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Dynamic evolution of precise regulatory encodings creates the clustered site signature of enhancers

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  • Justin Crocker

    (Dartmouth College
    Present address: Howard Hughes Medical Institute and Department of Ecology and Evolutionary Biology, Princeton University, Princeton, New Jersey 08544, USA.)

  • Nathan Potter

    (Dartmouth College)

  • Albert Erives

    (Dartmouth College)

Abstract

Concentration gradients of morphogenic proteins pattern the embryonic axes of Drosophila by activating different genes at different concentrations. The neurogenic ectoderm enhancers (NEEs) activate different genes at different threshold levels of the Dorsal (Dl) morphogen, which patterns the dorsal/ventral axis. NEEs share a unique arrangement of highly constrained DNA-binding sites for Dl, Twist (Twi), Snail (Sna) and Suppressor of Hairless (Su(H)), and encode the threshold variable in the precise length of DNA that separates one well-defined Dl element from a Twi element. However, NEEs also possess dense clusters of variant Dl sites. Here, we show that these increasingly variant sites are eclipsed relic elements, which were superseded by more recently evolved threshold encodings. Given the divergence in egg size during Drosophila lineage evolution, the observed characteristic clusters of divergent sites indicate a history of frequent selection for changes in threshold responses to the Dl morphogen gradient and confirm the NEE structure/function model.

Suggested Citation

  • Justin Crocker & Nathan Potter & Albert Erives, 2010. "Dynamic evolution of precise regulatory encodings creates the clustered site signature of enhancers," Nature Communications, Nature, vol. 1(1), pages 1-9, December.
  • Handle: RePEc:nat:natcom:v:1:y:2010:i:1:d:10.1038_ncomms1102
    DOI: 10.1038/ncomms1102
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