Abstract
Background
The homeobox gene Gsx2 (formerly Gsh2) is known to regulate patterning in the lateral ganglionic eminence (LGE) of the embryonic telencephalon. In its absence, the closely related gene Gsx1 (previously known as Gsh1) can partially compensate in the patterning and differentiation of ventral telencephalic structures, such as the striatum. However, the cellular and molecular mechanisms underlying this compensation remain unclear.
Results
We show here that in the Gsx2 mutants Gsx1 is expressed in only a subset of the ventral telencephalic progenitors that normally express Gsx2. Based on the similarities in the expression of Gsx1 and Ascl1 (Mash1) within the Gsx2 mutant LGE, we examined whether Ascl1 plays an integral part in the Gsx1-based recovery. Ascl1 mutants show only modest alterations in striatal development; however, in Gsx2;Ascl1 double mutants, striatal development is severely affected, similar to that seen in the Gsx1;Gsx2 double mutants. This is despite the fact that Gsx1 is expressed, and even expands, in the Gsx2;Ascl1 mutant LGE, comparable to that seen in the Gsx2 mutant. Finally, Notch signaling has recently been suggested to be required for normal striatal development. In spite of the fact that Notch signaling is severely disrupted in Ascl1 mutants, it actually appears to be improved in the Gsx2;Ascl1 double mutants.
Conclusion
These results, therefore, reveal a non-proneural requirement of Ascl1 that together with Gsx1 compensates for the loss of Gsx2 in a subset of LGE progenitors.
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Background
The homeobox gene Gsx2 (formerly known as Gsh2) has been shown to be required for correct dorsal-ventral patterning in the embryonic mouse telencephalon [1–3]. Gsx2 accomplishes this by repressing dorsal telencephalic genes such as Pax6 and promoting the expression of ventral regulators such as Ascl1 (Mash1) and Dlx genes within ventricular zone (VZ) and subventricular zone (SVZ) progenitors of the lateral ganglionic eminence (LGE). Although Gsx2 mutants do not survive after birth [4], analyses at late embryonic stages have demonstrated severe reductions in markers of striatal projection neurons as well as olfactory bulb interneurons [1–3, 5, 6], both of which are derived from the LGE [7–10].
The closely related Gsx1 (Gsh1) is also expressed in the embryonic ventral telencephalon [11], although no telencephalic phenotype has been reported [5, 6]. Despite this, removal of Gsx1 on the Gsx2 mutant background eliminates nearly all striatal projection neurons and olfactory bulb interneurons, suggesting that Gsx1 can, at least in part, compensate for the loss of Gsx2 in the development of these ventral telencephalic structures. This compensation, however, is complex because Gsx1 is normally only present in the medial ganglionic eminence and the ventral-most portion of the LGE. In Gsx2 mutants, Gsx1 expression spreads dorsally to encompass the mutant LGE at mid-neurogenesis time points (for example, embryonic day (E)14), which is coincident with the re-establishment of ventral identity (for example, Ascl1 and Dlx expression) in the mutant LGE [5, 6]. Both Ascl1 and Dlx genes are known to be required for normal development of the striatum and olfactory bulb interneurons [12–16]. Moreover, a recent study [17] suggests that Ascl1 and Dlx genes control distinct and parallel pathways that act in the specification of olfactory bulb interneurons. The mechanism by which Gsx1 compensates for the loss of Gsx2 has not been fully elucidated. Moreover, the requirement for Ascl1 or Dlx genes in this process is unclear.
In this study we have examined the molecular mechanisms underlying Gsx1-mediated recovery of ventral telencephalic development in Gsx2 mutants. To do this, we have generated and analyzed Gsx2EGFPmice as well as Gsx2;Ascl1 double mutants at multiple embryonic stages. Removal of Ascl1 from the Gsx2 mutant background results in a telencephalic phenotype nearly identical to the Gsx1:Gsx2 double mutant [5, 6]. These results thus indicate that Ascl1 is an essential component of the Gsx1-mediated recovery in a subset of LGE progenitors within the Gsx2 mutant telencephalon.
