Biosynthesis of a New Fusaoctaxin Virulence Factor in Fusarium graminearum Relies on a Distinct Path To Form a Guanidinoacetyl Starter Unit Priming Nonribosomal Octapeptidyl Assembly

Fusarium graminearum is a pathogenic fungus causing huge economic losses worldwide via crop infection leading to yield reduction and grain contamination. The process through which the fungal invasion occurs remains poorly understood. We recently characterized fusaoctaxin A in F. graminearum, where t...

Full description

Saved in:
Bibliographic Details
Published in:Journal of the American Chemical Society 2021-12, Vol.143 (47), p.19719-19730
Main Authors: Tang, Zhijun, Tang, Haoyu, Wang, Wanqiu, Xue, Yufeng, Chen, Dandan, Tang, Weihua, Liu, Wen
Format: Article
Language:English
Subjects:
Amidohydrolases - metabolism
Carbon-Carbon Lyases - metabolism
Cytochrome P-450 Enzyme System - metabolism
Fungal Proteins - biosynthesis
Fungal Proteins - genetics
Fusarium - genetics
Fusarium - metabolism
Multigene Family
Oligopeptides - biosynthesis
Oligopeptides - genetics
Virulence Factors - biosynthesis
Virulence Factors - genetics
Citations: Items that this one cites
Items that cite this one
Online Access:Get full text
Tags: Add Tag
No Tags, Be the first to tag this record!
Description
Summary:Fusarium graminearum is a pathogenic fungus causing huge economic losses worldwide via crop infection leading to yield reduction and grain contamination. The process through which the fungal invasion occurs remains poorly understood. We recently characterized fusaoctaxin A in F. graminearum, where this octapeptide virulence factor results from an assembly line encoded in fg3_54, a gene cluster proved to be involved in fungal pathogenicity and host adaptation. Focusing on genes in this cluster that are related to fungal invasiveness but not to the biosynthesis of fusaoctaxin A, we here report the identification and characterization of fusaoctaxin B, a new octapeptide virulence factor with comparable activity in wheat infection. Fusaoctaxin B differs from fusaoctaxin A at the N-terminus by possessing a guanidinoacetic acid (GAA) unit, formation of which depends on the combined activities of the protein products of fgm1–3. Fgm1 is a cytochrome P450 protein that oxygenates l-Arg to 4­(R)-hydroxyl-l-Arg in a regio- and stereoselective manner. Then, Cβ–Cγ bond cleavage proceeds in the presence of Fgm3, a pyridoxal-5′-phosphate-dependent lyase, giving guanidinoacetaldehyde and l-Ala. Rather than being directly oxidized to GAA, the guanidine-containing aldehyde undergoes spontaneous cyclization and subsequent enzymatic dehydrogenation to provide glycociamidine, which is linearized by Fgm2, a metallo-dependent amidohydrolase. The GAA path in F. graminearum is distinct from that previously known to involve l-Arg:l-Gly aminidotransferase activity. To provide this nonproteinogenic starter unit that primes nonribosomal octapeptidyl assembly, F. graminearum employs new chemistry to process l-Arg through inert C–H bond activation, selective C–C bond cleavage, cyclization-based alcohol dehydrogenation, and amidohydrolysis-associated linearization.
ISSN:0002-7863
1520-5126
DOI:10.1021/jacs.1c07770