Assuming that BunA and Madm interact, they should at least partially co-localize. Immunofluorescence studies in S2 cells revealed that GFP-BunA and HA-Madm signals in fact largely overlapped (Figure 2b, c). Interestingly, the HA-Madm signal was less dispersed when GFP-BunA was expressed in the same cell, indicating that the interaction with BunA altered the subcellular localization of HA-Madm (Figure ​(Figure2c).2c). A statistical analysis (Materials and methods) revealed that HA-Madm was only localized in punctae when co-overexpressed with GFP-BunA (100%, n = 50) but not when co-overexpressed with GFP (0%, n = 50). Moreover, when a mutated HA-Madm protein (R525H, see below) was expressed, the localization in punctae was lost in 66% of cells co-overexpressing GFP-BunA (n = 50). The GFP-BunA signal largely overlapped with the Golgi marker GMAP210 [38] but not with an endoplasmic reticulum (ER) marker (Figure ​(Figure2d,2d, and data not shown), indicating that GFP-BunA localizes to the Golgi. The localization of BunA and Madm was not dependent on their tag because GFP- and HA-tagged BunA and Madm behaved similarly (data not shown). Furthermore, GFP-tagged BunA and Madm proteins were functional because they rescued the lethality of bun and Madm mutants, respectively, when expressed in the fly (Materials and methods). Taken together, our AP-MS and co-localization studies demonstrate that the adapter molecule Madm associates with BunA.

As a second measurement of the strength of the Madm alleles, the severity of the pinhead phenotypes was judged. Consistent with the first assay, alleles 2D2, 2U3, and 3G5 produced the most severe pinhead phenotypes (Figure ​(Figure3c);3c); alleles 3Y2, 4S3, and 7L2 displayed pinhead phenotypes of intermediate strength (Figure ​(Figure3b);3b); and allele 3T4 led to a very mild reduction in head and eye size in the eyFLP/FRT assay (data not shown).

Thus, Madm controls cell number and cell size and also controls patterning processes in the eye and the wing. These phenotypes strongly resemble phenotypes displayed by bunA mutant cells and flies [12] [see Additional file 5 for wing notches], although the pinhead phenotype and the eye-patterning defects caused by the strong Madm alleles 2D2 and 3G5 are more severe.

In mammalian cells, both IP/MS and Y2H experiments provided evidence for a physical interaction between Madm and TSC22DF proteins [42,43]. Our study extends these findings in two ways. We demonstrate that only long TSC22DF proteins directly bind to Madm, and we also provide evidence for the biological significance of this interaction in growth control.

Madm is an adapter molecule that has several interaction partners in mammals. Originally, it was proposed that Madm - also named nuclear receptor binding protein 1 (NRBP1) in humans - binds to nuclear receptors because of the presence of two putative nuclear-receptor-binding motifs [39]. However, Madm has never been experimentally shown to bind to any nuclear receptor. Furthermore, the nuclear-receptor-binding motifs are not conserved in Drosophila. From studies in mammalian cells, it is known that Madm can bind to murine Mlf1 [40], Jab1 (Jun activation domain-binding protein 1) [50], activated Rac3 (Ras-related C3 botulinum toxin substrate 3) [47], Elongin B [51], and the host cellular protein NS3 of dengue virus type 2 [52]. Indeed, in our AP-MS experiment where HA-Madm was used as bait, we identified Elongin B but not Mlf1 (dMlf in Drosophila), Jab1 (CSN5 in Drosophila) or Rac3 (RhoL in Drosophila). It is possible that these interactions are not very prominent or even absent in Drosophila S2 cells.

Madm cDNA was cleaved by EcoRI and HindIII double digestion from expressed sequence tag (EST) clone LD28567 (Berkeley Drosophila Genome Project) and subcloned into pUAST using the same restriction sites to generate the UAS-Madm construct. Madm genomic DNA (from 559 bp upstream of Madm exon 1 (containing exon 1 of the neighboring gene CG2097) to 1,681 bp downstream of Madm exon 2) was amplified by PCR using forward primer GCTCTAGAAGGCGATGCGATGACCAGCTC and reverse primer GAGATCTTC-ATGACGTTTTCCGCGCACTCGAGT. The PCR product was digested with BglII and XbaI and subcloned into the transformation vector pCaspeR.

