Transport systems, intracellular traffic of intermediates and secretion of β-lactam antibiotics in fungi.

Fungal Biol Biotechnol

Área de Microbiología, Departamento de Biología Molecular, Universidad de León, León, Spain.

Published: April 2020

AI Article Synopsis

  • Fungal secondary metabolites, like β-lactam antibiotics penicillin and cephalosporin C, are produced through complex enzyme systems that require movement of materials across different cell compartments for efficiency.
  • Key enzymes in the penicillin pathway are localized in specific cell areas: early enzymes are in the cytoplasm, while later ones are found in peroxisomes, with specific transporters facilitating the import of necessary intermediates.
  • While transport and localization mechanisms for penicillin production are well-studied, the secretion process from peroxisomes to outside the cell is still not fully understood, with ongoing research aimed at identifying the responsible proteins.

Article Abstract

Fungal secondary metabolites are synthesized by complex biosynthetic pathways catalized by enzymes located in different subcellular compartments, thus requiring traffic of precursors and intermediates between them. The β-lactam antibiotics penicillin and cephalosporin C serve as an excellent model to understand the molecular mechanisms that control the subcellular localization of secondary metabolites biosynthetic enzymes. Optimal functioning of the β-lactam biosynthetic enzymes relies on a sophisticated temporal and spatial organization of the enzymes, the intermediates and the final products. The first and second enzymes of the penicillin pathway, ACV synthetase and IPN synthase, in and are cytosolic. In contrast, the last two enzymes of the penicillin pathway, phenylacetyl-CoA ligase and isopenicillin N acyltransferase, are located in peroxisomes working as a tandem at their optimal pH that coincides with the peroxisomes pH. Two MFS transporters, PenM and PaaT have been found to be involved in the import of the intermediates isopenicillin N and phenylacetic acid, respectively, into peroxisomes. Similar compartmentalization of intermediates occurs in two enzymes isopenicillin N-CoA ligase and isopenicillin N-CoA epimerase, that catalyse the conversion of isopenicillin N in penicillin N, are located in peroxisomes. Two genes encoding MFS transporters, and are located in the early cephalosporin gene cluster. These transporters have been localized in peroxisomes by confocal fluorescence microscopy. A third gene of , , encodes an MFS protein, located in the cell membrane involved in the secretion of cephalosporin C, although -disrupted mutants are still able to export cephalosporin by redundant transporters. The secretion of penicillin from peroxisomes to the extracellular medium is still unclear. Attempts have been made to identify a gene encoding the penicillin secretion protein among the 48 ABC-transporters of . The highly efficient secretion system that exports penicillin against a concentration gradient may involve active penicillin extrusion systems mediated by vesicles that fuse to the cell membrane. However, there is no correlation of pexophagy with penicillin or cephalosporin formation since inactivation of pexophagy leads to increased penicillin or cephalosporin biosynthesis due to preservation of peroxisomes. The penicillin biosynthesis finding shows that in order to increase biosynthesis of novel secondary metabolites it is essential to adequately target enzymes to organelles.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7183595PMC
http://dx.doi.org/10.1186/s40694-020-00096-yDOI Listing

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