Quick versus Quantitative: Evaluation of Two Commercial Real-Time PCR Assays for the Detection of Pneumocystis jirovecii from Bronchoalveolar Lavage Fluids
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作者:
Belanger, Corrie R.
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Vancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, CanadaVancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Belanger, Corrie R.
[1
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Locher, Kerstin
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Vancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Univ British Columbia, Dept Pathol & Lab Med, Vancouver, BC, CanadaVancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Locher, Kerstin
[1
,2
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Velapatino, Billie
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Vancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, CanadaVancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Velapatino, Billie
[1
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Dufresne, Philippe J.
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Inst Natl Sante Publ Quebec, Lab Sante Publ Quebec, Ste Anne De Bellevue, PQ, CanadaVancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Dufresne, Philippe J.
[3
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Eckbo, Eric
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Vancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Childrens Hosp Eastern Ontario, Div Microbiol, Ottawa, ON, CanadaVancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Eckbo, Eric
[1
,4
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Charles, Marthe
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Vancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Univ British Columbia, Dept Pathol & Lab Med, Vancouver, BC, CanadaVancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Charles, Marthe
[1
,2
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机构:
[1] Vancouver Coastal Hlth, Div Med Microbiol, Vancouver, BC, Canada
Two commercial real-time PCR assays for the detection of Pneumocystis jirovecii were compared, the quantitative RealStar P. jirovecii assay and the qualitative DiaSorin P. jirovecii assay, the latter of which can be used without nucleic acid extraction. Archived bronchoalveolar lavage (BAL) specimens (n = 66), previously tested by molecular methods, were tested by both assays, and the results were compared to the respective original result. The RealStar P. jirovecii assay demonstrated good positive percent agreement (PPA) (90% [95% confidence interval (CI), 72 to 97%]; 27/30) and negative percent agreement (NPA) (100% [95% CI, 88 to 100%]; 36/36) with the reference method. The DiaSorin P. jirovecii assay concordantly detected P. jirovecii in 19 of 24 positive BAL samples (PPA = 73% [95% CI, 52 to 88%]). All negative BAL samples gave concordant results (NPA = 100% [95% CI, 87 to 100%]; 34/34). Discordant results occurred mostly in samples with low fungal loads. In conclusion, the RealStar assay demonstrated good concordance with reference results, and the DiaSorin P. jirovecii assay performed well for negative BAL and positive BAL samples with P. jirovecii concentrations of greater than 260 copies/mL.IMPORTANCE Pneumonia, caused by the opportunistic fungus Pneumocystis jirovecii, poses a significant risk for immunocompromised individuals. Laboratory testing for P. jirovecii is progressively shifting toward the use of molecular tests such as real-time PCR; however, this is often performed at reference laboratories. Many frontline laboratories are looking into improving their service and reducing turnaround times for obtaining P. jirovecii results by bringing molecular P. jirovecii testing in-house. We evaluated and compared two commercial real-time PCR assays with different workflows for the detection of P. jirovecii from bronchoalveolar lavage specimens. The RealStar P. jirovecii assay requires nucleic acid extraction and provides a quantification of fungal load for positive samples. The DiaSorin P. jirovecii assay offers a simple workflow without nucleic extraction from patient samples and qualitative results. Results from this study provide valuable information on performance and workflow considerations for laboratories that wish to implement P. jirovecii molecular testing. Pneumonia, caused by the opportunistic fungus Pneumocystis jirovecii, poses a significant risk for immunocompromised individuals. Laboratory testing for P. jirovecii is progressively shifting toward the use of molecular tests such as real-time PCR; however, this is often performed at reference laboratories.
机构:
Univ Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R ChinaUniv Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R China
Lam, Jason Tszhin
Lui, Edwin
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Hong Kong Govt Environm Protect Dept, Environm Compliance Div, Wan Chai, Hong Kong, Peoples R ChinaUniv Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R China
Lui, Edwin
Chau, Simon
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Hong Kong Govt Environm Protect Dept, Environm Compliance Div, Wan Chai, Hong Kong, Peoples R ChinaUniv Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R China
Chau, Simon
Kueh, Cathie Show Wu
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Hong Kong Govt Environm Protect Dept, Water Policy & Planning Div, Wan Chai, Hong Kong, Peoples R ChinaUniv Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R China
Kueh, Cathie Show Wu
Yung, Ying-kit
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Hong Kong Govt Environm Protect Dept, Water Policy & Planning Div, Wan Chai, Hong Kong, Peoples R ChinaUniv Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R China
Yung, Ying-kit
Yam, Wing Cheong
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Univ Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R ChinaUniv Hong Kong, Dept Microbiol, Queen Mary Hosp Compound, Hong Kong, Hong Kong, Peoples R China
机构:
Univ Cape Town, Div Med Microbiol, ZA-7925 Cape Town, South Africa
Natl Hlth Lab Serv, Cape Town, South AfricaUniv Cape Town, Div Med Microbiol, ZA-7925 Cape Town, South Africa
Samuel, Catherine M.
Whitelaw, Andrew
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Univ Cape Town, Div Med Microbiol, ZA-7925 Cape Town, South Africa
Natl Hlth Lab Serv, Cape Town, South AfricaUniv Cape Town, Div Med Microbiol, ZA-7925 Cape Town, South Africa
Whitelaw, Andrew
Corcoran, Craig
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Natl Hlth Lab Serv, Cape Town, South Africa
Univ Cape Town, Div Clin Virol, ZA-7925 Cape Town, South AfricaUniv Cape Town, Div Med Microbiol, ZA-7925 Cape Town, South Africa
Corcoran, Craig
Morrow, Brenda
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Univ Cape Town, Dept Paediat & Child Hlth, Red Cross War Mem Childrens Hosp, ZA-7925 Cape Town, South AfricaUniv Cape Town, Div Med Microbiol, ZA-7925 Cape Town, South Africa