Nanoflow-LC-MS/MS was performed by coupling an UltiMate HPLC system (LC-Packings/Dionex) in-line with a Probot (LC-Packings/Dionex) autosampler system and an LTQ ion trap (Thermo Electron). Samples were automatically injected into a 10-μl sample-loop and loaded onto an analytical column (9 cm × 75 μm; packed with Magic C18 AQ beads 5 μm, 100 Å (Michrom BioResources)). Peptide mixtures were delivered to the analytical column at a flow rate of 300 nl/minute of buffer A (5% acetonitrile, 0.2% formic acid) for 25 minutes and then eluted using a gradient of acetonitrile (10-45%; 0.5%/minutes) in 0.2% formic acid. Peptide ions were detected in a survey scan from 400 to 2,000 atomic mass units (amu; one to two μscans) followed by three to six data-dependent MS/MS scans (three μscans each, isolation width 2 amu, dynamic exclusion list 250, dynamic exclusion time 240 sec, two repeats) in an automated fashion. Following analysis, raw MS/MS data were converted to Mascot generic format (MGF) files that were used to identify the corresponding peptides using the Mascot database search tool (MatrixScience) [59,60]. MS/MS spectra were searched against the Drosophila protein database (dmel_r5.18_FB2009_05 released 20090529) [60] with the following criteria: requirement for trypsin digestion; peptide mass tolerance 2 Da; fragment mass tolerance 0.6 Da; missed cleavage for trypsin 3; fixed modification carbamidomethyl (C); variable modifications acetyl (N-term), oxidation (M), CAM-thiopropanoyl (K) (derived from DSP crosslinker). All peptide assignments with Mascot ion score larger than the homology score and with Mascot expect score smaller than 0.05 (significant ion score) were considered as good hits.

Statistical analysis of the dependence of HA-Madm localization on GFP-BunA was carried out in S2 cells transiently transfected two days before analysis. Cells were co-transfected with pMT-HA-Madm or pMT-HA-Madm(R525H) and with either empty pMT-GW-Blast (for control GFP expression) or with pMT-GFP-bunA. Fifty cells were analyzed for each combination. The expressed HA-Madm and HA-Madm(R525H) proteins showed a similar diffuse localization in the cytoplasm of cells strongly expressing GFP (50 out of 50 each). By contrast, HA-Madm localized to dots (punctae) in cells displaying a readily detectable GFP-BunA signal (50 out of 50). In 17 out of 50 cells, GFP-BunA directed HA-Madm(R525H) localization in punctae.

The rabbit anti-BunA antibody was generated using the following peptide to immunize rabbits: H₂N-TNRKPKTTSSFEC-CONH₂ (Eurogentec). The serum was double-affinity purified against the peptide coupled to a column. Specificity of the antibody was shown by western blotting: Drosophila S2 cells were incubated for 2 days with dsRNA [61] that targets either the ORF of bunA (500 bp long dsRNA) or of GFP as a control (700 bp long dsRNA). Primer sequences are available on request.

The UAS/Gal4 system [34] was used to test whether ubiquitous expression of a UAS-Madm construct during development - achieved by the arm-Gal4, da-Gal4, and Act5C-Gal4 driver lines - rescued the recessive lethality of the EMS alleles. Using arm-Gal4, the viability of combinations of EMS alleles (2U3, 3G5, 3Y2, and 7L2) with the deletion Df(3R)Exel7283 was completely restored and the lethality of heteroallelic combinations among EMS alleles was partially rescued. One copy of genomic Madm rescue construct (LCQ139) - comprising 559 bp of the upstream region, the two Madm exons and the intron, and 1,681 bp of downstream sequences - was sufficient to entirely rescue the lethality of heteroallelic combinations of EMS alleles (2U3 and 3G5) and of the hemizygous alleles (tested with the deficiency Df(3R)Exel7283). In addition, the pinhead phenotypes of the EMS alleles 2U3 and 3G5 were reverted by one copy of the genomic construct.