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鉴定HeLa细胞中一种对EIA诱导型腺病毒启动子上游转录控制序列具有特异性的因子及其在感染和未感染细胞中的相对丰度。

Identification of a factor in HeLa cells specific for an upstream transcriptional control sequence of an EIA-inducible adenovirus promoter and its relative abundance in infected and uninfected cells.

作者信息

SivaRaman L, Subramanian S, Thimmappaya B

出版信息

Proc Natl Acad Sci U S A. 1986 Aug;83(16):5914-8. doi: 10.1073/pnas.83.16.5914.

Abstract

Utilizing the gel electrophoresis/DNA binding assay, a factor specific for the upstream transcriptional control sequence of the EIA-inducible adenovirus EIIA-early promoter has been detected in HeLa cell nuclear extract. Analysis of linker-scanning mutants of the promoter by DNA binding assays and methylation-interference experiments show that the factor binds to the 17-nucleotide sequence 5' TGGAGATGACGTAGTTT 3' located between positions -66 and -82 upstream from the cap site. This sequence has been shown to be essential for transcription of this promoter. The EIIA-early-promoter specific factor was found to be present at comparable levels in uninfected HeLa cells and in cells infected with either wild-type adenovirus or the EIA-deletion mutant dl312 under conditions in which the EIA proteins are induced to high levels [7 or 20 hr after infection in the presence of arabinonucleoside (cytosine arabinoside)]. Based on the quantitation in DNA binding assays, it appears that the mechanism of EIA-activated transcription of the EIIA-early promoter does not involve a net change in the amounts of this factor.

摘要

利用凝胶电泳/DNA结合分析,在HeLa细胞核提取物中检测到一种对EIA诱导型腺病毒EIIA早期启动子上游转录控制序列具有特异性的因子。通过DNA结合分析和甲基化干扰实验对启动子的接头扫描突变体进行分析,结果表明该因子与位于帽位点上游-66至-82位之间的17个核苷酸序列5'TGGAGATGACGTAGTTT 3'结合。该序列已被证明对该启动子的转录至关重要。在EIA蛋白被诱导至高水平的条件下(即在感染后7或20小时,在阿拉伯核苷存在下),发现未感染的HeLa细胞以及感染野生型腺病毒或EIA缺失突变体dl312的细胞中,EIIA早期启动子特异性因子的含量相当。基于DNA结合分析中的定量结果,EIA激活EIIA早期启动子转录的机制似乎并不涉及该因子数量的净变化。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6208/386407/6a82b19dc6e5/pnas00320-0171-a.jpg

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