CONSTRUCTION AND EXPRESSION OF PLASMIDS CONTAINING MUTATED DIPHTHERIA-TOXIN A-CHAIN-CODING SEQUENCES

被引:2
作者
FISHER, KS
MAXWELL, IH
MURPHY, JR
COLLIER, J
GLODE, LM
机构
[1] UNIV COLORADO,CTR CANC,DEPT MED,DIV MED ONCOL,DENVER,CO 80262
[2] HARVARD UNIV,SCH MED,DEPT MICROBIOL & MOLEC GENET,BOSTON,MA 02115
[3] SHIPLEY INST MED,BOSTON,MA 02115
[4] UNIV COLORADO,CTR CANC,DEPT PREVENT MED & BIOMET,DENVER,CO 80262
关键词
D O I
10.1128/IAI.59.10.3562-3565.1991
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
We previously demonstrated that cells can be killed through transfection of an expression plasmid that encodes the diphtheria toxin A-chain fragment (DT-A). This report describes the construction of expression plasmids containing three mutant DT-A-coding sequences substituting glutamic acid 148 with aspartic acid, serine, or glutamine which are known to have 100- to 300-fold-reduced ADP-ribosylation activity measured in vitro. The toxicity of these constructs was determined in cotransfection experiments using HeLa and 293 cells with a luciferase expression plasmid as the reporter. Dose responses were compared for the three new DT-A mutant plasmids and for the corresponding plasmids containing wild-type DT-A and the previously characterized tox 176 mutant. The dose required to produce 50% inhibition of control luciferase expression in 293 embryonic kidney cells for the five plasmids ranged from 0.01-mu-g for wild-type DT-A to 1.2-mu-g for the least toxic plasmid, which replaces glutamic acid 148 with glutamine. In conclusion, a wide range of DT-A toxicity can be achieved by using plasmid expression vectors that encode different DT-A mutations.
引用
收藏
页码:3562 / 3565
页数:4
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