Results
Gsx1 expression in the Gsx2 mutant telencephalon
Previous studies have shown that Gsx1 expands in the LGE of the Gsx2 mutant [3, 5, 6]. Normally, the cells expressing Gsx1 are confined to the ventral-most portion of the LGE; however, in Gsx2 mutants the expression of this gene expands throughout the entire dorsal-ventral extent of the LGE between E11 and E14. We have generated mice in which the first exon of Gsx2 is interrupted by an IRES-enhanced green fluorescent protein (EGFP) cassette so that EGFP is expressed in place of Gsx2. These mice appear to faithfully reproduce Gsx2 expression and provide a short-term fate map of Gsx2 derived cells that no longer express the protein (Figure 1A–C). Moreover, the Gsx2EGFP/EGFPembryos lack Gsx2 protein expression, while still delineating the portion of the LGE that the targeted Gsx2 gene is being transcribed in by virtue of the EGFP staining (Figure 1F–H). These mutants exhibit identical patterning defects to those reported for the previously available Gsx2 mutant allele [1–4] (data not shown). Using these mice together with an antibody that detects both Gsx1 and Gsx2 [18], we were able to examine the Gsx1 recovery on a cellular level, within the context of the Gsx2 expression domain.
While the Gsx1/2 antibody staining looks very similar to that of Gsx2 in the Gsx2EGFP/+embryos (Figure 1A–E), it reveals a rather different pattern in the Gsx2EGFP/EGFPembryos (Figure 1I, J). At E12.5, the cells expressing Gsx1 in the mutant LGE are few in number and largely confined to its ventral half. This finding is in agreement with previous Gsx1 gene expression studies [3, 5]; however, the cellular resolution afforded by the immunohistochemical approach revealed that the Gsx1 cells appear mostly at the border between the VZ and SVZ (Figure 1I, J). This is different from Gsx2 expression in the wild-type LGE where cells throughout the apical-basal extent of the VZ express this protein, albeit at different levels of expression (Figure 1B). Previous studies have shown that the expansion of Gsx1 throughout the Gsx2 mutant LGE is complete between E14.5 and E16.5 [3, 5, 6]. This is clearly revealed by Gsx1/2 staining in the Gsx2EGFP/EGFPmutants at E16.5 (Figure 2G). At this stage, only around half the LGE cells that would normally express Gsx2 contain Gsx1 staining. Again, the majority of the Gsx1 expressing cells appear to line up at the VZ/SVZ boundary (Figure 2H). This is similar to Gsx1/2 staining in the remnant of the medial ganglionic eminence in Gsx2EGFP/+brains (Figure 2B), and since this staining does not coincide with the EGFP from the Gsx2 locus (Figure 2A–C), it is likely to reflect Gsx1 expression in the wild-type medial ganglionic eminence. Thus, although Gsx1 can at least partially compensate for Gsx2 [5, 6], it does not do so in all cells of the LGE that would normally express Gsx2 but only in a subpopulation positioned at the VZ/SVZ boundary.
Relationship between Gsx1 and Ascl1 in the Gsx2 mutant LGE
Ascl1 (Mash1) is known to be required for the normal development of the ventral telencephalon [14–16]. Furthermore, Ascl1 is dependent on Gsx2 for its normal expression in LGE progenitor cells [1–3], at least at early stages, before Gsx1 expression expands into the mutant LGE. Ascl1 is expressed by many cells within the Gsx2EGFP/+VZ, although they are mainly located at the VZ/SVZ boundary (Figure 2D, E). Interestingly, the pattern of Ascl1 expression in the Gsx2 mutants is very similar to that of Gsx1 (as revealed by Gsx1/2 staining; Figure 2G–J), with scattered cells in the VZ and the majority accumulated along the VZ/SVZ boundary. In Gsx1;Gsx2 double mutants, Ascl1 is not expressed in the LGE at early stages (for example, E12.5) but at later stages (for example, E15.5–16.5) it is found at low levels within the presumptive LGE region [5, 6]. This suggests that although Gsx proteins are not absolutely required for Ascl1 expression in the LGE, they are positive regulators of its expression. The overlap in Gsx1 and Ascl1 expression in the Gsx2 mutant LGE (Figure 2H, J) therefore suggests that Ascl1 may act in concert with Gsx1 for the compensation observed in Gsx2 mutants.
