 |
|||||
|
|||||
|
|||||
|
|||||
|
|||||
The Journal of Neuroscience, August 13, 2003, 23(19):7246-7254
Previous Article | Next Article
Formation of Whisker-Related Principal Sensory Nucleus-Based Lemniscal Pathway Requires a Paired Homeodomain Transcription Factor, Drg11
Yu-Qiang Ding,1,2,3 Jun Yin,1,2,3 Hai-Ming Xu,1,2,3 Mark F. Jacquin,4 andZhou-Feng Chen1,2,3 Departments of 1Anesthesiology, 2Psychiatry, 3Molecular Biology and Pharmacology, and 4Neurology, School of Medicine, Washington University, St. Louis, Missouri 63110
Abstract
Top
Abstract
Introduction
Little is known about the molecular mechanisms underlying the formation of the principal sensory nucleus (PrV) of the trigeminal nerve, a major relay station for somatotopic pattern formation in the trigeminal system. Here, we show that mice lacking Drg11, a homeodomain transcription factor, exhibit defects within the PrV, which include an aberrant distribution of Drg11-/- cells, altered expression of a molecular marker, unusual projections of primary afferents from trigeminal ganglion cells, and, subsequently, increased cell death. In addition, surviving PrV cells exhibit delayed and more spatially restricted ascending projections to the ventral posterior medial nucleus of the thalamus (VPm). These early embryonic abnormalities in the PrV lead to the failure to develop whisker-related patterns in the PrV, VPm, and somatosensory cortex. By contrast, somatotopic patterns exist in the spinal trigeminal subnuclei interpolaris (SpVi) and subnuclei caudalis (SpVc) and the dorsal column nucleus-based lemniscal and cortical pathway. Thus, the deficits in the trigeminal system of Drg11-/- mice are specific to the PrV. Our results demonstrate that Drg11 is essential for proper cellular differentiation and, subsequently, for the formation of the whisker-related lemniscal and cortical structures.
Key words: transcription factor; Drg11; barrel; principal sensory nucleus; subnucleus interpolaris; subnucleus caudalis; subnucleus oralis; morphogenesis
Introduction
The somatosensory map of the periphery is represented at different levels of the brainstem, thalamus, and somatosensory (S1) cortex. On the face of rodents, whiskers are organized in a reliable array. This pattern is relayed via the axons of trigeminal ganglion (TG) neurons to the cells in the trigeminal brainstem nuclei, which in turn project to the thalamus and to the S1 cortex via the thalamocortical afferents (TCAs) (Woolsey and Van der Loos, 1970; Woolsey, 1990
The well described somatotopic pattern in the trigeminal brainstem complex and its convenient detection make it one of the most attractive systems for studying fundamental mechanisms that control neuronal connection and pattern formation. Insofar as the whisker-related patterns are clearest during early postnatal periods, much of our knowledge regarding the formation of whisker-related patterns has been obtained by surgical manipulation of the periphery in postnatal animals (Woolsey, 1990
Drg11, a paired homeodomain transcription factor, is necessary for the assembly of the nociceptive circuitry in the dorsal spinal cord (Saito et al., 1995
Materials and Methods
Generation, maintenance, and genotyping of Drg11 mutant mice. Drg11+/- and Drg11-/- mice were generated and genotyped as described previously (Chen et al., 2001Histochemical staining. For cytochrome oxidase (CO) and NADPH stains, animals were perfused with 4% paraformaldehyde (PFA) at E18.5, E19.5, postnatal day (P) 1, P3, P7, or P14, and the brains were removed. After cryoprotection with 20% sucrose in 0.1 M PBS, pH 7.4, the brains were sectioned transversely at 50 µm or at 35 µm thickness tangentially (for viewing the barrels) in the S1 cortex, and then subjected to CO (Wong-Riley and Welt, 1980
For X-gal staining, embryos (E10.5-E13.5) were fixed with 4% PFA for 5 min, rinsed in PBS for 10 min, and incubated in PBS containing 0.15 M NaCl, 1 mM MgCl2, 0.003% Triton X-100, 0.001% potassium ferricyanide, 0.001% potassium ferrocyanide, and 1 mg/ml X-gal at 37°C for 1.5-2 hr. Some of embryos were sectioned at a thickness of 12 µm, and the sections were observed under the light microscope.
