Strain-specific proteogenomics accelerates the discovery of natural products via their biosynthetic pathways

Author:

Albright Jessica C1,Goering Anthony W1,Doroghazi James R2,Metcalf William W2,Kelleher Neil L1

Affiliation:

1. grid.16753.36 0000000122993507 Departments of Chemistry, Molecular Biosciences, and the Feinberg School of Medicine Northwestern University 2170 Campus Drive 60208 Evanston IL USA

2. grid.35403.31 0000000419369991 Department of Microbiology and the Institute of Genomic Biology University of Illinois at Urbana-Champaign 61801 Urbana IL USA

Abstract

Abstract The use of proteomics for direct detection of expressed pathways producing natural products has yielded many new compounds, even when used in a screening mode without a bacterial genome sequence available. Here we quantify the advantages of having draft DNA-sequence available for strain-specific proteomics using the latest in ultrahigh-resolution mass spectrometry for both proteins and the small molecules they generate. Using the draft sequence of Streptomyces lilacinus NRRL B-1968, we show a >tenfold increase in the number of peptide identifications vs. using publicly available databases. Detected in this strain were six expressed gene clusters with varying homology to those known. To date, we have identified three of these clusters as encoding for the production of griseobactin (known), rakicidin D (an orphan NRPS/PKS hybrid cluster), and a putative thr and DHB-containing siderophore produced by a new non-ribosomal peptide sythetase gene cluster. The remaining three clusters show lower homology to those known, and likely encode enzymes for production of novel compounds. Using an interpreted strain-specific DNA sequence enables deep proteomics for the detection of multiple pathways and their encoded natural products in a single cultured bacterium.

Publisher

Oxford University Press (OUP)

Subject

Applied Microbiology and Biotechnology,Biotechnology,Bioengineering

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