Expression of Gsx2 in the Ascl1 mutant
Although Ascl1 expression in LGE progenitors has been shown to require Gsx2 [1–3], the role (if any) of Ascl1 in regulating Gsx2 expression has not been reported. In E12.5 Ascl1-/- mutants, we found that Gsx2 (and Gsx1/2) staining in the LGE was not significantly different from that observed in wild types (Figure 3A, D and data not shown). Conversely, at E18.5 we observed a large increase in the numbers of cells expressing Gsx2 along the dorsal-ventral aspect of the VZ in the Ascl1 mutants and in certain cases clusters of Gsx2 expressing cells were found in the forming striatum (Figure 3E). The expression of Gsx2 coincided with Ki67 staining in many of these clusters (Figure 3E, F) on closely adjacent sections, suggesting that despite their ectopic location, these Gsx2 cells may remain in the cell cycle. Gsx1 expression was not changed in the LGE of Ascl1 mutants [19] (data not shown). These findings could indicate that, in addition to being downstream of Gsx genes, Ascl1 may also serve a negative feedback function to repress Gsx2 in LGE progenitors, particularly at late embryonic stages.
Gsx2;Ascl1 double mutants exhibit severe striatal defects
To examine the possibility that Ascl1 is required for the Gsx1-mediated recovery observed in the Gsx2 mutant, we generated Gsx2;Ascl1 double homozygous mutants and analyzed the striatum at E18.5. The expression of FoxP1 can be used to mark striatal neurons and, thus, the forming striatum at this stage [20, 21]. Staining for this marker shows that the size of the striatum in Gsx2 mutants is severely reduced compared to wild types (Figure 4A, B), which is consistent with previous studies [1–3, 5, 6]. Unlike the Gsx2 mutants, however, Ascl1 mutants exhibit more subtle defects in striatal development [14] and, accordingly, showed a more modest reduction in FoxP1 expression (Figure 4C). Interestingly, the Gsx2;Ascl1 double mutants showed an even more severe reduction in FoxP1 staining than the Gsx2 mutants (Figure 4D), indicating that only a rudimentary striatum is present in these brains.
The striatum is composed of two anatomically and neurochemically distinct compartments termed the patch and matrix [22]. The striatum-enriched phosphoprotein DARPP-32 has been shown to mark the forming patch compartment at perinatal time points [23] (Figure 4E). DARPP-32 is severely reduced in the Gsx2 mutant striatum (Figure 4F) [1, 2, 5, 24] while its expression was only moderately reduced in the Ascl1 mutants (Figure 4G). Interestingly, no DARPP-32-positive neurons were observed in the Gsx2;Ascl1 double mutant striatum (Figure 4H), a finding that is identical to that previously observed in the Gsx1;Gsx2 double mutant striatum [5]. Calbindin is known to mark the matrix compartment in the mature striatum [22]. As previously reported [5], calbindin expression is increased in the forming Gsx2 mutant striatum (Figure 4J) while a clear reduction in its expression was seen in the Ascl1 mutant striatum (Figure 4K). The rudimentary striatum present in the Gsx2;Ascl1 double mutant striatum did express calbindin (Figure 4L). Again, this was similar to that previously observed in the Gsx1;Gsx2 double mutant striatum [5]. Thus, the similarities in the phenotypes observed in the Gsx2;Ascl1 and Gsx1;Gsx2 double mutants suggest that Ascl1 is required for the Gsx1-based striatal recovery in Gsx2 mutants.
In order to determine whether Ascl1 is required downstream of Gsx1 in a Gsx2 mutant, we examined the expression of Gsx1 in Gsx2;Ascl1 double mutants. If Ascl1 is required for Gsx1 to expand throughout the Gsx2 mutant LGE, then the similarities in the Gsx2;Ascl1 and Gsx1;Gsx2 double mutant phenotypes would be easily explained by the lack of Gsx1 in LGE progenitors. However, this is not the case, because we observed both Gsx1 gene expression and Gsx1/2 staining in the Gsx2;Ascl1 double mutant LGE (Figure 5C, F). Indeed, the level and extent of this expression was very similar to that seen in the Gsx2 mutant (Figure 5B, E). This allows us to conclude that Ascl1 acts downstream of Gsx1 in the Gsx2 mutant LGE.
