Lysate-based
cell-free expression (CFE) systems are accessible
platforms for expressing proteins that are difficult to synthesize in vivo, such as nonribosomal peptide synthetases (NRPSs).
NRPSs are large (>100 kDa), modular enzyme complexes that synthesize
bioactive peptide natural products. This synthetic process is analogous
to transcription/translation (TX/TL) in lysates, resulting in potential
resource competition between NRPS expression and NRPS activity in
cell-free environments. Moreover, CFE conditions depend on the size
and structure of the protein. Here, a reporter system for rapidly
investigating and optimizing reaction environments for NRPS CFE is
described. This strategy is demonstrated in E. coli lysate reactions using blue pigment synthetase A (BpsA), a model
NRPS, carrying a C-terminal tetracysteine (TC) tag which forms a fluorescent
complex with the biarsenical dye, FlAsH. A colorimetric assay was
adapted for lysate reactions to detect the blue pigment product, indigoidine,
of cell-free expressed BpsA-TC, confirming that the tagged enzyme
is catalytically active. An optimized protocol for end point TC/FlAsH
complex measurements in reactions enables quick comparisons of full-length
BpsA-TC expressed under different reaction conditions, defining unique
requirements for NRPS expression that are related to the protein’s
catalytic activity and size. Importantly, these protein-dependent
CFE conditions enable higher indigoidine titer and improve the expression
of other monomodular NRPSs. Notably, these conditions differ from
those used for the expression of superfolder GFP (sfGFP), a common
reporter for optimizing lysate-based CFE systems, indicating the necessity
for tailored reporters to optimize expression for specific enzyme
classes. The reporter system is anticipated to advance lysate-based
CFE systems for complex enzyme synthesis, enabling natural product
discovery.
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