9PC6

Antibody (1B2) Bound Crosslinked Rifamycin Synthetase Module 1 with a C-terminal Type II Thioesterase

これはPDB形式変換不可エントリーです。

9PC6 の概要

• エントリーDOI: 10.2210/pdb9pc6/pdb
• EMDBエントリー: 71497
• 分子名称: 6-deoxyerythronolide-B synthase,RifR, Antibody Fragment 1B2 Heavy Chain, Antibody Fragment 1B2 Light Chain (3 entities in total)
• 機能のキーワード: polyketide synthase module, antibody (fab), transferase-immune system complex, transferase/immune system
• 由来する生物種: Amycolatopsis mediterranei; 詳細
• タンパク質・核酸の鎖数: 6
• 化学式量合計: 496343.17

構造登録者

Cogan, D.P.,Liu, C.,West, R.C.,Chen, M. (登録日: 2025-06-27, 公開日: 2025-07-23)

主引用文献

Liu, C.,West, R.C.,Chen, M.,Cohn, W.,Wang, G.,Mandot, A.M.,Kim, S.,Cogan, D.P.
Molecular Basis for Asynchronous Chain Elongation During Rifamycin Antibiotic Biosynthesis.
Biorxiv, 2025

PubMed Abstract: The rifamycin synthetase (RIFS) from the bacterium is a large (3.5 MDa) multienzyme system that catalyzes over 40 chemical reactions to generate a complex precursor to the antibiotic rifamycin B. It is considered a hybrid enzymatic assembly line and consists of an N-terminal nonribosomal peptide synthetase loading module followed by a decamodular polyketide synthase (PKS). While the biosynthetic functions are known for each enzymatic domain of RIFS, structural and biochemical analyses of this system from purified components are relatively scarce. Here, we examine the biosynthetic mechanism of RIFS through complementary crosslinking, kinetic, and structural analyses of its first PKS module (M1). Thiol-selective crosslinking of M1 provided a plausible molecular basis for previously observed conformational asymmetry with respect to ketosynthase (KS)-substrate carrier protein (CP) interactions during polyketide chain elongation. Our data suggest that C-terminal dimeric interfaces-which are ubiquitous in bacterial PKSs-force their adjacent CP domains to co-migrate between two equivalent KS active site chambers. Cryogenic electron microscopy analysis of M1 further supported this observation while uncovering its unique architecture. Single-turnover kinetic analysis of M1 indicated that although removal of C-terminal dimeric interfaces supported 2-fold greater KS-CP interactions, it did not increase the partial product occupancy of the homodimeric protein. Our findings cast light on molecular details of natural antibiotic biosynthesis that will aid in the design of artificial megasynth(et)ases with untold product structures and bioactivities.

PubMed: 40631255
DOI: 10.1101/2025.07.05.663307

実験手法

ELECTRON MICROSCOPY (3.96 Å)