High survivin expression in the primary tumor is related to poor prognosis in many cancer types [15–20]. As p53 leads to the repression of survivin expression selleck chemicals llc [21], p53 AIP1 might act inversely against survivin in the same manner as p53. It is interesting to evaluate both the expression of the p53AIP1 gene and survivin in primary non-small cell lung cancer. In this study, we demonstrated the expression of these

genes in non-small cell lung cancer and normal lung tissue, and the combination of p53AIP1 with survivin may be a prognostic marker. Methods Patients and Samples This study was approved by the Institutional Review Board of the National Hospital Organization Kumamoto Medical Center (Kumamoto, Japan) and all patients completed informed consent forms. Forty-seven operative samples from non-small cell lung cancer (NSCLC) patients were obtained at the National Hospital Organization Kumamoto Medical Center (Kumamoto, Japan) between May 1997 and September 2003. The samples were histologically diagnosed as primary non-small cell lung cancer according

to the WHO classification. None of the cases had received radiation therapy or chemotherapy before Fludarabine in vitro surgery. Adjacent normal lung tissue was also taken from all cases. Tissue specimens were frozen immediately with RNA later™(QIAGEN) and stored at -80°C until LY3039478 purchase RNA extraction. RNA from tissue samples was prepared using TRIzol reagents (Invitrogen). To evaluate cigarette consumption, a smoking index (SI) was used: cigarette consumption per day multiplied by smoking years. Referring to this index, smokers were divided into 2 groups, heavy smokers with indices ≥ 400, and light smokers < 400. Quantitative PCR analysis For quantitative evaluation of the RNA expression by PCR, we used Taqman PCR methods (TaqMan® Gene Expression Assays; Applied Biosystems, Tokyo, Japan) as previously reported [22]. The p53AIP1 gene was amplified by the following primer set as follows, reverse: ggggacttctcaggtcgtgt, forward: tggacttcttcatgccccga. The p53AIP1 gene internal probe was ttgcggtgcgagtcgtggaagtaa. Survivin was amplified by the following primer set: reverse: ggggacttctcaggtcgtgt, forward: tggacttctt

catgccccga. The survivin internal probe was ttgcggtgcgagtcgtgg aagtaa. PCR amplification condition were one cycle of 50°C, 2 min, and 95°C, 10 Idoxuridine min followed by 50 cycles of 95°C, 15 sec and 60°C, 1 min. The measured value was calculated by comparative Ct methods [22] and GAPDH gene amplification was used as a control. All reactions were duplicated. The amounts of p53AIP1 and survivin mRNA were expressed as n-fold GAPDH mRNA and the levels were compared relative to adjacent normal lung tissues. A tumor/normal ratio of p53AIP1 and survivin mRNA expression greater than 1 was identified as a positive expression, and the others as negative. Statistical analysis All statistical analysis was performed using Stat View J5.0 (SAS Institute Inc.).

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