In situ hybridization, immunocytochemistry, and cell counting. For in situ hybridization, embryos (E10.5-E15.5, E18.5) were fixed in 4% PFA overnight and sunk in 15% sucrose. The embryos were frozen, sectioned, and kept on frosted slides. In situ hybridization was performed according to a procedure described previously (Birren et al., 1993
Terminal deoxynucleotidyl transferase-mediated biotinylated UTP nick end labeling (TUNEL) staining. After fixation with 4% PFA, the embryos (E14.5, E15.5, E16.5, E17.5, E18.5) were cryoprotected with 15% sucrose overnight, and serial 12-µm-thick sections were cut with a cryostat. The sections were directly mounted onto glass slides and then subjected to TUNEL examination (Gavrieli et al., 1992
DiI and DiI/DiA labeling. Embryos at different stages and postnatal mouse brains were fixed with 4% PFA. For the study of projections from the whisker follicle to the PrV, a small amount of 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate (DiI) or 4-[4-(dihexadecylamino)styryl]-N-methylpyridium iodide (DiA) (Molecular Probes) crystals were placed in the follicle(s). Tissues were kept in fixative at 37°C for 3-4 d (E12.5), 2 weeks (E13.5-E15.5), or 3-4 weeks (E16.5-E18.5). After the removal of the brainstems, they were vibratome sectioned transversely at 100 µm. Labeling was observed under an epifluorescent or laser confocal microscopy. The projections from the TG to the vibrissae follicles were examined by DiI labeling (E12.5-E15.5). DiI crystals were placed into the TG and kept between 5 d and 1 week. The projection from the PrV to the ventrobasal thalamus was studied at different stages as well (E14.5-E18.5). After the removal of the brains, they were cut in half at the level of the caudal pole of the PrV. DiI crystals were inserted into the PrV and stored for
1 week (E15.5) or 2-3 weeks (E16.5-E18.5). Placement of DiI crystals into the ventrobasal thalamus was performed in a similar way, and the materials were kept for 5-7 d (E14.5, E15.5) or 1-2 weeks (E18.5, P3, P10) for tracer diffusion.
Results
Drg11 exhibits spatially restricted expression in the trigeminal brainstem complex
To determine the spatiotemporal pattern of Drg11 expression in the developing trigeminal system, we examined the expression of Drg11 in the trigeminal nuclei at different embryonic stages by in situ hybridization or X-gal staining. An IRES-tau-lacZ marker was previously introduced into the Drg11 locus (Chen et al., 2001
View larger version (96K):
[in this window]
[in a new window]
Figure 1. Expression of Drg11 in the PrV, SpVi, and SpVc. Drg11 expression detected by X-gal staining (A,B) and in situ hybridization (C-F) in transverse sections through the hindbrain. A, At E10.5, Drg11 is expressed in presumptive PrV cells that begin to emerge from the ventricular zone of the ventral hindbrain (arrow). B, At E11.5, Drg11 expression increases as more PrV cells emerge from the ventricular zone (arrow). C, At E12.5, Drg11 expression is concentrated in the presumptive PrV region. D, At E15.5, Drg11 expression encompasses PrV. E, No Drg11 expression is detected in the SpVi. F, Drg11 is expressed in laminae I-II but not in III-IV of the SpVc. Mo, Motor trigeminal nucleus, t: spinal trigeminal tract. Scale bars, 100 µm.
Abnormal distribution of Drg11-/- cells and increased cell death in the PrV of Drg11-/- mice
To study the role of Drg11 in the development of the PrV, we first stained the PrV of Drg11+/- and Drg11-/- embryos with X-gal at different stages. Up to E12.5, no difference in the staining pattern of migrating PrV cells was detected between Drg11+/- and Drg11-/- embryos (data not shown). Over the next few days, presumptive PrV cells continued their ventrolateral migration, as described previously (al-Ghoul and Miller, 1993To assess the distribution of Drg11-/- cells in Drg11-/- mutants, Drg11-/- cells in the PrV were monitored by the use of anti-Neo immunocytochemistry (Chen et al., 2001
View larger version (90K):
[in this window]
[in a new window]
Figure 2. Immunocytochemical staining of neo+ cells and TUNEL studies of the PrV in wild-type and Drg11-/- mice. A, B, Neo staining (red) and Hoechst countstaining (green) of the PrV in wild-type (A,C) and Drg11 (B,D) mutants at E14.5. Arrowheads indicate the region where few Drg11-/-/neo+ cells were found. C,D, Higher magnification of A,B. E, Comparison of the number of Drg11+/- and Drg11-/- cells in the PrV at E14.5. Neo+ cells in Drg11+/- embryos at E14.5, 143.7 ± 8.1; in Drg11-/- embryos, 135.4 ± 5.2; p = 0.061 (p > 0.05). F,G, Neo staining (red) in the PrV of the wild-type embryos (F) and the mutant (G) at E16.5, Note that in the most ventral aspect (arrowheads) of the mutant PrV, Drg11-/- cells appear to avoid certain regions. H, Comparison of the number of Drg11+/- and Drg11-/- cells in the PrV at E14.5. Neo+ cells in Drg11+/- embryos at E16.5, 153.6 ± 8.7; in Drg11-/- embryos, 160.3 ± 13.7; p = 0.72 (p > 0.05). I,J, At E18.5, TUNEL studies revealed increased cell death in the mutant PrV (J, arrow) compared with the wild-type PrV (I, arrows). K, Comparison of the number of apoptotic cells in the PrV between wild-type and Drg11 mutant embryos at E18.5. The average number of apoptotic cells in the PrV. Wild-type embryo, 5.3 ± 1.4; Drg11 mutant, 15.0 ± 2.3; p = 0.015 (p < 0.05). Scale bars, 100 µm.
To ascertain whether an abnormally increased cell death occurs in the PrV of Drg11-/- embryos, TUNEL staining was performed. Whereas TUNEL staining was normal before E18.5 (data not shown), the number of TUNEL+ cells in the mutant PrV was significantly increased in the mutants at E18.5 (Fig. 2I-K). By contrast, no abnormal cell death was noted in the SpVi and in the deep laminae of the SpVc of Drg11-/- embryos at this stage (data not shown). Therefore, the earliest stage when we could identify a morphological abnormality in the PrV is at E14.5, and abnormal PrV cell death was first detected at E18.5.
