group, International Centre for Genetic Engineering and Biotechnology, New Delhi, India.

Synthetic Biology and Biofuels Group, International Centre for Genetic Engineering and Biotechnology, New Delhi, India; DBT-ICGEB Centre for Advanced Bioenergy Research, International Centre for Genetic Engineering and Biotechnology, New Delhi, India.

出版信息

Metab Eng. 2016 Sep;37:35-45. doi: 10.1016/j.ymben.2016.04.003. Epub 2016 Apr 28.

Abstract

Long chain fatty alcohols have wide application in chemical industries and transportation sector. There is no direct natural reservoir for long chain fatty alcohol production, thus many groups explored metabolic engineering approaches for its microbial production. Escherichia coli has been the major microbial platform for this effort, however, terminal endogenous enzyme responsible for converting fatty aldehydes of chain length C14-C18 to corresponding fatty alcohols is still been elusive. Through our in silico analysis we selected 35 endogenous enzymes of E. coli having potential of converting long chain fatty aldehydes to fatty alcohols and studied their role under in vivo condition. We found that deletion of ybbO gene, which encodes NADP(+) dependent aldehyde reductase, led to >90% reduction in long chain fatty alcohol production. This feature was found to be strain transcending and reinstalling ybbO gene via plasmid retained the ability of mutant to produce long chain fatty alcohols. Enzyme kinetic study revealed that YbbO has wide substrate specificity ranging from C6 to C18 aldehyde, with maximum affinity and efficiency for C18 and C16 chain length aldehyde, respectively. Along with endogenous production of fatty aldehyde via optimized heterologous expression of cyanobaterial acyl-ACP reductase (AAR), YbbO overexpression resulted in 169mg/L of long chain fatty alcohols. Further engineering involving modulation of fatty acid as well as of phospholipid biosynthesis pathway improved fatty alcohol production by 60%. Finally, the engineered strain produced 1989mg/L of long chain fatty alcohol in bioreactor under fed-batch cultivation condition. Our study shows for the first time a predominant role of a single enzyme in production of long chain fatty alcohols from fatty aldehydes as well as of modulation of phospholipid pathway in increasing the fatty alcohol production.

摘要

长链脂肪醇在化学工业和交通运输领域有着广泛应用。长链脂肪醇的生产没有直接的天然储存库,因此许多研究团队探索了通过代谢工程方法进行微生物生产。大肠杆菌一直是这项工作的主要微生物平台,然而,负责将碳链长度为C14 - C18的脂肪醛转化为相应脂肪醇的末端内源酶仍然难以捉摸。通过我们的计算机模拟分析,我们选择了35种大肠杆菌内源酶,它们具有将长链脂肪醛转化为脂肪醇的潜力,并研究了它们在体内条件下的作用。我们发现,编码NADP(+)依赖性醛还原酶的ybbO基因缺失导致长链脂肪醇产量降低>90%。这一特性具有菌株通用性,通过质粒重新导入ybbO基因可使突变体保留生产长链脂肪醇的能力。酶动力学研究表明,YbbO具有广泛的底物特异性,范围从C6到C18醛,对C18和C16链长醛的亲和力和效率最高。通过优化蓝细菌酰基-ACP还原酶(AAR)的异源表达实现脂肪醛的内源生产,同时过表达YbbO,可产生169mg/L的长链脂肪醇。进一步对脂肪酸以及磷脂生物合成途径进行工程改造,使脂肪醇产量提高了60%。最终,工程菌株在补料分批培养条件下的生物反应器中生产了1989mg/L的长链脂肪醇。我们的研究首次表明了单一酶在从脂肪醛生产长链脂肪醇以及调节磷脂途径以提高脂肪醇产量方面的主要作用。

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