共 51 条
Performance evaluation of multiplex PCR including Aspergillus - not so simple!
被引:18
作者:

Alanio, Alexandre
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机构:
Sorbonne Paris Cite Univ, Paris Diderot, Paris, France
St Louis Hosp, AP HP, Parasitol Mycol Lab, Paris, France
Inst Pasteur, Mycol Unit, CNRS URA3012, Natl Reference Ctr Invas Mycoses & Antifungals, Paris, France Sorbonne Paris Cite Univ, Paris Diderot, Paris, France

Bretagne, Stephane
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Sorbonne Paris Cite Univ, Paris Diderot, Paris, France
St Louis Hosp, AP HP, Parasitol Mycol Lab, Paris, France
Inst Pasteur, Mycol Unit, CNRS URA3012, Natl Reference Ctr Invas Mycoses & Antifungals, Paris, France Sorbonne Paris Cite Univ, Paris Diderot, Paris, France
机构:
[1] Sorbonne Paris Cite Univ, Paris Diderot, Paris, France
[2] St Louis Hosp, AP HP, Parasitol Mycol Lab, Paris, France
[3] Inst Pasteur, Mycol Unit, CNRS URA3012, Natl Reference Ctr Invas Mycoses & Antifungals, Paris, France
关键词:
Aspergillus;
multiplex PCR;
microarray;
multiplexed PCR and liquid-phase array;
electrospray-ionization mass spectrometry;
azole resistance detection;
REAL-TIME PCR;
AZOLE RESISTANCE;
INVASIVE ASPERGILLOSIS;
TRIAZOLE RESISTANCE;
DNA CONTAMINATION;
FUNGAL PATHOGENS;
IDENTIFICATION;
FUMIGATUS;
ASSAY;
DIAGNOSIS;
D O I:
10.1093/mmy/myw080
中图分类号:
R51 [传染病];
学科分类号:
100401 ;
摘要:
Multiplex PCRs have been designed for including species other than Aspergillus fumigatus for the diagnosis of invasive aspergillosis, such as microarrays, liquid-phase array, and electrospray-ionization mass spectrometry (PCR/ESI MS). These methods are based on the selection of multiple primers to amplify different species with the specificity checked by hybridization to a probe or by base composition of the amplicon for the PCR/ESI MS. When testing complex samples such as respiratory specimens, some clinically relevant species can be missed. Indeed, it is impossible to design primers able to amplify all the known fungal species with the same efficiency. Therefore, the best amplified species may not be the most clinically relevant. Multiplex assays have also been proposed to detect A. fumigatus DNA and azole resistance. Since the gene responsible for azole resistance is single copy and the gene used for detection is multicopy, only the high fungal loads can be evaluated. Thus, although interesting for investigating mycobiome, the multiplex assays should be used with cautious for the diagnosis of IA or the detection of resistance. For the diagnosis of invasive aspergillosis, validated quantitative PCRs specifically targeting A. fumigatus or a limited set of species to increase sensitivity is a safer option.
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页码:56 / 62
页数:7
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