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大鼠肿瘤中特异性表达序列的克隆。

Cloning of sequences expressed specifically in tumors of rat.

作者信息

Yamamoto M, Maehara Y, Takahashi K, Endo H

出版信息

Proc Natl Acad Sci U S A. 1983 Dec;80(24):7524-7. doi: 10.1073/pnas.80.24.7524.

Abstract

The sequences specifically transcribed in tumor cells are believed to be closely related to transformed phenotypes. For the isolation of such sequences, a cDNA clone library was constructed by using poly(A)+ RNAs from azo-dye-induced rat ascites hepatomas. Thirty-one tumor RNA-responsive clones were isolated by screening 4,000 clones of this library with conventional techniques, differential colony hybridization, and RNA blot hybridization. These clones were categorized into two groups with respect to their size distribution of mRNAs from which clones were derived. The first group was complementary to a single distinct species, either about 1.5 or 0.6 kilobases in length, of poly(A)+ RNA, and the second showed no distinct bands but a smear on a RNA blot. Semiquantitative RNA dot blot assays revealed that the sequences of these clones were expressed very little, if at all, in normal and regenerating livers, while generally high in ascites hepatomas. This specificity was also true for other solid lines of tumors, such as Morris hepatoma 5123D of Buffalo rat and Walker 256 carcinosarcoma of Wistar rat. The smear class sequences were transcribed from middle-repetitive sequences of DNA, indicating that a class of middle-repetitive sequences is specifically transcribed in tumor cells.

摘要

据信,肿瘤细胞中特异性转录的序列与转化表型密切相关。为了分离此类序列,利用偶氮染料诱导的大鼠腹水肝癌的聚腺苷酸加尾(poly(A)+)RNA构建了一个cDNA克隆文库。通过使用常规技术、差异菌落杂交和RNA印迹杂交对该文库的4000个克隆进行筛选,分离出31个肿瘤RNA反应性克隆。根据这些克隆所源自的mRNA的大小分布,将这些克隆分为两组。第一组与长度约为1.5或0.6千碱基的单一独特种类的聚腺苷酸加尾RNA互补,第二组在RNA印迹上没有明显条带,而是呈现一片模糊。半定量RNA斑点印迹分析表明,这些克隆的序列在正常肝脏和再生肝脏中即使有表达也非常少,而在腹水肝癌中通常表达较高。这种特异性在其他实体瘤细胞系中也成立,如布法罗大鼠的莫里斯肝癌5123D和Wistar大鼠的沃克256癌肉瘤。模糊类序列是从DNA的中度重复序列转录而来,这表明一类中度重复序列在肿瘤细胞中特异性转录。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0043/389984/4233b1852f33/pnas00650-0158-a.jpg

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