In Vitro Module Editing Of NRPS Enables Production Of Highly Potent Gq‐Signaling Inhibitor FR900359 Derived From Unculturable Plant Symbiont

Author:

Hashimoto Takuya12ORCID,Suenaga Hikaru1,Amagai Keita3,Hashimoto Junko4,Kozone Ikuko4,Takahashi Shunji3,Shin‐ya Kazuo1ORCID

Affiliation:

1. National Institute of Advanced Industrial Science and Technology 2-4-7 Aomi Koto-ku Tokyo 135-0064 Japan

2. National Institute of Advanced Industrial Science and Technology 1-1-1 Higashi Tsukuba Ibaraki 305-8566 Japan

3. Natural Product Biosynthesis Research Unit RIKEN Center for Sustainable Resource Science 2-1 Hirosawa Wako Saitama 351-0198 Japan

4. Japan Biological Informatics Consortium 2-4-7 Aomi Koto-ku Tokyo 135-0064 Japan

Abstract

AbstractHeterotrimeric G proteins are key mediators in the signaling of G protein‐coupled receptors (GPCR) that are involved in a plethora of important physiological processes and thus major targets of pharmaceutical drugs. The cyclic depsipeptides YM‐254890 and FR900359 are strong and selective inhibitors of the Gq subfamily of G proteins. FR900359 was first reported to be produced by unculturable plant symbiont, however, a culturable FR900359 producer was discovered recently by the standard strategy, screening of the producing strain from the environment. As another strategy, we introduce herein the different way to supply natural compounds of unculturable microorganism origin. We therefore embarked on constructing an artificial biosynthetic gene cluster (BGC) for FR900359 with YM‐254890 BGC as a template using “in vitro module editing” technology, first developed for the modification of type‐I PKS BGCs, to edit YM‐254890 BGC. The resulting artificial BGCs coding FR900359 were heterologously expressed in the Pseudomonas putida KT2440 host strain.

Funder

Japan Agency for Medical Research and Development

Japan Society for the Promotion of Science

Publisher

Wiley

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