Performance characteristics of seven neuron-specific enolase assays
Language English Country United States Media print-electronic
Document type Comparative Study, Journal Article, Research Support, N.I.H., Extramural
Grant support
MH 64165
NIMH NIH HHS - United States
PubMed
17259755
DOI
10.1159/000098441
PII: 000098441
Knihovny.cz E-resources
- MeSH
- Adenocarcinoma blood enzymology MeSH
- Biological Assay * MeSH
- Enzyme-Linked Immunosorbent Assay MeSH
- Phosphopyruvate Hydratase blood MeSH
- Humans MeSH
- Carcinoma, Small Cell blood enzymology MeSH
- Biomarkers, Tumor metabolism MeSH
- Lung Neoplasms blood enzymology MeSH
- Carcinoma, Non-Small-Cell Lung blood enzymology MeSH
- Sensitivity and Specificity MeSH
- Carcinoma, Squamous Cell blood enzymology MeSH
- Case-Control Studies MeSH
- Carcinoma, Large Cell blood enzymology MeSH
- Check Tag
- Humans MeSH
- Publication type
- Journal Article MeSH
- Research Support, N.I.H., Extramural MeSH
- Comparative Study MeSH
- Names of Substances
- Phosphopyruvate Hydratase MeSH
- Biomarkers, Tumor MeSH
BACKGROUND/AIMS: The determination of neuron-specific enolase (NSE) is relatively frequently requested in the differential diagnosis of small-cell lung carcinoma and non-small-cell lung carcinoma. The individual results of different immunoassays are often not comparable, which has been confirmed by long-term external quality assessments. In this study, we assessed the possible sources of these differences. METHODS: More than 3,000 NSE analyses were performed using seven different immunoassays: DELFIA (PerkinElmer), Elecsys 2010 or Modular Analytics E 170 (Roche), Kryptor (B.R.A.H.M.S.), the enzyme-linked immunosorbent assay DRG and three assays based on immunoradiometric assays (DiaSorin, Immunotech and Schering-CIS). The following parameters were evaluated: precision profile of the individual methods, linearity on dilution and modified recovery, comparability and discrimination of immunoassays, sensitivity, and specificity. RESULTS: There were differences in the correlation of values of certain low-concentration specimens. Some assays correlate well while others do not (up to fivefold difference), especially in the case of controls prepared synthetically. Therefore, the current non-standardized preparation of controls is questionable in our opinion. In the cutoff range, the difference in the results of native samples did not exceed its double value. The variation in values >100 microg/l obtained with different assays is <40%. CONCLUSION: Our results confirmed expected matrix interferences especially in the range of normal and cutoff NSE concentrations. Another source of discrepancies can be attributed to different antibody affinity to alphagamma- and gammagamma-enolase isoenzymes. Finally, improper settings of cutoff values also contribute to the different discrimination of the methods.
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