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鼠A型逆转录病毒可促进胚胎癌细胞中高水平的基因表达。

Murine A type retroviruses promote high levels of gene expression in embryonal carcinoma cells.

作者信息

Morgan R A, Christy R J, Huang R C

机构信息

Department of Biology, Johns Hopkins University, Baltimore, MD 21218.

出版信息

Development. 1988 Jan;102(1):23-30. doi: 10.1242/dev.102.1.23.

Abstract

The expression of Intracisternal A Particle (IAP) genes in the mouse embryonal carcinoma cell line PCC3 was investigated by cDNA cloning and transient gene expression assays. A group of 26 IAP cDNA clones, products of transcriptionally active IAP proviruses, were selected from a cDNA library made from undifferentiated PCC3 cell RNA. Several of these clones were characterized by restriction enzyme mapping and DNA sequence analysis. The DNA sequence in both the promoter and structural regions of two cDNAs closely resembles those of IAP genomic clones. Three new sequence elements were identified within the U3 region, an Sp1 transcription-factor-binding site, an adenovirus E1a enhancer sequence and a region of homology to a promoter element of adenovirus E4 gene. Hybrid constructs were made that place the U3/R region of the IAP cDNAs immediately 5' to the chloramphenicol acetyl transferase (CAT) gene. IAP-CAT constructs were transfected into PCC3 cells, and cell extracts prepared and analysed for CAT enzyme activity and CAT RNA levels. IAP-CAT transfected cells were shown to contain substantial levels of CAT enzyme activity and to accumulate much greater levels of CAT RNA than two standard promoters, pRSVcat and pSV2cat. The ability of these A type retroviral promoters to function in PCC3 cells is in direct contrast to the near total restriction of normal C type retroviral expression in EC cells.

摘要

通过cDNA克隆和瞬时基因表达分析,研究了小鼠胚胎癌细胞系PCC3中脑内A颗粒(IAP)基因的表达。从由未分化的PCC3细胞RNA构建的cDNA文库中,挑选出一组26个IAP cDNA克隆,它们是转录活性IAP前病毒的产物。其中几个克隆通过限制性酶切图谱和DNA序列分析进行了表征。两个cDNA的启动子和结构区域中的DNA序列与IAP基因组克隆的序列非常相似。在U3区域内鉴定出三个新的序列元件,一个Sp1转录因子结合位点、一个腺病毒E1a增强子序列以及一个与腺病毒E4基因启动子元件同源的区域。构建了杂交体,将IAP cDNA的U3/R区域置于氯霉素乙酰转移酶(CAT)基因的紧邻5'端。将IAP-CAT构建体转染到PCC3细胞中,制备细胞提取物并分析CAT酶活性和CAT RNA水平。结果显示,与两个标准启动子pRSVcat和pSV2cat相比,转染IAP-CAT的细胞含有大量的CAT酶活性,并且积累了更高水平的CAT RNA。这些A型逆转录病毒启动子在PCC3细胞中发挥功能的能力与EC细胞中正常C型逆转录病毒表达几乎完全受限形成直接对比。

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