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The Journal of Neuroscience, October 15, 2000, 20(20):7664-7671
Facial Visceral Motor Neurons Display Specific Rhombomere Origin and Axon Pathfinding Behavior in the Chick
John Jacob and Sarah Guthrie Medical Research Council Centre for Developmental Neurobiology, King's College, Guy's Campus, London SE1 1UL, United Kingdom
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
In the chick embryo, facial motor neurons comprise branchiomotor and visceral motor subpopulations, which innervate branchial muscles and parasympathetic ganglia, respectively. Although facial motor neurons are known to develop within hindbrain rhombomere 4 (r4) and r5, the precise origins of branchiomotor and visceral motor neuron subpopulations are unclear. We investigated the organization and axon pathfinding of these motor neurons using axonal tracing and rhombomere transplantation in quail-chick chimeras. Our results show that a large majority of branchiomotor neurons originate in r4 but that a cohort of these neurons undergoes a caudal migration from r4 into r5. By contrast, visceral motor neurons develop exclusively in r5. We found that a striking property of facial visceral motor neurons is the ability of their axons to navigate back to appropriate ganglionic targets in the periphery after heterotopic transplantation. These results complement previous studies in which heterotopic facial branchiomotor neurons sent axons to their correct, branchial arch, target. By contrast, when trigeminal branchiomotor neurons were transplanted heterotopically, we found that they were unable to pathfind correctly, and instead projected to an inappropriate target region. Thus, facial and trigeminal motor neuron populations have different axon pathfinding characteristics.
Key words: facial nerve; branchiomotor neuron; visceral motor neuron; rhombomere; hindbrain; axon pathfinding
INTRODUCTION
Cranial motor neurons innervate a variety of muscles and ganglia in the vertebrate head. Within the embryonic chick hindbrain, trigeminal motor neurons occupy rhombomere 2 (r2) and r3, whereas facial motor neurons occupy r4 and r5 (Lumsden and Keynes, 1989
; Lumsden 1990
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Figure 1. Distribution of motor neurons in the hindbrain and summary of rhombomere transplants. A, Diagram of the ventral aspect of a stage 21 chick embryo showing the motor nuclei of the branchial nerves (V, trigeminal; VII, facial; IX, glossopharyngeal; and X/XI, vagus/cranial accessory) and the somatic motor nuclei (III, oculomotor; IV, trochlear; VI, abducens; and XII, hypoglossal) based on axon tracing (modified after Lumsden, 1990
In the rodent embryo, BM and VM neurons occupy r4 and r5, respectively (Fritzsch and Nichols, 1993
BM and VM axons from particular axial levels actively pathfind to target regions that are populated by neural crest cells derived from the same axial level (Lumsden et al., 1991
We have investigated the distribution of facial BM and VM neurons in chick embryos, by axon tracing, and by testing the repertoire of axon projections derived from r4 and r5 when these were transplanted orthopically in quail-chick chimeras. Orthotopic r4 transplants were also used to examine whether BM neurons migrate caudally from r4 into r5. Heterotopic rhombomere transplants were then used to discover whether graft-derived BM or VM axons navigated to appropriate or inappropriate targets in the periphery.
MATERIALS AND METHODS
Retrograde labeling. Rhode Island Red hens' eggs were incubated at 38°C to stage 20-28 (Hamburger and Hamilton, 1951
Retrograde labeling of the hyoid nerve in stage 25 embryos with an r4 orthotopic graft was performed in a few cases, to track the migration pattern of BM neurons in this rhombomere. These embryos were fixed in Dent's fixative (1:4 DMSO-methanol) before immunofluorescence using QCPN antibody (which recognizes a quail-specific perinuclear antigen; Developmental Hybridoma Bank, Iowa City, IA).
