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	Figure 3. Expression of OSR1 and Osr2A leads to an increase of pronephros size in Xenopus laevis larvae. (A) Enlargement of pronephros: Dorsal view of stage 45 larvae [36] injected with 200 pg OSR1 mRNA and whole-mount immunostained with antibodies 3G8 and 4A6 [37]. The injected side is marked by an arrow. Bar = 200 μm (B) Ectopic kidney cell patches (marked by arrow heads): Lateral view of a stage 45 larvae [36] expressing OSR1 and prepared as in A. Bar = 200 μm (C) Pronephros size on injected versus control side in OSR1 or Osr2A injected embryos was determined in lateral views by measuring the area through the widest part of the immunostained pronephros. The Student's t-test was used to score significant differences. The p-value is given by comparing embryos injected with gene of interest plus GFP mRNA as marker with those injected with GFP mRNA taken from previous data [23]. *** denotes p-value ≤ 0.001. The vertical line in the middle represents the mean and the small bars the standard deviation. N is the number of animals investigated.
	Figure 4. Expression of human OSR1 in animal caps. Animal caps derived from embryos injected with OSR1 mRNA were cultured in Steinberg's solution, retinoic acid (RA, 10-4M) and/or activin A (ActA, 10 ng/ml) as indicated. To avoid a too high lethality only 150 pg mRNA was injected. (A) Classification of whole-mount immunostained animal caps used for the analysis of pronephric tissue induction. The immunostaining was done with a mixture of the antibodies 3G8 and 4A6: - no pronephric tissue, + two or more pronephric cell patches or a small area of pronephric cells, +++ pronephric tubule like structures. Bar = 200 μm (B) Exogenous OSR1 is expressed in injected embryos. After cutting the animal caps protein extracts of the remaining late blastula stage embryos injected with OSR1 mRNA were used for Western blot analysis with myc-tag specific antibody. Lane 1 and 2 refer to two pools of ten embryos. The exogenous myc-OSR1 is marked by an arrow. (C) The pronephros induction potential in animal caps was assayed after four days using the categories given in panel A. N refers to the number of animal caps investigated. (D) Quantitative RT-PCR analysis for the expression of early nephrogenic transcription factors (TFs) of animal caps after three hours and treated as indicated in (C). The bar represents the values of two independent animal cap pools (N = 30) tested. The results of OSR1 injection with retinoic acid treatment alone or in combination with activin A are each from one animal cap pool. Data obtained for hnf1b expression were only from one pool tested except for OSR1 injection alone.
	Figure 5. Expression of human LHX1, PAX8 and HNF1B in animal caps. Animal caps of LHX1 and/or PAX8 (250 pg alone or 125 pg each) or HNF1B (150 pg) injected embryos were cultured in Steinberg's solution for three hours and analysed after four days by whole-mount immunostaining using a mixture of the antibodies 3G8 and 4A6. Activin A (ActA, 10 ng/ml) and retinoic acid (RA, 10-4M) were added as given. (A) and (B) The pronephric tissue induction in animal caps treated as indicated on the left was scored using the categories given in Figure 4A. The number of animal caps (N) is given.
	Figure 1. Time dependent induction of the early nephrogenic transcription factors in retinoic acid and activin A treated animal caps. (A) Animal caps were cut at the late blastula stage 9 [36] and incubated for 1.5 or 3 hours in retinoic acid (10-4M) and activin A (10 ng/ml). For 5, 7 and 13 hours treatments retinoic acid and activin A was replaced after three hours with Steinberg's solution [15]. The mRNA levels were analysed by quantitative RT-PCR using the primers given in Additional file 2. The standard deviations from four independent animal cap pools (N = 30) are given and alterations are indicated by an upward arrow, if all four induction values were higher than one for a given probe. To detect osr2 transcripts primers targeting osr2B, the splice variant predominantly expressed in Xenopus laevis (compare Figure 2Bs) were used for two animal cap pools analyzed after 3, 5 and 7 hours and three after 13 hours In all other experiments primers targeting both splice variants were used. (B) Animal caps cut at the late blastula stage 9 were incubated with or without cycloheximide (CHX, 5 μg/ml) for 30 min and then stimulated for 1.5 hours in retinoic acid (10-4M) and activin A (10 ng/ml). RNA was quantified from six pools (N = 30) and upward arrows indicate induction for all six experiments. (C) Animal caps were cultured for three hours in retinoic acid (RA, 10-4M), activin A (ActA, 10 ng/ml) or both inducers together (RA+ActA) and then analysed by quantitative RT-PCR. The standard deviations from five (RA) or four (ActA or RA+ActA) independent animal cap pools (N = 30) are given and reproducible induction or reduction is indicated by an upward or downward arrow, if increased or decreased in all samples, respectively.
