Literature DB >> 19801486

Accurate quantification of microorganisms in PCR-inhibiting environmental DNA extracts by a novel internal amplification control approach using Biotrove OpenArrays.

R van Doorn1, M M Klerks, M P E van Gent-Pelzer, A G C L Speksnijder, G A Kowalchuk, C D Schoen.   

Abstract

PCR-based detection assays are prone to inhibition by substances present in environmental samples, thereby potentially leading to inaccurate target quantification or false-negative results. Internal amplification controls (IACs) have been developed to help alleviate this problem but are generally applied in a single concentration, thereby yielding less-than-optimal results across the wide range of microbial gene target concentrations possible in environmental samples (J. Hoorfar, B. Malorny, A. Abdulmawjood, N. Cook, M. Wagner, and P. Fach, J. Clin. Microbiol. 42:1863-1868, 2004). Increasing the number of IACs for each quantitative PCR (qPCR) sample individually, however, typically reduces sensitivity and, more importantly, the reliability of quantification. Fortunately, current advances in high-throughput qPCR platforms offer the possibility of multiple reactions for a single sample simultaneously, thereby allowing the implementation of more than one IAC concentration per sample. Here, we describe the development of a novel IAC approach that is specifically designed for the state-of-the-art Biotrove OpenArray platform. Different IAC targets were applied at a range of concentrations, yielding a calibration IAC curve for each individual DNA sample. The developed IACs were optimized, tested, and validated by using more than 5,000 unique qPCR amplifications, allowing accurate quantification of microorganisms when applied to soil DNA extracts containing various levels of PCR-inhibiting compounds. To our knowledge, this is the first study using a suite of IACs at different target concentrations to monitor PCR inhibition across a wide target range, thereby allowing reliable and accurate quantification of microorganisms in PCR-inhibiting DNA extracts. The developed IAC is ideally suited for high-throughput screenings of, for example, ecological and agricultural samples on next-generation qPCR platforms.

Entities:  

Mesh:

Substances:

Year:  2009        PMID: 19801486      PMCID: PMC2786501          DOI: 10.1128/AEM.00796-09

Source DB:  PubMed          Journal:  Appl Environ Microbiol        ISSN: 0099-2240            Impact factor:   4.792


  31 in total

1.  Purification and characterization of a common soil component which inhibits the polymerase chain reaction.

Authors:  R J Watson; B Blackwell
Journal:  Can J Microbiol       Date:  2000-07       Impact factor: 2.419

2.  Making internal amplification control mandatory for diagnostic PCR.

Authors:  Jeffrey Hoorfar; Nigel Cook; Burkhard Malorny; Martin Wagner; Dario De Medici; Amir Abdulmawjood; Patrick Fach
Journal:  J Clin Microbiol       Date:  2003-12       Impact factor: 5.948

Review 3.  Practical considerations in design of internal amplification controls for diagnostic PCR assays.

Authors:  J Hoorfar; B Malorny; A Abdulmawjood; N Cook; M Wagner; P Fach
Journal:  J Clin Microbiol       Date:  2004-05       Impact factor: 5.948

4.  Novel internal controls for real-time PCR assays.

Authors:  Frederick S Nolte
Journal:  Clin Chem       Date:  2004-05       Impact factor: 8.327

5.  Inhibitory effects of urine on the polymerase chain reaction for cytomegalovirus DNA.

Authors:  G Khan; H O Kangro; P J Coates; R B Heath
Journal:  J Clin Pathol       Date:  1991-05       Impact factor: 3.411

6.  Comparison of real-time PCR methods for detection of Salmonella enterica and Escherichia coli O157:H7, and introduction of a general internal amplification control.

Authors:  M M Klerks; C Zijlstra; A H C van Bruggen
Journal:  J Microbiol Methods       Date:  2004-12       Impact factor: 2.363

7.  Development of an internal control for the detection of the African swine fever virus by PCR.

Authors:  M Gonzague; C Plin; L Bakkali-Kassimi; A Boutrouille; C Cruciere
Journal:  Mol Cell Probes       Date:  2002-06       Impact factor: 2.365

8.  Robust detection and identification of multiple oomycetes and fungi in environmental samples by using a novel cleavable padlock probe-based ligation detection assay.

