To identify novel transcriptional targets of Shox2, we performed microarray analysis and compared gene expression levels in right atria of wildtype and Shox2 ^−/− hearts. Only right atria comprising the Shox2 expressing sinus venosus myocardium and venous valves were dissected from murine E11.5 hearts to increase the specificity of the array analysis. Genes were considered to be up- or downregulated if they showed log2 ratios of ≥0.35 or ≤−0.4 with a significance of P ≤ 0.0001. Using these selection criteria, we identified 321 genes with significantly altered gene expression (80 up- and 241 downregulated genes). As expected, Shox2 was among the highest negatively regulated genes. Classification of the 321 genes into gene families using the Gene Set Enrichment Analysis (GSEA) revealed that the highest proportion of regulated genes belongs to the group of transcription factors. Among these, the LIM homeodomain transcription factor Isl1 showed a reduced expression in right atria of Shox2 ^−/− embryos.

To verify Isl1 as a putative target gene, we carried out qRT-PCR analyses using right atrial tissue samples of wildtype and Shox2 knockout embryos and confirmed the downregulation of Isl1 expression in a second independent pool of embryonic heart tissue (Fig. 1A). To further investigate Isl1 as a putative target gene of Shox2, we compared the spatial expression of both genes and found that Shox2 and Isl1 expression overlap in embryonic mouse hearts. Isl1 expression was detected in the SAN of wildtype hearts, which corresponds to the area where Shox2 normally is expressed (Fig. 1B). Whole-mount in situ hybridization on isolated E11.5 wildtype and knockout hearts demonstrated that Isl1 transcripts are completely absent in the SAN region of Shox2 mutants (Fig. 1C b’), while normal expression was observed in the outflow tract (Fig. 1C b). The lack of Isl1 expression in the SAN, but unaffected Isl1 expression in the outflow tract of Shox2-null mice could be also confirmed at embryonic stage E12.5 (Fig. S1A). In situ analyses revealed a complete loss of Isl1 expression in the right atrium (SAN) of knockout hearts, suggesting that the residual Isl1 expression detected in Shox2 knockout tissue by qRT-PCR and microarray experiments is likely due to some remaining outflow tract tissue following microdissection. Quantitative expression analysis using outflow tract tissue samples showed high and consistent Isl1 expression levels in both wildtype and Shox2 knockout embryos (Fig. S1B).

To validate that the loss of Isl1 expression in the SAN of Shox2 knockout hearts is not due to incorrect formation of SAN tissue, we examined the expression of SAN markers in wildtype and knockout hearts using in situ hybridization and immunohistochemistry. While Tbx18 is mainly expressed in the SAN head, Hcn4 is a very prominent marker of the complete developing SAN [45, 56]. Double in situ hybridization experiments using an Isl1 antisense probe together with Hcn4 showed coexpression in the SAN of E12.5 and E13.5 wildtype hearts (Fig. 2A a, a’, c, c’). In Shox2 ^−/− mouse hearts Isl1 expression is completely absent in this region, while Hcn4 transcripts are still detectable (Fig. 2A b, b’, d, d’). Double immunostainings revealed that Hcn4 and Tbx18 colocalize with Isl1 in the SAN of E11.5 wildtype embryos (Fig. 2B a, g). While both markers could be detected in the SAN of wildtype and knockout hearts (Fig. 2B c, f, i, l), Isl1 staining is not detectable in this region in Shox2 ^−/− embryos (Fig. 2B e, k). Together, these stainings confirm the loss of Isl1 expression in the SAN of Shox2 mutants on transcript and protein level at different embryonic stages, while the presence of Hcn4 and Tbx18 confirm that the SAN is formed. The loss of Isl1 expression is thereby very likely linked to Shox2 deficiency and does not constitute an indirect effect due to disrupted development of SAN tissue in knockout embryos.

