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Identification of a novel transcript up-regulated in a clinically aggressive prostate carcinoma.

机译:在临床侵袭性前列腺癌中上调的新型转录本的鉴定。

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OBJECTIVES: To identify differentially expressed genes in tumor cells of patients with prostate cancer by means of tissue microdissection and targeted differential display. METHODS: RNA was recovered from pure populations of microdissected normal epithelium and invasive tumor from frozen tissue sections of a radical prostatectomy specimen. Reverse transcription-polymerase chain reaction (PCR) using arbitrary and zinc finger PCR primers was performed. RESULTS: A 130-base pair product was identified that appeared selectively in the tumor sample. DNA sequence analysis revealed it to be a clone from the expressed sequence tag database (GenBank accession R00504). Microdissection of normal epithelium and the corresponding invasive tumor was subsequently performed on a test panel of 10 prostate carcinoma specimens. Comparison of R00504 levels in normal epithelium and invasive carcinoma, using beta-actin as an internal control, showed the transcript to be substantially overexpressed in 5 of 10 carcinomas. Northern blotting revealed R00504 to be a 2.6-kilobase gene. CONCLUSIONS: A novel transcript up-regulated in an aggressive prostate carcinoma was identified using degenerate zinc finger primers in microdissected tissue samples. The approach used in this study may be helpful in quantitative comparison of known genes and identification of novel genes in microdissected human tissue samples.
机译:目的:通过组织显微解剖和靶向差异显示技术鉴定前列腺癌患者肿瘤细胞中差异表达的基因。方法:从前列腺癌根治术标本的冷冻组织切片中的正常解剖上皮和浸润性肿瘤的纯种群中提取RNA。使用任意和锌指PCR引物进行了逆转录聚合酶链反应(PCR)。结果:鉴定出一种130碱基对的产物,选择性地出现在肿瘤样品中。 DNA序列分析表明,它是来自表达的序列标签数据库(GenBank登录号R00504)的克隆。正常上皮和相应的浸润性肿瘤的显微解剖随后在10个前列腺癌标本的测试板上进行。使用β-肌动蛋白作为内部对照,比较正常上皮和浸润性癌中R00504的水平,表明该转录本在10个癌中的5个中基本上过表达。 Northern印迹显示R00504是2.6-碱基碱基的基因。结论:在显微解剖组织样品中使用简并的​​锌指引物鉴定了在侵略性前列腺癌中上调的新转录本。这项研究中使用的方法可能有助于定量比较人体组织样本中的已知基因和鉴定新基因。

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