Improving the diagnosis of invasive aspergillosis by the detection of Aspergillus in broncho-alveolar lavage fluid: Comparison of non-culture-based assays

Guegan, Hélène; Robert‐Gangneux, Florence; Camus, Christophe; Belaz, Sorya; Marchand, Tony; Baldeyrou, M.; Gangneux, Jean‐Pierre

doi:10.1016/j.jinf.2017.11.011

Cited by 39 publications

(50 citation statements)

References 44 publications

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“…In our cohort, the specificity of Aspergillus and panfungal PCR was similar or better to previous reports with 36%‐94% and 67%‐86% in BAL‐fluid, respectively, while their sensitivities were much lower . There are several potential explanations for the poor sensitivities of our PCR in the BAL‐fluid.…”

Section: Discussionsupporting

confidence: 83%

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Diagnosis of invasive mold diseases in patients with hematological malignancies using Aspergillus, Mucorales, and panfungal PCR in BAL

Wehrle-Wieland

Affolter

Goldenberger

et al. 2018

Transplant Infectious Dis

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Section: Discussionsupporting

confidence: 83%

“…When test performance was re‐evaluated disregarding GM to define probable disease, sensitivity of Aspergillus and panfungal PCRs increased to 50% and 25%. This illustrates the difficulty of the diagnosis of IMD in this and many other studies . Among the 167 patients included in this study, only 6 had proven IMD.…”

Section: Discussionmentioning

confidence: 59%

Diagnosis of invasive mold diseases in patients with hematological malignancies using Aspergillus, Mucorales, and panfungal PCR in BAL

Wehrle-Wieland

Affolter

Goldenberger

et al. 2018

Transplant Infectious Dis

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“…19 Also a recent study comparing various diagnostic methods, which reported the sensitivity of MycoGenie R of 73.7% in 38 patients with proven/probable IA, had a very high (22/38, 58%) rate of positivity of culture for Aspergillus. 12 In addition, in that cohort, the sensitivity was lower in 41 hematological patients than in those from intensive care unit (ICU) suggesting a lower fungal burden sufficient to cause IFD in highly immunocompromised hosts. 12 Indeed, also the low yield of fungal cultures and rather low median BAL GM ODI confirm the low burden of viable moulds in this study.…”

Section: Discussionmentioning

confidence: 75%

“…Molecular methods such as polymerase chain reaction (PCR) are able to detect Aspergillus DNA in BAL samples with good sensitivity (77.2%) and specificity (93.5%). 10 Although in recent years many publications [11][12][13] focused on the diagnostic role of Aspergillus PCR, its use is not yet recommended in the 2016 update of IDSA Guidelines on the diagnosis and management of Aspergillosis, mostly because of the lack of standardised and validated assays. 2,3 Their advantages include the possibility to detect fungal DNA also if it is no longer viable, such as after antifungal treatment has been started, and to confirm the presence of Aspergillus with higher sensitivity than culture, similarly to GM.…”

Section: Introductionmentioning

confidence: 99%

Use of Aspergillus fumigatus real-time PCR in bronchoalveolar lavage samples (BAL) for diagnosis of invasive aspergillosis, including azole-resistant cases, in high risk haematology patients: the need for a combined use with galactomannan