Loss of Ebf1 expression in the PrV of Drg11-/- mice
To determine whether Drg11 is required for expression of other transcription factors in PrV cells, a panel of molecular markers were examined in the PrV of Drg11-/- embryos. Early B-cell factors (Ebf)/olfactory factor 1 are members of the helix-loop-helix transcription factors and play multiple roles in a variety of developmental processes (Dubois and Vincent, 2001
View larger version (100K):
[in this window]
[in a new window]
Figure 3. Expression of molecular markers in the PrV detected by in situ hybridization. Transverse sections of the E14.5 PrV of wild-type (A,C,E,G)andDrg11-/-(B, D, F, H)embryos. A,B, Ebf1 expression is detected in the wild type (A), but not in the mutant (B). No significant changes are found in the expression pattern of Ebf2 (C,D), Ebf3 (E,F), and Rnx (G,H) between the wild-type and mutant PrV at E14.5. Scale bar, 100 µm.
Abnormal central projections of TG afferents in Drg11-/- mice
To assess the central projections of TG afferents, rows of vibrissal follicles of Drg11-/- embryos were labeled with DiI. At E11.5, afferents in Drg11-/- embryos have reached the brainstem on a normal time schedule (data not shown). On arriving at the brainstem, TG afferents bifurcate: the rostral branches enter the PrV, whereas the caudal branches innervate the trigeminal spinal nuclei. By E14.5, both wild-type and mutant TG afferents from the b2 vibrissae follicle penetrated the PrV, and no major difference in the projection pattern was found between wild-type and Drg11-/- mice (Fig. 4A,B). One day later, afferents from the c2 and d2 vibrissal follicles grow toward the more inner medial region of the PrV (Fig. 4C,D). The density and morphology of DiI-labeled collaterals in the mutant PrV were indistinguishable from those in the wild-type controls. By E16.5, in wild-type embryos, DiI-labeled fibers from the b2 and b3 follicles were much more abundant and have reached the inner portion of the PrV (Fig. 4E). However, in the mutants, the projections of TG afferents were abnormal (Fig. 4F). Most fibers had unusual orientations for the b row axons in having more ventromedial trajectories in the PrV than normal controls. A few fibers had aberrant dorsolateral trajectories (Fig. 4F). At E18.5, wild-type fibers from the c2 vibrissae follicle gave rise to collaterals that aggregated into a single cluster that is confined to the ventromedial region of the PrV (Fig. 4G). In the mutant, consistent with the aforementioned E16.5 projection pattern, DiI-labeled fibers from the c2 follicle did not enter the inner medial region of the PrV (Fig. 4H). Rather, they were confined to a ventrolateral position (Fig. 4H). These aberrant projections suggest that there are pathfinding errors for immature trigeminal afferents in the mutants. In contrast, mutant TG afferents appeared to innervate the SpVi in a normal manner at this stage (Fig. 4I,J).
View larger version (85K):
[in this window]
[in a new window]
Figure 4. Central and peripheral projections of TG afferents in wild-type and Drg11 mutant embryos as revealed by DiI staining. A,B, At E14.5, both wild-type (A) and mutant (B) TG afferents enter the PrV (arrows). Note that DiI crystals were applied to the b2 vibrissal follicle. C,D, At E15.5, more DiI-labeled axons are observed within the wild-type (C) and mutant (D) PrV. Most afferents have a dorsomedial trajectory (C,D, arrows). No major abnormality is noted in the mutant (D). Note that DiI crystals were applied to the c2 and d2 vibrissal follicles. E,F, At E16.5, DiI-labeled wild-type afferents further reach the inner region of the PrV with a dorsomedial trajectory (E, arrow). The mutant afferents display ventromedial trajectories (F, arrow). A few afferent fibers grow aberrantly in a dorsolateral direction (F, arrowheads). Note that DiI crystals were applied in the b2 and b3 vibrissal follicles. G,H, At E18.5, TG afferents become clustered (G, arrow) in the inner region of the PrV in wild-type mice (G, arrow). By contrast, mutant afferent clusters are located in more ventrolateral regions (H, arrow). Note that DiI crystals were placed in the c2 vibrissal follicle. These images were obtained through the use of a laser confocal microscope. I,J, No difference in the projection patterns of TG afferents is found between the SpVi of wild-type (I, arrow) and mutant (J, arrow). Note that DiI crystals were placed in the b2 and b3 follicles. K,L, DiI tracing of TG afferents to the vibrissal follicles of E15.5 wild-type (K, arrow) and mutant (L, arrow). Note that DiI-labeled fibers surround the base of the follicles and exhibit a circumferential profile (K,L, arrows). Scale bars, 100 µm.
We also assessed the projections of TG afferents to the vibrissae follicles by labeling of TG cells with DiI crystals. Between E12.5 and E14.5, TG axons appeared to normally grow toward the periphery in Drg11-/- embryos (data not shown). By E15.5, DiI tracing revealed mutant afferents encircling individual follicles as in wild-type afferents (Fig. 4K,L). The density of TG afferents enveloping vibrissal follicles also appeared similar between wild-type and Drg11-/- embryos. In addition, X-gal staining also failed to distinguish wild-type and mutant projections (data not shown). These results suggest that the peripheral projections of TG afferents are grossly normal in Drg11-/- embryos.
