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Abstract
Objective: The objective of this study was to determine
the genes that may be associated with malignant transformation of
ovarian endometrioma.
Methods: Endometriotic epithelial cells were isolated
from tissues derived from chocolate cyst linings by laser capture
microdissection. A Gene Chip Human Genome U133 Plus 2.0 Array was
applied to evaluate levels of gene expression in 3 different groups of
epithelial cells: epithelial cells of endometrioma, epithelial cells of
endometrioma adjacent to clear cell carcinoma, and epithelial cells of
clear cell carcinoma. As a validation assay, real-time reverse
transcriptase-polymerase chain reaction and immunohistochemical analyses
were performed.
Results: Gene expression analysis identified differential
expressions among the 3 groups of epithelial cells.
Using the classification of a signaling pathways database, 9 genes (12 gene probes) were selected from among 39 up-regulated genes indicating more than 2-fold higher expression between any comparisons of the 3 groups in the comprehensive microarray. Enhancement of fibroblast growth factor receptor 2 (FGFR2) gene expression was detected by microarray using 3 distinct probes. Gene and protein expression of FGFR2 differed significantly between epithelial cells of endometrioma and the epithelial component of clear cell carcinoma.
Using the classification of a signaling pathways database, 9 genes (12 gene probes) were selected from among 39 up-regulated genes indicating more than 2-fold higher expression between any comparisons of the 3 groups in the comprehensive microarray. Enhancement of fibroblast growth factor receptor 2 (FGFR2) gene expression was detected by microarray using 3 distinct probes. Gene and protein expression of FGFR2 differed significantly between epithelial cells of endometrioma and the epithelial component of clear cell carcinoma.
Conclusions: We demonstrated that FGFR2 may play a
significant role in the carcinogenesis of endometriosis and thus
represents a potential therapeutic target.
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