Reactivity-based screening for citrulline-containing natural products reveals a family of bacterial peptidyl arginine deiminases

Harris, Lonnie A.; Saint-Vincent, Patricia M. B.; Guo, Xiaorui; Hudson, Graham A.; Mitchell, Douglas A.

doi:10.1101/2020.07.16.207027

Cited by 3 publications

(2 citation statements)

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“…3,17,24,25 Beyond the minimal BGC required for lasso peptide biosynthesis and commonly associated transporters and isopeptidases, genome mining of the ever-growing database of bacterial genome sequences 12 has revealed tailoring enzymes that subject lasso peptides to further post-translational modifications (PTMs). Modifications that have been confirmed experimentally include disulfide bonds, 26,27 C-terminal methylation, 19,28 acetylation, 29 citrullination, 30 phosphorylation, 31 glycosylation, 32 epimerization, 26,33 and β-hydroxylation. 6,34 All previously described lasso peptide PTMs occur in either the loop or tail regions of the lasso peptide, and these auxiliary enzymes recognize the linear precursor rather than the matured lasso as a substrate.…”

Section: ■ Introductionmentioning

confidence: 93%

Cellulonodin-2 and Lihuanodin: Lasso Peptides with an Aspartimide Post-Translational Modification

et al. 2021

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Lasso peptides are a family of ribosomally synthesized and post-translationally modified peptides (RiPPs) defined by their threaded structure. Besides the class-defining isopeptide bond, other post-translational modifications (PTMs) that further tailor lasso peptides have been previously reported. Using genome mining tools, we identified a subset of lasso peptide biosynthetic gene clusters (BGCs) that are colocalized with genes encoding protein l-isoaspartyl methyltransferase (PIMT) homologues. PIMTs have an important role in protein repair, restoring isoaspartate residues formed from asparagine deamidation to aspartate. Here we report a new function for PIMT enzymes in the post-translational modification of lasso peptides. The PIMTs associated with lasso peptide BGCs first methylate an l-aspartate side chain found within the ring of the lasso peptide. The methyl ester is then converted into a stable aspartimide moiety, endowing the lasso peptide ring with rigidity relative to its unmodified counterpart. We describe the heterologous expression and structural characterization of two examples of aspartimide-modified lasso peptides from thermophilic Gram-positive bacteria. The lasso peptide cellulonodin-2 is encoded in the genome of actinobacterium Thermobifida cellulosilytica, while lihuanodin is encoded in the genome of firmicute Lihuaxuella thermophila. Additional genome mining revealed PIMT-containing lasso peptide BGCs in 48 organisms. In addition to heterologous expression, we have reconstituted PIMT-mediated aspartimide formation in vitro, showing that lasso peptide-associated PIMTs transfer methyl groups very rapidly as compared to canonical PIMTs. Furthermore, in stark contrast to other characterized lasso peptide PTMs, the methyltransferase functions only on lassoed substrates.

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Section: ■ Introductionmentioning

confidence: 93%

Cellulonodin-2 and Lihuanodin: Lasso Peptides with an Aspartimide Post-Translational Modification

et al. 2021

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“…This chemistry-based approach can be guided by genomic prioritization to only include strains capable of installing the targeted functional group, thus expediting natural product discovery. We have used reactivity-based screening to identify α/β-unsaturated carbonyl-containing natural products via 1,4-nucleophilic addition, reactive carbonyl-containing compounds via oxime ligation, and primary ureido-group-containing compounds via nucleophilic addition onto glyoxal-based probes. − Other research groups have reported related approaches for elucidating the proteomic targets of natural products, chemoselective natural product enrichment, and methodology to covalently target di/trienes using a nitrosopyridine-based probe. − To target the electron-rich polyene common to all GPMs (Supplemental Figure S1), we co-opted the well-known tetrazine ligation that was recently employed to detect isonitrile-containing natural products. , …”

Section: Introductionmentioning

confidence: 99%

Sterol Sponge Mechanism Is Conserved for Glycosylated Polyene Macrolides

Guo

Zhang

et al. 2021

ACS Cent. Sci.

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Amphotericin-like glycosylated polyene macrolides (GPMs) are a clinically and industrially important family of natural products, but the mechanisms by which they exert their extraordinary biological activities have remained unclear for more than half a century. Amphotericin B exerts fungicidal action primarily via self-assembly into an extramembranous sponge that rapidly extracts ergosterol from fungal membranes, but it has remained unclear whether this mechanism is applicable to other GPMs. Using a highly conserved polyene–hemiketal region of GPMs that we hypothesized to represent a conserved ergosterol-binding domain, we bioinformatically mapped the entirety of the GPM sequence-function space and expanded the number of GPM biosynthetic gene clusters (BGCs) by 10-fold. We further leveraged bioinformatic predictions and tetrazine-based reactivity screening targeting the electron-rich polyene region of GPMs to discover a first-in-class methyltetraene- and diepoxide-containing GPM, kineosporicin, and to assign BGCs to many new producers of previously reported members. Leveraging a range of structurally diverse known and newly discovered GPMs, we found that the sterol sponge mechanism of fungicidal action is conserved.

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Cellulonodin-2 and Lihuanodin: Lasso Peptides with an Aspartimide Post-translational Modification

Cao

Beiser

Koos

et al. 2021

Preprint

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Lasso peptides are a family of ribosomally synthesized and post-translationally modified peptides (RiPPs) defined by their threaded structure. Besides the class-defining isopeptide bond, other post-translational modifications (PTMs) that further tailor lasso peptides have been previously reported. Using genome mining tools, we identified a subset of lasso peptide biosynthetic gene clusters (BGCs) that are colocalized with protein L-isoaspartyl methyltransferase (PIMT) homologs. PIMTs have an important role in protein repair, restoring isoaspartate residues formed from asparagine deamidation to aspartate. Here we report a new function for PIMT enzymes in the post-translational modification of lasso peptides. The PIMTs associated with lasso peptide BGCs first methylate an L-aspartate sidechain found within the ring of the lasso peptide. The methyl ester is then converted into a stable aspartimide moiety, endowing the lasso peptide ring with rigidity relative to its unmodified counterpart. We describe the heterologous expression and structural characterization of two examples of aspartimide-modified lasso peptides from thermophilic Gram-positive bacteria. The lasso peptide cellulonodin-2 is encoded in the genome of actinobacterium Thermobifida cellulosilytica, while lihuanodin is encoded in the genome of firmicute Lihuaxuella thermophila. Additional genome mining revealed PIMT-containing lasso peptide BGCs in 48 organisms. In addition to heterologous expression, we have reconstituted PIMT-mediated aspartimide formation in vitro, showing that lasso peptide-associated PIMTs transfer methyl groups very rapidly as compared to canonical PIMTs. Furthermore, in stark contrast to other characterized lasso peptide PTMs, the methyltransferase functions only on lassoed substrates.

show abstract

Reactivity-based screening for citrulline-containing natural products reveals a family of bacterial peptidyl arginine deiminases

Cited by 3 publications

References 51 publications

Cellulonodin-2 and Lihuanodin: Lasso Peptides with an Aspartimide Post-Translational Modification

Cellulonodin-2 and Lihuanodin: Lasso Peptides with an Aspartimide Post-Translational Modification

Sterol Sponge Mechanism Is Conserved for Glycosylated Polyene Macrolides

Cellulonodin-2 and Lihuanodin: Lasso Peptides with an Aspartimide Post-translational Modification

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