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工程改造毕赤酵母以高效生产高价值甾体中间体15α-羟基-D-乙基孕烯醇酮。

Engineering Pichia pastoris for the efficient production of the high-value steroid intermediate 15α-OH-D-ethylgonendione.

作者信息

Zeng Yu-Long, Li Yang-Yang, Zheng Bei-Feng-Chu, Xie Dong-Qi, Tong Sheng-Qiang, Yuan Yuan, Wang Ya-Jun, Xue Bin, Liu Xiao-Guang

机构信息

College of Pharmaceutical Science, Zhejiang University of Technology, Hangzhou, 310032, Zhejiang, China.

Zhejiang Key Laboratory of Green Manufacturing Technology for Chemical Drugs, Deqing, 313200, Zhejiang, China.

出版信息

Microb Cell Fact. 2025 Jul 21;24(1):170. doi: 10.1186/s12934-025-02796-9.

Abstract

15α-OH-D-ethylgonendione (15α-OH-DE) is a key intermediate for the synthesis of steroid drug gestodene, a major component of a new generation of powerful contraceptives. Synthetic access to 15α-OH-DE by chemical means is limited by low titers and generation of toxic byproducts. To develop a sustainable process for 15α-OH-DE production, a whole-cell catalyst was constructed by engineering Pichia pastoris co-overexpressing the PRH gene from filamentous fungus Penicillium raistrickii, which encodes a steroid 15α-hydroxylase capable of selectively 15α-hydroxylating DE, and the glucose-6-phosphate dehydrogenase gene ZWF1 from the baker's yeast for enhanced NADPH production. Shake-flask cultivation was performed to optimize fermentation parameters and assess the potential of the engineered P. pastoris strains for 15α-OH-DE production. Subsequently, production was scaled up using a fed-batch strategy in a 5-L stirred-tank bioreactor, with pure methanol serving as both the carbon source and inducer. This process achieved a product titer of 5.79 g L⁻¹ with DE feeding of 10 g L after 170 h of methanol feeding (196 h fermentation), representing the highest reported titer of 15α-OH-DE to date. The above results highlight the potential of developing P. pastoris-based biotransformation systems for the efficient production of key intermediates of steroid pharmaceuticals and other high-value fine chemicals.

摘要

15α-羟基-D-乙基孕烯二酮(15α-OH-DE)是合成甾体药物孕二烯酮的关键中间体,孕二烯酮是新一代强效避孕药的主要成分。通过化学方法合成15α-OH-DE受到低产率和有毒副产物生成的限制。为了开发一种可持续的15α-OH-DE生产工艺,通过对巴斯德毕赤酵母进行工程改造构建了一种全细胞催化剂,该酵母共过表达了丝状真菌雷斯垂克青霉的PRH基因,该基因编码一种能够选择性地将DE进行15α-羟基化的甾体15α-羟化酶,以及面包酵母的葡萄糖-6-磷酸脱氢酶基因ZWF1以增强NADPH的产生。进行摇瓶培养以优化发酵参数并评估工程化毕赤酵母菌株生产15α-OH-DE的潜力。随后,在5-L搅拌罐生物反应器中采用补料分批策略进行放大生产,使用纯甲醇作为碳源和诱导剂。在甲醇补料170小时(发酵196小时)后,当DE进料为10 g/L时,该工艺实现了5.79 g/L的产物滴度,这是迄今为止报道的15α-OH-DE的最高滴度。上述结果突出了开发基于毕赤酵母的生物转化系统用于高效生产甾体药物关键中间体和其他高价值精细化学品的潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/45c2/12278525/8b71a17b9d35/12934_2025_2796_Fig1_HTML.jpg

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