Kern F G, Dailey L, Basilico C
Mol Cell Biol. 1985 Aug;5(8):2070-9. doi: 10.1128/mcb.5.8.2070-2079.1985.
In a previous report we showed that transcripts initiating from the late promoter of integrated polyoma plasmids could be detected at significant levels when neomycin resistance (neo) coding sequences were linked to this promoter. In this report we used chimeric plasmids that contain either a limited portion of the polyoma genome or deletions within the polyoma noncoding regulatory region to determine the sequence requirements for late promoter activity in this system. We observed no absolute requirement for either the polyoma early coding region or the origin of DNA replication for Neo-r colony formation. We were therefore able to independently assess the effects of deletions in the polyoma enhancer region on gene activity in both the early and late directions. We measured the ability of cells transfected with plasmids containing deletions in this region to form colonies in either semisolid or G418-containing medium under nonreplicative conditions. Our results indicate that either the PvuII 4 fragment, which contains the simian virus 40 core enhancer sequence, or a region from nucleotides 5099 to 5142, which contains the adenovirus type 5 E1A core enhancer sequence, can be deleted without significantly affecting gene expression in either direction. However, a deletion of nucleotides 5099 to 5172 reduced activities to similar extents in both directions, and a plasmid containing a larger deletion of nucleotides 5055 to 5182 showed a further reduction in activity. Although having no effect by itself, a second origin region deletion of nucleotides 5246 to 127 when present in these mutant backgrounds caused either a further reduction or elimination, respectively, of both G418 and agar colony-forming ability, suggesting the presence of an additional common regulatory element within this region. A comparison of 5' ends of neo transcripts present in cells transformed by these plasmids suggested that the reduction in activity was due to deletion of regulatory rather than structural elements of the late promoter. Our results indicate that the noncoding region of polyoma contains multiple complementing regulatory elements that control the level of both early and late gene expression.
在之前的一份报告中我们表明,当新霉素抗性(neo)编码序列与该启动子相连时,可从整合多瘤病毒质粒的晚期启动子起始的转录本能够以显著水平被检测到。在本报告中,我们使用了嵌合质粒,这些质粒要么包含多瘤病毒基因组的有限部分,要么在多瘤病毒非编码调控区域内有缺失,以确定该系统中晚期启动子活性的序列要求。我们观察到,对于新霉素抗性克隆形成,多瘤病毒早期编码区或DNA复制起点均无绝对要求。因此,我们能够独立评估多瘤病毒增强子区域缺失对早期和晚期方向基因活性的影响。我们测量了用在该区域有缺失的质粒转染的细胞在非复制条件下于半固体或含G418的培养基中形成菌落的能力。我们的结果表明,要么包含猿猴病毒40核心增强子序列的PvuII 4片段,要么包含腺病毒5型E1A核心增强子序列的核苷酸5099至5142区域,可以被缺失而不会显著影响任一方向的基因表达。然而,核苷酸5099至5172的缺失在两个方向上均使活性降低到相似程度,并且包含更大缺失(核苷酸5055至5182)的质粒显示活性进一步降低。尽管自身无影响,但当存在于这些突变背景中时,第二个核苷酸5246至127的起始区域缺失分别导致G418和琼脂菌落形成能力进一步降低或消除,这表明该区域内存在额外的共同调控元件。对由这些质粒转化的细胞中存在的neo转录本5'端的比较表明,活性降低是由于晚期启动子调控元件而非结构元件的缺失。我们的结果表明,多瘤病毒的非编码区域包含多个互补的调控元件,这些元件控制早期和晚期基因表达的水平。