Site-specific deficits in somatotopic pattern formation in Drg11-/- mice
The abnormal development of the PrV promoted examination of whisker-related pattern formation in Drg11-/- mice by CO staining. Histochemical staining of CO activity in somata, dendrites, and axonal terminals in different subcortical and cortical regions identifies individual cell aggregates, or patches, each corresponding to single whiskers in rodents (Wong-Riley and Welt, 1980
View larger version (141K):
[in this window]
[in a new window]
Figure 5. Somatotopic patterns in Drg11-/- and wild-type mice. A-J, CO staining of the whisker-like patterns in the PrV (A,B), VPm (C,D), S1 cortex (E,F, tangential section), SpVi (G,H), and SpVc (I,J). Note the absence of CO-stained patterns in the mutant PrV (B), VPm (D), and S1 cortex (F) but the presence of the patterns in the SpVi (H) and SpVc (J) of Drg11-/- mice. In the VPl thalamus and S1 cortex of the mutant, forepaw digit patterns were present (C,F, arrows). M,O, NADPH expression exhibits whisker-like patterns in the PrV (M) and S1 cortex (O) of wild-type mice and their absence in Drg11-/- mice (N, P). K,L, CO staining of the hindpaw digit patterns in the gracile nucleus (GN) of wild-type (K) mice and in the mutant (L). I-II, laminae I and II of the SpVc; III-IV, laminae III and IV of the SpVc; wp, whiskerpad representation; fp, forepaw representation. Scale bars, 100 µm.
The lack of patterning in specific portions of the barrel neuraxis, as revealed by CO staining, could also be because of a lack of CO activity or a metabolic abnormality in CO synthesis, as opposed to a lack of neuronal patterning. To assess this possibility, we used an alternative staining method: expression of NADPH (Mitrovic and Schachner, 1996
To assess whether lack of CO and NADPH patterning was because of a failure in either pattern formation or pattern maintenance in Drg11-/- mutants, we performed CO and NADPH histochemistry from the earliest stage at which patterns are normally visible. In wild-type controls, the patterns first emerge in the brainstem at E18.5, as detected by CO staining, in the VPm at P2 and in the S1 cortex at P3 (Ma, 1993
We next assessed pattern formation in the DCN-based lemniscal pathway. In wild-type mice, forepaw and hindpaw digits were recognizable as discrete patches in the VPl and S1 cortex by CO staining (Fig. 5C,E) (data not shown). Forepaw and hindpaw digit patches were also identified in the VPl thalamus and S1 cortex of Drg11-/- mice (Fig. 2D,F) (data not shown). The digit patterns were also present in the gracile nucleus and cuneate nucleus of the mutant DCN (Fig. 5K, L). Thus, both hindpaw and forepaw digit patterns developed in Drg11-/- mice.
Delayed thalamic projections of PrV cells in Drg11-/- mice
The abnormal distribution of PrV cells, the loss of Ebf1 expression, and increased TUNEL staining indicated that the development of the PrV is severely impaired in Drg11-/- mice. Do PrV cells project normally to the contralateral VPm in Drg11-/- embryos? To address this question, PrV axons were anterogradely labeled with DiI. To exclude the possibility that labeling may spuriously include the SpVi, the caudal brainstem at the level of the caudal pole of the PrV was removed before applying DiI to the PrV. At E17.5, PrV axons have reached the VPm and outline the contour of the VPm (Fig. 6A). However, at this stage, PrV axons labeled by DiI were not detected in the VPm of Drg11-/- embryos (Fig. 6B). By E19.5, the mutant PrV axons have reached the VPm, but the intensity and areal expanse of labeling was much less (Fig. 6C,D), suggesting that the projections of PrV axons were greatly reduced in number and area. We next examined the morphology of the VPm by Nissl staining. No difference in the gross morphology of the VPm between Drg11-/- and wild-type embryos was found up to E18.5 (data not shown). These data demonstrated a delayed projection of PrV efferents to the VPm and a resultant projection that is reduced in areal extent. Given that Drg11 is not expressed in the VPm, the projection abnormalities of PrV cells must reflect an abnormal development of PrV cells, rather than a target field defect.
View larger version (77K):
[in this window]
[in a new window]
Figure 6. Projections of PrV efferents and TCAs revealed by DiI tracing. A-D, DiI tracing of PrV projections in the VPm. A,B, Whereas PrV efferents are present in the E17.5 wild-type VPm (A), no DiI-labeled axons are present in the mutant VPm (B). C,D, At E19.5, DiI-labeled PrV efferents are found in both the wild-type (C) and mutant (D) VPm, but the extent of DiI labeling in the mutant is much reduced (D). E-H, DiI tracing of TCAs in the S1 cortex. E,F, At E15.5, TCAs of wild-type and mutants labeled by DiI are found in the S1 cortex. Arrows point to the growth cones of TCAs that arrive at S1 cortex. No major difference is found in the projection patterns. G,H, The projection of TCAs in layer IV of the cortex at P10. In wild-type mice (G), DiI-labeled axons aggregate to form individual patches corresponding to single barrels (G, arrows), but in the mutant (H), DiI-labeled axons are distributed evenly. Scale bar, 100 µm.
