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Fig. 2. Parasegment-specific activation and repression of slp1 by Runt. (A) Wild-type slp1 expression in a gastrula stage embryo as visualized by in situ hybridization. (B) The phasing of slp1 expression relative to the expression of different pair-rule transcription factors. A strip of cells along the anteroposterior axis is depicted across the bottom with slp1-expressing cells indicated by shading. The higher expression level of the even-numbered stripes is indicated by darker shading. The four-cell wide Runt stripes are depicted above this strip as a trapezoid, reflecting the higher expression levels in the center of the stripes. By contrast, Eve and Ftz stripes are depicted as triangles with peak expression in the most anterior cells, whereas the uniform expression of Opa is depicted as a broad rectangle that spans the presegmental region. The regulatory circuitry responsible for generating the slp1 pattern is also depicted. Activation by Runt + Opa is indicated with an arrowhead, whereas repression by either Eve, or the combination of Runt + Ftz, is indicated with a horizontal bar. (C) Transient elimination of runt activity in an embryo hemizygous for the temperature-sensitive runt[YP17] mutation leads to loss of odd-numbered slp1 stripes and expansion of some of the even-numbered stripes. These changes are interpreted to be due to loss of Runt-dependent activation and repression as indicated in D. (E) Double in situ hybridization showing the complementary expression of slp1 (blue) and ftz (brown) mRNAs in embryos with a high-level of NGT-driven Runt. This embryo was obtained by crossing homozygous NGT40 females with homozygous UAS-runt[232] males. As indicated in F, slp1 expression in these embryos fills the presumptive odd-numbered parasegments and is repressed throughout the even-numbered parasegments.





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