首页> 美国卫生研究院文献>Journal of Virology >In vitro transactivation of baculovirus early genes by nuclear extracts from Autographa californica nuclear polyhedrosis virus-infected Spodoptera frugiperda cells.
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In vitro transactivation of baculovirus early genes by nuclear extracts from Autographa californica nuclear polyhedrosis virus-infected Spodoptera frugiperda cells.

机译:杆状病毒原核多角体病毒感染的斜纹夜蛾细胞核提取物对杆状病毒早期基因的体外反式激活。

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摘要

Nuclear extracts, prepared from Autographa californica nuclear polyhedrosis virus-infected Spodoptera frugiperda cells during a time course of infection, were analyzed for activation of early gene transcription and for late gene transcription. The templates used in the in vitro transcription assays contained promoters for baculovirus genes that have been classified as immediate early, delayed early, and late. The promoters were derived from the baculovirus 39K, p26, gp64, and DNA polymerase genes. In addition, the adenovirus major late promoter was included in these studies. We found that transcription from promoters classified as immediate early or delayed early was accurately initiated by using extracts from uninfected cells. Furthermore, transcription from all early promoters tested was found to be transactivated by nuclear extracts prepared at 4 and 8 h postinfection. However, baculovirus enhancer-dependent transcriptional activation was not observed in tests with templates containing the hr5 enhancer sequence. Transcription from baculovirus late promoters was also not observed. A decline in transcription by nuclear extracts prepared from cells late in infection was associated with the presence of DNase activity.
机译:分析了在感染的一段时间过程中,从加州白粉虱核多角体病毒感染的斜纹夜蛾细胞中制备的核提取物的早期基因转录激活和晚期基因转录。体外转录测定中使用的模板包含杆状病毒基因的启动子,这些启动子已被分类为立即早期,延迟早期和晚期。启动子来自杆状病毒39K,p26,gp64和DNA聚合酶基因。此外,这些研究还包括腺病毒主要的晚期启动子。我们发现,通过使用未感染细胞的提取物可以准确地启动分类为立即早期或延迟早期的启动子的转录。此外,发现所有被测试的早期启动子的转录都被感染后4和8 h制备的核提取物反式激活。但是,在含有hr5增强子序列的模板的测试中未观察到杆状病毒增强子依赖性转录激活。也未观察到杆状病毒晚期启动子的转录。从感染后期的细胞制备的核提取物的转录下降与DNase活性的存在有关。

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