Lack of a barrel-like distribution of TCAs in Drg11-/- mice
To determine whether TCAs project to the S1 cortex and form whisker-like patterns in Drg11-/- mice, the projections of TCAs to the cortex were examined by applying DiI crystals to the ventrobasal thalamus and anterogradely labeling their projections during development. TCAs originating in the ventrobasal thalamus grow ventrally, project through the internal capsule, and then turn dorsally to reach the neocortex before they branch off to the nascent layer IV of the S1 cortex (Bernardo and Woolsey, 1987TCAs branch to layer IV of the S1 cortex initially in a uniform distribution pattern and later are sculpted into whisker-related patches (Rebsam et al., 2002
Normal gross topography of TG afferents in Drg11-/- mice
Somatotopic pattern formation in subcortical regions requires topographic projections of primary afferents. Although patterns first develop during the late embryonic stages or early postnatal periods, the topography of afferent projections is established much earlier (Erzurumlu and Jhaveri, 1992
View larger version (76K):
[in this window]
[in a new window]
Figure 7. Topographic organization of the TG projections revealed by DiI and DiA double labeling. A-D, DiI and DiA were applied in the dorsal and ventral vibrissae follicles of wild-type (A,C) and mutant (B,D) embryos, respectively, at E12.5. DiI-labeled (red; arrows) and DiA-labeled (green; arrowheads) axons are segregated in the TG (A,B), PrV (A,B), and SpVi (C,D). No major difference between the wild type and mutant is noted. E,H, DiI crystals were applied to distinct vibrissae follicles of wild-type (E,G) and mutant (F,H) embryos, respectively, at E15.5. Two well separated foci of DiI-labeled afferents mark distinct clusters of TG afferents in the PrV (E,F, arrowheads) and SpVi (G,H, arrowheads). Note the equivalent locations and densities of labeled afferents in the wild type and mutants. Scale bar, 100 µm.
Discussion
The molecular mechanisms underlying the development of the PrV-based lemniscal pathway are poorly understood. In this study, we have characterized the development of the PrV in Drg11-/- mice and found that in the absence of Drg11, Drg11-/- cells distribute abnormally and PrV efferents project to VPm aberrantly, followed by an increase of abnormal cell death in the PrV. Moreover, the projections of TG afferents to the PrV are aberrant. As a result, whisker-related patterns fail to form in the PrV, VPm, and S1 cortex. By contrast, such patterns form in the SpVi, SpVc, DCN, and associated VPl and limb cortex. Together, our results demonstrate that Drg11 is essential for the proper development of the PrV cells and is the first identified molecule that distinguishes the PrV-based lemniscal pathway from the SpVi-based paralemniscal pathway.Drg11 is required for the development of the PrV
Drg11 is the earliest known marker that marks the birth of PrV cells (Fig. 1). Insofar as the onset of Drg11 expression coincides with the migration of PrV cells, Drg11 could be involved in migration. By the use of tau-lacZ as a marker, no notable difference in the migratory behavior of PrV cells was observed in the absence of Drg11 function between E11.5 and E13.5. Nevertheless, one cannot completely rule out the possibility that a subset of the mutant PrV cells may migrate aberrantly. Once the cells have reached their destination, and begin to form the PrV, several prominent molecular and cellular abnormalities occur in Drg11-/- embryos: an abnormal distribution of Drg11-/- cells, the loss of Ebf1 expression, aberrant thalamic projections, and abnormal cell death (Figs. 2, 3, 6). In addition, aberrant projections of TG afferents within the PrV are also found (Fig. 4). The timing of each defect that occurs is significant because it permits reasonable interpretation of the primary locus of the action of the mutation. The latter is believed to be PrV morphogenesis in light of the following: the first sign of abnormal distribution of the PrV cells and loss of Ebf1 gene expression are detected at E14.5, abnormal projections of TG afferents to the PrV at E16.5, a delayed and reduced thalamic projections at E17.5, followed by an increased cell death in the PrV at E18.5. The finding that there is a segregation of Drg11-/- cells from non-Drg11-expressing cells in the outermost PrV, as reflected in neo expression pattern, strongly suggests that Drg11 is involved in the morphogenesis of the PrV cells (Fig. 2). This phenotype is reminiscent of the abnormal dorsal horn morphology detected in Drg11-/- embryos, suggesting that Drg11 may control the similar cellular events in both regions (Chen et al., 2001Because Drg11 is expressed in both the TG and PrV, one important issue to consider is whether the abnormal projections of TG primary afferents reflect a primary requirement for Drg11 in the TG or PrV, or both. Several lines of evidence support the notion that a lack of whisker-related patterning primarily reflects the defects in the PrV, rather than a defect in the TG. First, intra-axonal labeling of hundreds of TG afferents revealed that the same axons of TG neurons always innervate both the PrV and SpVi (Hayashi, 1980
