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首页> 外文期刊>British Journal of Cancer >Semiquantification of circulating hepatocellular carcinoma cells by reverse transcriptase polymerase chain reaction
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Semiquantification of circulating hepatocellular carcinoma cells by reverse transcriptase polymerase chain reaction

机译:逆转录聚合酶链反应半定量循环肝癌细胞

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Hepatocellular carcinoma (HCC) is one of the most common and rapidly fatal malignancies worldwide. Treatment options are severely limited by the frequent presence of metastases. If hepatocyte-specific mRNAs are detected in the circulation, it is possible to infer the presence of circulating, presumably malignant, liver cells. If these can be quantified, it is possible to predict the likelihood of haematogenous metastasis. In this investigation, we have attempted to gain an index of the mass of circulating HCC cells (with reference to the number of hepatoblastoma cells) by measuring the amounts of PCR products for albumin (alb) mRNA and alpha-fetoprotein (afp) mRNA by reverse transcriptase polymerase chain reaction (RT-PCR) and Southern blot analysis. For calibration, total RNA from 1-10(6) HepG2 cells was mixed with total RNA from 10(6) normal peripheral mononuclear cells. A linear relationship was demonstrated between the amount of alb- or afp PCR product and the level of HepG2 total RNA spiked. The assay is sensitive down to a detection level of one HepG2 cell. Alb mRNA was detected in 50% of 18 normal subjects and afp mRNA in only two normal subjects. The alb mRNA cut-off level for the normal was exceeded by seven normal subjects and 34 out of 64 HCC patients, and that for afp mRNA was exceeded by six HCC patients but none of the normal subjects. The level of alb mRNA detected was not linearly proportional to the amount of afp mRNA detected in peripheral blood of the same patients, suggesting heterogeneous expression of alb and afp genes in different circulating tumour cells. In addition, no significant linear association between the levels of afp mRNA and serum AFP was observed. Semiquantification of both mRNA markers for HCC cell detection may prove useful in prediction of metastases.
机译:肝细胞癌(HCC)是世界上最常见,最致命的恶性肿瘤之一。转移灶的频繁出现严重限制了治疗的选择。如果在循环中检测到肝细胞特异的mRNA,则有可能推断循环的肝细胞可能是恶性的。如果这些可以量化,则可以预测发生血源性转移的可能性。在这项研究中,我们试图通过测量白蛋白(alb)mRNA和甲胎蛋白(afp)mRNA的PCR产物的量来获得循环HCC细胞质量的指数(参考肝母细胞瘤细胞的数量)。逆转录聚合酶链反应(RT-PCR)和Southern印迹分析。为了进行校准,将来自1-10(6)HepG2细胞的总RNA与来自10(6)正常外周单核细胞的总RNA混合。在alb-或afp PCR产物的量与掺入的HepG2总RNA的水平之间显示出线性关系。该测定法敏感度低至一个HepG2细胞的检测水平。在18个正常受试者中有50%检测到Alb mRNA,仅在两个正常受试者中检测到afp mRNA。 7名正常受试者和64名HCC患者中的34名超过了正常人的alb mRNA截止水平,而6名HCC患者超出了abp mRNA的阈值,但没有一名正常受试者。在同一患者外周血中检测到的alb mRNA的水平与检测到的afp mRNA的数量不是线性比例的,表明alb和afp基因在不同的循环肿瘤细胞中异质表达。另外,在afp mRNA水平和血清AFP之间没有观察到显着的线性关联。用于HCC细胞检测的两种mRNA标记的半定量可证明对转移预测有用。

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