A metagenomic library cloning strategy that promotes high-level expression of captured genes to enable efficient functional screening

Author:

Rich Michelle HORCID,Sharrock Abigail VORCID,Mulligan Timothy S,Matthews Frazer,Brown Alistair SORCID,Lee-Harwood Hannah R,Williams Elsie M,Copp Janine NORCID,Little Rory FORCID,Francis Jenni JB,Horvat Claire N,Stevenson Luke JORCID,Owen Jeremy GORCID,Saxena Meera T,Mumm Jeff SORCID,Ackerley David FORCID

Abstract

SummaryFunctional screening of environmental DNA (eDNA) libraries is a potentially powerful approach to discover enzymatic “unknown unknowns”, but is usually heavily biased toward the tiny subset of genes preferentially transcribed and translated by the screening strain. We have overcome this by preparing an eDNA library via partial digest with restriction enzyme Fatl (cuts CATG), causing a substantial proportion of ATG start codons to be precisely aligned with strong plasmid-encoded promoter and ribosome-binding sequences. Whereas we were unable to select nitroreductases from standard metagenome libraries, our Fatl strategy yielded 21 nitroreductases spanning eight different enzyme families, each conferring resistance to the nitro-antibiotic niclosamide and sensitivity to the nitro-prodrug metronidazole. We showed expression could be improved by co-expressing rare tRNAs and encoded proteins purified directly using an embedded Hisg-tag. In a transgenic zebrafish model of metronidazole-mediated targeted cell ablation, our lead MhqN-family nitroreductase proved ∼5- fold more effective than the canonical nitroreductase NfsB.

Publisher

Cold Spring Harbor Laboratory

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