A previous study showed that a homeodomain transcription factor, Rnx, is required for the maintenance of Drg11 expression (Qian et al., 2002
Drg11-dependent formation of PrV-based lemniscal pathway
In Drg11-/- mice, somatotopic patterning in the PrV, VPm, and S1 cortex is disrupted, as demonstrated by histochemical and Nissl staining and DiI labeling (Fig. 5) (data not shown). Whereas abnormal morphogenesis of PrV cells and central projection deficits in the PrV are first detected in Drg11-/- mice between E14.5 and E16.5, abnormal patterning is only apparent a few days later, when patterns are first visible normally (Chiaia et al., 1992The delay in arrival of PrV-thalamic projections must reflect an intrinsic impairment of PrV cells because Drg11 is not expressed in the VPm (Fig. 6). Furthermore, the reduced areal expanse of PrV-thalamic projections at E19.5 may simply reflect the reduced number of PrV cells caused by early cell death (Fig. 2) (data not shown). Despite the seeming absence of PrV inputs to the thalamus before E19.5, TCAs do navigate to layer IV of the S1 cortex without delay (Fig. 6). This is consistent with previous observations that the navigation of TCAs toward the cortex is a target- and environment-dependent process and does not require PrV-relayed, whisker-related inputs (Molnar and Blakemore, 1995
Drg11: a key molecular determinant that distinguishes the formation of the PrV-based leminscal pathway from SpViand SpVc-based pathway
An important finding in the present study is that the PrV-based whisker-related lemniscal and cortical patterns fail to form in Drg11-/- mice, whereas somatotopic patterns form in the SpVi-based paralemniscal pathway and in the SpVc. Moreover, forepaw and hindpaw digit patterning also develops in the DCN, VPl, and S1 cortex (Fig. 5). Therefore, the patterning effect in Drg11-/- mice displays an unprecedented specificity.The SpVi-based lemniscal and the SpVi-based paralemniscal pathways are parallel pathways that take origin in patterned nuclei. However, their thalamic projection patterns are different: the PrV cells terminate preferentially in the VPm, whereas the SpVi thalamic-projecting cells terminate preferentially in the posterior nucleus of the thalamus (Williams et al., 1994
Footnotes
Received Apr. 22, 2003; revised Jun. 5, 2003; accepted Jun. 17, 2003.This work was supported by a National Institutes of Health (NIH) RO1 grant and a grant from McDonnell Center for Molecular and Cellular Neurobiology to Z-F.C., and NIH Grant PO1-DE07734 to M.F.J. We thank Dr. Thomas Woolsey for critical comments on this manuscript and discussion.
Correspondence should be addressed to Dr. Zhou-Feng Chen, Departments of Anesthesiology, Psychiatry, and Molecular Biology and Pharmacology, School of Medicine, Washington University, St. Louis, MO 63110. E-mail: chenz{at}morpheus.wustl.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/237246-09$15.00/0
References
Agmon A, Yang LT, O'Dowd DK, Jones EG (1993) Organized growth of thalamocortical axons from the deep tier of terminations into layer IV of developing mouse barrel cortex. J Neurosci 13: 5365-5382.[Abstract]
al-Ghoul WM, Miller MW (1993) Orderly migration of neurons to the principal sensory nucleus of the trigeminal nerve of the rat. J Comp Neurol 330: 464-475.[Web of Science][Medline]
Bates CA, Killackey HP (1985) The organization of the neonatal rat's brainstem trigeminal complex and its role in the formation of central trigeminal patterns. J Comp Neurol 240: 265-287.[Web of Science][Medline]
Bates CA, Erzurumlu RS, Killackey HP (1982) Central correlates of peripheral pattern alterations in the trigeminal system of the rat. III. Neurons of the principal sensory nucleus. Brain Res 281: 108-113.[Medline]
Bernardo KL, Woolsey TA (1987) Axonal trajectories between mouse somatosensory thalamus and cortex. J Comp Neurol 258: 542-564.[Web of Science][Medline]
Birren SJ, Lo L, Anderson DJ (1993) Sympathetic neuroblasts undergo a developmental switch in trophic dependence. Development 119: 597-610.
[Abstract/Free Full Text] Braisted JE, Tuttle R, O'Leary DD (1999) Thalamocortical axons are influenced by chemorepellent and chemoattractant activities localized to decision points along their path. Dev Biol 208: 430-440.[Web of Science][Medline]
Braisted JE, Catalano SM, Stimac R, Kennedy TE, Tessier-Lavigne M, Shatz CJ, O'Leary DD (2000) Netrin-1 promotes thalamic axon growth and is required for proper development of the thalamocortical projection. J Neurosci 20: 5792-5801.
