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Polymerase chain reaction for verification of fluorescent colonies of Erwinia chrysanthemi and Pseudomonas putida WCS358 in immunofluorescence colony staining
Author(s) -
Wolf J.M.,
Beckhoven J.R.C.M.,
Vries Ph.M.,
Raaijmakers J.M.,
Bakker P.A.H.M.,
Bertheau Y.,
Vuurde J.W.L.
Publication year - 1995
Publication title -
journal of applied bacteriology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.889
H-Index - 156
eISSN - 1365-2672
pISSN - 0021-8847
DOI - 10.1111/j.1365-2672.1995.tb03178.x
Subject(s) - pseudomonas putida , immunofluorescence , fluorescent staining , erwinia , staining , polymerase chain reaction , microbiology and biotechnology , pseudomonas , biology , fluorescence , indirect immunofluorescence , bacteria , antibody , biochemistry , gene , genetics , physics , quantum mechanics
The potential of polymerase chain reaction (PCR) for verifying the identity of colonies stained by the immunofluorescence colony‐staining (IFC) procedure was investigated. Using primers directed against conserved sequences of the pectate lyase‐genes coding for isozymes PLa, PLd and PLe of Erwinia chrysanthemi , the authors confirmed the identity of 96% of 20 fluorescent target colonies, punched from IFC‐stained samples with pure cultures. In pour plates with mixtures of Erw. chrysanthemi and non‐target colonies from potato peel extracts, the identity of 90% of 113 target colonies was confirmed. Using primers directed against sequences of the ferric‐pseudobactin receptor gene pupA of Pseudomonas putida WCS358, the identity of 96% of 22 target colonies was confirmed in IFC‐stained samples with pure cultures. In pour plates with mixtures of Ps. putida WCS358 and non‐target bacteria from compost extracts, the identity of 59% of 108 fluorescent colonies was confirmed by PCR. It was shown that components from non‐target bacteria lowered the threshold level of PCR for Ps. putida WCS358