 |
|||||
|
|||||
|
|||||
|
|||||
|
|||||
Previous Article | Next Article
Volume 16, Number 20, Issue of October 15, 1996 pp. 6463-6475
Copyright ©1996 Society for NeuroscienceDifferential Expression of Bone Morphogenetic Proteins in the Developing Vestibular and Auditory Sensory Organs
Seung-Ha Oh1, Randy Johnson2, and Doris K. Wu1 1 National Institute on Deafness and Other Communication Disorders, Rockville, Maryland 20850, and 2 M. D. Anderson Cancer Center, Department of Biochemistry and Molecular Biology, Houston, Texas 77030
ABSTRACT
The genes responsible for the formation of various sensory organs in the inner ear are not known. There are eight sensory organs in the chick inner ear, and our previous study showed that all presumptive sensory organs initially express bone morphogenetic protein 4 (BMP4), a member of the transforming growth factor (TGF)-
Key words: BMP4; BMP5; BMP7; crista ampullaris; basilar papilla; maculagene family. To address the potential role of BMPs in the patterning of different sensory organ structures, we investigated the expression of BMP4, BMP5, and BMP7 during sensory organ differentiation in the chick inner ear. The gene expression pattern of BMP5, although similar to that of BMP4, was transient and disappeared by embryonic day 3.5 (E3.5). In contrast, BMP7 gene expression was quite extensive, starting in the otic placode. By E5, gene expression patterns of BMP4 and BMP7 differed among vestibular and auditory sensory organs. In the vestibular sensory organs, BMP7 gene expression segregated from the main sensory tissue areas at the onset of differentiation, whereas BMP4 expression concentrated in supporting cells. In the cochlea, however, BMP7 gene expression became restricted to sensory tissue over time and eventually concentrated in supporting cells, whereas BMP4 gene expression was localized to hair cells. The different BMP expression patterns in developing auditory and vestibular sensory organs may help to shape each respective sensory structure. Furthermore, the expression of BMP4 in the cochlea also revealed an interesting pattern of sensory cell differentiation: the distal portion of the cochlea differentiates first, and the tall hair cells develop before the short hair cells.
INTRODUCTION
Bone morphogenetic proteins (BMPs) belong to theecapentaplegic
eg-
elated (DVR) subgroup within the transforming growth factor (TGF)-
). In the DVR subgroup, BMPs can be subdivided further into at least two subfamilies, including decapentaplegic (dpp) and 60A. The dpp subfamily includes the Drosophila dpp gene and its mammalian homologs BMP2 and BMP4. The 60A subfamily includes the Drosophila 60A gene and its mammalian homologs BMP5, BMP6, BMP7, and BMP8. Genes within the same subfamily are highly conserved and in some cases can substitute for each other functionally (Padgett et al., 1993
The roles of BMPs during embryogenesis are quite extensive, including patterning in Drosophila (Capdevila and Guerrero, 1994
The membranous portion of the inner ear is derived from the otocyst. Genes such as Hoxa-1 (Carpenter et al., 1993
MATERIALS AND METHODS
Embryos. Fertilized White Leghorn eggs (Truslow Farm) were incubated for designated times, and embryos were staged according to Hamburger and Hamilton (1951)PCR amplification. Total RNA from E3 chick otocysts was isolated as described (Chirgwin et al., 1979
In situ hybridization. In situ hybridization of whole embryos and frozen sections was performed as described (Wu and Oh, 1996
Isolation of chicken BMP5 cDNA clones. From a stage 22 limb bud library (Roberts et al., 1995
