Literature DB >> 2280781

Multiplex PCR amplification and immobilized capture probes for detection of bacterial pathogens and indicators in water.

A K Bej1, M H Mahbubani, R Miller, J L DiCesare, L Haff, R M Atlas.   

Abstract

Detection of pathogens (Legionella species) and indicator bacteria (coliform bacteria) was achieved by multiplex (simultaneous) PCR amplification of diagnostic gene sequences and by hybridization to immobilized poly-dT-tailed capture probes using a dot- or slot-blot approach. Complex manipulations of primer concentrations and staggered additions of primers were required in order to achieve equal amplification of multiple genes. Multiplex PCR amplification of two different Legionella genes, one specific for L. pneumophila (mip) and the other for the genus Legionella (5S rRNA), was achieved by staggered amplification. Multiplex PCR amplification using differing amounts of primers specific for lacZ and lamB genes permitted the detection of coliform bacteria and those associated with human faecal contamination, including the indicator bacterial species E. coli and enteric pathogens Salmonella and Shigella. Hybridization of biotin-labelled amplified DNA, in which the biotin was incorporated during PCR amplification from biotinylated-dUTP, to immobilized 400-dT-tailed capture probes permitted specific and sensitive detection of target gene sequences. The sensitivity of colorimetric detection achieved by PCR amplification of target DNA was at a level equivalent to 1-2 bacterial cells, which is the same level of sensitivity obtained with radioactive detection. The simultaneous amplification of several genes and hybridization to immobilized capture probes with colorimetric detection is an effective, efficient and rapid detection method for various human bacterial pathogens.

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Year:  1990        PMID: 2280781     DOI: 10.1016/0890-8508(90)90026-v

Source DB:  PubMed          Journal:  Mol Cell Probes        ISSN: 0890-8508            Impact factor:   2.365


  30 in total

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Review 2.  Molecular biology and infections of the gut.

Authors:  N P Mapstone; P Quirke
Journal:  Gut       Date:  1992-11       Impact factor: 23.059

3.  Rapid detection of avian influenza virus a and subtype H5N1 by single step multiplex reverse transcription-polymerase chain reaction.

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4.  Polymerase chain reaction-gene probe detection of microorganisms by using filter-concentrated samples.

Authors:  A K Bej; M H Mahbubani; J L Dicesare; R M Atlas
Journal:  Appl Environ Microbiol       Date:  1991-12       Impact factor: 4.792

5.  Electrochemical nanoparticle-enzyme sensors for screening bacterial contamination in drinking water.

Authors:  Juhong Chen; Ziwen Jiang; Jonathan D Ackerman; Mahdieh Yazdani; Singyuk Hou; Sam R Nugen; Vincent M Rotello
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6.  Use of heteroduplex analysis to classify legionellae on the basis of 5S rRNA gene sequences.

Authors:  A Pinar; S Ahkee; R D Miller; J A Ramirez; J T Summersgill
Journal:  J Clin Microbiol       Date:  1997-06       Impact factor: 5.948

7.  The elimination of primer-dimer accumulation in PCR.

Authors:  J Brownie; S Shawcross; J Theaker; D Whitcombe; R Ferrie; C Newton; S Little
Journal:  Nucleic Acids Res       Date:  1997-08-15       Impact factor: 16.971

8.  Enzyme-linked immunoassay for detection of PCR-amplified DNA of legionellae in bronchoalveolar fluid.

Authors:  D Jonas; A Rosenbaum; S Weyrich; S Bhakdi
Journal:  J Clin Microbiol       Date:  1995-05       Impact factor: 5.948

9.  Identification of Bordetella pertussis infection by shared-primer PCR.

Authors:  Z Li; D L Jansen; T M Finn; S A Halperin; A Kasina; S P O'Connor; T Aoyama; C R Manclark; M J Brennan
Journal:  J Clin Microbiol       Date:  1994-03       Impact factor: 5.948

10.  Detection of Giardia cysts by using the polymerase chain reaction and distinguishing live from dead cysts.

Authors:  M H Mahbubani; A K Bej; M Perlin; F W Schaefer; W Jakubowski; R M Atlas
Journal:  Appl Environ Microbiol       Date:  1991-12       Impact factor: 4.792

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