Uas arm s10

Fly culcture and crosses were performed according to standard procedures. Drosophila stocks used in this study include: UAS-Cut (#36496; Bloomington stock center (BDSC)); FRT19A, cut^C145 (#36496; BDSC); UAS-Wg-HA (#5918; BDSC); UAS-Arm-S10 (#4782; BDSC); UAS-cut-RNAi (#33967; BDSC); UAS-br-RNAi (#27272; BDSC); esg-Gal4, tubP-Gal80^ts, UAS-GFP (Biteau et al., 2008 (link); Micchelli and Perrimon, 2006 (link)); wg-Gal4 (Alexandre et al., 2014 (link)); wg(KO; NRT–Wg) (Alexandre et al., 2014 (link)); UAS-TCF-ΔN (#4785; BDSC); wg-lacZ (#1672; BDSC); Rab3-GFP (#62541; BDSC); UAS-CD8-RFP (#27392, BDSC); cut-intron2-Gal4 (#49818, BDSC); NRE-GFP (#30727; BDSC); UAS-Sgg.S9A (#5255; BDSC); UAS-EcR-DN (#6872; BDSC); UAS-wg-RNAi (#33902; BDSC); UAS-Br-Z1 (#51190; BDSC); UAS-Br-Z3 (#51192; BDSC); UAS-Br-Z4 (#51193; BDSC); FRT19A, dsh³ (#6331; BDSC); UAS-TCF (#4838; BDSC); UAS-Nipped-B-RNAi (#32406; BDSC); UAS-SA-RNAi (#33395; BDSC); UAS-Eip74EF-RNAi (#29353; BDSC); UAS-Eip75B (#26717; BDSC); UAS-white-RNAi (#33623; BDSC); Act5C-FRT>stop>FRT-lacZ.nls (#6355; BDSC).
wg-Gal4 transgenic flies were generated by integrating the Gal4 containing plasmid RIVGal4 (Baena-Lopez et al., 2013 (link)) into the attP site of wg flies (Alexandre et al., 2014 (link)).

Two ago RNAi lines, #31501 and #34802, were obtained from Bloomington Drosophila stock center (BDSC). The targeting regions for BDSC#31501 and #34802 are 2504-2913th and 5538-5558th nucleotide, respectively (Additional file: Fig. S1 a). Two ago overexpression fly lines used are: FlyORF library #F001828 and line generated with pUAS-myc-ago construct from our laboratory. To make pUAS-myc-ago, an ago cDNA clone (Drosophila Genomics Resource Center clone #LD30271) was sequenced and cloned into pUAST-myc.
All Gal4 lines were obtained from BDSC except ci-Gal4 (gift from R. A. Holmgren). wg-LacZ [37 (link)], tub-Gal80^ts (BDSC#7017), UAS-wg RNAi (NIG#4889R-3), UAS-arm^S10 (BDSC#4782), UAS-cyc E (BDSC#4781), UAS-dmyc (BDSC#9674), UAS-nuclear lacZ (BDSC#3955) and UAS-GFP (BDSC#1522) lines were also used. All cultures were carried out at either 18 °C or 25 °C. For conditional induction of Gal4, flies with tub-Gal80^ts were incubated at 18 °C until induction at 29 °C.