end of the open reading frame was obtained by PCR amplification of plasmid DNA obtained from a random-primed limb bud library (see the following section for details of library construction). All PCR reactions were carried out using pfu Taq polymerase (Boehringer Mannheim, Indianapolis, IN). A ~500 bp fragment was obtained in a PCR reaction using a primer directed against the Bluescript vector (Stratagene) and a BMP5 gene-specific primer directed against the 5
Fig. 1. Nucleotide and deduced amino acid sequence of the chicken BMP5 cDNA and comparison with the human and mouse BMP5 genes. A, The sequence of chicken BMP5 cDNA. The in-frame translational stop codon at63 upstream to the first methionine is indicated in italics. Sequences used to design gene-specific primers in the PCR reactions are underlined. The putative polyA site (AATAAA) is also underlined at the 3
[View Larger Version of this Image (73K GIF file)]
Random-primed library construction. Messenger RNA was isolated from stage 22 limb bud cells using the acid-phenol method followed by poly(A+) selection (PolyATtract, Promega, Madison, WI). Approximately 4 µg of mRNA was reverse-transcribed using random hexamers (160 ng) and Superscript reverse transcriptase (Life Technologies). After second-strand synthesis and incubation with T4 polymerase to generate blunt ends, the double-stranded cDNA was ligated to nonpalindromic BstXI hemiphosphorylated adaptors (Duguid and Dinauer, 1990
Three-dimensional reconstruction. Three-dimensional reconstruction of frozen sections was performed as described (Wu and Oh, 1996
RESULTS
Identification of BMPs in chick otocyst and isolation of chicken BMP5 cDNA
Using the RT-PCR technique, we found BMP4, BMP5, BMP6, and BMP7 transcripts in E3 chick otocysts, with BMP7 transcripts being the most abundant. cDNA clones for BMP4, BMP5, and BMP7 were subsequently isolated from a stage 22 limb bud library as described (Roberts et al., 1995BMP5 mRNA distribution in the developing inner ear
The following whole-mount in situ hybridization results were summarized from 69 embryos ranging from stage 8 to 24 (E1-E4) during six experiments. BMP5 mRNA was not detected in the developing inner ear until stage 13 (E2) (Fig. 2A,B, arrowhead). The BMP5 expression was similar to that of BMP4 (Wu and Oh, 1996
Fig. 2. Gene expression of BMP5 and BMP7 in developing chick inner ear by whole-mount in situ hybridization. Embryos shown in A-D and I were hybridized with a BMP5 cRNA; embryos in E-H and J were hybridized with a BMP7 cRNA. The embryo shown in K is a control hybridized with a sense BMP5 RNA probe. The control for BMP7 was similar to that shown in K. A is a side view and B is a dorsal view of a stage 13 (21 somites, E2) embryo showing positive BMP5 expression in the dorsal and posterior margins of the otic cup. I is a transverse section of the embryo in A, showing expression in the dorsal margin of the otic cup as well as the dorsal portion of the hind brain (arrow in I). By stage 16 (C, 26 somites, E2.5), BMP5 mRNA became restricted to two foci. The anterior focus (arrow in C) disappeared by stage 17 (D, 32 somites), but the posterior focus (arrowhead in C and D) remained until stage 22 (E3.5). BMP7 mRNA was present in the otic placode (E, 8.5 somites, E1.5). As the otic placode invaginated to form the otic pit, positive BMP7 expression was present in the dorsal and posterior portions of the otic cup (F, 21 somites, E2). G is a transverse section of F showing that the BMP7-positive area was much broader than that of BMP5 (I). Positive BMP7 expression was also present in the first pharyngeal pouch (arrow in G). By stage 16 (H, 28 somites, E2.5), most of the otic epithelium was positive for BMP7, except the ventral portion of the otic cup shown in J. BMP7 mRNA was also found in the eye (black arrow in H), the ectoderm of branchial arches (white arrowhead in H), the heart (white arrow in H), and the dorsal part of the neural tube (black arrow in J). Scale bars: A-F, H, K, 100 µm; G, I, J, 50 µm.