Authors:  R van Doorn; M Slawiak; M Szemes; A M Dullemans; P Bonants; G A Kowalchuk; C D Schoen
Journal:  Appl Environ Microbiol       Date:  2009-04-24       Impact factor: 4.792

9.  Primary structure of the Aequorea victoria green-fluorescent protein.

Authors:  D C Prasher; V K Eckenrode; W W Ward; F G Prendergast; M J Cormier
Journal:  Gene       Date:  1992-02-15       Impact factor: 3.688

10.  Application of a real-time polymerase chain reaction with internal positive control for detection and quantification of enterovirus in cerebrospinal fluid.

Authors:  S Monpoeho; M Coste-Burel; M Costa-Mattioli; B Besse; J J Chomel; S Billaudel; V Ferré
Journal:  Eur J Clin Microbiol Infect Dis       Date:  2002-07-13       Impact factor: 3.267
View more
  9 in total

1.  Simultaneous quantification of multiple food- and waterborne pathogens by use of microfluidic quantitative PCR.

Authors:  Satoshi Ishii; Takahiro Segawa; Satoshi Okabe
Journal:  Appl Environ Microbiol       Date:  2013-02-22       Impact factor: 4.792

2.  Nanoliter multiplex PCR arrays on a SlipChip.

Authors:  Feng Shen; Wenbin Du; Elena K Davydova; Mikhail A Karymov; Janmajay Pandey; Rustem F Ismagilov
Journal:  Anal Chem       Date:  2010-06-01       Impact factor: 6.986

3.  Microfluidic quantitative PCR for simultaneous quantification of multiple viruses in environmental water samples.

Authors:  Satoshi Ishii; Gaku Kitamura; Takahiro Segawa; Ayano Kobayashi; Takayuki Miura; Daisuke Sano; Satoshi Okabe
Journal:  Appl Environ Microbiol       Date:  2014-09-26       Impact factor: 4.792

4.  Re-evaluation of dioxygenase gene phylogeny for the development and validation of a quantitative assay for environmental aromatic hydrocarbon degraders.

Authors:  Paola Meynet; Ian M Head; David Werner; Russell J Davenport
Journal:  FEMS Microbiol Ecol       Date:  2015-05-04       Impact factor: 4.194

Review 5.  Fabrication challenges and perspectives on the use of carbon-electrode dielectrophoresis in sample preparation.

Authors:  Rodrigo Martinez-Duarte
Journal:  IET Nanobiotechnol       Date:  2017-03       Impact factor: 1.847

6.  Establishment of a reborn MMV-microarray technology: realization of microbiome analysis and other hitherto inaccessible technologies.

Authors:  Harshita Sharma; Yasunori Kinoshita; Seiichi Fujiu; Shota Nomura; Mizuho Sawada; Shamim Ahmed; Masaki Shibuya; Kosaku Shirai; Syota Takamatsu; Tsuyoshi Watanabe; Hitoshi Yamazaki; Ryohei Kamiyama; Tetsuya Kobayashi; Hidenao Arai; Miho Suzuki; Naoto Nemoto; Ki Ando; Hidekazu Uchida; Koichiro Kitamura; Osamu Takei; Koichi Nishigaki
Journal:  BMC Biotechnol       Date:  2014-08-21       Impact factor: 2.563

Review 7.  Detection of pathogens in water: from phylochips to qPCR to pyrosequencing.

Authors:  Tiong Gim Aw; Joan B Rose
Journal:  Curr Opin Biotechnol       Date:  2011-12-05       Impact factor: 9.740

8.  Design and Performance Testing of a DNA Extraction Assay for Sensitive and Reliable Quantification of Acetic Acid Bacteria Directly in Red Wine Using Real Time PCR.

Authors:  Cédric Longin; Michèle Guilloux-Benatier; Hervé Alexandre
Journal:  Front Microbiol       Date:  2016-06-01       Impact factor: 5.640

9.  The identification and semi-quantitative assessment of gastrointestinal nematodes in faecal samples using multiplex real-time PCR assays.

Authors:  Nikol Reslova; Lucie Skorpikova; Iveta Angela Kyrianova; Jaroslav Vadlejch; Johan Höglund; Philip Skuce; Martin Kasny
Journal:  Parasit Vectors       Date:  2021-08-09       Impact factor: 3.876
  9 in total

北京卡尤迪生物科技股份有限公司 © 2022-2023.