Olfactory bulb defects in Gsx2;Ascl1 double mutants
Unlike striatal neurons that are largely produced at embryonic stages, olfactory bulb interneurons are generated over a protracted period, starting around E14 and with the majority produced during the first 2 weeks after birth [25]. Since Gsx2 mutants die shortly after birth [4], only the olfactory bulb interneurons that are generated at embryonic stages can be assayed. Previous studies [1, 3, 5, 6] have shown that Gsx2 mutants exhibit defects in the development of these neurons at birth. The olfactory bulb interneurons produced at embryonic time points have been suggested to originate, at least in part, from the dorsal (d)LGE [26]. We have recently shown that the zinc finger transcription factor Sp8 marks the dLGE as well as olfactory bulb interneurons [27] (Figure 6A, E). In Gsx2 mutants, the number of Sp8 expressing cells is dramatically reduced in both the dLGE and olfactory bulb (Figure 6B, F) [27]. Although Ascl1 mutants have been shown to have olfactory bulb interneuron defects [14, 28], the expression of Sp8 in these mutants is not reduced in the dLGE at E15.5 [17]; rather, it appears as if more cells are seen in this region streaming laterally towards the ventrolateral telencephalon by E18.5 (Figure 6C). Moreover, there appear to be similar numbers of Sp8-positive cells within the Ascl1 mutant olfactory bulb compared to wild type, although their distribution appears somewhat disorganized (Figure 6G). Conversely, in the Gsx2;Ascl1 double mutants the expression of Sp8 is reduced, even when compared to the Gsx2 mutants (Figure 6B, D). Indeed, most sections of the double mutant olfactory bulb lack any Sp8-positive cells (Figure 6H).
Sp8 is required for normal development of the calretinin (CR)-expressing subtype of olfactory bulb interneurons [27]. In addition to the dLGE, the septum has also been suggested to give rise to olfactory bulb interneurons [29], and more recent results suggest that the septum may also represent a region where the CR interneurons originate [30, 31]. Indeed, CR positive neurons can be seen in the wild-type dLGE and even more so in the septum at E18.5 (Figure 7A) as well as in the forming glomerular layer of the olfactory bulb (Figure 7E). As might be predicted from the Sp8 staining, the Gsx2 mutants showed reductions in CR interneurons (Figure 7B, F), while the Ascl1 mutants did not appear to exhibit reduced numbers of CR positive cells (Figure 7G) and at least in portions of the dLGE may even contain increased numbers of these cells (Figure 7C). Furthermore, the Gsx2;Ascl1 double mutants showed a more severe reduction in CR staining than the Gsx2 mutants (Figure 7D, H). Previous studies [1, 3, 5, 6, 14, 28] have shown that Gsx2 (Figure 7J) and Ascl1 mutants (Figure 7K) exhibit reductions in glutamic acid decarboxylase (67 kDa) (GAD67)-positive olfactory bulb interneurons (GAD67 is a rate limiting enzyme in GABA production). These appear to be compounded in the Gsx2;Ascl1 double mutants where essentially no GAD67-positive cells were observed in the olfactory bulb at this time point (Figure 7L). Taken together, these data suggest that Ascl1 functions downstream of Gsx2 to regulate aspects of olfactory bulb interneuron diversity. Indeed, it appears that Gsx2 is required for many, if not all, of the interneuron subtypes to be properly generated, while Ascl1 is more crucial for the generation of GAD67 (that is, GABAergic) and dopaminergic interneurons [28].
