Validation of novel promoter sequences derived from two endogenous ubiquitin genes in transgenic Aedes aegypti

被引:76
作者
Anderson, M. A. E.
Gross, T. L.
Myles, K. M.
Adelman, Z. N.
机构
[1] Virginia Polytech Inst & State Univ, Fralin Life Sci Inst, Blacksburg, VA 24061 USA
[2] Virginia Polytech Inst & State Univ, Dept Entomol, Blacksburg, VA 24061 USA
关键词
Aedes; promoter; mosquito; ubiquitin; transgenic; YELLOW-FEVER MOSQUITO; DENGUE VIRUS TYPE-2; DROSOPHILA-MELANOGASTER; TRANSPOSON VECTOR; EXPRESSION; TRANSFORMATION; MARKER; EFFICIENT; EXCISION; PATHWAY;
D O I
10.1111/j.1365-2583.2010.01005.x
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
To date, only a limited number of promoter sequences have been described to drive transgene expression in the disease vector Aedes aegypti. We sought to increase this repertoire by characterizing the ability of upstream sequences derived from the Ae. aegypti Ub(L40) and polyubiquitin genes to drive the expression of marker proteins. Both genomic fragments were able to drive robust expression of luciferase in cultured mosquito cells. Following Mos1-transformation, the Ub(L40) promoter drove strong expression of a fluorescent marker in early larvae and in ovaries, while the polyubiquitin promoter drove robust EGFP expression in all stages of development, including constitutive expression throughout the midgut. These promoter fragments provide two new expression profiles for future Ae. aegypti genetic experiments.
引用
收藏
页码:441 / 449
页数:9
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