[Abstract/Free Full Text] Cases O, Vitalis T, Seif I, De Maeyer E, Sotelo C, Gaspar P (1996) Lack of barrels in the somatosensory cortex of monoamine oxidase A-deficient mice: role of a serotonin excess during the critical period. Neuron 16: 297-307.[Web of Science][Medline]
Chen ZF, Rebelo S, White F, Malmberg AB, Baba H, Lima D, Woolf CJ, Basbaum AI, Anderson DJ (2001) The paired homeodomain protein DRG11 is required for the projection of cutaneous sensory afferent fibers to the dorsal spinal cord. Neuron 31: 59-73.[Web of Science][Medline]
Chiaia NL, Bennett-Clarke CA, Rhoades RW (1991) Effects of cortical and thalamic lesions upon primary afferent terminations, distributions of projection neurons, and the cytochrome oxidase pattern in the trigeminal brainstem complex. J Comp Neurol 303: 600-616.[Web of Science][Medline]
Chiaia NL, Bennett-Clarke CA, Eck M, White FA, Crissman RS, Rhoades RW (1992) Evidence for prenatal competition among the central arbors of trigeminal primary afferent neurons. J Neurosci 12: 62-76.[Abstract]
Cohen-Tannoudji M, Babinet C, Wassef M (1994) Early determination of a mouse somatosensory cortex marker. Nature 368: 460-463.[Medline]
Diamond ME, Armstrong-James M, Budway MJ, Ebner FF (1992) Somatic sensory responses in the rostral sector of the posterior group (POm) and in the ventral posterior medial nucleus (VPM) of the rat thalamus: dependence on the barrel field cortex. J Comp Neurol 319: 66-84.[Web of Science][Medline]
Ding YQ, Wang YQ, Qin BZ, Li JS (1993) The major pelvic ganglion is the main source of nitric oxide synthase-containing nerve fibers in penile erectile tissue of the rat. Neurosci Lett 164: 187-189.[Medline]
Dubois L, Vincent A (2001) The COE-Collier/Olf1/EBF-transcription factors: structural conservation and diversity of developmental functions. Mech Dev 108: 3-12.[Web of Science][Medline]
Erzurumlu RS, Jhaveri S (1992) Trigeminal ganglion cell processes are spatially ordered prior to the differentiation of the vibrissa pad. J Neurosci 12: 3946-3955.[Abstract]
Erzurumlu RS, Kind PC (2001) Neural activity: sculptor of 'barrels' in the neocortex. Trends Neurosci 24: 589-595.[Web of Science][Medline]
Gavrieli Y, Sherman Y, Ben-Sasson SA (1992) Identification of programmed cell death in situ via specific labeling of nuclear DNA fragmentation. J Cell Biol 119: 493-501.
[Abstract/Free Full Text] Hayashi H (1980) Distributions of vibrissae afferent fiber collaterals in the trigeminal nuclei as revealed by intra-axonal injection of horseradish peroxidase. Brain Res 183: 442-446.[Web of Science][Medline]
Henderson TA, Woolsey TA, Jacquin MF (1992) Infraorbital nerve blockade from birth does not disrupt central trigeminal pattern formation in the rat. Brain Res Dev Brain Res 66: 146-152.[Medline]
Henderson TA, Johnson EM, Osborne PA, Jacquin MF (1994) Fetal NGF augmentation preserves excess trigeminal ganglion cells and interrupts whisker-related pattern formation. J Neurosci 14: 3389-3403.[Abstract]
Iwasato T, Erzurumlu RS, Huerta PT, Chen DF, Sasaoka T, Ulupinar E, Tonegawa S (1997) NMDA receptor-dependent refinement of somatotopic maps. Neuron 19: 1201-1210.[Web of Science][Medline]
Jacquin MF, Chiaia NL, Haring JH, Rhoades RW (1990) Intersubnuclear connections within the rat trigeminal brainstem complex. Somatosens Mot Res 7: 399-420.[Web of Science][Medline]
Jhaveri S, Erzurumlu RS, Chiaia N, Kumar TR, Matzuk MM (1998) Defective whisker follicles and altered brainstem patterns in activin and follistatin knockout mice. Mol Cell Neurosci 12: 206-219.[Medline]
Killackey HP, Fleming K (1985) The role of the principal sensory nucleus in central trigeminal pattern formation. Brain Res 354: 141-145.[Medline]
Killackey HP, Jacquin MF, Rhoades RW (1990) The somatosensory system. In: Development of sensory systems in mammals (Coleman JR, ed). New York: Wiley.R. W.
Kutsuwada T, Sakimura K, Manabe T, Takayama C, Katakura N, Kushiya E, Natsume R, Watanabe M, Inoue Y, Yagi T, Aizawa S, Arakawa M, Takahashi T, Nakamura Y, Mori H, Mishina M (1996) Impairment of suckling response, trigeminal neuronal pattern formation, and hippocampal LTD in NMDA receptor epsilon 2 subunit mutant mice. Neuron 16: 333-344.[Web of Science][Medline]
Li Y, Erzurumlu RS, Chen C, Jhaveri S, Tonegawa S (1994) Whisker-related neuronal patterns fail to develop in the trigeminal brainstem nuclei of NMDAR1 knockout mice. Cell 76: 427-437.[Web of Science][Medline]
Logan C, Wingate RJ, McKay IJ, Lumsden A (1998) Tlx-1 and Tlx-3 homeobox gene expression in cranial sensory ganglia and hindbrain of the chick embryo: markers of patterned connectivity. J Neurosci 18: 5389-5402.
[Abstract/Free Full Text] Ma PM (1993) Barrelettes-architectonic vibrissal representations in the brainstem trigeminal complex of the mouse. II. Normal post-natal development. J Comp Neurol 327: 376-397.[Web of Science][Medline]
Mitrovic N, Schachner M (1996) Transient expression of NADPH diaphorase activity in the mouse whisker to barrel field pathway. J Neurocytol 25: 429-437.[Web of Science][Medline]
Molnar Z, Blakemore C (1995) How do thalamic axons find their way to the cortex? Trends Neurosci 18: 389-397.[Web of Science][Medline]
Pereira A, Freire MAM, Bahia CP, Franca JG, Picanco-Diniz CW (2000) The barrel field of the adult mouse SmI cortex as revealed by NADPH-diaphorase histochemistry. Neuroreport 11: 1889-1892.[Medline]
Qian Y, Shirasawa S, Chen CL, Cheng L, Ma Q (2002) Proper development of relay somatic sensory neurons and D2/D4 interneurons requires homeobox genes Rnx/Tlx-3 and Tlx-1. Genes Dev 16: 1220-1233.
