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非洲猪瘟病毒DNA的分子克隆

Molecular cloning of African swine fever virus DNA.

作者信息

Ley V, Almendral J M, Carbonero P, Beloso A, Viñuela E, Talavera A

出版信息

Virology. 1984 Mar;133(2):249-57. doi: 10.1016/0042-6822(84)90392-1.

Abstract

African swine fever virus DNA (about 170 kbp) was cleaved with the restriction endonuclease EcoRI and most of the resulting 31 fragments were cloned in either the phage vector lambda WES lambda B or the plasmid pBR325. Three fragments were not cloned in those vectors, the largest fragment EcoRI-A (21.2 kbp) and the two crosslinked terminal fragments, EcoRI-K' and D'. Endonuclease SalI cut fragment EcoRI-A into three pieces which were cloned in plasmid pBR322. The two terminal EcoRI fragments were cloned after removal of the crosslinks with nuclease S1 and addition of EcoRI linkers to the fragment ends. The complete library of the cloned fragments accounted for about 98% of ASF virus genome, the missing sequences being those removed by the nuclease S1 in the process of cloning the terminal fragments.

摘要

非洲猪瘟病毒DNA(约170千碱基对)用限制性内切酶EcoRI切割,产生的31个片段中的大多数被克隆到噬菌体载体λWESλB或质粒pBR325中。有三个片段未克隆到这些载体中,即最大的片段EcoRI-A(21.2千碱基对)以及两个交联的末端片段EcoRI-K'和D'。内切酶SalI将片段EcoRI-A切成三段,这些片段被克隆到质粒pBR322中。在用核酸酶S1去除交联并在片段末端添加EcoRI接头后,将两个末端EcoRI片段进行克隆。克隆片段的完整文库约占非洲猪瘟病毒基因组的98%,缺失的序列是在克隆末端片段过程中被核酸酶S1去除的那些序列。

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