Microsurgery. Stage 10-12 embryos were used in stage-matched quail-to-chick orthotopic and heterotopic grafting experiments. Operations were performed as previously described (Guthrie and Lumsden, 1992
Immunohistochemistry. Fixed embryonic tissues for whole-mount immunostaining were washed extensively in 1% Triton X-100 (Tx; Sigma, Poole, UK) in PBS, and endogenous peroxidases were inactivated using 0.1% hydrogen peroxide solution, before a blocking step in 10% sheep serum and 0.1% Tx-PBS for 2 d at 4°C; all subsequent steps were done at this temperature. Embryos were then incubated in a 1:4 dilution of both the quail-specific antibodies QCPN and QN (which recognizes a quail axon antigen; a generous gift of Dr. H. Tanaka; Tanaka et al., 1990
RESULTS
Anatomy of the facial nerve in the chick
In the chick, motor neurons that project into the facial nerve develop in r4 and r5 (Fig. 1A) and comprise BM and VM classes (Lumsden and Keynes, 1989
Retrograde labeling reveals that BM neurons are present in r4 and r5, whereas VM neurons are restricted to r5
The development of motor neurons in r4 and r5 in the chick was investigated using fluorescein- or rhodamine-dextran as a retrograde tracer (Glover et al., 1986
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Figure 2. Retrograde labeling of motor neurons in r4 and r5 over a series of developmental stages. A-K, Ventral views of flat-mounted hindbrains showing retrograde labeling of facial BM and/or VM neurons. A, B, E, F, H, I, L, M, Labeling of BM neurons after fluorescein-dextran fills of the hyoid nerve (L, green bar) at st. 22 (A), st. 23 (B), st. 24 (E, F), st. 25 (H), and st. 27 (I). Between three and five embryos were labeled at each stage. Note the presence of BM neurons in r5 from stage 23 onward. Many of the BM neurons in r5 occupy lateral positions (B, E, arrowheads), whereas others lie closer to the floor plate in a medial position (E, F, arrows). Higher power views of these medially positioned BM neurons are shown in the insets in E and F. C, G, J, Labeling of VM neurons after fluorescein-dextran fills of the palatine nerve (N, green bar) at st. 25 (C), st. 27 (G), and st. 28 (J). Four or five embryos were labeled at each stage. Note the curved trajectory of VM axons (G, arrow). D, K, Double-labeling of BM and VM subpopulations after fluorescein-dextran fills of the palatine nerve (O, green bar) and rhodamine-dextran fills of the hyoid nerve (O, red bar) at st. 25 (D) (n = 3) and st. 27 (K) (n = 5). D, Within r5 a single BM neuron in a medial position has been labeled (arrow), but the majority of facial motor neurons in r5 are located laterally. K, Motor neuron cell bodies at st. 27 occupy the same mediolateral position. The straight or slightly curved axon trajectories of r4 BM neurons are clearly seen (arrow). Presence of apparently double-labeled cells (yellow) in D and K is an artifact caused by the superposition of labeled neurons at different depths when generating the confocal z-series shown here. Double-labeled cells were never observed in any single focal plane at all depths (data not shown). L, N, O, Schematics of ventral aspect of facial nerve and hindbrain indicating dextran labeling, and quantification of the mean (+SEM) number of BM neurons labeled in r5 at st. 22, 23, and 24 (M). Scale bar (in A): A, B, C, E, F, H, 100 µm. Scale bar (in D): G, I-K, 50 µm. fp, Floor plate; ep, exit point; gVII, geniculate ganglion; ov, otic vesicle; p, palatine nerve; ct, chorda tympani; h, hyoid nerve; Mx, maxilla; Ba1, first branchial arch; Ba2, second branchial arch. Dashed lines in A-C, E, F, and H indicate margins of floor plate and rhombomere boundaries.
From stage 20-22, BM neurons projecting via the hyoid nerve were located exclusively in r4 (Fig. 2A; data not shown), whereas from stage 23 to 27, there was a progressive increase in the number of facial BM neurons located in r5 (Fig. 2A,B,E,F,H,I). At stage 23 these neurons appeared confined to rostral r5 (Fig. 2B), but at later stages they were observed throughout the rostrocaudal extent of r5. Quantitation of the number of BM neurons in r5 was possible at stage 23 and 24, owing to the ease of counting individual labeled neurons with minimal overlap of adjacent cells and clear boundary demarcation. An approximately fourfold increase in the number of labeled BM neurons in r5 was observed between stages 23 and 24 (Fig. 2M). No BM neurons labeled via the hyoid nerve were present caudal to r5. Most of the labeled BM neurons in r5 were located laterally and did not form a genu. These experiments reveal that facial BM neurons are initially restricted to r4, but are later detected in r5. At earlier stages, BM neuron cell bodies showed considerable mediolateral spread within r4, whereas at later stages they were restricted to more lateral domains (Fig. 2I).
