Mutational analysis in Corynebacterium stationis MFS transporters for improving nucleotide bioproduction

Author:

Kinose Keita,Shinoda Keiko,Konishi Tomoyuki,Kawasaki HisashiORCID

Abstract

Abstract Product secretion from an engineered cell can be advantageous for microbial cell factories. Extensive work on nucleotide manufacturing, one of the most successful microbial fermentation processes, has enabled Corynebacterium stationis to transport nucleotides outside the cell by random mutagenesis; however, the underlying mechanism has not been elucidated, hindering its applications in transporter engineering. Herein, we report the nucleotide-exporting major facilitator superfamily (MFS) transporter from the C. stationis genome and its hyperactive mutation at the G64 residue. Structural estimation and molecular dynamics simulations suggested that the activity of this transporter improved via two mechanisms: (1) enhancing interactions between transmembrane helices through the conserved “RxxQG” motif along with substrate binding and (2) trapping substrate-interacting residue for easier release from the cavity. Our results provide novel insights into how MFS transporters change their conformation from inward- to outward-facing states upon substrate binding to facilitate efflux and can contribute to the development of rational design approaches for efflux improvements in microbial cell factories. Keypoints • An MFS transporter from C. stationis genome and its mutation at residue G64 were assessed • It enhanced the transporter activity by strengthening transmembrane helix interactions and trapped substrate-interacting residues • Our results contribute to rational design approach development for efflux improvement Graphical Abstract

Funder

The research center for computational science, Okazaki

Japan Society for the Promotion of Science

Institute for Fermentation, Osaka

Oriental Yeast Co., Ltd.

Program for Promoting Research on the Supercomputer Fugaku

The University of Tokyo

Publisher

Springer Science and Business Media LLC

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