Shoemaker C, Goff S, Gilboa E, Paskind M, Mitra S W, Baltimore D
Proc Natl Acad Sci U S A. 1980 Jul;77(7):3932-6. doi: 10.1073/pnas.77.7.3932.
Closed circular Moloney murine leukemia virus (M-MuLV) DNA was prepared from recently infected cells and cloned in a lambda vector. Four classes of cloned M-MuLV inserts were found: Class I, full length 8.8-kilobase (kb) inserts with two tandem long terminal repeats (LTRs) of 600 base pairs; class 2, 8.2-kb inserts with a single copy of a LTR; class 3, M-MuLV DNA inserts with various portions deleted; and class 4, an 8.8-kb insert with an internal sequence inversion. Determination of nucleotide sequence at the junction between the two LTRs from a class 1 insert suggested that circularization occurred by blunt-end ligation of an 8.8-kb linear DNA. The class 4 molecule had an inversion that was flanked by inverted LTRs, each of which had lost two terminal base pairs at the inversion end points. Also, four base pairs that were present only once in standard M-MuLV DNA were duplicated at either end of the inversion. This molecule was interpreted as resulting from an integrative inversion in which M-MuLV DNA has integrated into itself. Its analysis thus provided explicit information concerning the mechanism by which retrovirus DNA integrates into host cell DNA. Models of retrovirus integration based on bacterial DNA transposition mechanisms are proposed.
闭合环状莫洛尼鼠白血病病毒(M-MuLV)DNA是从近期感染的细胞中制备的,并克隆到λ载体中。发现了四类克隆的M-MuLV插入片段:I类,全长8.8千碱基(kb)的插入片段,带有两个600个碱基对的串联长末端重复序列(LTR);II类,8.2-kb的插入片段,带有单个LTR拷贝;III类,缺失不同部分的M-MuLV DNA插入片段;IV类,一个8.8-kb的插入片段,其内部序列发生了倒位。对I类插入片段中两个LTR之间连接处的核苷酸序列测定表明,环化是由一个8.8-kb线性DNA的平端连接产生的。IV类分子的倒位两侧是反向LTR,每个LTR在倒位端点处都丢失了两个末端碱基对。此外,在标准M-MuLV DNA中仅出现一次的四个碱基对在倒位的两端都发生了重复。该分子被解释为是由M-MuLV DNA整合到自身中的整合性倒位产生的。因此,对其分析提供了有关逆转录病毒DNA整合到宿主细胞DNA中的机制的明确信息。提出了基于细菌DNA转座机制的逆转录病毒整合模型。