[View Larger Version of this Image (65K GIF file)]
BMP7 mRNA distribution in the developing inner ear from stage 8 to 24
The following whole-mount in situ hybridization results were summarized from 80 embryos ranging from stage 8 (E1) to 24 (E4) during eight experiments. Among the three BMPs characterized so far, BMP7 was the earliest one to be expressed in the inner ear. BMP7 mRNA was detected in the otic placode, with concentration in the otic epithelium next to the hind brain (Fig. 2E, arrowhead). As the otic placode invaginated to form the otic cup, BMP7 expression concentrated in the dorsal and posterior portions of the otic cup (Fig. 2F, arrowhead). This expression pattern in the otic cup (Fig. 2G), although similar to that of BMP4 (Wu and Oh, 1996
Fig. 3. Top. Three-dimensional reconstruction of BMP4 and BMP7 gene expression of a stage 24 (E4) chick otocyst. A and B are medial views and C and D are lateral views of the same otocyst. This otocyst was reconstructed from a total of 44 horizontal, serial cryosections of 12 µm thickness. The most dorsal sections of the otocyst were missing, which resulted in a flattened image at the top. All odd-number sections were probed for BMP4, and all even-number sections were probed for BMP7. In A and C, all of the BMP4-positive, presumptive sensory organs are shown. Identification of each presumptive sensory organ was as described (Wu and Oh, 1996
[View Larger Version of this Image (94K GIF file)]
Comparison of BMP4 and BMP7 mRNA distribution in the developing inner ear
Previous data suggest that BMP4 is an early marker for all sensory organs of the inner ear (Wu and Oh, 1996
Fig. 7. Comparison of BMP4 and BMP7 gene expression patterns in maculae from E4 to E7. A and B, C and D, and E and F are pairs of 12 µm adjacent sections. Sections shown in A, C, and E were probed for BMP4; B, D, and F were probed for BMP7. A section similar to that in E and F was probed for BDNF (G). A and B are horizontal sections from an E4 embryo; C and D are transverse sections from an E5 embryo, and E-G are transverse sections of E7 embryos. At E4, most presumptive sensory organs were within a subset of the BMP7-positive area, except for a portion of the macula utriculi (A, B). By E5, BMP4 expression in the macula utriculi was much more restricted (C). Only a portion of the BMP4-positive area in the macula utriculi (u) overlapped with that of BMP7 (D). Arrows in D point to the nonsensory portion of basilar papilla that was positive for BMP7. By E7, BMP7 expression had segregated from the main sensory tissue areas (F), and BMP4 transcripts had localized largely in supporting cells (E), in contrast to the expression pattern of BDNF (G), which was in hair cells. The arrow in E points to the BMP4-positive area in the roof of lateral ampulla. Brackets in A and D mark the presumptive macula utriculi. Orientation: A, anterior; D, dorsal; M, medial. bp, Basilar papilla; s, macula sacculi; u, macula utriculi; sc, superior crista; lc, lateral crista. Scale bar, 50 µm.
[View Larger Version of this Image (47K GIF file)]
Fig. 6. Comparison of BMP4 and BMP7 gene expression patterns in superior crista ampullaris from E4 to E16. A and B, C and D, E and F, G and H, and I and J are pairs of adjacent 12 µm sections. Sections shown in A, C, E, G, and I were probed for BMP4; B, D, F, J, and K were probed for BMP7; and H was probed for BDNF. A and B were sections from stage 24 (E4) embryos; C and D from E5; E-H from E7; I, J, L, M from E8; and K, N from E16. At E4, (A) BMP4- and (B) BMP7-positive areas overlapped in the presumptive crista (sc). Arrows in B point to the thin epithelium at the dorsolateral portion of the otocyst that was negative for BMP7. By E5, BMP7 (D) has begun to segregate from the presumptive sensory area. Arrowhead in C points to the cruciatum that was negative for BMP4. The arrow points to the part of the otic epithelium with weak BMP4 expression next to the strong expression in the surrounding mesenchyme. This weak epithelial signal became the positive signal in the roof of the ampulla by E7 (arrow in E, G). At E7, BMP7 expression was restricted mostly to the nonsensory portion of the ampulla (F). On the other hand, the BMP4-positive area within the crista concentrated in supporting cells (E, G) rather than in hair cells, as contrasted by the pattern of BDNF expression (H). The areas within the rectangles in I, J, and K are enlarged in L, M, and N, respectively. BMP4 transcripts spanned the entire epithelium in one area of the ampulla (bracket in L), and this area was also positive for BMP7 (bracket in M). By E16, positive hybridization was found in the planum semilunatum (ps) and the crista ampullaris (bracket in N). Orientation: D, dorsal; M, medial. Refer to orientation axis in A for B-H and orientation axis in I for J-N. ca, Crista ampullaris; ed, endolymphatic apparatus; sc, superior crista; ps, planum semilunatum. Scale bars: A-J, 100 µm; K, 200 µm; L-N, 25 µm.