et al. 2019

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Diagnosis of invasive aspergillosis (IA) is challenging, particularly in high-risk patients with lung lesions other than typical according to 2008-EORTC/MSG criteria. Even if microbiology is positive, they still remain unclassified according to 2008-EORTC/MSG. Quantitative polymerase chain reaction (qPCR) provides new mycological documentation of IA. This retrospective study assessed Aspergillus fumigatus real time qPCR (MycoGENIE R ) in BAL to diagnose IA and identify azole-resistant strains. Clinical, radiological, and microbiological data from 114 hematology patients (69% HSCT recipients; 29% on mould active agents) from years 2012-2017 were collected; and 123 BAL samples were tested with qPCR (cutoff: Ct < 40) and galactomannan (GM, Platelia R , cutoff: 0.5 ODI). Patients were classified as proven/probable, possible, and no-IA. "Atypical-IA" referred to patients with lesions other than typical according to 2008-EORTC/MSG and positive mycology. Proven IA was diagnosed in two cases (1.6%), probable in 28 (22.8%), possible in 27 (22%), atypical in 14 (11.4%). qPCR was positive in 39 samples (31.7%). Sensitivity and specificity of qPCR for proven/probable IA (vs no-IA; atypical-IA excluded) were 40% (95% confidence interval [CI]: 23-59) and 69% (95%CI: 55-81), respectively. Sensitivity of qPCR was higher when combined with GM (83%, 95%CI: 65-94) and in those receiving mould-active agents at BAL (61%, 95%CI: 32-86). One sample had TR34/L98H mutation. In conclusion, in high-risk hematology patients with various lung lesions, A. fumigatus qPCR in BAL contributes to diagnosing IA, particularly if combined with GM and in patients receiving mould-active agents might allow detecting azole-resistant mutations in culture negative samples. C The Author(s)

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“…The validity of other, non‐culture‐based methods for the detection of Aspergillus has gained traction over recent years, such that current proposals for the second revision of the EORTC/MSG definitions for IMI include consideration of Aspergillus PCR assays . PCR‐based assays have a wide range of reported sensitivities and have been suggested as a way to improve diagnostic accuracy when combined with other modalities, detect azole resistance and guide judicious use of preemptive antifungal treatment . Grancini et al suggested that BAL real‐time PCR, when performed in conjunction with routine BAL culture and GM, can have a NPV of 99% in immunocompromised patients, while Hoenigl et al reported 100% sensitivity and 98% specificity when combining PCR with GM.…”

Section: Discussionmentioning

confidence: 99%

False positive bronchoalveolar lavage galactomannan: Effect of host and cut‐off value

Farmakiotis

Weiss

et al. 2018

Mycoses

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Summary Objectives Bronchoalveolar lavage galactomannan (BAL‐GM) is a mycological criterion for diagnosis of probable invasive aspergillosis (IA) per European Organization for Research and Treatment of Cancer/Mycoses Study Group (EORT‐MSG) consensus criteria, but its real‐world positive predictive value (PPV) has not been well‐studied. Our aim was to estimate the PPV of BAL‐GM in a contemporary cohort of patients with positive BAL‐GM. Methods We identified consecutive patients with ≥1 positive BAL‐GM value (index ≥ 0.5) at Brigham and Women's Hospital from 11/2009 to 3/2016. We classified patients as having no, possible, probable, or proven IA, excluding BAL‐GM as mycological criterion. Results We studied 134 patients: 54% had hematologic malignancy (HM), and 10% were solid organ transplant (SOT) recipients. A total of 42% of positive (≥0.5) BAL‐GM results were falsely positive (PPV 58%). The number of probable IA cases was increased by 23% using positive BAL‐GM as mycologic criterion alone. PPV was higher in patients with HM or SOT (P < 0.001) and with use of higher thresholds for positivity (BAL‐GM ≥ 1 vs 1‐0.8 vs 0.8‐0.5: P = 0.002). Conclusions 42% of positive BAL‐GM values were falsely positive. We propose a critical reassessment of BAL‐GM cutoff values in different patient populations. Accurate noninvasive tests for diagnosis of IA are urgently needed.

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Improving the diagnosis of invasive aspergillosis by the detection of Aspergillus in broncho-alveolar lavage fluid: Comparison of non-culture-based assays

Abstract: The molecular detection of Aspergillus directly in BAL samples greatly improved the diagnosis of IA, particularly in non-hematological patients.

Cited by 39 publications

References 44 publications

Diagnosis of invasive mold diseases in patients with hematological malignancies using Aspergillus, Mucorales, and panfungal PCR in BAL

Diagnosis of invasive mold diseases in patients with hematological malignancies using Aspergillus, Mucorales, and panfungal PCR in BAL

Use of Aspergillus fumigatus real-time PCR in bronchoalveolar lavage samples (BAL) for diagnosis of invasive aspergillosis, including azole-resistant cases, in high risk haematology patients: the need for a combined use with galactomannan

False positive bronchoalveolar lavage galactomannan: Effect of host and cut‐off value

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