Abstract

Using consensus regions in gene sequences encoding the two forms of nitrite reductase (Nir), a key enzyme in the denitrification pathway, we designed two sets of PCR primers to amplify cd(1)- and Cu-nir. The primers were evaluated by screening defined denitrifying strains, denitrifying isolates front wastewater treatment plants, and extracts from activated sludge. Sequence relationships of nir genes were also established. The ed, printers were designed to amplify a 778 to 799-bp region of cd(1)-nir in the six published sequences. Likewise, the Cu primers amplified a 473-bp region in seven of the eight published Cu-nir sequences. Together, the two sets of PCR primers amplified nir genes in nine species within four genera, as well as in four of the seven sludge isolates. The primers did not amplify genes of nondenitrifying strains. The Cu primers amplified the expected fragment in all 13 sludge samples, but cd(1)-nir fragments were only obtained in five samples. PCR products of the expected sizes were verified as nir genes after hybridization to DNA probes, except in one case. The sequenced nir fragments were related to other nir sequences, demonstrating: that the primers amplified the correct gene. The selected primer sites for Cu-nir were conserved, while broad-range primers targeting conserved regions of cd(1)-nir seem to be difficult to find. We also report on the existence of Cu-nir in Paracoccus denitrificans Pd1222.

Published in

Applied and Environmental Microbiology
1999, Volume: 65, number: 4, pages: 1652-1657
Publisher: AMER SOC MICROBIOLOGY

SLU Authors

• Hallin, Sara

  • Department of Molecular Sciences, Swedish University of Agricultural Sciences
    

UKÄ Subject classification

Microbiology


Permanent link to this page (URI)

https://res.slu.se/id/publ/78304