[View Larger Version of this Image (146K GIF file)]
Basilar papilla The gene expression patterns of BMP4 and BMP7 in the basilar papilla were different from those of other sensory organs in the inner ear. We demonstrated previously that the presumptive sensory tissue for the papilla develops from a cluster of three other sensory organs: posterior crista, lagena, and macula neglecta (Wu and Oh, 1996
Fig. 5. Comparison of BMP4 and BMP7 gene expression pattern in the basilar papilla from E6.5 to E16. Transverse sections in A, C, E, I, and K and the sagittal section in G were probed for BMP4. Transverse sections in B, D, F, J, and L and the sagittal section in H were probed for BMP7. A and B, C and D, and E and F are 12 µm adjacent sections. At E6.5, the BMP4 expression in the lagena and the sensory portion (anterior arm) of the papilla spanned the entire epithelium (A) and overlapped with that of BMP7 (B). C is one of the transverse sections illustrated in Figure 4A showing the three areas of BMP4 hybridization signals: the strong anterior (area marked by bracket), the weak middle (area marked by arrowheads), and the posterior (area marked by arrows). Because BMP4 hybridization signals of the posterior arm expanded laterally in the papilla, the positive BMP4 signal can be observed in some sections opposite the sensory epithelium, as shown in C. D is an adjacent section of C probed for BMP7 and shows a hybridization pattern similar to that of BMP4. By E9, the structure of the papilla was more mature, and the three BMP4-positive areas were still evident in a longitudinal (E) as well as a cross-sectional (G) view of the papilla. The hybridization pattern of BMP7 was still similar to that of BMP4, except that there was a restricted area within the posterior arm with stronger BMP7 expression (arrow in F and H). By E12, BMP4 transcripts concentrated in the hair cells (I), whereas BMP7 expression still spanned the entire epithelium (J). By E16, BMP4 transcripts were located in hair cells (K), and BMP7 transcripts were located in supporting cells only (L). Also, some adjacent mesenchyme was positive for BMP4 (K). Brackets in K and L indicate the height of the sensory epithelium. Orientation for A, B: D, distal; P, proximal. Orientation for C-F: D, dorsal; L, lateral. Orientation for G, H: A, anterior; D, dorsal. Orientation for I-L: D, dorsal; L, lateral. Scale bars: A, B, I-L, 50 µm; C, D, G, H, 50 µm; E, F, 50 µm.
[View Larger Version of this Image (75K GIF file)]
In the papilla, BMP7 gene expression became more restricted to the sensory tissue during differentiation. At E5, the entire papilla was positive for BMP7, including the nonsensory portion (an example of the nonsensory portion of papilla is shown in Fig. 7D, indicated by arrows). At E6.5, restriction of BMP7 expression could be observed in the papilla, with the majority of the positive area overlapping with that of BMP4 (compare Fig. 5A with 5B and 5C with 5D). The similarity in patterns was most obvious in the anterior portion of the papilla (anterior arm of the BMP4-positive area), and the hybridization signals spanned the height of the epithelium (Fig. 5A,B). At E9, BMP7 gene expression remained similar to that of BMP4 (compare Fig. 5E with 5F and 5G with 5H), except that there was a portion of epithelium within the posterior arm that has a stronger BMP7 expression (5F,H, arrow). This concentration of BMP7 expression was transient, and the identity of these cells is not clear. By E12, BMP4 transcripts were concentrated in hair cells (Fig. 5I), and this pattern was much more evident by E16 (Fig. 5K; bracket marks the height of the sensory epithelium). On the other hand, BMP7 transcripts were still distributed across the entire epithelium at E12 (Fig. 5J) and became restricted to supporting cells by E16 (Fig. 5L; bracket marks the height of the sensory epithelium). This pattern of BMP4 in hair cells and BMP7 in supporting cells of the papilla remained at least until the eggs hatched.
