摘要
Objective. To understanding the molecular mechanisms in invasion and metastasis of the ovarian car-cinoma, we investigate a novel candidate metastasis-associated gene (MTA1) and nm23H1 mRNA ex-pression and mutation in ovarian carcinoma.Methods. Twenty primary ovarian carcinoma specimens, 20 corresponding lymph nodes and 8 normalovarian was examined for mRNA expression and mutation of MTA1 and nm23H1 genes by revere-tran-scription ploymerase chain reaction(RT-PCR) and RT-PCR-SSCP analysis. The level of the expressionwas determined by the relative optic desity (ROD) of the PCR products.Results. The frequency of MAT1 overexpression was 100%(7/7) in primary ovarian carcinoma withmetastasis but only 38.5% (5/13) in those without metastasis (P=0.0103 ). Overexpression of MAT1 wasobserved in 87.5%(6/7) of lymph nodes with metastasis but only 23%(3/13) of lymph nodes withoutmetastasis (P=0.0118). In contrast with MAT1, low expression of nm23H1 mRNA was seen in 7 of 7 o-varian carcinoma with metastasis but only in 4 of 13(30%) of those without metastassis (P=0.0043). Lownm23H1 expression was also seen in 7 of 7 lymph nodes with metastasis but only in 5 of 13 (38.5%)nonmetastatic lymph nodes (P=0.0102). The ROD ratio of MAT1 to nm23H1 increased with the develop-ment of metastasis. No mutation of MAT1 and nm23H1 genes was found by SSCP analysis.Conclusion. The mRNA expression of MTA1 and nm23H1 is positively and negatively correlated withlymph node metastasis, respectively. Expression abnormalities but not mutation of the two genes are fre-quent events related to lymph node metastasis of ovarian cancer.
Objective. To understanding the molecular mechanisms in invasion andmetastasis of the ovarian carcinoma, we investigate a novel candidate metastasis―associated gene (MTA1) and nm23Hl mRNA expression and mutation in ovarian carcinoma. Methods. Twenty primary ovariancarcinoma specimens, 20 corresponding lymph nodes and 8 normal ovarian was examined for mRNAexpression and mutation of MTA1 and nm23Hl genes by reverse-transcription ploymerase chain reaction(RT―PCR) and RT―PCR―SSCP analysis. The level of the expression was determined by the relativeoptic desity (ROD) of the PCR products. Results. The frequency of MAT1 overexpression was 100% (7/7)in primary ovarian carcinoma with metastasis but only 38.5% (5/13) in those without metastasis(P=0.0103). Overexpression of MAT1 was observed in 87.5% (6/7) of lymph nodes with metastasis butonly 23% (3/13). of lymph nodes without metastasis (P=0.0118). In contrast with MAT1, low expressionof nm23H1 mRNA was seen in 7 of 7 o-varian carcinoma with metastasis but only in 4 of 13(30%) ofthose without metastassis (P=0.0043). Low nm23H1 expression was also seen in 7 of 7 lymph nodes withmetastasis but only in 5 of 13 (38.5%) nonmetastatic lymph nodes (P=0.0102). The ROD ratio of MAT1to nm23Hl increased with the development of metastasis. No mutation of MAT1 and nm23H1 genes wasfound by SSCP analysis. Conclusion. The mRNA expression of MTA1 and nm23H1 is positively andnegatively correlated with lymph node metastasis, respectively. Expression abnormalities but notmutation of the two genes are frequent events related to lymph node metastasis of ovarian cancer.
