Gorman C M, Moffat L F, Howard B H
Mol Cell Biol. 1982 Sep;2(9):1044-51. doi: 10.1128/mcb.2.9.1044-1051.1982.
We constructed a series of recombinant genomes which directed expression of the enzyme chloramphenicol acetyltransferase (CAT) in mammalian cells. The prototype recombinant in this series, pSV2-cat, consisted of the beta-lactamase gene and origin of replication from pBR322 coupled to a simian virus 40 (SV40) early transcription region into which CAT coding sequences were inserted. Readily measured levels of CAT accumulated within 48 h after the introduction of pSV2-cat DNA into African green monkey kidney CV-1 cells. Because endogenous CAT activity is not present in CV-1 or other mammalian cells, and because rapid, sensitive assays for CAT activity are available, these recombinants provided a uniquely convenient system for monitoring the expression of foreign DNAs in tissue culture cells. To demonstrate the usefulness of this system, we constructed derivatives of pSV2-cat from which part or all of the SV40 promoter region was removed. Deletion of one copy of the 72-base-pair repeat sequence in the SV40 promoter caused no significant decrease in CAT synthesis in monkey kidney CV-1 cells; however, an additional deletion of 50 base pairs from the second copy of the repeats reduced CAT synthesis to 11% of its level in the wild type. We also constructed a recombinant, pSV0-cat, in which the entire SV40 promoter region was removed and a unique HindIII site was substituted for the insertion of other promoter sequences.
我们构建了一系列重组基因组,这些基因组可在哺乳动物细胞中指导氯霉素乙酰转移酶(CAT)的表达。该系列中的原型重组体pSV2-cat由来自pBR322的β-内酰胺酶基因和复制起点与猿猴病毒40(SV40)早期转录区域相连组成,CAT编码序列插入其中。将pSV2-cat DNA导入非洲绿猴肾CV-1细胞后,在48小时内即可检测到CAT水平的积累。由于CV-1细胞或其他哺乳动物细胞中不存在内源性CAT活性,且有快速、灵敏的CAT活性检测方法,这些重组体为监测组织培养细胞中外源DNA的表达提供了一个极为便利的系统。为证明该系统的实用性,我们构建了pSV2-cat的衍生物,其中部分或全部SV40启动子区域被去除。在SV40启动子中删除一个72碱基对重复序列拷贝,对猴肾CV-1细胞中CAT的合成没有显著影响;然而,从第二个重复拷贝中再删除50个碱基对,使CAT的合成降至野生型水平的11%。我们还构建了一个重组体pSV0-cat,其中整个SV40启动子区域被去除,并用一个独特的HindIII位点替代,用于插入其他启动子序列。