Ampulla As mentioned above, at stage 24 (E4), all three presumptive cristae were positive for BMP4 (Fig. 6A) and were well within the BMP7-positive area (Fig. 6B; see also Fig. 3 for composite). BMP4 transcripts were also present in the mesenchyme surrounding the dorsolateral portion of the inner ear (Fig. 6A). At E5, BMP4 expression in the sensory tissue was interrupted in the middle by the nonsensory tissue known as the cruciatum (Fig. 6C, arrowhead). The cruciatum was present only in the superior and posterior cristae but not in the lateral crista (Dohlman, 1964By E7, the crista ampullaris was more differentiated, and BMP4 transcripts were more concentrated in supporting cells of the crista (Fig. 6E,G). Previous studies showed that brain-derived neurotrophic factor (BDNF) is expressed by hair cells of all sensory organs in the rat inner ear (Pirvola et al., 1992
At E8, the typical dome-shaped morphology of the crista was much more evident. BMP4 transcripts concentrated in supporting cells (Fig. 6I), except at the periphery of the crista where BMP4 mRNA still spanned the entire epithelium (Fig. 6L, bracket). All BMP4 hybridization signals in the ampulla became very weak at E12 and disappeared by E16 (data not shown). At E8, BMP7 transcripts remained concentrated in the side wall of the ampulla, whereas the structure of the planum semilunatum became more defined (Fig. 6J). In addition, a small portion of the epithelium in the periphery of the crista was positive for BMP7 (Fig. 6M, bracket) and overlapped with that of BMP4 (Fig. 6L, bracket). By E16, the structure of the planum semilunatum was quite evident and remained positive for BMP7 (Fig. 6N, ps). This positive expression persisted at least until E19. In addition, there was some weaker BMP7 hybridization signal in the crista (Fig. 6N, bracket). The positive cells in the crista were most likely hair cells, based on their apical locations within the epithelium and results obtained from probing adjacent sections of the cristae for BMP7 and BDNF (data not shown); however, the BMP7 hybridization signals in the crista were not always consistent. Additional characterization using an antibody specific for BMP7 may help to identify unequivocally these cells in the crista.
The epithelium lining the semicircular canals was also positive for BMP7 at E7, and the hybridization signals eventually disappeared by E12 (data not shown).
Maculae utriculi and sacculi An earlier study indicates that the presumptive macula sacculi is generated at stage 20 (E3.5), and the presumptive macula utriculi is generated at stage 24 (E4), based on BMP4 gene expression (Wu and Oh, 1996BMP4 expression in the macula neglecta is discrete at E6 (stage 29) (Wu and Oh, 1996
DISCUSSION
BMP5 gene expression in the inner ear
BMP5 gene expression in the otocyst, although associated with presumptive sensory areas, was transient. In addition, BMP5 was expressed in the furrow of the first branchial arch, which gives rise to the external auditory meatus. In the chick, the external ear consists of an auditory canal but no pinna. In the mouse, defects in the BMP5 gene cause malformation of the pinna (Kingsley et al., 1992BMP4 and 7 gene expression in the otocyst up to E4
Thus far, among all of the different BMP genes that we have characterized in the chick inner ear, BMP7 was the earliest one to be expressed, starting in the otic placode. By E4 (stage 24), the majority of the otocyst was positive for BMP7, including the presumptive sensory organs, except for part of the macula utriculi. At this age, there are two BMP7-negative areas within the otocyst: an anteromedial area and a dorsolateral area. It is not know whether the BMP7-negative anteromedial area is associated with any particular structure in the mature inner ear; however, the dorsolateral area normally gives rise to the semicircular canals. By E7, when semicircular canals were formed, the epithelia of the canals became positive for BMP7 (data not shown).Within the BMP7-positive area, subsequent gene expression of BMP7 showed different patterns, depending on whether that portion of tissue was vestibular or auditory (which is discussed below).