Notch signaling in Gsx2;Ascl1 double mutants
Previous studies have shown that Notch signaling is required for normal LGE/striatal development [16, 32]. Moreover, Ascl1 mutants exhibit reduced Notch signaling [14, 16]. It is possible, therefore, that the phenotypes observed in the Gsx2;Ascl1 double mutants are a result of compound effects of a loss of Notch signaling together with distinct Gsx2 requirements. To address this, we examined the expression of factors in the Notch signaling pathway, Ngn2, Dll1 and Hes5, in relation to Gsx1/2 expression. In Gsx2 mutants, Ngn2 was shifted ventrally into the LGE as previously described (Figure 8F) [1–3], although it appeared to be directly abutting the ventrally shifted Gsx1/2 staining (Figure 8B). Indeed, both Dll1 (Figure 8J) and Hes5 (Figure 8N) were continuously expressed throughout the Gsx2 mutant LGE. In the Ascl1 mutants, Gsx1/2 staining was present up to the normal pallio-subpallial boundary (Figures 3A and 8C) and Ngn2 staining abutted it at its normal ventral position (compare Figure 8E and 8G). This theoretically leaves no proneural gene expression in the LGE and, in fact, both Dll1 (Figure 8K) and Hes5 (Figure 8O) staining was absent, as previously described [14]. This is not the case in Gsx2;Ascl1 double mutants, where Ngn2 was observed to extend ventrally into the double mutant LGE and improvement in Dll1 (Figure 8L) and Hes5 (Figure 8P) expression was observed, at least within the presumptive LGE region, compared to Ascl1 mutants. This indicates that the Notch signaling defects observed in Ascl1 mutants are, in part, due to Gsx2 expression remaining in the LGE. Thus, it appears that Ascl1 performs a non-proneural function in the Gsx1-mediated recovery observed in the Gsx2 mutant. Interestingly, it also seems that Ascl1 plays a role in the timing of the Gsx1 expansion into the Gsx2 mutant LGE as the Gsx2;Ascl1 double mutants showed much less Gsx1 (as marked by Gsx1/2 staining) expression in the presumptive LGE at E12.5 (Figure 8D) when compared to later time points (for example, E16.5; Figure 5C, F).
Discussion
The study of knock-out mice is essentially an investigation into the compensatory mechanisms (or lack thereof) when any given gene is inactivated. In the case of Gsx2, it has previously been shown that Gsx1 is involved in the partial recovery observed in these mutants [5, 6]. What remained unclear was why the Gsx1-dependent compensation was not more effective in restoring normal development. In addition to a delayed upregulation of Gsx1 in the Gsx2 mutant LGE [5, 6], we provide novel data here showing that Gsx1 is expressed only in a subset of LGE cells that would normally express Gsx2. Interestingly, these cells are largely located at the boundary between the VZ and SVZ, similar in location to that of Ascl1 expressing cells. Based on the facts that the striatal phenotype of the Gsx2;Ascl1 mutants is nearly identical to that observed in Gsx1;Gsx2 mutants [5, 6] and that Gsx1 expands in the Gsx2;Ascl1 mutants in a similar way to that observed in Gsx2 mutants, we conclude that Ascl1 is required downstream of Gsx1 for this recovery. These findings suggest that there are Ascl1-dependent and Ascl1-independent pathways for LGE development. This is in agreement with recent studies by Long et al. [17, 19] showing that Dlx1/2 and Ascl1 regulate parallel and overlapping pathways in LGE specification. Furthermore, our results indicate that the Ascl1-dependent pathway for LGE specification appears to be independent of its well-known role in regulating the Notch signaling pathway.
The mechanism by which Gsx1 is upregulated in the Gsx2 mutant LGE has been unclear. It does not appear that Gsx2 represses Gsx1 expression because only a subset of the cells that normally express Gsx2, particularly those at the VZ/SVZ boundary, are Gsx1-positive in the Gsx2 mutant LGE. It seems possible, therefore, that Gsx1 can only be expressed in certain cell types or in cells that have reached a particular level of maturation (that is, cells transitioning from the VZ to the SVZ). Indeed, it appears that Gsx1-positive cells in the medial ganglionic eminence region also reside largely in the VZ/SVZ boundary region (for example, Figure 2C). Interestingly, at early stages (that is, E12.5) in the Gsx2 mutants, the LGE SVZ does not form, and only after Gsx1 has expanded throughout the mutant LGE (that is, by E14–15) does the it do so in this mutant [2, 3, 5]. Together with the current findings, these results suggest that Gsx1 may be expressed in more mature progenitors and might even play a role in the maturation process.
