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Triosephosphate isomerase and peroxiredoxin 6, two novel serum markers for human lung squamous cell carcinoma

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There is currently substantial interest in the identification of human tumor antigens for the diagnosis and immunotherapy of cancer. In our previous study, secretion character and up‐regulation of triosephosphate isomerase were observed in lung squamous cell carcinoma, and autoantibodies against triosephosphate isomerase and peroxiredoxin 6 were detected in the sera from over 25% of patients, but in none of the healthy controls. In this study, peroxiredoxin 6 was also found at higher levels in the sera of the patients. Up‐regulated triosephosphate isomerase and peroxiredoxin 6 were further validated by enzyme‐linked immunosorbent assay in an additional 61 lung squamous cell carcinoma patients, 23 lung adenocarcinoma patients, 56 other types of carcinoma patients, 12 benign lung disease patients, and 59 healthy controls. We found that both triosephosphate isomerase and peroxiredoxin 6 were specifically elevated in lung squamous cell carcinoma sera compared with other groups, with the exception of peroxiredoxin 6 in lung adenocarcinoma patients. Positive correlation between triosephosphate isomerase and distant metastasis was found. At the cut‐off point 0.221 (optical density value) on the receiver operating characteristic curve, triosephosphate isomerase could comparatively discriminate lung squamous cell carcinoma from healthy controls with a sensitivity of 65.6%, specificity 84.7%, and total accuracy 75%. For peroxiredoxin 6, at the cut‐off point 0.151, it could discriminate the two groups with a sensitivity of 70.5%, specificity 62.7%, and total accuracy 65.8%. With both triosephosphate isomerase and peroxiredoxin 6, discriminant analysis results showed that 68.9% of the lung squamous cell carcinoma and 83.1% of healthy controls were correctly classified. We concluded that triosephosphate isomerase and peroxiredoxin 6 could be markers for lung squamous cell carcinoma. (Cancer Sci 2009; 100: 2396–2401)
Title: Triosephosphate isomerase and peroxiredoxin 6, two novel serum markers for human lung squamous cell carcinoma
Description:
There is currently substantial interest in the identification of human tumor antigens for the diagnosis and immunotherapy of cancer.
In our previous study, secretion character and up‐regulation of triosephosphate isomerase were observed in lung squamous cell carcinoma, and autoantibodies against triosephosphate isomerase and peroxiredoxin 6 were detected in the sera from over 25% of patients, but in none of the healthy controls.
In this study, peroxiredoxin 6 was also found at higher levels in the sera of the patients.
Up‐regulated triosephosphate isomerase and peroxiredoxin 6 were further validated by enzyme‐linked immunosorbent assay in an additional 61 lung squamous cell carcinoma patients, 23 lung adenocarcinoma patients, 56 other types of carcinoma patients, 12 benign lung disease patients, and 59 healthy controls.
We found that both triosephosphate isomerase and peroxiredoxin 6 were specifically elevated in lung squamous cell carcinoma sera compared with other groups, with the exception of peroxiredoxin 6 in lung adenocarcinoma patients.
Positive correlation between triosephosphate isomerase and distant metastasis was found.
At the cut‐off point 0.
221 (optical density value) on the receiver operating characteristic curve, triosephosphate isomerase could comparatively discriminate lung squamous cell carcinoma from healthy controls with a sensitivity of 65.
6%, specificity 84.
7%, and total accuracy 75%.
For peroxiredoxin 6, at the cut‐off point 0.
151, it could discriminate the two groups with a sensitivity of 70.
5%, specificity 62.
7%, and total accuracy 65.
8%.
With both triosephosphate isomerase and peroxiredoxin 6, discriminant analysis results showed that 68.
9% of the lung squamous cell carcinoma and 83.
1% of healthy controls were correctly classified.
We concluded that triosephosphate isomerase and peroxiredoxin 6 could be markers for lung squamous cell carcinoma.
(Cancer Sci 2009; 100: 2396–2401).

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