To determine the distribution of facial VM neurons, we retrogradely labeled motor neurons projecting into the palatine nerve, which was possible from stage 25 onward (Fig. 2C,G,J,N). At stage 25, VM neurons were confined to r5 in a lateral position (Fig. 2C). This tight clustering of VM cell bodies within r5 was maintained at later stages when rhombomere boundaries had disappeared (Fig. 2J). Thus, from stage 25 onward, r5 contains both facial BM and VM neurons, a spatial overlap that could be demonstrated by double labeling of the hyoid and palatine divisions of the facial nerve at stages 25 and 27 (Fig. 2D,K,O). These results show that from the time when they can first be labeled selectively, BM and VM neurons are confined to r4 and r5, respectively, but that eventually r5 contains both BM and VM subpopulations.
Facial BM neurons develop in r4 and r5, whereas VM neurons develop exclusively in r5
To investigate the rhombomere origin of facial BM and VM neurons, orthotopic transplants of r4 or r5 were performed at stages 10-12 using the quail-chick chimera system (Figs. 1B,C, 3). By this developmental stage certain key aspects of rhombomere identity have already been established, including Hox gene expression patterns and some aspects of cranial motor neuron phenotype (Guthrie and Lumsden, 1992
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Figure 3. Quail-to-chick orthotopic grafts of r4 and r5. A-G, Anti-neurofilament immunohistochemistry of control (A) and QCPN-QN immunohistochemistry of chimeric (B-G) embryos analyzed at st. 25-30. A, Ventral view of flat-mounted control chick embryo showing the pathways of the branchial nerves V, trigeminal; VII, facial; and IX, glossopharyngeal. Rostral (r) is to the top, and medial (m) is to the right. B, C, Parasagittal vibratome sections of a chimera with an orthotopic graft of r4. B, Hindbrain with grafted rhombomere (asterisk). Note that many quail cells from the graft have migrated posteriorly (black arrowheads). Rostral and dorsal (d) are indicated by orthogonal arrows. C, Quail axons from motor neurons in r4 innervate the muscle plate of the second branchial arch, which contains quail neural crest cells in the peripheral region. D-G, Parasagittal vibratome sections (D-F) and flat-mount (G) of chimeras with an orthotopic graft of r5. D, Quail graft is visible (asterisk) along with QN+ axons of the ventrally projecting abducens nerve (arrow). Orientation is the same in D-F. E-G, Three examples of the axonal projection patterns of motor neurons in r5. E, In this embryo, motor axons project along the palatine pathway of the facial nerve. An abducens nerve is also visible (arrow). F, This embryo has a palatine nerve and a hyoid projection that terminates abruptly at the level of the first branchial cleft (arrowhead), between the first and second branchial arches. QN+ axons do not reach the core of the second branchial arch (data not shown). G, Ventral view of a st. 25 embryo showing a palatine nerve and a hyoid nerve that terminates proximal to the second branchial arch and caudal to the first branchial cleft (arrowhead). The graft is marked with an asterisk. Scale bar: A, 400 µm; B, C, 100 µm; and D-G, 250 µm. gV, Trigeminal ganglion; gIX, glossopharyngeal ganglion; o, m, ophthalmic and mandibular divisions of trigeminal nerve; ldp, lesser deep petrosal branch of glossopharyngeal nerve.
In 100% of chimeras containing an orthotopic r4 graft, we observed the projection of quail-derived axons along exclusively the hyoid pathway (n = 16; Fig. 3B,C; Table 1). Quail axons filled the hyoid pathway, which was morphologically indistinguishable from that in control embryos (Fig. 3A), curving caudally from the geniculate ganglion to innervate the second branchial arch (summarized in Fig. 5E).
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Table 1. Frequency with which quail axons were observed in various axon pathways after orthotopic and heterotopic quail to chick rhombomere transplants For orthotopic r5 transplants, analysis was initially done at stage 23-24 (n = 6; data not shown), but no quail-derived axons were observed in the periphery. This is likely to be attributable to the late formation of facial VM projections along the palatine nerve relative to BM projections (see above). We therefore confined all subsequent analyses to chimeras of stage 25 or older. In all operated embryos at stage 25-30, a quail-derived abducens nerve was detected (22 of 22 of r5 grafts; Table 1). The abducens nucleus lies within r5 and 6 in the chick embryo and is formed by somatic motor (SM) neurons that project ventrally (Fig. 1A; Lumsden and Keynes, 1989
After orthotopic transplantation of r5, 95% of embryos contained quail axons within the palatine nerve (n = 21 of 22; Fig. 3D-G; Table 1). In 4 of 22 chimeras, only a quail-derived palatine nerve was present, whereas in a further 17 of 22 cases, both a palatine and a hyoid projection were present. In just one chimera, dorsal projections of quail-derived axons grew via the hyoid nerve exclusively. The pattern of quail palatine projections was normal, extending rostrally past the first branchial arch and then over the palate to its target, the sphenopalatine ganglion. By contrast, in these embryos, r5 quail neurons formed only sparse projections within the hyoid nerve, and often failed to reach the branchial arch muscle plate (Fig. 3F, Table 1). The motor axon pathways resulting from these orthotopic grafts are summarized in Figure 5, E and F.