[Abstract/Free Full Text] Rebsam A, Seif I, Gaspar P (2002) Refinement of thalamocortical arbors and emergence of barrel domains in the primary somatosensory cortex: a study of normal and monoamine oxidase a knock-out mice. J Neurosci 22: 8541-8552.
[Abstract/Free Full Text] Saito T, Greenwood A, Sun Q, Anderson DJ (1995) Identification by differential RT-PCR of a novel paired homeodomain protein specifically expressed in sensory neurons and a subset of their CNS targets. Mol Cell Neurosci 6: 280-292.[Web of Science][Medline]
Senft SL, Woolsey TA (1991) Growth of thalamic afferents into mouse barrel cortex. Cereb Cortex 1: 308-335.
[Abstract/Free Full Text] Shortland PJ, Demaro JA, Shang F, Waite PM, Jacquin MF (1996) Peripheral and central predictors of whisker afferent morphology in the rat brainstem. J Comp Neurol 375: 481-501.[Web of Science][Medline]
Tracey DJ, Waite PME (1995) Somatosensory system. In: The rat nervous system (Paxinos G, ed). San Diego: Academic.
Wang MM, Reed RR (1993) Molecular cloning of the olfactory neuronal transcription factor Olf-1 by genetic selection in yeast. Nature 364: 121-126.[Medline]
Wang SS, Tsai RYL, Reed RR (1997) The characterization of the Olf-1/EBF-like HLH transcription factor family: implications in olfactory gene regulation and neuronal development. J Neurosci 17: 4149-4158.
[Abstract/Free Full Text] Williams MN, Zahm DS, Jacquin MF (1994) Differential foci and synaptic organization of the principal and spinal trigeminal projections to the thalamus in the rat. Eur J Neurosci 6: 429-453.[Web of Science][Medline]
Willis WD, Coggeshall RE (1991) Sensory mechanisms of the spinal cord. London: Plenum.
Wong-Riley MT, Welt C (1980) Histochemical changes in cytochrome oxidase of cortical barrels after vibrissal removal in neonatal and adult mice. Proc Natl Acad Sci USA 77: 2333-2337.
[Abstract/Free Full Text] Woolsey TA (1990) Peripheral alteration and somatosensory development. In: Development of sensory systems in mammals (Coleman JR, ed), pp 461-516. New York: Wiley.
Woolsey TA, Van der Loos H (1970) The structural organization of layer IV in the somatosensory region (SI) of mouse cerebral cortex. The description of a cortical field composed of discrete cytoarchitectonic units. Brain Res 17: 205-242.[Web of Science][Medline]
This article has been cited by other articles:
M. F. Jacquin, J. J. A. Arends, C. Xiang, L. A. Shapiro, C. E. Ribak, and Z.-F. Chen
In DRG11 Knock-Out Mice, Trigeminal Cell Death Is Extensive and Does Not Account for Failed Brainstem Patterning
J. Neurosci., April 2, 2008; 28(14): 3577 - 3585.
[Abstract] [Full Text] [PDF]
C.-L. Wang, L. Zhang, Y. Zhou, J. Zhou, X.-J. Yang, S.-m. Duan, Z.-Q. Xiong, and Y.-Q. Ding
Activity-Dependent Development of Callosal Projections in the Somatosensory Cortex
J. Neurosci., October 17, 2007; 27(42): 11334 - 11342.
[Abstract] [Full Text] [PDF]
F. Oury, Y. Murakami, J.-S. Renaud, M. Pasqualetti, P. Charnay, S.-Y. Ren, and F. M. Rijli
Hoxa2- and Rhombomere-Dependent Development of the Mouse Facial Somatosensory Map
Science, September 8, 2006; 313(5792): 1408 - 1413.
[Abstract] [Full Text] [PDF]
L.-J. Lee, F.-S. Lo, and R. S. Erzurumlu
NMDA Receptor-Dependent Regulation of Axonal and Dendritic Branching
J. Neurosci., March 2, 2005; 25(9): 2304 - 2311.
[Abstract] [Full Text] [PDF]
S. M. Adams, J. C. de Rivero Vaccari, and R. A. Corriveau
Pronounced Cell Death in the Absence of NMDA Receptors in the Developing Somatosensory Thalamus
J. Neurosci., October 20, 2004; 24(42): 9441 - 9450.
[Abstract] [Full Text] [PDF]
This Article Abstract 
Full Text (PDF) Submit an eLetter Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager 
Citing Articles Citing Articles via HighWire Citing Articles via Web of Science (14) Citing Articles via Google Scholar Google Scholar Articles by Ding, Y.-Q. Articles by Chen, Z.-F. Search for Related Content PubMed PubMed Citation Articles by Ding, Y.-Q. Articles by Chen, Z.-F.
|
|
|
|
 |
|