Evaluation of PCR for Detection of DNA Specific for
            <i>Aspergillus</i>
            Species in Sera of Patients with Various Forms of Pulmonary Aspergillosis

Yamakami, Yuriko; Hashimoto, Atsuro; Yamagata, Eiji; Kamberi, Perparim; Karashima, Reiko; Nagai, Hirokazu; Nasu, Masaru

doi:10.1128/jcm.36.12.3619-3623.1998

Cited by 64 publications

(12 citation statements)

References 22 publications

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“…It does appear that, as in case of patient O, the infection is detected one week and not the next. This phenomenon has been reported (Van Burik et al , 1998; Yamakami et al , 1998; Lass‐Flörl et al, 2001). The ability of the PCR to detect Aspergillus may have been affected by the presence of antifungal drugs.…”

Section: Discussionsupporting

confidence: 69%

The prospective evaluation of a nested polymerase chain reaction assay for the early detection of Aspergillus infection in patients with leukaemia or undergoing allograft treatment

Ferns¹,

Fletcher

Bradley³

et al. 2002

Br J Haematol

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Summary. Patients with acute leukaemia or undergoing allogenic bone marrow transplantation at University College London Hospital Trust were screened for the presence of aspergillosis by polymerase chain reaction (PCR). Aspergillus DNA, from whole blood samples, was amplified by nested PCR to detect a 135 bp fragment in the mitochondrial region of Aspergillus fumigatus or A. flavus (121 bp). One colony‐forming unit (CFU) per 2 ml of blood or 1–10 fg DNA could be detected. Patients at risk of aspergillosis were classified as probable or possible based on the European Organization for Research and Treatment of Cancer definitions. Antifungal drugs given were recorded. In four of 17 patients studied, infection was not suspected and the PCR was negative. Four patients were considered to have possible aspergillosis infection and were PCR positive on at least one occasion. Of the three patients in the probable group, four of the nine samples tested PCR positive from one patient and in another patient only one of nine samples tested positive. The remaining six patients were not suspected of having fungal infection but each had one or two PCR‐positive results. In summary, six of seven patients thought to have clinical evidence of infection were PCR positive on at least one occasion and treatment with antifungals may have reduced infection below detectable levels.

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Section: Discussionsupporting

confidence: 69%

The prospective evaluation of a nested polymerase chain reaction assay for the early detection of Aspergillus infection in patients with leukaemia or undergoing allograft treatment

Ferns¹,

Fletcher

Bradley³

et al. 2002

Br J Haematol

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“…Tests are also available to detect aspergillus antibodies (120,121); however, these tests depend on a normal host immune response, which is absent in immunosupressed patients. A polymerase chain reaction test to detect DNA of Aspergillus species has been developed (122)(123)(124).…”

Section: Invasive Aspergillosismentioning

confidence: 99%

Aspergillus‐Related Lung Disease

Al-Alawi

Ryan

Flint

et al. 2005

Canadian Respiratory Journal

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Aspergillus is a ubiquitous dimorphic fungus that causes a variety of human diseases ranging in severity from trivial to life-threatening, depending on the host response. An intact host defence is important to prevent disease, but individuals with pre-existing structural lung disease, atopy, occupational exposure or impaired immunity are susceptible. Three distinctive patterns of aspergillus-related lung disease are recognized: saprophytic infestation of airways, cavities and necrotic tissue; allergic disease including extrinsic allergic alveolitis, asthma, allergic bronchopulmonary aspergillosis, bronchocentric granulomatosis and chronic eosinophilic pneumonia; and airway and tissue invasive disease -- pseudomembranous tracheobronchitis, acute bronchopneumonia, angioinvasive aspergillosis, chronic necrotizing aspergillosis and invasive pleural disease. A broad knowledge of these clinical presentations and a high index of suspicion are required to ensure timely diagnosis and treatment of the potentially lethal manifestations of aspergillus-related pulmonary disease. In the present report, the clinical, radiographic and pathological aspects of the various aspergillus-related lung diseases are briefly reviewed.