Although we could not precisely quantify the number of QN+ axons in the different pathways, these observations imply that the majority of dorsally projecting motor neurons in r5 follow VM rather than BM axon pathways. Taken together, the results of these orthotopic grafts show that r4 and r5 both generate facial BM neurons, but that the majority originate in r4. By contrast, facial VM neurons develop exclusively in r5.
A subpopulation of facial BM neurons that originate in r4 migrates into r5
Between stages 23 and 25, our retrograde labeling studies show that there is a dramatic increase in the number of facial BM neurons within r5. This period corresponds to the onset of rhombomere boundary disappearance, and is in line with previous observations that inter-rhombomeric cell mixing occurs among differentiated neurons of the mantle zone at these stages (Hemond and Glover, 1993
To determine whether facial BM neurons migrate from r4 to r5, we examined some chimeras containing orthotopic r4 grafts for evidence of neuronal migration from r4 to r5 (n = 3). These embryos were analyzed at stage 26-27 by dextran labeling the hyoid nerve, and the hindbrains were immunostained using QCPN antibodies to detect quail cells, before vibratome sectioning (Fig. 4). Quail-derived, dextran-labeled facial BM neurons (arrowheads) were observed in r5 as well as in r4, suggesting that facial BM neurons in r4 indeed migrate caudally into r5 (Fig. 4B,C). Some dextran-labeled BM neurons in r5 were not QCPN-positive, implying that they were derived from the chick host, and consistent with the generation of BM neurons in r5 demonstrated earlier. Some QCPN-positive cells in r5 were not labeled with dextrans, and probably represent other cell or neuronal types with a similar migration pattern. Thus, avian embryos display cell migrations from r4 into r5, and a proportion of these cells are facial BM neurons.
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Figure 4. Retrograde labeling of the hyoid nerve in a chimera with an orthotopic graft of r4. A-C, Parasagittal vibratome sections through the hindbrain of a st. 26 embryo with an orthotopic r4 graft, after a fluorescein-dextran (green) fill of the hyoid nerve and whole-mount QCPN immunohistochemistry (red). A, Quail cells (red) that have migrated posteriorly from r4 into r5 are clearly seen near the pial surface (arrow). B, QCPN+-dextran-labeled cells are quail BM neurons that are present in r4 (arrow) and r5 (arrowheads). C, Higher power view of the boxed area in B to show quail BM neurons (yellow or red center and green surround) in r5 that have migrated posteriorly from r4 (arrowheads). Also visible are QCPN -dextran-labeled endogenous chick BM neurons (arrows) that originate in r5. p, Pial surface; v, ventricular surface. Scale bar: A, B, 100 µm; C, 25 µm.