BMP4 and BMP7 gene expressions in the basilar papilla
Our previous study (Wu and Oh, 1996BMP7 gene expression in the auditory component of the inner ear was quite different from that of the vestibular portion. Instead of segregating away from the sensory tissues, BMP7 gene expression became restricted to the sensory tissue in the papilla as development continued. Later in development, BMP7 was expressed only in supporting cells of the basilar papilla, whereas BMP4 localized to hair cells. During this period of segregation, from E12 to E16, the basilar papilla exhibits the spatula shape of a mature papilla (Cotanche and Sulik, 1985
BMP4 and BMP7 gene expression in the vestibular organs
In the vestibular portion of the inner ear, BMP7 gene expression segregated from the sensory tissue proper as sensory organs started to differentiate. For example, in the superior crista, the segregation of BMP7 from the main sensory area at E5 coincided with the beginning of histological differentiation (Knowlton, 1967Relationship of BMP4 and BMP7 coordinate expression in the inner ear
At the moment, we do not know the functions of these BMPs in the inner ear, nor do we know the significance of different BMP gene expression patterns among auditory and vestibular sensory organs. Nevertheless, these various expression patterns may contribute to the ultimate difference in structures and functions of the sensory organs. Functions that have been ascribed to the TGF-Another question concerning BMP function is whether specific coordination among different BMPs is required to bring about normal morphogenesis of the inner ear. During embryogenesis, BMP4 and BMP7 were colocalized in many tissues, such as the allantois, apical epidermal ridge, and mesenchyme of limb bud (Jones et al., 1991
FOOTNOTES
Received April 26, 1996; revised July 24, 1996; accepted July 29, 1996.
We are indebted to the staff in the Biocomputation Center at Ames Research Center, NASA, for their help with ROSS software. We thank Dr. Manning Correia for consultation on the structure of crista ampullaris and Dr. Fabio Nunes in our laboratory for repeating some of the results presented. We also thank Regeneron Pharmaceutical Company for the gift of the chicken BDNF probe; Drs. Connie Cepko, James Battey, Susan Wray, and Daniel Choo for critical reading of this manuscript; and Ms. Mirene Boerner for editing.
Correspondence should be addressed to Doris K. Wu, National Institute on Deafness and Other Communication Disorders, 5 Research Court, Room 2B34, Rockville, MD 20850.
Dr. Oh's present address: Department of Otolaryngology, Seoul National University, 28 Yongon-Dong Chono-Gu, Seoul, Korea 110-744.
REFERENCES
- Anniko M (1983) Embryonic development of vestibular sense organs and their innervation. In: Development of auditory and vestibular system (Romand, RS, eds) , p. 375. New York: Academic.
- Bartolami S, Goodyear R, Richardson G (1991) Appearance and distribution of the 275 kDa hair-cell antigen during development of the avian inner ear. J Comp Neurol 314:777-788 . [Web of Science][Medline]
- Basler K, Edlund T, Jessell TM, Yamada T (1993) Control of cell pattern in the neural tube: regulation of cell differentiation by dosalin-1, a novel TGF
- Capdevila J, Guerrero I (1994) Targeted expression of the signalling molecule decapentaplegic induces pattern duplications and growth alterations in Drosophila wings. EMBO J 13:4459-4468 . [Web of Science][Medline]
- Capovilla M, Brandt M, Botas J (1994) Direct regulation of decapentaplegic by ultrabithorax and its role in Drosophila midgut morphogenesis. Cell 76:461-475 . [Web of Science][Medline]
- Carpenter EM, Goddard JM, Chisaka O, Manley NR, Capecchi MR (1993) Loss of Hox-a1 (Hox-1.6) function results in the reorganization of the murine hindbrain. Development 118:1063-1075 . [Abstract]
- Chirgwin JM, Przbyla AE, MacDonald RJ, Rutter WJ (1979) Isolation of biologically active ribonucleic acid from sources enriched in ribonucleases. Biochemistry 18:5294-5299 . [Medline]
- Cohen GM, Cotanche DA (1992) Development of the sensory receptors and their innervation in the chick cochlea. In: Development of auditory and vestibular systems, Vol 2 (Romand, AL, eds) , p. 101. New York: Elsevier.
