Lactams are an important
class of commodity chemicals used in the
manufacture of nylons, with millions of tons produced every year.
Biological production of lactams could be greatly improved by high-throughput
sensors for lactam biosynthesis. To identify biosensors of lactams,
we applied a chemoinformatic approach inspired by small molecule drug
discovery. We define this approach as analogue generation toward catabolizable
chemicals or AGTC. We discovered a lactam biosensor based on the ChnR/Pb
transcription factor-promoter pair. The microbial biosensor is capable
of sensing ε-caprolactam, δ-valerolactam, and butyrolactam
in a dose-dependent manner. The biosensor has sufficient specificity
to discriminate against lactam biosynthetic intermediates and therefore
could potentially be applied for high-throughput metabolic engineering
for industrially important high titer lactam biosynthesis.
Tightly regulated promoters are essential for numerous biological applications, where strong inducibility, portability, and scalability are desirable. Current systems are often incompatible with large-scale fermentations due to high inducer costs and strict media requirements. Here, we describe the bottom-up engineering of ‘Jungle Express’, an expression system that enables efficient gene regulation in diverse proteobacteria. This system is guided by EilR, a multidrug-binding repressor with high affinity to its optimized operator and cationic dyes that act as powerful inducers at negligible costs. In E. coli, the engineered promoters exhibit minimal basal transcription and are inducible over four orders of magnitude by 1 µM crystal violet, reaching expression levels exceeding those of the strongest current bacterial systems. Further, we provide molecular insights into specific interactions of EilR with its operator and with two inducers. The versatility of Jungle Express opens the way for tightly controlled and efficient gene expression that is not restricted to host organism, substrate, or scale.
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