Temporal differences in the formation of BM and VM pathways
Our retrograde labeling and grafting studies also gave information about the timing of BM and VM peripheral axon outgrowth. Orthotopic r4 transplants revealed that axonal projections to the second branchial arch are well established by stage 25 (n = 4 chimeras; Fig. 3C), the earliest stage examined. These observations are in keeping with earlier reports that showed the formation of hyoid projections to the second branchial arch as early as stage 21 (Simon et al., 1994
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Figure 5. Summary diagram of the temporal order of development of motor pathways of the facial nerve in the chick, based on retrograde axon tracing and orthotopic grafts. A, St. 20-22: all BM neurons are confined to r4 and send their axons into the hyoid nerve. B, St. 23: BM neurons are also identified in r5. C, St. 25: BM neurons born in r5 extend axons along the hyoid pathway, and VM neurons in r5 project axons to form the anlage of the palatine nerve. D, St. 27: Cell bodies of BM and VM neurons occupy the same mediolateral position. The palatine nerve has extended to the maxilla to innervate the target ganglia. For abbreviations, see Figure 2 legend. E-J, Motor pathways that result from orthotopic (E, F) and heterotopic (G-J) quail to chick grafts. E, r4 orthotopic grafts: quail axons grow into the second branchial arch. 1 and 2 point out first and second branchial arches. F, r5 orthotopic grafts: quail axons grow into the palatine branch and into the second branchial arch. G, H, r5 to r3 grafts (G, whole rhombomere; H, basal plate graft only): quail axons that exit via the r2 dorsal exit point reroute to join the facial nerve pathway at the geniculate ganglion. Other quail axons exit the hindbrain via the exit point in r4. Axons are distributed in the palatine and hyoid nerves en route to the correct targets. For clarity, axons that traverse the trigeminal nerve in a small minority of chimeras have been omitted. I, r3 to r5 grafts: axons project to an incorrect target, the second branchial arch. J, r2 (basal plate) to r4 grafts: axons project to an incorrect target, the second branchial arch. For abbreviations, see Figure 2 legend.
Ectopic motor neurons with distinct segmental origins display different specificity in their axon pathfinding
To test the specificity of axon pathfinding of motor neurons with distinct segmental origins, heterotopic rhombomere transpositions were performed, and chimeras were analyzed as before, at stages 25-30 (Figs. 1D-G, 6, Table 1). When r5 was transposed to r3 position, quail-derived axons projected along several distinct pathways (n = 6; Figs. 1D, 5G, Table 1). The most striking observation was that in some cases an ectopic longitudinal QN-positive nerve bundle exited the hindbrain via the r2 exit point before turning caudally and projecting to the geniculate ganglion. This tract is likely to be composed of facial motor axons, which had navigated back to their intermediate target. Such a tract is unlikely to contain neural crest-derived neurons because r5 gives rise to few neural crest cells (Lumsden et al., 1991
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Figure 6. BM and VM axon pathfinding after heterotopic quail-to-chick transplants. A-G, QCPN and QN immunohistochemistry in embryos at st. 25-30 after heterotopic grafts of r5 basal plate to r3 (A, B), r3 to r5 (C, D), and r2 basal plate to r4 (E-G). A, B, Ventral views of two flat-mounted embryos showing ectopic QN+ axon tract (A, B, black arrows) projecting from the trigeminal nerve exit point in r2 to the geniculate ganglion. In B, QN+ axons also exit the hindbrain via the exit point in r4 and project to the geniculate ganglion in the facial nerve (f). A palatine nerve is recognizable in both cases and has bifurcated in B to supply both the sphenopalatine and ethmoidal ganglia (data not shown). Two other motor pathways additionally present in B are a hyoid nerve and mandibular projection (arrowhead), which is at the limit of detectability. In B, the connection of the ectopic bundle and facial nerve to the hindbrain was severed during flat-mounting, as indicated by black dashed lines. The grafted rhombomeres (data not shown) resembled the basal plate graft shown in E. C, D, Dorsal (C) and lateral (D) views of whole-mount embryo showing, respectively, the graft (C, black arrow) and axonal projection of trigeminal BM neurons to the second branchial arch (D, white arrow). E-G, Dorsal (E) and lateral (F, G) views of whole-mount embryo showing the grafted basal plate (E, black arrow), the projection of trigeminal BM axons to the second branchial arch (F, white arrow), and, at higher power, the second branchial arch, which is devoid of quail neural crest cells (G). Scale bar (in G): C, G, 200 µm; A, E, 300 µm; B, 500 µm; F, 1200 µm; and D, 1600 µm.
Nevertheless, to confirm that this ectopic fascicle was a motor rather than a sensory pathway we also grafted r5 basal plate alone in place of r3 (n = 8; Fig. 1E), thus eliminating possible contamination by neural crest cells. These chimeras showed the same ectopic nerve bundle directed from the r2 trigeminal nerve exit point to the geniculate ganglion in 9 of 14 cases, and data from both types of operation were subsequently pooled because the findings were identical (Figs. 5H, 6A,B, Table 1). Ectopic r5-derived motor axons also followed a second axon pathway, which turned caudally within the neuroepithelium, exited the hindbrain via the r4 facial exit point, and projected via the facial nerve to the geniculate ganglion (n = 9 of 14). Thus, r5-derived motor neurons were able to project back to their intermediate target either via the inappropriate (r2) exit point or by projecting aberrantly in a caudal direction toward the appropriate (r4) exit point. Overall, motor axons from r5 projected along novel pathways to the facial nerve or geniculate ganglion in 93% of cases.
