Ey flp

Drosophila lines were obtained from the Bloomington Drosophila Stock Center (BDSC) or the Vienna Drosophila RNAi Center (VDRC): UAS-Optix-RNAi (VDRC-KK110813), UAS-Dcr-2 (VDRC-60008), tsh[md621]-GAL4 (BDSC-3040), dpp[blk1]-GAL4 (BDSC-1553), UAS-Dcr-2; ey-FLP (BDSC-5580), UAS-GFP-nls (BDSC-4776), ato^5’EYE-GAL4 (Yu et al., 2015 (link)), the G-TRACE line UAS-FLP Ubi-p63E(FRT.STOP)Stinger (BDSC-28282; Evans et al., 2009 (link)) and Actin5C>y+>GAL4 (BDSC-3953); the latter two are referred to as UAS-FLP Ubi>IC>GFP and Act>IC>GAL4, respectively, in the text and figures (IC=interruption cassette). For reporter constructs, genomic DNA fragments were cloned into the vectors pCasper-β-gal (encoding cytoplasmic β-Galactosidase) or pStinger (encoding nuclear eGFP) (Pirrotta, 1988 (link); Barolo et al., 2000 ). Both vectors were first modified to contain a 1.1 kb fragment spanning the ato promoter region and 5’UTR (Sun et al., 1998 (link)). All constructs were confirmed by sequencing (data are available upon request) and injected into w CantonS for P-element transformation (Spradling and Rubin, 1982 (link)). All crosses for Fig. 4 were carried out at 30°C to enhance Optix gene silencing.