Gene amplification, laboratory evolution, and biosensor screening reveal MucK as a terephthalic acid transporter in Acinetobacter baylyi ADP1

Isabel Pardo; Ramesh K Jha; Ryan E Bermel; Felicia Bratti; Molly Gaddis; Emily McIntyre; William Michener; Ellen L Neidle; Taraka Dale; Gregg T Beckham; Christopher W Johnson

doi:10.1016/j.ymben.2020.09.009

Gene amplification, laboratory evolution, and biosensor screening reveal MucK as a terephthalic acid transporter in Acinetobacter baylyi ADP1

Metab Eng. 2020 Nov:62:260-274. doi: 10.1016/j.ymben.2020.09.009. Epub 2020 Oct 1.

Authors

Affiliations

¹ Renewable Resources and Enabling Sciences Center, National Renewable Energy Laboratory, Golden CO, USA; Agile BioFoundry, Emeryville CA, USA.
² Agile BioFoundry, Emeryville CA, USA; Bioscience Division, Los Alamos National Laboratory, Los Alamos NM, USA.
³ Department of Microbiology, University of Georgia, Athens GA, USA.
⁴ Renewable Resources and Enabling Sciences Center, National Renewable Energy Laboratory, Golden CO, USA; Agile BioFoundry, Emeryville CA, USA. Electronic address: gregg.beckham@nrel.gov.
⁵ Renewable Resources and Enabling Sciences Center, National Renewable Energy Laboratory, Golden CO, USA; Agile BioFoundry, Emeryville CA, USA. Electronic address: christopher.johnson@nrel.gov.

PMID: 32979486
DOI: 10.1016/j.ymben.2020.09.009

Abstract

Microbial terephthalic acid (TPA) catabolic pathways are conserved among the few bacteria known to turnover this xenobiotic aromatic compound. However, to date there are few reported cases in which this pathway has been successfully expressed in heterologous hosts to impart efficient utilization of TPA as a sole carbon source. In this work, we aimed to engineer TPA conversion in Acinetobacter baylyi ADP1 via the heterologous expression of catabolic and transporter genes from a native TPA-utilizing bacterium. Specifically, we obtained ADP1-derived strains capable of growing on TPA as the sole carbon source using chromosomal insertion and targeted amplification of the tph catabolic operon from Comamonas sp. E6. Adaptive laboratory evolution was then used to improve growth on this substrate. TPA consumption rates of the evolved strains, which retained multiple copies of the tph genes, were ~0.2 g/L/h (or ~1 g TPA/g cells/h), similar to that of Comamonas sp. E6 and almost 2-fold higher than that of Rhodococcus jostii RHA1, another native TPA-utilizing strain. To evaluate TPA transport in the evolved ADP1 strains, we engineered a TPA biosensor consisting of the transcription factor TphR and a fluorescent reporter. In combination with whole-genome sequencing, the TPA biosensor revealed that transport of TPA was not mediated by the heterologous proteins from Comamonas sp. E6. Instead, the endogenous ADP1 muconate transporter MucK, a member of the major facilitator superfamily, was responsible for TPA transport in several evolved strains in which MucK variants were found to enhance TPA uptake. Furthermore, the IclR-type transcriptional regulator DcaS was identified as a repressor of mucK expression. Overall, this work presents an unexpected function of a native protein identified through gene amplification, adaptive laboratory evolution, and a combination of screening methods. This study also provides a TPA biosensor for application in ADP1 and identifies transporter variants for use in metabolic engineering applications focused on plastic upcycling of polyesters.

Keywords: Acinetobacter baylyi ADP1; Adaptive laboratory evolution; Major facilitator superfamily transporter; Plastics bioconversion; Plastics upcycling; TPA biosensor; mucK.

Publication types

Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

Acinetobacter
Biosensing Techniques*
Gene Amplification*
Laboratories
Phthalic Acids
Rhodococcus

Substances

Phthalic Acids
terephthalic acid

Supplementary concepts

Acinetobacter baylyi
Rhodococcus jostii