Literature DB >> 9276419

PCR-enzyme-linked immunosorbent assay and partial rRNA gene sequencing: a rational approach to identifying mycobacteria.

S Patel1, M Yates, N A Saunders.   

Abstract

A PCR-enzyme-linked immunosorbent assay (ELISA) for amplification and rapid identification of mycobacterial DNA coding for 16S rRNA was developed. The PCR selectively targeted and amplified part of the 16S rRNA gene from all mycobacteria while simultaneously labelling one strand of the amplified product with a 5' fluorescein-labelled primer. The identity of the labelled strand was subsequently determined by hybridization to a panel of mycobacterial species-specific capture probes, which were immobilized via their 5' biotin ends to a streptavidin-coated microtiter plate. Specific hybridization of a 5' fluorescein-labelled strand to a species probe was detected colorimetrically with an anti-fluorescein enzyme conjugate. The assay was able to identify 10 Mycobacterium spp. A probe able to hybridize to all Mycobacterium species (All1) was also included. By a heminested PCR, the assay was sensitive enough to detect as little as 10 fg of DNA, which is equivalent to approximately three bacilli. The assay was able to detect and identify mycobacteria directly from sputa. The specificities of the capture probes were assessed by analysis of 60 mycobacterial strains corresponding to 18 species. Probes Avi1, Int1, Kan1, Xen1, Che1, For1, Mal1, Ter1, and Gor1 were specific. The probe Tbc1 cross-hybridized with the Mycobacterium terrae amplicon. Analysis of 35 strains tested blind resulted in 34 strains being correctly identified. This method could be used for rapid identification of early cultures and may be suitable for the detection and concurrent identification of mycobacteria within clinical specimens.

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Year:  1997        PMID: 9276419      PMCID: PMC229971          DOI: 10.1128/jcm.35.9.2375-2380.1997

Source DB:  PubMed          Journal:  J Clin Microbiol        ISSN: 0095-1137            Impact factor:   5.948


  34 in total

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Authors:  J O Falkinham
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Authors:  B Springer; L Stockman; K Teschner; G D Roberts; E C Böttger
Journal:  J Clin Microbiol       Date:  1996-02       Impact factor: 5.948

5.  Heminested inverse PCR for IS6110 fingerprinting of Mycobacterium tuberculosis strains.

Authors:  S Patel; S Wall; N A Saunders
Journal:  J Clin Microbiol       Date:  1996-07       Impact factor: 5.948

6.  Detection and identification of mycobacteria by amplification of rRNA.

Authors:  B Böddinghaus; T Rogall; T Flohr; H Blöcker; E C Böttger
Journal:  J Clin Microbiol       Date:  1990-08       Impact factor: 5.948

7.  Detection and identification of mycobacteria by amplification of mycobacterial DNA.

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8.  Phylogenetic analysis and identification of different serovars of Mycobacterium intracellulare at the molecular level.

Authors:  B Böddinghaus; J Wolters; W Heikens; E C Böttger
Journal:  FEMS Microbiol Lett       Date:  1990-07       Impact factor: 2.742

9.  PCR assay based on DNA coding for 16S rRNA for detection and identification of mycobacteria in clinical samples.

Authors:  L F Kox; J van Leeuwen; S Knijper; H M Jansen; A H Kolk
Journal:  J Clin Microbiol       Date:  1995-12       Impact factor: 5.948

Review 10.  Mycobacteria other than Mycobacterium tuberculosis: review of microbiologic and clinical aspects.

Authors:  G L Woods; J A Washington
Journal:  Rev Infect Dis       Date:  1987 Mar-Apr
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6.  Assessment of partial sequencing of the 65-kilodalton heat shock protein gene (hsp65) for routine identification of Mycobacterium species isolated from clinical sources.

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7.  PCR-enzyme-linked immunosorbent assay for detection and identification of Campylobacter species: application to isolates and stool samples.

Authors:  L A Metherell; J M Logan; J Stanley
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8.  In situ study of abundant expression of proinflammatory chemokines and cytokines in pulmonary granulomas that develop in cynomolgus macaques experimentally infected with Mycobacterium tuberculosis.

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10.  The conservation and application of three hypothetical protein coding gene for direct detection of Mycobacterium tuberculosis in sputum specimens.

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