- Cordes SP, Barsh GS (1994) The mouse segmentation gene kr encodes a novel basic domain-leucine zipper transcription factor. Cell 79:1025-1034 . [Web of Science][Medline]
- Cotanche DA, Sulik KK (1983) Early differentiation of hair cells in the embryonic chick basilar papilla: a preliminary report. Arch Otorhinolaryngol 237:191-195 . [Medline]
- Cotanche DA, Sulik KK (1984) The development of stereociliary bundles in the cochlear duct of chick embryos. Dev Brain Res 16:181-193.
- Cotanche DA, Sulik KK (1985) Parameters of growth in the embryonic and neonatal chick basilar papilla. Scanning Electron Microsc 1:407-417.
- Dohlman G (1964) Secretin and absorption of endolymph. Ann Otol Rhinol Laryngol 73:708-723. [Web of Science][Medline]
- Dudley AT, Lyons KM, Robertson EJ (1995) A requirement for bone morphogenetic protein-7 during development of the mammalian kidney and eye. Gene Dev 9:2795-2807.
[Abstract/Free Full Text] - Duguid JR, Dinauer MC (1990) Library subtraction of in vitro cDNA libraries to identify differentially expressed genes in scrapie infection. Nucleic Acids Res 18:2789-2792 .
[Abstract/Free Full Text] - Fermin CD, Cohen GM (1984) Developmental gradients in the embryonic chick's basilar papilla. Acta Otolaryngol 97:39-51 . [Medline]
- Francis PH, Richardson MK, Brickell PM, Tickle C (1994) Bone morphogenetic proteins and a signalling pathway that controls patterning in the developing chick limb. Development 120:209-218 . [Abstract]
- Frohman MA, Martin GR, Corder SP, Halamek LP, Barsh GS (1993) Altered rhombomere-specific gene expression and hyoid bone differentiation in the mouse segmentation mutant, kreisler (kr). Development 117:925-936 . [Abstract]
- Ginzberg RD, Gilula NB (1979) Modulation of cell junctions during differentiation of the chicken otocyst sensory epithelium. Dev Biol 68:110-129 . [Web of Science][Medline]
- Ginzberg RD, Gilula NB (1980) Synaptogenesis in the vestibular sensory epithelium of the chick embryo. J Neurocytol 9:405-424 . [Web of Science][Medline]
- Green M (1968) Mechanism of the pleiotropic effects of the short-ear mutant gene in the mouse. J Exp Zool 167:129-150 . [Web of Science][Medline]
- Hamburger V, Hamilton H (1951) A series of normal stages in the development of the chick embryo. J Morphol 88:49-52. [Web of Science]
- Hawley SH, Wunnenberg-Stapleton K, Hashimoto C, Laurent MN, Watabe T, Blumberg BW, Cho KWY (1995) Disruption of BMP signals in embryonic Xenopus ectoderm leads to direct neural induction. Genes Dev 9:2923-2935 .
[Abstract/Free Full Text] - Houston B, Thorp BH, Burt DW (1994) Molecular cloning and expression of bone morphogenetic protein-7 in the chick epiphyseal growth plate. J Mol Endocrinol 13:289-301 .
