Carmichael G G, Schaffhausen B S, Dorsky D I, Oliver D B, Benjamin T L
Proc Natl Acad Sci U S A. 1982 Jun;79(11):3579-83. doi: 10.1073/pnas.79.11.3579.
We have constructed a transformation-defective polyoma virus mutant (Py 1387-T) that directs the synthesis of a normal small tumor antigen, a functional large tumor antigen, and a truncated (51,000-dalton) middle-sized tumor (mT) antigen that lacks 37 amino acids at its COOH terminus. The shortened mT polypeptide is missing the hydrophobic "tail" thought to be responsible for the anchorage of this protein into the plasma membrane and is in fact in cytosol fractions. This truncated mT polypeptide is inactive in an in vitro protein kinase assay and is altered in its phosphorylation in vivo. Mutant 1387-T differs from wild-type virus in having a T.A base pair instead of a C.G base at nucleotide position 1387. This change was introduced into viral DNA by using a synthetic undecanucleotide as a specific mutagen. Wild-type polyoma DNA was rendered single stranded by molecular cloning into coliphage M13. The oligonucleotide, which hybridizes with a mismatch at the site to be altered, was used to prime the synthesis of double-stranded closed circular DNA. Progeny recombinant phage were screened by DNA sequence analysis for the desired base change. The polyoma mutant was reconstructed from recombinant phage replicative form DNA molecules containing the mutation.
我们构建了一种转化缺陷型多瘤病毒突变体(Py 1387-T),它能指导合成正常的小肿瘤抗原、功能性大肿瘤抗原以及一种截短的(51,000道尔顿)中等大小肿瘤(mT)抗原,该抗原在其COOH末端缺少37个氨基酸。缩短的mT多肽缺少被认为负责将该蛋白锚定到质膜中的疏水“尾巴”,实际上存在于胞质溶胶组分中。这种截短的mT多肽在体外蛋白激酶测定中无活性,并且在体内其磷酸化发生了改变。突变体1387-T与野生型病毒的不同之处在于,在核苷酸位置1387处有一个T.A碱基对而非C.G碱基。通过使用合成的十一核苷酸作为特异性诱变剂,将这种变化引入病毒DNA中。野生型多瘤DNA通过分子克隆到大肠杆菌噬菌体M13中而变成单链。与待改变位点存在错配杂交的寡核苷酸用于引发双链闭环DNA的合成。通过DNA序列分析筛选子代重组噬菌体,以寻找所需的碱基变化。从含有该突变的重组噬菌体复制形式DNA分子中重建多瘤突变体。