Ascl1 has previously been implicated in the development of the striatum and olfactory bulb interneurons [14–17, 28]. In general, however, the requirement for Ascl1 in striatal and olfactory bulb development is not as great as that for Gsx2. In fact, the striatum of the Ascl1 mutant is only slightly reduced in size when compared to the wild type [14] (Figure 4). Moreover, the reduction in dopaminergic and GABAergic olfactory bulb interneurons [28] is not as severe as that observed in Gsx2 mutants [5, 6]. Although striatal development is only modestly affected by the loss of Ascl1, we show here that the added loss of Gsx2 results in a nearly complete loss of striatal development. This result is identical to that previously reported for Gsx1;Gsx2 double mutants [5, 6]. Thus, Ascl1 is absolutely essential for the Gsx1-mediated recovery observed in Gsx2 mutants. While Ascl1 appears to be downstream of Gsx2 [1–3], the relationship between Gsx1 and Ascl1 appears to be more complex. The loss of Gsx1 and Gsx2 severely depletes the expression of Ascl1 throughout embryogenesis [5, 6], suggesting that both are genetically upstream; however, our findings here also demonstrate a delay in the expression of Gsx1 in Gsx2;Ascl1 double mutants at early stages (for example, Figure 8D), potentially implicating Ascl1 in feedback regulation of Gsx1 expression.
Ascl1 is a known regulator of the Notch signaling pathway [14, 16] and Notch signaling has previously been implicated in controlling striatal development [16, 32]. It does not seem that the striatal defects observed in the Gsx2;Ascl1 double mutants, described here, are simply due to compound effects of the loss of Gsx2 and impaired Notch signaling because we observed an improvement in Notch signaling (as indicated by Hes5 and Dll1 expression) within LGE progenitors of the Gsx2;Ascl1 double mutants compared to Ascl1 mutants. Our interpretation of this result is that Gsx2;Ascl1 mutants are similar to Gsx2 mutants in that Ngn2 is allowed to expand ventrally into the LGE and, as a result, Notch signaling is improved. Clearly, Ascl1 plays a role in regulating Notch signaling within LGE progenitors [14, 16]; however, the fact that striatal development is not more severely affected in the Ascl1 mutant could suggest that Gsx2 normally works through another gene encoding a basic helix-loop-helix (bHLH) factor to regulate aspects of LGE neurogenesis.
A somewhat surprising finding that we observed in the Ascl1 mutants was that Gsx2 expression appeared to be increased at perinatal stages. This is not the case at early time points (for example, E12.5) and suggests that Ascl1 may play a role in depleting the Gsx2 progenitors during embryogenesis. The increased Gsx2 in the Ascl1 mutant LGE correlated well with the expression of Sp8, a zinc finger transcription factor that has previously been shown to be dependent on Gsx2 expression [27].
Previous studies have described a reduction in dopaminergic and GABAergic interneurons in the Ascl1 mutants [14, 28]; however, no data on other subtypes have been provided. We show here that unlike the dopaminergic and GABAergic subtypes, the CR interneurons are not reduced and may, in fact, be increased. The neurotransmitter of this subtype remains somewhat unclear. Recent reports suggests that as few as 14% are GABAergic [33], while others suggest that most if not all are GABAergic [30, 34]. Our data seem to support the former possibility (at least at this stage of development) since the reduction in GABAergic neurons (as marked by GAD67) is not paralleled by CR-positive cells in the Ascl1 mutant olfactory bulb. We have recently shown that the zinc finger transcription factor Sp8 is required for the normal development of the CR interneurons in the olfactory bulb [27]. Accordingly, we found that in Ascl1 mutants at late stages of development, Sp8 staining is maintained in the dLGE and olfactory bulbs. Because Gsx2 is required for Sp8 expression in the dLGE and the latter is essential for normal CR interneuron production, it seems likely that the sequential expression of these two transcription factors cooperate to generate this interneuron subtype. However, despite that Gsx2 appears to function upstream of Ascl1, this bHLH factor does not actively promote CR interneuron development.
The origin of distinct subtypes of olfactory bulb interneurons has recently been the subject of considerable attention. Kohwi et al. [30] have recently suggested that CR interneurons arise from pallial and septal regions but not the dLGE. On the other hand, De Marchis et al. [35] found that these interneurons were generated from the postnatal region of the SVZ that directly derives from the dLGE. In support of this, Merkle et al. [31] showed that at least some CR neurons are derived from the rostral dorsal SVZ (a likely derivative of the dLGE). Although CR interneurons start to be produced at embryonic time points, a recent study by Batista-Brito et al. [36] have shown that most are generated at postnatal time points. Our data show that at least a few CR neurons are present in the late embryonic dLGE and that Ascl1 mutants appear to exhibit enhanced CR neuron production in the dLGE and possibly olfactory bulb. Thus, Ascl1 may play a role in the temporal regulation of CR interneuron production from the dLGE and its SVZ derivatives. In any case, our findings clearly demonstrate that the dLGE is a significant source of CR interneurons that are generated at embryonic time points; however, we cannot exclude the contribution of the septum in the generation of these interneurons as shown by Merkle et al. [31], particularly at early postnatal stages. Indeed, Gsx2 is expressed at high levels in both the dLGE as well as in the dorsal portion of the septum (Figure 2) and CR staining in the septal region is also lost in the Gsx2 mutant (Figure 7). Regardless of their origin, it seems that all subtypes of olfactory bulb interneurons, at least at embryonic time points, require Gsx2 for their normal production.
