Home > Research > Publications & Outputs > Studies on MWFs in America and Europe

Research

Links

Keywords

View graph of relations

Studies on MWFs in America and Europe: The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids

Research output: Contribution to conference - Without ISBN/ISSN Conference paperpeer-review

Published

Standard

Studies on MWFs in America and Europe: The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids. / Rhodes, Glen; Fluri, Alexandra; Rfenacht, Andrea et al.
2008. Paper presented at 2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008, Cleveland, OH, United States.

Research output: Contribution to conference - Without ISBN/ISSN Conference paperpeer-review

Harvard

Rhodes, G, Fluri, A, Rfenacht, A & Pickup, R 2008, 'Studies on MWFs in America and Europe: The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids', Paper presented at 2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008, Cleveland, OH, United States, 18/05/08 - 22/05/08. <https://www.proceedings.com/17364.html>

APA

Rhodes, G., Fluri, A., Rfenacht, A., & Pickup, R. (2008). Studies on MWFs in America and Europe: The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids. Paper presented at 2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008, Cleveland, OH, United States. https://www.proceedings.com/17364.html

Vancouver

Rhodes G, Fluri A, Rfenacht A, Pickup R. Studies on MWFs in America and Europe: The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids. 2008. Paper presented at 2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008, Cleveland, OH, United States.

Author

Rhodes, Glen ; Fluri, Alexandra ; Rfenacht, Andrea et al. / Studies on MWFs in America and Europe : The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids. Paper presented at 2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008, Cleveland, OH, United States.

Bibtex

@conference{93461d483f864a78b6099d0151f21e2c,
title = "Studies on MWFs in America and Europe: The development of a quantitative real-time PCR assay for Mycobacterium immunogenum in metal working fluids",
abstract = "In recent years nontuberculous mycobacteria (NTM) have reportedly been on the increase caused by opportunistic infections. The bacteria within the M. chelonae complex (MCC; M. chelonae, M. abscessus and M. immunogenum) have been under investigation as to their role with respect to hypersensitivity pneumonitis in automobile workers and other occupational workers. Detection of these bacteria in metal working fluids (MWFs) has traditionally been by culture complemented by PCR and restriction digests of products to discriminate at the species level. Real-time PCR assays have to date only been able to distinguish to the genus level using a SYBR Green labelling assay. Here we describe a novel quantitative real-time 5-Nuclease (Taqman) PCR technique was developed to specifically detect M. immunogenum. The specific primers and Taqman probe were designed to amplify a 60 bp region of the rpoB gene. Specificity for M. immunogenum was confirmed when tested against close mycobacterial relatives and Rhodocccous equi strains. The sensitivity of detection of M. immunogenum genomic DNA was shown to be approximately 9 fg (2 cell equivalents). The assay was successfully applied to the detection of M. immunogenum in industrial metal working fluids from the U.K. and the U.S.A demonstrating its applicability to industry. In particular, this method permits the detection of M. immunogenum and to clarify the possible link to hypersensitive pneumonitis, which is under investigation since more than 15 years.",
keywords = "Biocides, Metalworking, Metalworking fluids",
author = "Glen Rhodes and Alexandra Fluri and Andrea Rfenacht and Roger Pickup",
year = "2008",
month = may,
day = "22",
language = "English",
note = "2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008 ; Conference date: 18-05-2008 Through 22-05-2008",

}

RIS

TY - CONF

T1 - Studies on MWFs in America and Europe

T2 - 2008 Annual Meeting of the Society of Tribologists and Lubrication Engineers, STLE 2008

AU - Rhodes, Glen

AU - Fluri, Alexandra

AU - Rfenacht, Andrea

AU - Pickup, Roger

PY - 2008/5/22

Y1 - 2008/5/22

N2 - In recent years nontuberculous mycobacteria (NTM) have reportedly been on the increase caused by opportunistic infections. The bacteria within the M. chelonae complex (MCC; M. chelonae, M. abscessus and M. immunogenum) have been under investigation as to their role with respect to hypersensitivity pneumonitis in automobile workers and other occupational workers. Detection of these bacteria in metal working fluids (MWFs) has traditionally been by culture complemented by PCR and restriction digests of products to discriminate at the species level. Real-time PCR assays have to date only been able to distinguish to the genus level using a SYBR Green labelling assay. Here we describe a novel quantitative real-time 5-Nuclease (Taqman) PCR technique was developed to specifically detect M. immunogenum. The specific primers and Taqman probe were designed to amplify a 60 bp region of the rpoB gene. Specificity for M. immunogenum was confirmed when tested against close mycobacterial relatives and Rhodocccous equi strains. The sensitivity of detection of M. immunogenum genomic DNA was shown to be approximately 9 fg (2 cell equivalents). The assay was successfully applied to the detection of M. immunogenum in industrial metal working fluids from the U.K. and the U.S.A demonstrating its applicability to industry. In particular, this method permits the detection of M. immunogenum and to clarify the possible link to hypersensitive pneumonitis, which is under investigation since more than 15 years.

AB - In recent years nontuberculous mycobacteria (NTM) have reportedly been on the increase caused by opportunistic infections. The bacteria within the M. chelonae complex (MCC; M. chelonae, M. abscessus and M. immunogenum) have been under investigation as to their role with respect to hypersensitivity pneumonitis in automobile workers and other occupational workers. Detection of these bacteria in metal working fluids (MWFs) has traditionally been by culture complemented by PCR and restriction digests of products to discriminate at the species level. Real-time PCR assays have to date only been able to distinguish to the genus level using a SYBR Green labelling assay. Here we describe a novel quantitative real-time 5-Nuclease (Taqman) PCR technique was developed to specifically detect M. immunogenum. The specific primers and Taqman probe were designed to amplify a 60 bp region of the rpoB gene. Specificity for M. immunogenum was confirmed when tested against close mycobacterial relatives and Rhodocccous equi strains. The sensitivity of detection of M. immunogenum genomic DNA was shown to be approximately 9 fg (2 cell equivalents). The assay was successfully applied to the detection of M. immunogenum in industrial metal working fluids from the U.K. and the U.S.A demonstrating its applicability to industry. In particular, this method permits the detection of M. immunogenum and to clarify the possible link to hypersensitive pneumonitis, which is under investigation since more than 15 years.

KW - Biocides

KW - Metalworking

KW - Metalworking fluids

M3 - Conference paper

AN - SCOPUS:77954939514

Y2 - 18 May 2008 through 22 May 2008

ER -