Abstract
The organic polymer lignin is a component of plant cell walls, which like (hemi)-cellulose is highly abundant in nature and relatively resistant to degradation. However, extracellular enzymes released by natural microbial consortia can cleave the β-aryl ether linkages in lignin, releasing monoaromatic phenylpropanoids that can be further catabolised by diverse species of bacteria. Biodegradation of lignin is therefore important in global carbon cycling, and its natural abundance also makes it an attractive biotechnological feedstock for the industrial production of commodity chemicals. Whilst the pathways for degradation of lignin-derived aromatics have been extensively characterised, much less is understood about how they are recognised and taken up from the environment. The purple phototrophic bacterium Rhodopseudomonas palustris can grow on a range of phenylpropanoid monomers and is a model organism for studying their uptake and breakdown. R. palustris encodes a tripartite ATP-independent periplasmic (TRAP) transporter (TarPQM) linked to genes encoding phenylpropanoid-degrading enzymes. The periplasmic solute-binding protein component of this transporter, TarP, has previously been shown to bind aromatic substrates. Here, we determine the high-resolution crystal structure of TarP from R. palustris as well as the structures of homologous proteins from the salt marsh bacterium Sagittula stellata and the halophile Chromohalobacter salexigens, which also grow on lignin-derived aromatics. In combination with tryptophan fluorescence ligand-binding assays, our ligand-bound co-crystal structures reveal the molecular basis for high-affinity recognition of phenylpropanoids by these TRAP transporters, which have potential for improving uptake of these compounds for biotechnological transformations of lignin.
Highlights
High-affinity solute uptake is an essential requirement for the survival of microorganisms in low nutrient environments
Enrichment of tripartite ATP-independent periplasmic (TRAP) transporters with potential specificity for HCMs in marine proteobacteria TRAP transporters are widespread across the bacterial domain, we have previously noted their enrichment in phylogenetically diverse marine bacteria, presumably to enable scavenging of a diverse range of organic acids present at low concentrations in the ocean/aquatic environments [33]
To assess the potential diversity of the transporters within these organisms, we extracted the sequences for all full-length TRAP solute-binding protein (SBP) from a subset of marine bacteria enriched for TRAP transporters [33], namely C. salexigens DSM 3043, Aurantimonas manganoxydans
Summary
High-affinity solute uptake is an essential requirement for the survival of microorganisms in low nutrient environments. The FEBS Journal published by John Wiley & Sons Ltd on behalf of The tripartite tricarboxylate transporters and the tripartite ATP-independent periplasmic (TRAP) transporters are SBP-dependent secondary transporters that use either the proton motive force or sodium (Na+) ions for solute uptake [3]. Since their discovery by Forward et al in 1997 [4], the advent of mass genome sequencing has revealed that TRAP transporters are widely encoded in bacteria and archaea [5]. They are key to the survival of human pathogens such as Vibrio cholerae [6] and Haemophillus influenzae [7] as well as being involved in plant virulence [8] and uptake of carbon sources in many environmental bacteria [9,10,11]
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