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“…A number of previous studies evaluating PCR‐mediated detection of Aspergillus species showed significantly improved sensitivity but involved assays with different methods and objectives, partly to optimize culture assays, partly for typing in epidemiological studies (Aufauvre‐Brown et al , 1992; van Belkum et al , 1993; Girardin et al , 1994; Anderson et al , 1996; Rath et al , 1996; Brandt et al , 1998; Fletcher et al , 1998; Radford et al , 1998). Studies with clinical samples, such as blood or BAL, were mostly done retrospectively and, with few exceptions, with small numbers of patients (Spreadbury et al , 1993; Tang et al , 1993; Makimura et al , 1994; Melchers et al , 1994; Bretagne et al , 1995, 1998; Verweij et al , 1995a; Walsh et al , 1995; Kappe et al , 1996; Yamakami et al , 1996, 1998; Einsele et al , 1997, 1998; Jones et al , 1998; Van Burik et al , 1998; Kawamura et al , 1999; Skladny et al , 1999). Results from recent studies screening blood samples from high‐risk patients with PCR assays seem promising to identify a population at highest risk for invasive fungal disease (Einsele et al , 1998; Hebart et al , 2000a,b; Lass‐Flörl et al , 2001).…”

mentioning

confidence: 99%

Clinical evaluation of a polymerase chain reaction assay to detect Aspergillus species in bronchoalveolar lavage samples of neutropenic patients

et al. 2002

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Summary. The increasing incidence of invasive aspergillosis, a life-threatening infection in immunocompromised patients, emphasizes the need to improve the currently limited diagnostic tools. Using a recently developed two-step polymerase chain reaction (PCR) assay to detect 10 fg of Aspergillus DNA, corresponding to 1-5 colony-forming units (CFU)/ml of spiked samples in vitro, we prospectively examined 197 bronchoalveolar lavage (BAL) samples from 176 subjects, including 141 neutropenic, febrile patients with lung infiltrates, at risk for invasive fungal disease. Underlying diseases of these patients were haematological malignancies; 93 patients suffered from acute leukaemias. Thirty-one of these immunocompromised patients (17AE6%) were PCR positive, correlating with positive BAL culture, positive histology from lung surgery or from autopsy, positive computerized tomography scans or positive galactomannan enzyme-linked immunosorbent assay. Six patients (4AE3%) of this group had positive PCR results without any correlation to clinical or other diagnostic data, probably owing to contamination of the samples by ubiquitous Aspergillus spores. The samples of two patients (1AE4%) with a subsequent histologically proven mould infection were PCR negative. All 102 immunocompromised patients (72AE3%) with a negative PCR showed no evidence of invasive fungal disease. From 35 patients without immunodeficiency, four (11AE4%) showed positive results, without evidence of invasive or non-invasive pulmonary aspergillosis. In this haematological population, the sensitivity and specificity values of the test reached 93AE9% and 94AE4%, the positive predictive value 83AE8%, the negative predictive value 98AE1%. Our data support the considerable clinical value of this PCR assay for confirming and improving diagnosis of pulmonary aspergillosis in high-risk patients.

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Evaluation of PCR for Detection of DNA Specific for Aspergillus Species in Sera of Patients with Various Forms of Pulmonary Aspergillosis

Cited by 64 publications

References 22 publications

The prospective evaluation of a nested polymerase chain reaction assay for the early detection of Aspergillus infection in patients with leukaemia or undergoing allograft treatment

The prospective evaluation of a nested polymerase chain reaction assay for the early detection of Aspergillus infection in patients with leukaemia or undergoing allograft treatment

Aspergillus‐Related Lung Disease

Clinical evaluation of a polymerase chain reaction assay to detect Aspergillus species in bronchoalveolar lavage samples of neutropenic patients

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