EMBRYONIC STEM-CELLS STABLY TRANSFECTED WITH MRAR-BETA-2-LACZ EXHIBIT SPECIFIC EXPRESSION IN CHIMERIC EMBRYOS

被引:0
作者
SHEN, S [1 ]
VANDENBRINK, CE [1 ]
KRUIJER, W [1 ]
VANDERSAAG, PT [1 ]
机构
[1] NETHERLANDS INST DEV BIOL,HUBRECHT LAB,UPPSALALAAN 8,3584 CT UTRECHT,NETHERLANDS
关键词
CHIMERIC EMBRYOS; EMBRYONIC STEM CELLS; MRAR-BETA-2-LACZ EXPRESSION; RETINOIC ACID;
D O I
暂无
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Using the embryonic stem (ES) cell/chimera approach, we have studied the activity of the mouse retinoic acid receptor beta2 (mRARbeta2) promoter during ES cell differentiation and during embryonic development. Stable ES clones were isolated after introduction of a 1.8 kb mRARbeta2-lacZ expression cassette. LacZ expression in these stable clones was specifically induced by retinoic acid (RA) in a similar fashion as the endogenous RARbeta2 gene Following introduction of three different ES clones into blastocysts, an integration-independent mRARbeta2-lacZ expression pattern was obtained in chimeric embryos similar to that described by in situ hybridization and transgenic studies. Moreover, mRARbeta2-lacZ expression was also detected at some additional sites not described before, e.g. body wall, ureter, mesonephric duct and optic stalk. Maternal RA administration at 8.5 days of pregnancy extended lacZ expression to more anterior and posterior regions. Transgenic mice were generated from germ-line transmission of the transfected ES cells; expression pattern and changes in expression upon RA induction in these transgenic embryos were identical to those in chimeric embryos. We conclude that by using the ES/chimera approach, the proximal 1.8 kb of the mRARbeta2 promoter produces a reliable and reproducible expression pattern of the reporter gene, and that the ES cell/chimera approach is invaluable for the study of gene expression and regulation.
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页码:465 / 476
页数:12
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