Conclusion
Our data show that Gsx1 compensates for the loss of Gsx2 gene function in only a subpopulation of the LGE progenitors that normally express Gsx2, which may explain why the compensation is not more complete. Additionally, we show that Ascl1 is an obligate factor for Gsx1 in the recovery process and that this is independent of its well-known proneural function.
Methods
Gsx2 [4] and Ascl1 [37] mice were genotyped as previously described [2, 14]. Interbreeding between Gsx2 and Ascl1 heterozygotes was performed to generate Ascl1;Gsx2 double heterozygotes, which were subsequently crossed to generate Ascl1;Gsx2 double homozygous mutants.
Gsx2EGFPknock-in mice were generated by inserting an IRES-EGFP-pA cassette (Clonetech, Mountain View, CA, USA) into the first exon of Gsx2 between the Not I and Nco I sites (Figure 9A). Specifically, a 9-kb genomic fragment encompassing the Gsx2 locus was isolated by a Hin dIII digest of a Gsx2-positive 129 BAC and subcloned into the Hin dIII site of pBluescript SK (Stratagene, La Jolla, CA, USA). The targeting vector backbone was previously described in Bell et al. [38]. A 6.4-kb Nco 1/Spe 1 fragment from the 9-kb Gsx2 genomic region was blunted and subcloned into the Hpa 1 site of cre/lox targeting vector to be used as the 3' homology arm. A 1-kb Hin dIII/Not 1 fragment from the 9-kb Gsx2 genomic region was blunted and subcloned into the Sma 1 site of pBluescript SK (called 5'arm-PBS). The pIRES2-EGFP vector (Clonetech) was digested with Afl II, blunted, and redigested with Nhe 1 to release IRES-EGFP. IRES-EGFP was cloned into 5'arm-PBS, which was digested with Sal 1, blunted, and redigested with Spe 1 (5'arm-EGFP-PBS). The 5'arm-IRES-EGFP was released with a Xho 1 digest that was blunted and subcloned into the Pme 1 site of the cre/lox targeting vector. The Gsx2EGFPvector was linearized with Sal 1 and electroporated in W4 embryonic stem (ES) cells (reviewed in [39]) and selected with G418 and gancyclovir. Correctly targeted cells were identified by PCR (Figure 9A, B) using the following primer pairs to generate products specific for the correctly targeted Gsx2EGFP/+allele: internal primer 1 (5'-cctccgcttctgttgtgact-3') with internal primer 2 (5'-cctaggaatgctcgtcaagaag-3'), which gave an 837 bp product, and an external primer (5'-cctccactacaaggccacatac3') with internal primer 2, which generated a 1,170 bp product, specific for the correctly targeted Gsx2EGFP/+allele. Two different targeted ES cell lines were used for blastocyst injection by the Cincinnati Children's Hospital Medical Center transgenic facility. Germline transmission was tested by crossing the chimeras with C57/B6 mice to obtain agouti offspring. F1 Gsx2EGFP/+mice were bred to β-actin-FLPe (enhanced Flpase) mice [40] obtained from Jackson Laboratory, Bar Harbor, ME, which resulted in the Neomyocin cassette flanked by FLP recombinase target (FRT) sites to be removed (Figure 9A). Embryos derived from Gsx2EGFP/+crosses were genotyped with the following primers: internal 2 (5'-cctaggaatgctcgtcaagaag-3') with Gsx2 int5A (5'-catcaccatcaccagcccc-3'), which generated a 225 bp product specific for the knock-in allele; and Gsx2-Int5B (5'-ccacggagattccactgcc 3') with Gsx2-1437 (5'-gcatccaccccaaatctcagtc-3'), which generated a 298 bp product specific for the Gsx2 wild-type allele (Figure 9C). The Gsx2-Int5b primer binds in the deleted region of exon 1 before the Nco 1 site so homozygous mutants Gsx2EGFP/EGFPdo not have a wild-type band.
