Cell-Free Biosynthesis to Evaluate Lasso Peptide Formation and Enzyme-Substrate Tolerance

Si, Yuan; Kretsch, Ashley M; Daigh, Laura M.; Burk, Mark J.; Mitchell, Douglas A.

doi:10.1101/2020.11.25.399105

Cited by 11 publications

(19 citation statements)

References 65 publications

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“…We chose the lasso peptide biosynthetic system from T. fusca , as the structure of the B1 protein (TfuB1) was successfully determined 5 and in vitro synthesis of the lasso peptide (fusilassin/fuscanodin) in the PURE system was reported. 21 Synthetic genes of TfuB1, TfuB2, and the precursor peptide fused with sfGFP (TfuA_sfGFP) were amplified by PCR using primers containing a T7 promoter and an appropriately positioned ribosome binding site (Supplementary Tables 1–3). Proteins encoded by resulting DNA molecules were co-expressed in the PURE system at 37 ºC for 1 hour and then incubated at 50 ºC, the temperature for the TfuB2 activity test.…”

Section: Resultsmentioning

confidence: 99%

Cell-free mutant analysis combined with structure prediction of a lasso peptide biosynthetic protein B2

Alfi

Popov

Kumar

et al. 2022

Preprint

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Biochemical and structural analyses of purified proteins are essential for the understanding of their properties. However, many proteins are unstable and difficult to purify, hindering their characterization. The B2 proteins of the lasso peptide biosynthetic pathways are cysteine proteases that cleave precursor peptides during the maturation process. The B2 proteins are poorly soluble and no experimentally-solved structures are available. Here, we performed a rabid semi-comprehensive mutational analysis of the B2 protein from the thermophilic actinobacterium, Thermobifida fusca (TfuB2) using a cell-free transcription/translation system, and compared the results with the structure prediction by AlphaFold2. Analysis of 34 TfuB2 mutants with substitutions of hydrophobic residues confirmed the accuracy of the predicted structure, and revealed a hydrophobic patch on the protein surface, which likely serves as the binding site of the partner protein, TfuB1. Our results suggest that the combination of rapid cell-free mutant analyses with precise structure predictions can greatly accelerate structure-function research of proteins for which no structures are available.

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Section: Resultsmentioning

confidence: 99%

Cell-free mutant analysis combined with structure prediction of a lasso peptide biosynthetic protein B2

Alfi

Popov

Kumar

et al. 2022

Preprint

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“…The role of hydrophobic enzymesubstrate interactions in RiPP biosynthesis is well-documented, but most studies on the topic to date have focused on the LP-enzyme interactions (vide infra). The preference for hydrophobic amino acids in substrate CPs for promiscuous biosynthetic enzymes has also been noted, 44,45,[47][48][49] but to our knowledge, never clearly articulated. Thorough biophysical studies on LazF and other RiPP enzymes will be needed to further evaluate this idea.…”

Section: Substrate Specificity Of Edsmentioning

confidence: 94%

Site-specific nonenzymatic peptide S/O–glutamylation reveals the extent of substrate promiscuity in glutamate elimination domains

Vinogradov

Suga

2021

Preprint

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Formation of dehydroalanine and dehydrobutyrine residues via tRNA-dependent dehydration of serine and threonine is a key post-translational modification in the biosynthesis of lanthipeptides and thiopeptides. The dehydration process involves two reactions, wherein the O–glutamyl Ser/Thr intermediate, accessed by a dedicated enzyme utilizing Glu-tRNAGlu as the acyl donor, is recognized by the second enzyme, referred to as the glutamate elimination domain (ED), which catalyses the eponymous reaction yielding a dehydroamino acid. Here, we report two complementary strategies based on a thiol-thioester exchange reaction for direct, nonenzymatic access to diverse ED substrates. These chemistries enabled us to dissect the substrate recognition requirements of three known EDs. Our results establish that EDs are uniquely promiscuous enzymes capable of acting on substrates with arbitrary amino acid sequences, and performing retro-Michael reaction beyond the canonical glutamate elimination. To aid in the substrate recruitment process, EDs apparently engage in nonspecific hydrophobic interactions with their substrates.

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“…We will not discuss these types of cyclization, as their biocatalytic applications have been developed to a less extent, in comparison with lanthipeptides and microviridins. On the other hand, lasso peptides consist of a macrolactam formed between the N -terminus of the peptide and a carboxylate sidechain in an ATP-dependent manner, and the production of these peptides with synthetic and biocatalytic methods has been reported previously ( Cheng and Hua, 2020 ; Hegemann et al., 2015 ; Maksimov et al., 2012 ; Si et al., 2020 ).…”

Section: Biocatalytic Approaches For the Synthesis Of Rippsmentioning

confidence: 99%

Biocatalytic synthesis of peptidic natural products and related analogues

et al. 2021

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Peptidic natural products (PNPs) represent a rich source of lead compounds for the discovery and development of therapeutic agents for the treatment of a variety of diseases. However, the chemical synthesis of PNPs with diverse modifications for drug research is often faced with significant challenges, including the unavailability of constituent nonproteinogenic amino acids, inefficient cyclization protocols, and poor compatibility with other functional groups. Advances in the understanding of PNP biosynthesis and biocatalysis provide a promising, sustainable alternative for the synthesis of these compounds and their analogues. Here we discuss current progress in using native and engineered biosynthetic enzymes for the production of both ribosomally and nonribosomally synthesized peptides. In addition, we highlight new in vitro and in vivo approaches for the generation and screening of PNP libraries.

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Cell-Free Biosynthesis to Evaluate Lasso Peptide Formation and Enzyme-Substrate Tolerance

Cited by 11 publications

References 65 publications

Cell-free mutant analysis combined with structure prediction of a lasso peptide biosynthetic protein B2

Cell-free mutant analysis combined with structure prediction of a lasso peptide biosynthetic protein B2

Site-specific nonenzymatic peptide S/O–glutamylation reveals the extent of substrate promiscuity in glutamate elimination domains

Biocatalytic synthesis of peptidic natural products and related analogues

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