首页> 外文期刊>Nucleic Acids Research >IDENTIFICATION OF RAPID TURNOVER TRANSCRIPTS OVEREXPRESSED IN THYROID TUMORS AND THYROID CANCER CELL LINES - USE OF A TARGETED DIFFERENTIAL RNA DISPLAY METHOD TO SELECT FOR MRNA SUBSETS
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IDENTIFICATION OF RAPID TURNOVER TRANSCRIPTS OVEREXPRESSED IN THYROID TUMORS AND THYROID CANCER CELL LINES - USE OF A TARGETED DIFFERENTIAL RNA DISPLAY METHOD TO SELECT FOR MRNA SUBSETS

机译:甲状腺癌和甲状腺癌细胞系中过表达的快速周转记录的鉴定-使用靶向差异RNA展示法选择MRNA亚基

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The mRNAs of transiently expressed proteins such as cytokines and proto-oncogenes are commonly subject to rapid transcriptional activation and degradation, Transcript turnover is determined in part by association of certain proteins with consensus AU-rich motifs (AUUUA) in the 3'-untranslated region of the transcripts, Here we report a modification of differential RNA display (DRD) to detect differentially expressed rapid turnover mRNAs containing AU-rich motifs from thyroid cancer tissues and cell lines, RNA of normal and thyroid cancer tissues was differentially displayed using a 3' anchor primer to the poly(A) tail and an arbitrary 5' primer incorporating an AUUUA sequence, The appropriateness of the strategy was established by its ability to display known early response genes, such as c-fos, using partially degenerate primers. To test whether the novel cDNAs isolated coded for transcripts subject to rapid turnover, they were used as probes for Northern blots of RNA from clonal human thyroid carcinoma cell lines treated for varying periods with either cycloheximide or actinomycin D, A number of novel differentially expressed cDNA fragments were isolated from human papillary thyroid carcinoma tissues, among them a cDNA with zinc finger motifs and homology to other zinc finger proteins, Using this fragment to probe a cDNA library, a full-length cDNA (ZnF20) was isolated that was 4333 bp in length and contained an open reading frame of 1029 amino acids, The ZnF20 cDNA hybridized to multiple transcripts in a thyroid cancer cell line (8.0, 4.5 and 2 kb) that increased after cycloheximide treatment and decayed <2 h after addition of actinomycin D, The ZnF20 mRNA was overexpressed in three of six thyroid papillary carcinomas as compared with paired normal thyroid tissue controls, The data presented here support the use of a targeted DRD approach for the isolation of rapid turnover mRNAs, many of which may be interesting candidate oncogenes.
机译:瞬时表达蛋白(例如细胞因子和原癌基因)的mRNA通常会经历快速转录激活和降解。转录产物的转换部分取决于某些蛋白与3'-非翻译区的共有AU富集基序(AUUUA)的关联。的转录本,我们在这里报告了一种差异RNA展示(DRD)的修饰方法,用于检测来自甲状腺癌组织和细胞系的含有AU富集基序的差异表达快速更新mRNA,使用3'差异显示了正常和甲状腺癌组织的RNA锚定到poly(A)尾巴上的引物和掺入AUUUA序列的任意5'引物,该策略的适当性是通过其使用部分简并引物展示已知的早期响应基因(例如c-fos)的能力来确定的。为了测试编码为转录物的新cDNA是否经历快速更新,它们被用作探针,用于不同时期用环己酰亚胺或放线菌素D处理的克隆人甲状腺癌细胞系RNA的RNA印迹,许多新颖的差异表达cDNA从人乳头状甲状腺癌组织中分离到cDNA片段,其中一个具有锌指基序且与其他锌指蛋白有同源性的cDNA。用该片段探测cDNA文库,分离出全长4333 bp的全长cDNA(ZnF20)。长度为1029个氨基酸的开放阅读框,该ZnF20 cDNA与甲状腺癌细胞系(8.0、4.5和2 kb)中的多个转录本杂交,在环己酰亚胺处理后增加,在加入放线菌素D后<2 h衰减。与配对的正常甲状腺组织对照相比,ZnF20 mRNA在6例甲状腺乳头状癌中有3例过表达。使用靶向DRD方法分离快速更新的mRNA,其中许多可能是有趣的候选癌基因。

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