For staging of embryos, the morning of vaginal plug detection was designated as E0.5. At least three embryos of each genotype were examined for every stage studied and marker used. Embryos were fixed overnight in 4% paraformaldehyde at 4°C, rinsed extensively in phosphate-buffered saline and cryoprotected in 30% sucrose before sectioning at 12–14 μm on a cryostat. Sections were thaw-mounted onto SuperFrost®/Plus slides (Fisher Scientific, Pittsburgh, PA, USA) and stored at -20°C until used.
For immunohistochemistry, primary antibodies were used at the following concentrations: rabbit anti-Ascl1 (Mash1; 1:1,000; provided by J Johnson); rabbit anti-calbindin (1:2,500; provided by P Emson); goat anti-calretinin (1:2,000; Millipore, Billerica, MA, USA); rabbit anti-Dll (pan DLX; 1:400; provided by J Khotz); rabbit anti-FoxP1 (1:4,000; provided by E Morissey); rabbit anit-GAD67 (1:1,000; Millipore); goat anti-GFP (1:5,000; Abcam, Cambridge, MA, USA); rabbit anti-Gsx2 (1:5,000; [2]); rabbit anti-Gsx1/2 (1:2,000; provided by M Goulding); rabbit anti-Ki67 (1:1,000; Novocastra, Newcastle, UK); rabbit anti-Ngn2 (1:1,000; provided by M Nakafuku); rabbit anti-Sp8 (1:500; [26]). The secondary antibodies for brightfield staining were biotinylated swine anti-rabbit antibodies (1:200; DAKO, Glostrup, Denmark) and biotinylated horse anti-goat antibodies (1:200; Vector Laboratories, Burlingame, CA, USA). For visualization, the ABC kit (Vector Laboratories) followed by diaminobenzidine (DAB; Sigma, St. Louis, MO, USA) as the final chromogen were utilized. The secondary antibodies for fluorescent staining were donkey anti-goat antibodies conjugated to Cy2 (Jackson Immunoresearch, West Grove, PA, USA), and donkey anti-rabbit antibodies conjugated to Cy3 (Jackson Immunoresearch).
In situ hybrization histochemistry was performed using digoxygenin-labeled cRNA probes as described in Toresson et al. [41]. Probes used were Gsx1 [5], Hes5 and Dll1 [14].
Abbreviations
- bHLH:
-
basic helix-loop-helix
- CR:
-
calretinin
- E:
-
embryonic day
- ES:
-
embryonic stem
- dLGE:
-
dorsal lateral ganglionic eminence
- EGFP:
-
enhanced green fluorescent protein
- GAD67:
-
glutamic acid decarboxylase (67 kDa)
- LGE:
-
lateral ganglionic eminence
- SVZ:
-
subventricular zone
- VZ:
-
ventricular zone.
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Acknowledgements
We gratefully acknowledge the kind gifts of antibodies and probes from P Emson, M Goulding, J Johnson, J Kohtz, E Morrisey and M Nakafuku. This work was supported by the NIH grants NS044080 and MH069643 to KC and by the HFSPO grant RG160-2000B to FG and KC. RRW is supported by an NIH training grant (HD046387) and ZJA is supported by an NIH NRSA (DC008928).
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Authors' contributions
BW generated the Gsx2EGFPmice and carried out most of the experiments. RRW helped generate and characterize the Gsx2EGFPmice. ZJA helped with some of the immunohistochemistry experiments. FG provided the Ascl1 mice and helped conceive the experiments. KC supervised the studies and wrote the manuscript. All authors read and commented on the manuscript.
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Wang, B., Waclaw, R.R., Allen, Z.J. et al. Ascl1 is a required downstream effector of Gsx gene function in the embryonic mouse telencephalon. Neural Dev 4, 5 (2009). https://doi.org/10.1186/1749-8104-4-5
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DOI: https://doi.org/10.1186/1749-8104-4-5