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[通过半定量和原位检测法检测端粒酶活性以及对膀胱癌中hTERT表达进行定量分析]

[Detection of telomerase activity by semi-quantitative and in situ assays and quantification of hTERT expression in bladder carcinomas].

作者信息

Longchampt Elisabeth, Lebret Thierry, Molinie Vincent, Bieche Ivan, Botto Henry, Lidereau Rosette

机构信息

Laboratoire d'Oncogénétique, INSERM E0017, Saint-Cloud, France.

出版信息

Prog Urol. 2003 Apr;13(2):238-45.

PMID:12765058
Abstract

OBJECTIVES

Several studies have reported the important role played by telomerase, an enzyme which maintains the length of telomeres, during carcinogenesis. The objective of this study was to detect telomerase activity by semiquantitative in situ methods and to quantify expression of the hTERT subunit in a group of bladder cancers in order to assess its diagnostic and prognostic value.

MATERIAL AND METHODS

Telomerase activity (TA) was detected by the TRAP method ("telomeric repeat amplification protocol") on a series of 29 bladder cancers and 3 samples of healthy mucosa. Levels of expression of the hTERT gene were studied by real-time quantitative RT-PCR. In situ detection of TA was performed by using the same kit as the TRAP method, applied to frozen tissue sections exclusively for cases with discordant results between TA detection and hTERT mRNA.

RESULTS

TA was detected by TRAP in 15 of the 29 bladder cancers. hTERT mRNA was detected and quantified in all tumour samples. A significant correlation was observed between TA and the level of hTERT mRNA expression. In situ detection of TA demonstrated heterogeneous TA in tumour tissue. A significant correlation was observed between the level of hTERT mRNA expression and tumour histological grades and stages.

CONCLUSION

hTERT mRNA detection by real-time quantitative RT-PCR appears to be a sensitive method for the diagnosis of bladder cancer with a good correlation with tumour grade and stage. Quantitative evaluation of hTERT mRNA could therefore be a useful marker of tumour progression for the early diagnosis and follow-up of bladder cancers.

摘要

目的

多项研究报道了端粒酶(一种维持端粒长度的酶)在致癌过程中所起的重要作用。本研究的目的是通过半定量原位方法检测端粒酶活性,并对一组膀胱癌中hTERT亚基的表达进行定量,以评估其诊断和预后价值。

材料与方法

采用端粒重复序列扩增法(TRAP法)检测29例膀胱癌及3例健康黏膜样本中的端粒酶活性(TA)。通过实时定量逆转录聚合酶链反应(RT-PCR)研究hTERT基因的表达水平。对于TA检测与hTERT mRNA结果不一致的病例,仅将用于TRAP法的同一试剂盒应用于冷冻组织切片进行TA的原位检测。

结果

29例膀胱癌中,15例通过TRAP法检测到TA。在所有肿瘤样本中均检测并定量了hTERT mRNA。观察到TA与hTERT mRNA表达水平之间存在显著相关性。TA的原位检测显示肿瘤组织中TA呈异质性。观察到hTERT mRNA表达水平与肿瘤组织学分级和分期之间存在显著相关性。

结论

通过实时定量RT-PCR检测hTERT mRNA似乎是诊断膀胱癌的一种敏感方法,与肿瘤分级和分期具有良好的相关性。因此,hTERT mRNA的定量评估可能是膀胱癌早期诊断和随访中肿瘤进展的一个有用标志物。

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