Cloning, expression, and nucleotide sequence of genes involved in production of pediocin PA-1, and bacteriocin from Pediococcus acidilactici PAC1.0.

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Appl Environ Microbiol. 1992 August; 58(8): 2360-2367

Cloning, expression, and nucleotide sequence of genes involved in production of pediocin PA-1, and bacteriocin from Pediococcus acidilactici PAC1.0.

J D Marugg, C F Gonzalez, B S Kunka, A M Ledeboer, M J Pucci, M Y Toonen, S A Walker, L C Zoetmulder and P A Vandenbergh

Unilever Research Laboratorium Vlaardingen, The Netherlands.

ABSTRACT

The production of pediocin PA-1, a small heat-stable bacteriocin,is associated with the presence of the 9.4-kbp plasmid pSRQ11in Pediococcus acidilactici PAC1.0. It was shown by subcloningof pSRQ11 in Escherichia coli cloning vectors that pediocinPA-1 is produced and, most probably, secreted by E. coli cells.Deletion analysis showed that a 5.6-kbp SalI-EcoRI fragmentderived from pSRQ11 is required for pediocin PA-1 production.Nucleotide sequence analysis of this 5.6-kbp fragment indicatedthe presence of four clustered open reading frames (pedA, pedB,pedC, and pedD). The pedA gene encodes a 62-amino-acid precursorof pediocin PA-1, as the predicted amino acid residues 19 to62 correspond entirely to the amino acid sequence of the purifiedpediocin PA-1. Introduction of a mutation in pedA resulted ina complete loss of pediocin production. The pedB and pedC genes,encoding proteins of 112 and 174 amino acid residues, respectively,are located directly downstream of the pediocin structural gene.Functions could not be assigned to their gene products; mutationanalysis showed that the PedB protein is not involved in pediocinPA-1 production. The mutation analysis further revealed thatthe fourth gene, pedD, specifying a relatively large proteinof 724 amino acids, is required for pediocin PA-1 productionin E. coli. The predicted pedD protein shows strong similaritiesto several ATP-dependent transport proteins, including the E.coli hemolysin secretion protein HlyB and the ComA protein,which is required for competence induction for genetic transformationin Streptococcus pneumoniae.(ABSTRACT TRUNCATED AT 250 WORDS)

Appl Environ Microbiol. 1992 August; 58(8): 2360-2367

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