To further study the transcriptional control mechanism of ISL1 by SHOX2, we investigated specific binding sites within the ISL1 locus. As a first step, we performed multispecies conservation analysis for the human ISL1 locus to identify evolutionary conserved regions. Conservation of DNA sequences provides a route for identifying functional elements in genomes [32]. Sequence comparison of human, frog, chicken, and mouse Isl1 revealed several highly conserved regions (Fig. S2A). Using luciferase assays, we functionally characterized these highly conserved elements. The reporter constructs used are depicted as black boxes below the conservation plot in Supplemental Material Fig. S2A and are referred to as ISL1-reporter-1 to ISL1-reporter-5. ISL1-reporter-3 and -4 include regulatory elements previously identified downstream of the translational stop codon [22, 23], while ISL1-reporter-1 contains a recently published minimal promoter of the Isl1 gene [31]. Cotransfections of the different ISL1 reporter constructs along with a SHOX2a expression plasmid revealed a strong increase in luciferase activity only for ISL1-reporter-2, compared to the basal level of the respective reporter alone (Fig. S2B). By transfection of serial gene deletion constructs (genomic locations of the constructs are depicted in Fig. 3A), we confined the SHOX2 transcriptional regulatory element to a 184-bp region located in the second intron of ISL1, corresponding to ISL1-reporter-2del 3 (Fig. 3A, B). To identify the precise SHOX2 binding site, EMSA was performed using four different oligonucleotide probes (Oligo1–Oligo4; Fig. S3A) that cover the respective intronic ISL1 sequence. We obtained a shift with both Oligo1 (strong binding) and 3 (weaker binding), but not with Oligo2 and 4 (Fig. 3C, Fig. S3B). Competitive EMSAs demonstrated that only high excess (150-fold) of unlabeled Oligo3 (SpC3) competitively affects binding of Oligo1 to SHOX2 (Fig. S4A, left panel), while already a low molar excess (50-fold) of unlabeled Oligo1 (SpC1) competitively inhibits binding of labeled Oligo3 to SHOX2 (Fig. S4A, right panel). Our luciferase assays also show that the sequence encompassing Oligo1 alone is not sufficient to activate ISL1 by SHOX2 (as this region was also partly included in the ISL1-reporter-2del 2 construct which did not show an increase in luciferase activity upon cotransfection with SHOX2) (Fig. 3B), suggesting that both sequences (encompassing Oligo1 and Oligo3) are necessary to activate the ISL1 gene by SHOX2. Oligo1 and Oligo3 both include AATT-palindromic sequences, which were mutated to CCGG (Oligo1 mut and Oligo3 mut) to confirm sequence specific binding. No shift was obtained using the mutated Oligos, confirming that the AATT motif is essential for SHOX2 binding (Fig. 3C). In addition, competition assays revealed that an excess of unlabeled wildtype Oligos (SpC1 and SpC3) reduce the DNA binding ability of SHOX2, whereas excess of mutant Oligos (MuC1 and MuC3) do not affect the binding (Fig. S4B).

To functionally assess whether Shox2 and Isl1 act in the same genetic pathway, we injected zebrafish embryos with morpholinos (MO). When injecting either 2.8 ng of shox2-MO or isl1-MO, 82.0 ± 2.6 % (n = 175; 2 independent experiments) and 79.1 ± 0.3 % (n = 182; 2 independent experiments) of injected embryos, respectively, displayed pericardial edema (Fig. 4A asterisk) and a severely reduced heart rate (Fig. 4B). Embryonic heart morphogenesis proceeds normally in shox2-MO and isl1-MO injected zebrafish. By 72-h post fertilization (hpf), morphant hearts consist of two heart chambers, atrium and ventricle, with properly developed myocardial and endocardial cell layers. The similarity of phenotypes between shox2 and isl1 deficiency in the fish raised the possibility that a close functional interaction between these two genes exists. To address whether the observed cardiac dysfunction caused by shox2 deficiency could depend on isl1 function, we examined the ability of isl1 to compensate the morpholino-mediated loss of shox2 function by transient rescue experiments. DNA constructs expressing isl1 and shox2 under the control of the cardiac myosin light chain 2 (cmlc2) promoter [18, 33], which drives myocardial-specific expression were used for the rescue experiment. The cmlc2 promoter also drove expression of GFP, which allowed monitoring of cardiomyocyte-specific expression (Fig. S5A). We coinjected 0.32 ng of the isl1-expression construct along with 2.8 ng shox2-MO, which was sufficient to induce the bradycardia phenotype and subsequently measured the heart rate of GFP positive embryos after 72 hpf. Myocardial-specific expression of isl1 could significantly rescue the reduced heart rate in shox2 morphant embryos. As a control, injection of the isl1- or shox2-expression construct alone did not cause any changes in embryonic heart rate (Fig. 4C). Histological sections of shox2-MO injected hearts rescued by isl1 overexpression show normal development of the heart without formation of pericardial edema (Fig. 4D), compared to those of shox2-MO injected embryos alone (Fig. 4A). In addition, we could show a downregulation of isl1 protein levels in embryos injected with shox2-MO (Fig. S5B). Both proteins, shox2 and isl1, are highly expressed during neural development and isl1 plays an important role during differentiation of neurons in the brain. To exclude that shox2 deficiency also affects differentiation of isl1 positive neurons, we analyzed the isl1 expression after shox2 knockdown by whole-mount in situ hybridization. Isl1 expression in the brains of shox2 morphants is indistinguishable from wildtype embryos (Fig. S6A and B). On the other hand, isl1 deficient embryos show a normal expression of shox2 in the head region (Fig. S6C and D). Furthermore, we performed immunostaining using acetylated Tubulin as neuronal marker (Fig. S6E and F). While the heart rate was reduced after shox2-MO injection, no alteration could be detected in neural development. Together, these results indicate an epistatic relationship and a direct functional link between shox2 and isl1 in the pacemaking system of zebrafish embryos.