Design of an effective small expression tag to enhance GPCR production in E. coli‐based cell‐free and whole cell expression systems

Author:

Cho Seongyeon1,Lee Haein1,Han Yong Hee2,Park Tae Shin3,Seo Sang Woo12,Park Tai Hyun124ORCID

Affiliation:

1. School of Chemical and Biological Engineering, Institute of Chemical Process Seoul National University Seoul Republic of Korea

2. Interdisciplinary Program in Bioengineering Seoul National University Seoul Republic of Korea

3. Receptech Research Institute, Receptech Inc. Siheung Republic of Korea

4. Department of Nutritional Science and Food Management Ewha Womans University Seoul Republic of Korea

Abstract

AbstractG protein‐coupled receptors (GPCRs) play crucial roles in sensory, immune, and tumor metastasis processes, making them valuable targets for pharmacological and sensing applications in various industries. However, most GPCRs have low production yields in Escherichia coli (E. coli) expression systems. To overcome this limitation, we introduced AT10 tag, an effective fusion tag that could significantly enhance expression levels of various GPCRs in E. coli and its derived cell‐free protein synthesis (CFPS) system. This AT10 tag consisted of an A/T‐rich gene sequence designed via optimization of translation initiation rate. It is translated into a short peptide sequence of 10 amino acids at the N‐terminus of GPCRs. Additionally, effector proteins could be utilized to suppress cytotoxicity caused by membrane protein expression, further boosting GPCR production in E. coli. Enhanced expression of various GPCRs using this AT10 tag is a promising approach for large‐scale production of functional GPCRs in E. coli‐based CFPS and whole cell systems, enabling their potential utilization across a wide range of industrial applications.

Funder

Ministry of Trade, Industry and Energy

Publisher

Wiley

Subject

Molecular Biology,Biochemistry

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