Functional analysis of eve stripe 2 enhancer evolution in Drosophila: rules governing conservation and change.

@article{citeulike:972650, abstract = {Experimental investigations of eukaryotic enhancers suggest that multiple binding sites and trans-acting regulatory factors are often required for wild-type enhancer function. Genetic analysis of the stripe 2 enhancer of even-skipped (eve), an important developmental gene in Drosophila, provides support for this view. Given the importance of even-skipped expression in early Drosophila development, it might be predicted that many structural features of the stripe 2 enhancer will be evolutionarily conserved, including the DNA sequences of protein binding sites and the spacing between them. To test this hypothesis, we compared sequences of the stripe 2 enhancer between four species of Drosophila: D. melanogaster, D. yakuba, D. erecta and D. pseudoobscura. Our analysis revealed a large number of nucleotide substitutions in regulatory protein binding sites for bicoid, hunchback, Kruppel and giant, as well as a systematic change in the size of the enhancer. Some of the binding sites in D. melanogaster are either absent or modified in other species. One functionally important bicoid-binding site in D. melanogaster appears to be recently evolved. We, therefore, investigated possible functional consequences of sequence differences among these stripe 2 enhancers by P-element-mediated transformation. This analysis revealed that the eve stripe 2 enhancer from each of the four species drove reporter gene expression at the identical time and location in D. melanogaster embryos. Double staining of native eve protein and transgene mRNA in early embryos showed that the reporter gene mimicked native eve expression and, in every case, produced sharply defined stripes at the blastoderm stage that were coincident with eve stripe 2 protein. We argue that stripe 2 eve expression in Drosophila evolution can be viewed as being under constant stabilizing selection with respect to the location of the anterior and posterior borders of the stripe. We further hypothesize that the stripe 2 enhancer is functionally robust, so that its evolution may be governed by the fixation of both slightly deleterious and adaptive mutations in regulatory protein binding sites as well as in the spacing between binding sites. This view allows for a slow but continual turnover of functionally important changes in the stripe 2 enhancer.}, address = {Department of Ecology and Evolution, University of Chicago, Chicago, IL 60637, USA. mludwig@midway.uchicago.edu}, author = {Ludwig, M. Z. and Patel, N. H. and Kreitman, M. }, citeulike-article-id = {972650}, issn = {0950-1991}, journal = {Development}, keywords = {cis\_regulatory\_evolution, drosophila, even-skipped\_enhancer, function\_study}, month = {March}, number = {5}, pages = {949--958}, posted-at = {2008-04-22 15:58:26}, priority = {2}, title = {Functional analysis of eve stripe 2 enhancer evolution in Drosophila: rules governing conservation and change.}, url = {http://view.ncbi.nlm.nih.gov/pubmed/9449677}, volume = {125}, year = {1998} }

TY - JOUR ID - citeulike:972650 L3 - citeulike-article-id:972650 TI - Functional analysis of eve stripe 2 enhancer evolution in Drosophila: rules governing conservation and change. JF - Development VL - 125 IS - 5 SP - 949 EP - 958 AD - Department of Ecology and Evolution, University of Chicago, Chicago, IL 60637, USA. mludwig@midway.uchicago.edu SN - 0950-1991 N2 - Experimental investigations of eukaryotic enhancers suggest that multiple binding sites and trans-acting regulatory factors are often required for wild-type enhancer function. Genetic analysis of the stripe 2 enhancer of even-skipped (eve), an important developmental gene in Drosophila, provides support for this view. Given the importance of even-skipped expression in early Drosophila development, it might be predicted that many structural features of the stripe 2 enhancer will be evolutionarily conserved, including the DNA sequences of protein binding sites and the spacing between them. To test this hypothesis, we compared sequences of the stripe 2 enhancer between four species of Drosophila: D. melanogaster, D. yakuba, D. erecta and D. pseudoobscura. Our analysis revealed a large number of nucleotide substitutions in regulatory protein binding sites for bicoid, hunchback, Kruppel and giant, as well as a systematic change in the size of the enhancer. Some of the binding sites in D. melanogaster are either absent or modified in other species. One functionally important bicoid-binding site in D. melanogaster appears to be recently evolved. We, therefore, investigated possible functional consequences of sequence differences among these stripe 2 enhancers by P-element-mediated transformation. This analysis revealed that the eve stripe 2 enhancer from each of the four species drove reporter gene expression at the identical time and location in D. melanogaster embryos. Double staining of native eve protein and transgene mRNA in early embryos showed that the reporter gene mimicked native eve expression and, in every case, produced sharply defined stripes at the blastoderm stage that were coincident with eve stripe 2 protein. We argue that stripe 2 eve expression in Drosophila evolution can be viewed as being under constant stabilizing selection with respect to the location of the anterior and posterior borders of the stripe. We further hypothesize that the stripe 2 enhancer is functionally robust, so that its evolution may be governed by the fixation of both slightly deleterious and adaptive mutations in regulatory protein binding sites as well as in the spacing between binding sites. This view allows for a slow but continual turnover of functionally important changes in the stripe 2 enhancer. KW - cis_regulatory_evolution KW - drosophila KW - even-skipped_enhancer KW - function_study AU - Ludwig, MZ AU - Patel, NH AU - Kreitman, M PY - 1998/03// UR - http://view.ncbi.nlm.nih.gov/pubmed/9449677 ER -