Projections along the distal, motor pathways of the facial and trigeminal nerves were also assessed; QN-positive projections were observed in the palatine (n = 11 of 14) and hyoid (n = 7 of 14) divisions of the facial nerve and along the mandibular branch of the trigeminal nerve (n = 4 of 14). A ventrally projecting abducens nerve was observed in all (14 of 14) chimeras, supporting the view that r5 identity is not altered when it is transposed rostrally, because SM abducens neurons are generated within it. The broad conclusion of this experiment is therefore that many ectopic VM axons were able to pathfind to their eventual target, by following novel pathways incorporating one or both of their bona fide intermediate targets, the r4 exit point and/or the geniculate ganglion.
After transposition of r3 to r5 position, in 100% of cases quail BM neurons extended their axons rostrally, exited the hindbrain via r4, and grew along the hyoid pathway to the second branchial arch (n = 9; Figs. 1F, 6C,D, Table 1). No quail-derived neural crest cells were identified in the periphery in these transplants, in accordance with observations that r3 is neural crest-depleted (Lumsden et al., 1991
DISCUSSION
Our study has revealed that facial branchiomotor and visceral motor neurons have different segmental origins in the chick embryo hindbrain. Visceral motor neurons are generated exclusively in rhombomere 5, whereas the majority of branchiomotor neurons originate in rhombomere 4. This early segmental ground plan is modified by the migration of a cohort of BM neurons from r4 into r5 and the generation of a smaller population of BM neurons within r5. When transplanted rostrally, r5 facial VM neurons displayed the ability to pathfind back to their correct targets. By contrast, r2 and r3 trigeminal BM neurons transplanted caudally did not pathfind back to the first branchial arch, but grew into the second branchial arch, an incorrect target region. Our findings thus suggest that facial motor axons are capable of rerouting to their targets, whereas trigeminal motor axons are not, consistent with previous experiments showing that ectopic r4 facial BM neurons could navigate back to the second branchial arch (Bell et al., 1999
Time course of the development of facial motor neurons in the chick
The sequence of motor neuron development in r4 and r5 can be inferred from the expression of markers, axonal tracing, and grafting experiments, derived from this and previous studies. Postmitotic facial motor neurons are first recognized in r4 and r5 by Islet-1 and SC1 expression at stage 14-15 (Simon et al., 1994
Based on axon tracing, r5 BM axons have reached the branchial arch by stage 23, even though the results of orthotopic r5 transplantation experiments show that projections from r5 BM neurons cannot be detected in the hyoid nerve until stage 25. Taken together, these results imply that the projections formed by BM neurons resident in r5 at stage 23 must originate from r4-derived BM neurons that have migrated caudally into r5. At approximately stage 25, BM neurons born in r5 then send projections to the branchial arch, and r5 VM neurons project into the palatine nerve. By stage 27, the cell bodies of BM and VM neurons have migrated laterally, and VM axons have reached their target parasympathetic ganglia (Fig. 5A-D).
