Evaluation of a commercial test based on ligase chain reaction for direct detection of Mycobacterium tuberculosis in respiratory specimens

“…Uptake of this technology to the routine environment has been slow, possibly due to the market dominance of PCR. Commercial LCR kits (LCx, Abbott laboratories) for Mycobacterium tuberculosis seem to perform adequately (Leon Muinos et al, 2004;Ribeiro et al, 2004), but the Chlamydia trachomatis LCx kit had problems with reproducibility and had to be withdrawn from the market due to ''high negative control rates resulting in invalid runs and non-repeating positives'' (FDA product recall Z-0859-1/Z-0860-1, http://www.fda.gov/bbs/topics/ ENFORCE/2001/ENF00709.html). This technology holds great promise, particularly for SNP detection and use in microchips (Lou et al, 2004) or with universal microarrays (Busti et al, 2002).…”

Section: Ligase Chain Reactionmentioning

confidence: 99%

Nucleic acid amplification-based techniques for pathogen detection and identification

Monis

Giglio

2006

Infection, Genetics and Evolution

134

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Nucleic acid amplification techniques have revolutionised diagnostic and research industries. Current technologies that allow the detection of amplification in real-time are fast becoming industry standards, particularly in a diagnostic context. In this review, we describe and explore the application of numerous real-time detection chemistries and amplification techniques for pathogen detection and identification, including the polymerase chain reaction, nucleic acid sequence-based amplification, strand displacement amplification and the ligase chain reaction. The emergence of newer technologies, such as lab-on-a-chip devices and photo-cleavable linkers, is also discussed.

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“…Further Gap-LCR takes advantage of the primer extension ability of DNA polymerase. A complete match between primers and DNA template will result in specific extension of primers and gap filling by DNA polymerase equivalent to allele-specific PCR or a single-base extension reaction [7][8][9][10]. This reaction is highly sensitive: as few as 50 copies of mutant DNA can be detected in the presence of a 10,000-fold excess of wild-type DNA when Gap-LCR and automated enzyme-linked immunoassay are utilized [7].…”

Section: Introductionmentioning

confidence: 99%

A New Genotyping Method for Detecting Low Abundance Single Nucleotide Mutations Based on Gap Ligase Chain Reaction and Quantitative PCR Assay

Jiang

et al. 2011

Cell Biochem Biophys

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We tested applicability of a new genotyping technique to detect a low abundance CD17 (A → T) mutation of β-globin gene. The technique utilized a combined gap ligase chain reaction (Gap-LCR) and quantitative PCR (qPCR) methods. One pair of Gap-LCR primers was modified by adding specific sequences to the 5' end of the upstream and the 3' end of the downstream primer which served as a combining sequence for qPCR. First, specific mutation is detected using Gap-LCR; then, ligation products are detected by qPCR. Our results show that the amount of LCR products is directly proportional to the amount of template DNA. We further demonstrate that this technique detects a low abundance mutant DNA with a mutant/normal allele ratio as low as 1:10000. This technique was applied to detect a paternally inherited CD17 mutation from 53 maternal plasma samples. The results were consistent with those obtained by PCR/reverse dot blot of amniotic fluid cell DNA. In conclusion, by combining Gap-LCR and qPCR technology we successfully established a highly sensitive technique to detect low abundance point mutations. This technique can be applied to detect fetal DNA point mutation in maternal plasma.

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Evaluation of a commercial test based on ligase chain reaction for direct detection of Mycobacterium tuberculosis in respiratory specimens

Cited by 8 publications

References 20 publications

Evolution of tuberculosis diagnostics: From molecular strategies to nanodiagnostics

Evolution of tuberculosis diagnostics: From molecular strategies to nanodiagnostics

Nucleic acid amplification-based techniques for pathogen detection and identification

A New Genotyping Method for Detecting Low Abundance Single Nucleotide Mutations Based on Gap Ligase Chain Reaction and Quantitative PCR Assay

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