Pomerantz B J, Mueller C R, Hassell J A
J Virol. 1983 Sep;47(3):600-10. doi: 10.1128/JVI.47.3.600-610.1983.
To map the polyomavirus large T antigen binding sites on the viral genome we employed a quantitative immunoassay. Defined, radiolabeled fragments of the viral genome were reacted with crude nuclear extracts prepared from lytically infected mouse 3T6 cells, and the fragments bound by large T antigen were immunoprecipitated with anti-T serum and Formalin-fixed Staphylococcus aureus. The immunoprecipitated DNA was then analyzed by gel electrophoresis and autoradiography. By the use of a variety of restriction endonuclease-generated fragments of wild-type and mutant viral DNAs, the region of high-affinity binding was localized to a 153-base-pair stretch between nucleotides 5292 and 152. At least two independent binding sites lie within this region, one upstream and the other downstream of the Bg/I site at nucleotide 87. One of the binding sites is located within sequences required in cis for DNA replication; the other overlaps the TATA box and cap sites of the early transcription unit. The two sites share a common sequence, A/TGAGGC-N4/5-A/TGAGGC, which may serve as the recognition sequence for large T antigen.
为了绘制多瘤病毒大T抗原在病毒基因组上的结合位点图谱,我们采用了一种定量免疫测定法。将确定的、经放射性标记的病毒基因组片段与从经裂解感染的小鼠3T6细胞制备的粗核提取物反应,然后用抗T血清和福尔马林固定的金黄色葡萄球菌对被大T抗原结合的片段进行免疫沉淀。接着,通过凝胶电泳和放射自显影分析免疫沉淀的DNA。利用野生型和突变型病毒DNA的多种限制性内切酶产生的片段,高亲和力结合区域被定位在核苷酸第5292位和152位之间的一段153个碱基对的序列上。该区域内至少有两个独立的结合位点,一个在核苷酸第87位的Bg/I位点上游,另一个在其下游。其中一个结合位点位于DNA复制所需的顺式作用序列内;另一个与早期转录单元的TATA盒和帽位点重叠。这两个位点共有一个共同序列,即A/TGAGGC-N4/5-A/TGAGGC,它可能是大T抗原的识别序列。