	Figure 2. Splice variants of Xenopus osr2. (A) Schematic representation of the Xenopus osr2 splicing variants A and B based on the mammalian data [35] shows alternative splice sites 2A and 2B indicated by arrowheads. Boxes represent exons and filled areas reflect open reading frames, while lines represent the promoter and introns. In the lower panel a scheme of the five and three zinc-finger domains (grey boxes) in osr2A and in osr2B protein is given, respectively. The black box in osr2B denotes the alternatively spliced exon 4. (B) Alignment of the nucleotide sequence around alternatively spliced exon 4 is based on a Xenopus laevis osr2B full-length cDNA sequence (accession no. BC108579), whereas the corresponding osr2A cDNA of Xenopus tropicalis (accession no. CU075721) is taken, as no corresponding Xenopus laevis cDNA is available. The nucleotide sequence around alternatively spliced sites 2A and 2B (indicated by arrowheads) is conserved in both species. The forward primer FP is identical for both splice variants, whereas the reverse primers distinguish between osr2A and osr2B. (C) Animal caps were cut at the late blastula stage 9 [36] and incubated for 1.5 or 3 hours in retinoic acid (10-4M) and activin A (10 ng/ml). For 5, 7 and 13 hours treatments retinoic acid and activin A was replaced after three hours with Steinberg's solution as originally described [15]. The mRNA levels were analysed by quantitative RT-PCR using the specific primers for osr2A and osr2B (see Additional file 2) and the results are normalized to odc expression levels. If two independent pools were analysed, the mean is given and the bar marks the two values.
	Figure 6. Functional identification of HNF1 binding sites in the promoter region of lhx1 in HEK293 cells and in animal caps. (A) HEK293(HNF1B) cells [45] were transfected with lhx1 gene firefly luciferase fusion constructs and HNF1B expression was induced by adding doxycycline. On the left panel schematic drawings of transfected lhx1 promoter luciferase fusion constructs (not to scale) are given. Lines represent promoter and intron regions, boxes are exons with protein coding (filled) or untranslated (open) regions (adapted from [42]). Arrows mark potential HNF1 binding sites identified by JASPAR [44]. The arrow head marks the ARE (activin response element) in intron 1 [42]. The Ex1(-120/+3) construct contains the complete HNF1 binding site in the promoter region of lhx1, whereas the binding site in the Ex1(-117/+3) construct is partially deleted (compare panel C). The HNF-4a P2-285 construct contains the P2-promoter of the HNF-4a gene which is regulated by HNF1B [46]. The fold change of luciferase activity of transfected constructs in doxycycline induced HEK293(HNF1B) versus untreated cells is given using the renilla luciferase reporter pRL-Con as an internal control. The Student's t-test was used and *, ** and *** refer to p-value of ≤ 0.05, ≤ 0.01 and ≤ 0.001, respectively and n.s. means not significant. N is the number of independent transfections made. (B) The luciferase reporter constructs (50 pg each) were tested in animal caps of controls or HNF1B (150 pg) injected embryos. The luciferase activity was measured in pools of four animal caps after four hours cultivation in Steinberg's solution. To calculate the increase of luciferase activity in HNF1B injected animal caps the ratio of firefly luciferase (FL) to renilla luciferase (RL) was used (FL/RL). The vertical line in the middle represents the mean and the small bars the standard deviation. Since experiments with different pools of animal caps were not comparable in quantitative terms, we used the Mann-Whitney-test to score significant differences. * and ** refer to p-value of ≤ 0.05 and ≤ 0.01, respectively and n.s. means not significant. N is the number of animal cap pools tested. (C) The upper panel shows the sequence logo of HNF1 binding site given in JASPAR [44] and the lower panel the sequences of the HNF1 binding site (capital letters) in Ex1(-120/+3) and Ex1(-117/+3) constructs. The vector sequence is indicated by italics.
	Figure 7. Induction of the early nephrogenic transcription factors and other genes in animal caps. osr1, osr2, hnf1b and lhx1 are induced already after 1.5 hours treatment with activin A (ActA) and retinoic acid (RA) suggesting that they are direct targets, whereas pax8 is first expressed after thirteen hours implying an indirect activation. osr2 and lhx1 (highlighted in grey) are induced after three hours by activin A alone. HNF1B overexpressed in animal caps induces after seven hours osr1, osr2, hnf1a, hnf4a, wnt11b, gdnf and tfe3. After fourteen hours pax2 and esd are increased and rbms1, fgfr4c and gsc are decreased suggesting secondary effects. HNF1B induces the expression of lhx1 by an HNF1 binding site in its promoter region (arrow). Furthermore, the lhx1 target genes cer1 and chrd are induced in HNF1B injected animal caps possibly via lhx1.

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