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一种利用[3H]鸟嘌呤掺入法检测转染果蝇细胞中瞬时基因表达的实验方法。

An assay for transient gene expression in transfected Drosophila cells, using [3H]guanine incorporation.

作者信息

Burke J F, Sinclair J H, Sang J H, Ish-Horowicz D

出版信息

EMBO J. 1984 Nov;3(11):2549-54. doi: 10.1002/j.1460-2075.1984.tb02172.x.

Abstract

We have developed an assay for transient gene expression using a dominant-selectable marker previously employed to transform Drosophila cultured cells. Drosophila hydei cells transfected with a functional Escherichia coli xanthine guanine phosphoribosyl transferase gene (gpt), under the control of the long terminal repeats (LTRs) of the copia transposable element, rapidly incorporate guanine into acid-precipitable counts. Autoradiographic analysis in situ shows that approximately 20% of cells take up, and express, the gpt gene. This transient gpt expression depends on the Drosophila promoter sequences since vectors with the gpt gene in reverse orientation to the copia LTRs fail to incorporate guanine. Deletion analysis confirms that the LTRs are essential for gpt gene expression. Similarly, cells transfected with gpt controlled by the Drosophila 70 000 mol. wt. heat-shock (hsp 70) promoter show regulated guanine incorporation when heat shocked. The efficiency of the copia LTRs varies considerably between the cell lines we tested, whereas that of the hsp 70 promoter does not. The heterologous promoters of the Rous sarcoma virus (RSV) and simian virus 40 (SV40) function poorly in these cells.

摘要

我们利用先前用于转化果蝇培养细胞的显性选择标记,开发了一种瞬时基因表达检测方法。用功能性大肠杆菌黄嘌呤鸟嘌呤磷酸核糖转移酶基因(gpt)转染的海德氏果蝇细胞,在copia转座元件的长末端重复序列(LTRs)控制下,能迅速将鸟嘌呤掺入酸不溶性计数中。原位放射自显影分析表明,约20%的细胞摄取并表达了gpt基因。这种瞬时gpt表达依赖于果蝇启动子序列,因为gpt基因与copia LTRs反向的载体无法掺入鸟嘌呤。缺失分析证实LTRs对gpt基因表达至关重要。同样,用果蝇70000分子量热休克(hsp 70)启动子控制的gpt转染的细胞,在热休克时显示出受调控的鸟嘌呤掺入。我们测试的细胞系中,copia LTRs的效率差异很大,而hsp 70启动子的效率则没有差异。劳斯肉瘤病毒(RSV)和猿猴病毒40(SV40)的异源启动子在这些细胞中的功能很差。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0469/557728/763493814f01/emboj00315-0104-a.jpg

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