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腺病毒基因在可溶性全细胞提取物中的DNA依赖性转录。

DNA-dependent transcription of adenovirus genes in a soluble whole-cell extract.

作者信息

Manley J L, Fire A, Cano A, Sharp P A, Gefter M L

出版信息

Proc Natl Acad Sci U S A. 1980 Jul;77(7):3855-9. doi: 10.1073/pnas.77.7.3855.

Abstract

We have developed a cell-free system for studying the synthesis of mRNA in mammalian cells. The system consists of a dialyzed and concentrated whole-cell extract derived from HeLa cells, small molecules and cofactors needed for transcription, and exogenously added DNA. Accurate transcription by RNA polymerase II is entirely dependent upon addition of promoter-containing eukaryotic DNA. At optimal DNA and extract concentrations, transcription initiation from the adenovirus serotype 2 late promoter is readily detectable, and specific transcripts over 4000 nucleotides in length are observed. The RNA synthesized in vitro contains the same 5' capped RNase T1 undecanucleotide as does the in vivo transcript. RNA synthesis also initiates accurately at both an early and an intermediate adenovirus promoter site.

摘要

我们开发了一种用于研究哺乳动物细胞中mRNA合成的无细胞系统。该系统由源自HeLa细胞的透析浓缩全细胞提取物、转录所需的小分子和辅因子以及外源添加的DNA组成。RNA聚合酶II的精确转录完全依赖于添加含启动子的真核DNA。在最佳DNA和提取物浓度下,很容易检测到腺病毒2型晚期启动子的转录起始,并且可以观察到长度超过4000个核苷酸的特异性转录本。体外合成的RNA与体内转录本含有相同的5' 帽化RNase T1十一核苷酸。RNA合成也在腺病毒早期和中期启动子位点准确起始。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d502/349725/f5fa4919a8d4/pnas00494-0147-a.jpg

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