Subpopulations of BM neurons in r5
We have demonstrated that, in addition to VM neurons, r5 contains two distinct subpopulations of BM neurons, one group that migrates caudally from r4, and a second that is intrinsic to r5. The caudal migration of a subset of facial BM neurons in the chick hindbrain appears highly directed, as in the rodent (Auclair et al., 1996
Two types of evidence support the existence of a subpopulation of BM neurons that is born in r5. First, retrograde axon tracing of the hyoid (BM) nerve in chimeras with an r4 orthotopic graft labels BM neurons that have originated in r5, in addition to those that migrate from r4. Second, in the great majority of embryos with an r5 orthotopic graft, dual palatine (VM) and hyoid (BM) pathways are detected. The latter pathway was observed less frequently, contained fewer axons, and sometimes could not be traced all the way to the second branchial arch. One explanation for this finding is that the later development of r5 BM neurons relative to r4 BM neurons could deprive them of limiting amounts of trophic support from the branchial arch (Oppenheim et al., 1988
Axon pathfinding of motor neurons after heterotopic grafts
When r5 was transplanted ectopically, we found that in the majority of cases, motor axons were able to reroute back to their intermediate target, the geniculate ganglion, and formed a palatine nerve en route to the sphenopalatine ganglion. In some cases axons formed an ectopic fascicle extending longitudinally from r2 exit point to the geniculate ganglion. This feature is reminiscent of the longitudinal fascicle observed after transplantation of r4 to r2 position, which resulted from the projection of r4 facial motor axons back to the second branchial arch (Bell et al., 1999
The axon pathfinding of r5 VM neurons contrasts with the lack of pathfinding selectivity of heterotopic trigeminal motor axons, which projected to the inappropriate ganglion and branchial arch. This behavior is unlikely to be explained by a change in the phenotype of the transposed segment, because previous studies using molecular markers have shown that neither rostral nor caudal transposition within the pre-otic region is associated with the respecification of rhombomere identity (Guthrie et al., 1992
Guidance cues for BM and VM axon pathfinding in the head
The normal topographic projection of motor neurons to the branchial arches may depend on the corresponding expression on motor axons and peripheral mesenchyme of molecules whose expression is governed by the same repertoire of Hox genes (Lumsden and Keynes, 1989
The guidance molecules that ensure selective pathfinding of VM and BM neurons at individual axial levels remain largely unidentified. The branchial arches have been shown to exert a growth-promoting and chemoattractive influence on cranial motor axons, mediated partly by the production of hepatocyte growth factor (HGF) (Caton et al., 2000
FOOTNOTES Received Feb. 28, 2000; revised June 23, 2000; accepted July 19, 2000.
This work was supported by grants from the Special Trustees of Guy's Hospital and the Wellcome Trust. J.J. is a Wellcome Clinical Training Fellow. We thank F. Prin for assistance with figures, C. Barrett for assistance with immunohistochemistry, and N. Pringle for antibodies. We are grateful to A. Lumsden, R. Wingate, and a helpful reviewer for insightful comments on this manuscript.
Correspondence should be addressed to Sarah Guthrie, Medical Research Council Centre for Developmental Neurobiology, Fourth Floor, New Hunt's House, King's College, Guy's Campus, London SE1 1UL, UK. E-mail: sarah.guthrie{at}kcl.ac.uk.
REFERENCES
- Auclair F, Valdes N, Marchand R (1996) Rhombomere-specific origin of branchial and visceral motoneurones of the facial nerve in the rat embryo. J Comp Neurol 369:451-461[Medline].
- Bell E, Wingate RJ, Lumsden A (1999) Homeotic transformation of rhombomere identity after localized Hoxb1 misexpression. Science 284:2168-2171
[Abstract/Free Full Text] .- Caton A, Hacker A, Naeem A, Livet J, Maina F, Klein R, Birchmeier C, Guthrie S (2000) The branchial arches and HGF are growth-promoting and chemoattractant for cranial motor axons. Development 127:1751-1766[Abstract].
- D'Amico-Martel A, Norden DM (1983) Contributions of placodal and neural crest cells to avian cranial peripheral ganglia. Am J Anat 166:445-468[ISI][Medline].
- Fritzsch B, Nichols DH (1993) DiI reveals a prenatal arrival of efferents at the differentiating otocyst of mice. Hear Res 65:51-60[ISI][Medline].
- Glover JC, Petursdottir G, Jansen JKS (1986) Fluorescent dextran-amines used as axonal tracers in the nervous system of the chicken embryo. J Neurosci Methods 18:243-254[ISI][Medline].
- Graham A, Lumsden A (1996) Interactions between rhombomeres modulate Krox-20 and follistatin expression in the chick embryo hindbrain. Development 122:473-480[Abstract].
- Guthrie S, Lumsden A (1992) Motor neuron pathfinding following rhombomere reversals in the chick embryo hindbrain. Development 114:663-673[Abstract].
- Guthrie S, Muchamore I, Kuroiwa A, Marshall H, Krumlauf R, Lumsden A (1992) Neuroectodermal autonomy of Hox-2.9 expression revealed by rhombomere transpositions. Nature 356:157-159[Medline].
- Hamburger V (1975) Cell death in the development of the lateral motor column of the chick embryo. J Comp Neurol 160:535-546[ISI][Medline].
- Hamburger V, Hamilton HL (1951) A series of normal stages in development of the chick embryo. J Morphol 88:49-87[ISI].
- Hemond SG, Glover JC (1993) Clonal patterns of cell proliferation migration, and dispersal in the brainstem of the chicken embryo. J Neurosci 13:1387-1402[Abstract].
