Quantification of Fungal DNA by Using Fluorescence Resonance Energy Transfer and the Light Cycler System

Loeffler, Juergen; Henke, Norbert; Hebart, Holger; Schmidt, Diethard; Hagmeyer, Lars; Schumacher, Ulrike; Einsele, Hermann

doi:10.1128/jcm.38.2.586-590.2000

Cited by 253 publications

(96 citation statements)

References 14 publications

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“…The new assay's analytical sensitivity of 100 fg DNA per 50 lL reaction volume is comparable to the sensitivities of published assays for the detection of Candida and Aspergillus in systemic infections. 17,18 It is superior to the sensitivity of 10-35 pg DNA per reaction found in PCR assays for detection of dermatophytes. 6,19 The combination of direct microscopy and culture, considered the gold standard in dermatophyte diagnostics, has an unsatisfactory sensitivity level, especially in onychomycosis, where studies show that 15-50% of microscopy positive nail specimens fail to yield positive cultures.…”

Section: Discussionmentioning

confidence: 99%

Diagnosis of common dermatophyte infections by a novel multiplex real-time polymerase chain reaction detection/identification scheme

et al. 2007

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Section: Discussionmentioning

confidence: 99%

Diagnosis of common dermatophyte infections by a novel multiplex real-time polymerase chain reaction detection/identification scheme

et al. 2007

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“…Several studies have described probes, restriction fragment length polymorphisms or other methods to identify unique ribosomal DNA (rDNA) sequences (Hopfer et al 1993;Prariyachatigul et al 1996;Kappe et al 1998;Turenne et al 1999;Velegraki et al 1999;Evertsson et al 2000;Kauffman et al 2000;Loeffler et al 2000;Martin et al 2000;Turin et al 2000). The most common approaches have targeted portions of the rDNA of species of yeast (Prariyachatigul et al 1996;Tanaka et al 1996;Elie et al 1998;Flahaut et al 1998;Walsh and Chanock 1998;Evertsson et al 2000;Baquero et al 2001).…”

Section: Introductionmentioning

confidence: 99%

Identification of pathogenic yeast species by polymerase chain reaction amplification of theRPS0gene intron fragment

Martínez

Gómez

Pemán

et al. 2009

Journal of Applied Microbiology

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Aims: This work focuses on the development of a method for the identification of pathogenic yeast. With this aim, we target the nucleotide sequence of the RPS0 gene of pathogenic yeast species with specific PCR primers. PCR analysis was performed with both the genomic DNA, whole cells of clinical isolates of Candida species and clinical samples. Methods and Results: A single pairs of primers, deduced from the nucleotide sequence of the RPS0 gene from pathogenic yeast, were used in PCR analysis performed with both the genomic DNA and whole cells of clinical isolates of Candida species and clinical samples. The primers designed are highly specific for their respective species and produce amplicons of the expected sizes and fail to amplify any DNA fragment from the other species tested. The set of primers was tested successfully for the identification of yeast from colonies, blood cultures and clinical samples. These results indicate that genes containing intron sequences may be useful for designing species‐specific primers for the identification of fungal strains by PCR. The sensitivity of the method with genomic DNA was evaluated with decreasing DNA concentrations (200 ng to 1 pg) and different cell amounts (107–105 cells). Conclusion: The results obtained show that the amplification of RPS0 sequences may be suitable for the identification of pathogenic and other yeast species. Significance and Impact of the Study: Identification of Candida species using molecular approaches with high discriminatory power is important in determining adequate measures for the interruption of transmission of this yeast. The approach described in this work is based on standard technology, and it is specific, sensitive and does not involve complex and expensive equipment. Furthermore, the method developed in this work not only can be used in eight yeast species, but also provides the basis to design primers for other fungi species of clinical, industrial or environmental interest.

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“…Primer sequences and hybridization probes for the detection of 18S rRNA gene for Candida spp. were used as previously described (Loeffler et al 2000b). Standard PCR was performed on a T gradient thermo block (Biometra, Göttingen, Germany) in a 50-ll reaction mix containing 1 ll of the isolated DNA, 0AE25 ll Taq DNA polymerase (5 U ll )1 , AmpliTaq Ò , 1AE25 ll PCR nucleotide mix (10 mmol l )1 of each dNTP) (all Roche, Mannheim, Germany), 0AE2 ll of each primer (0AE01 nmol ll )1 , Biometra), 5 ll 10 · PCR buffer (200 mmol l )1 Tris-HCl, 500 mmol l )1 KCl, pH 8AE4), 4 ll MgCl 2 (50 mmol l )1 , Invitrogen, Karlsruhe, Germany) and 38AE1 ll dH 2 0 (Sigma-Aldrich).…”

Section: Pcrmentioning

confidence: 99%

“…Early identification of Candida species improves the survival of individual patients and is necessary for initiation of an optimal antifungal therapy (Schabereiter-Gurtner et al 2007) or for the development of specific cell therapy strategies. However, current PCR protocols have been criticised because of poor sensitivity, lack of standardization and excessive time and labour efforts (Loeffler et al 2000b). Improvements of the methodology for clinical routine diagnostics are warranted.…”

Section: Introductionmentioning

confidence: 99%

A real-time PCR assay for the differentiation of Candida species

Stephan

Fricke²,

Schimmelpfennig

et al. 2010

Journal of Applied Microbiology

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Aims: We established a real-time PCR assay for the detection and strain identification of Candida species and demonstrated the ability to differentiate between Candida albicans the most common species, and also Candida parapsilosis, Candida glabrata, Candida tropicalis and Candida dubliniensis by LightCycler PCR and melting curve analysis. Methods and Results: The DNA isolation from cultures and serum was established using the QIAmp Tissue Kit. The sensitivity of the assay was >/= 2 genome equivalents/assay. It was possible to differentiate all investigated Candida species by melting curve analysis, and no cross-reaction to human DNA or Aspergillus species could be observed. Conclusions: The established real-time PCR assay is a useful tool for the rapid identification of Candida species and a base technology for more complex PCR assays. Significance and Impact of the Study: We carried out initial steps in validation of a PCR assay for the detection and differentiation of medically relevant Candida species. The PCR was improved by generating PCR standards, additional generation of melting curves for species identification and the possibility to investigate different specimens simultaneously

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Quantification of Fungal DNA by Using Fluorescence Resonance Energy Transfer and the Light Cycler System

Cited by 253 publications

References 14 publications

Diagnosis of common dermatophyte infections by a novel multiplex real-time polymerase chain reaction detection/identification scheme

Diagnosis of common dermatophyte infections by a novel multiplex real-time polymerase chain reaction detection/identification scheme

Identification of pathogenic yeast species by polymerase chain reaction amplification of theRPS0gene intron fragment

A real-time PCR assay for the differentiation of Candida species

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