Umair Z , Kumar S , Kim DH , Rafiq K , Kumar V , Kim S , Park JB , Lee JY , Lee U , Kim J .

	Fig. 1. Ventx1.1 represses early and late neural genes in Xenopus whole embryo and animal cap explantsVentx1.1 (500 pg/embryo) mRNA was co-injected with and without FoxD5b-En mRNA (280 pg/embryos) at the one-cell stage, followed by dissection of the animal cap explants (AC) at stage 8 and harvesting at stage 11 and 24 respectively. The relative gene expressions were analyzed by RT-PCR: (A and C) Ventx1.1 reduced the FoxD5b-induced expression of zic3 and foxD5b in both animal cap explants (A) and whole embryos (WE) (B) at stage 11. (B and D) Ventx1.1 reduced the FoxD5b-En-induced expression of ncam, Xngnr (pan-neural markers) and NeuroD (neuronal differentiation marker) while induced the expression of xK81 (keratin marker) at stage 24. EF1α loading control, non-injected animal caps (negative control), whole embryo (WE) (positive control), control reaction without reverse transcriptase (−RT).
	Fig. 2. Genome-wide Xenopus ChIP-Seq of Ventx1.1 identifies two Ventx1.1 response cisacting elements (VRE1 and VRE2) on the zic3 promoter(A) Putative Ventx1.1 response consensus binding elements (VREs) are presented within the upstream promoter region of zic3 gene. (B) ChIP-Seq coverage plot of 3Flag-Ventx1.1 on the zic3 promoter. (C) Putative VRE sequences and their locations within the zic3 promoter. (D) This plot is showing the similarity in structure between Chr8S and Chr8L of zic3 promoter with the VRE1 and VRE2 locations marked. (E) In the ChIP assay, 3Flag-Ventx1.1 construct (500 pg/embryos) was injected at the one-cell stage and the embryos were harvested at stage 11 in 30% MMR solution. Anti-Flag antibody was used to immune-precipitate the endogenous zic3 promoter region. VRE1 and VRE2 were measured by PCR with specific zic3 promoter primers. (F) Consensus binding motifs of VRE1 and VRE2 are fully matched in both Chr8S and Chr8L of the zic3 promoter regions.
	Fig. 3. Site-directed mutagenesis of VRE1 and VRE2 within the zic3 promoter-reporter construct abolishes the repressional activity of Ventx1.1. on the reporter(A) Schematic representation of serially-deleted zic3 promoter constructs. (A–I) Different serially-deleted zic3 (40 pg/embryos) promoter constructs were co-injected with and without Ventx1.1 (500 pg/embryos) at the one-cell stage and grown until stage 11 to measure the relative promoter activity. The data are shown as mean ± S.E. of the values from at least three independent experiments. Differences were considered significant at P < 0.05.
	Fig. 4. VRE1 mutation partially abolishes negative and positive effects of Xcad2 and FoxD5b-En, respectivelyDifferent serially-deleted zic3(40 pg/embryos) promoter constructs were co-injected with and without FoxD5b-En (280 pg/embryos) at the one-cell stage and grown until stage 11 to measure the relative promoter activity. (A) FoxD5b-En increased the relative promoter activity of zic3(−1805) promoter region compared to zic3(−1805) alone. (B) zic3(−517) and zic3(−517)mVRE1 promoter constructs were co-injected with and without FoxD5b-En in separate groups. The FoxD5b-mediated induction in the relative promoter activity of zic3(−517) was abolished in zic3(−517)mVRE1. (C) zic3(−517) and zic3(−517)mVRE1 promoter constructs were co-injected with and without Xcad2 in separate groups. The Xcad2-mediated reduction in the relative promoter activity of zic3(−517) was abolished in zic3(−517)mVRE1 reporter construct. The data are shown as mean ± S.E. of the values from at least three independent experiments. Differences were considered significant at P < 0.05.
	Fig. 5. Schematic diagram depicting Ventx1.1 as a key protein in the neural inhibitory circuit of BMP4/Smad1/Xcad2/Ventx1.1 and the reciprocal inhibitory circuit of FoxD5b/Ventx1.1Ventx1.1 seems play an essential role in the BMP4/Smad1/Xcad2/Ventx1.1-mediated neural inhibition in Xenopus embryos during gastrula.

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