- Hunt P, Gulisano M, Cook M, Sham MH, Faiella A, Wilkinson D, Boncinelli E, Krumlauf R (1991) A distinct Hox code for the branchial region of the vertebrate head. Nature 353:861-864[Medline].
- Jacob J, Tiveron M-C, Brunet J-F, Guthrie S (2000) Role of the target in the pathfinding of facial visceral motor axons. Mol Cell Neurosci 16:14-26[Medline].
- Kuratani SC, Eichele G (1993) Rhombomere transplantation repatterns the segmental organisation of cranial nerves and reveals cell-autonomous expression of a homeodomain protein. Development 117:105-117[Abstract].
- Lumsden A (1990) The cellular basis of segmentation in the developing chick hindbrain. Trends Neurosci 13:329-335[ISI][Medline].
- Lumsden A, Keynes R (1989) Segmental patterns of neuronal development in the chick hindbrain. Nature 337:424-428[Medline].
- Lumsden A, Sprawson N, Graham A (1991) Segmental origin and migration of neural crest cells in the hindbrain region of the chick embryo. Development 113:1281-1291[Abstract].
- Maina F, Hilton MC, Ponzetto C, Davies AM, Klein R (1997) Met receptor signaling is required for sensory nerve development and HGF promotes axonal growth and survival of sensory neurons. Genes Dev 11:3341-3350
[Abstract/Free Full Text] .- Marin F, Puelles L (1995) Morphological fate of rhombomeres in quail/chick chimaeras: a segmental analysis of hindbrain nuclei. Eur J Neurosci 7:1714-1738[ISI][Medline].
- McKay I, Lewis J, Lumsden A (1997) Organisation and development of facial motor neurons in the kreisler mutant mouse. Eur J Neurosci 9:1499-1506[Medline].
- Moody SA, Heaton MB (1983) Developmental relationships between trigeminal ganglia and trigeminal motoneurons in chick embryos. III. Ganglion perikarya direct motor axon growth in the periphery. J Comp Neurol 213:350-364[Medline].
- Noden DM (1983) The role of the neural crest in patterning of avian cranial skeletal, connective, and muscle tissues. Dev Biol 96:144-165[ISI][Medline].
- Oppenheim RW, Haverkamp LJ, Prevette D, McManaman JL, Appel SH (1988) Reduction of naturally occurring motoneuron death in vivo by a target-derived neurotrophic factor. Science 240:919-922
[Abstract/Free Full Text] .- Simon H, Lumsden A (1993) Rhombomere-specific origin of the contralateral vestibulo-acoustic efferent neurons and their migration across the embryonic midline. Neuron 11:209-220[ISI][Medline].
- Simon H, Guthrie S, Lumsden A (1994) Regulation of SC1/DM-GRASP during the migration of motor neurons in the chick embryo brain stem. J Neurobiol 25:1129-1143[ISI][Medline].
- Simon H, Hornbruch A, Lumsden A (1995) Independent assignment of antero-posterior and dorso-ventral positional values in the developing chick hindbrain. Curr Biol 5:205-214[ISI][Medline].
- Studer M, Lumsden A, ArizaMcNaughton L, Bradley A, Krumlauf R (1996) Altered segmental identity and abnormal migration of motor neurons in mice lacking Hoxb-1. Nature 384:630-634[Medline].
- Tanaka H, Kinutani M, Agata A, Takashima Y, Obata K (1990) Pathfinding during spinal tract formation in the chick-quail chimaera analysed by species-specific monoclonal antibodies. Development 110:565-571
[Abstract/Free Full Text] .- Tucker A, Lumsden A, Guthrie S (1996) Cranial motor axons respond differentially to the floor plate and sensory ganglia in collagen gel co-cultures. Eur J Neurosci 8:906-916[Medline].
- Varela-Echavarría A, Pfaff SL, Guthrie S (1996) Differential expression of LIM homeobox genes among motor neuron subpopulations in the developing chick brain stem. Mol Cell Neurosci 8:242-257[ISI][Medline].
- Warrilow J, Guthrie S (1999) Rhombomere origin plays a role in the specificity of cranial motor axon projections in the chick. Eur J Neurosci 11:1403-1413[Medline].
- Wingate RJ, Lumsden A (1996) Persistence of rhombomeric organisation in the postsegmental hindbrain. Development 122:2143-2152[Abstract].
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