[Abstract/Free Full Text] - Jones MC, Lyons KM, Hogan BLM (1991) Involvement of bone morphogenetic protein-4 (BMP-4) and Vgr-1 in morphogenesis and neurogenesis in the mouse. Development 111:531-542. [Abstract]
- Katayama A, Corwin JT (1989) Cell production in the chicken cochlea. J Comp Neurol 281:129-135 . [Web of Science][Medline]
- Katayama A, Corwin JT (1993) Cochlear cytogenesis visualized through pulse labeling of chick embryos in culture. J Comp Neurol 333:28-40 . [Web of Science][Medline]
- King JA, Marker PC, Seung KJ, Kingsley DM (1994) BMP5 and the molecular, skeletal, and soft-tissue alterations in short ear mice. Dev Biol 166:112-122 . [Web of Science][Medline]
- Kingsley DM (1994) The TGF-
[Free Full Text] - Kingsley DM, Bland AE, Grubber JM, Marker PC, Russell LB, Copeland NG, Jenkins NA (1992) The mouse short ear skeletal morphogenesis locus is associated with defects in a bone morphogenetic TGF
- Knowlton VY (1967) Correlation of the development of membranous and bony labyrinths, acoustics ganglia, nerves, and brain centers of the chick embryos. J Morphol 121:179-208. [Web of Science]
- Landolt JP, Correia MJ, Young ER, Cardin RPS, Sweet RC (1975) A scanning electron microscopic study of the morphology and geometry of neural surfaces and structures associated with the vestibular apparatus of the pigeon. J Comp Neurol 159:257-288 . [Web of Science][Medline]
- Luo G, Hofmann C, Bronckers ALJJ, Sohocki M, Bradley A, Karsenty G (1995) BMP-7 is an inducer of nephrogenesis, and is also required for eye development and skeletal patterning. Genes Dev 9:2808-2820 .
[Abstract/Free Full Text] - Lyons KM, Pelton RW, Hogan BLM (1990) Organogenesis and pattern formation in the mouse: RNA distribution patterns suggest a role for bone morphogenetic protein-2A (BMP-2A). Development 109:833-844 .
[Abstract/Free Full Text] - Lyons KM, Hogan BLM, Robertson EJ (1995) Colocalization of BMP 7 and BMP 2 RNAs suggests that these factors cooperatively mediate tissue interactions during murine development. Mech Dev 50:71-83 . [Web of Science][Medline]
- Maisonpierre PC, Belluscio L, Conover JC, Yancopoulos GD (1992) Gene sequences of chicken BDNF and NT-3. DNA Sequence 3:49-54 . [Medline]
- Mansour SL, Goddard JM, Capecchi MR (1993) Mice homozygous for a targeted disruption of the proto-oncogene int-2 have developmental defects in the tail and inner ear. Development 117:13-28 .
[Abstract/Free Full Text] - Mark M, Lufkin T, Vonesch J-L, Ruberte E, Olivo J, Dolle P, Gorry P, Lumsden A, Chambon P (1993) Two rhombomeres are altered in Hoxa-1 mutant mice. Development 119:319-338 . [Abstract]
- Massague J (1990) The transforming growth factor-
- Padgett RW, Wozney J, Gelbart WM (1993) Human BMP sequences can confer normal dorsal-ventral patterning in the Drosophila embryo. Proc Natl Acad Sci USA 90:2905-2909 .
[Abstract/Free Full Text] - Pirvola U, Ylikoski J, Palgi J, Lehtonen E, Arumae U, Saarma M (1992) Brain-derived neurotrophic factor and neurotrophin 3 mRNAs in the peripheral target fields of developing inner ear ganglia. Proc Natl Acad Sci USA 89:9915-9919 .
[Abstract/Free Full Text] - Riddle RD, Johnson RL, Laufer E, Tabin C (1993) Sonic hedgehog mediates the polarizing activity of the ZPA. Cell 75:1401-1416 . [Web of Science][Medline]
- Roberts DJ, Johnson RL, Burke AC, Nelson CE, Morgan BA, Tabin C (1995) Sonic hedgehog is an endodermal signal inducing Bmp-4 and Hox genes during induction and regionalization of the chick hindgut. Development 121:3163-3174 . [Abstract]
- Sampath TK, Rashka KE, Doctor JS, Tucker RF, Hoffmann FM (1993) Drosophila transforming growth factor beta superfamily proteins induce endochondral bone formation in mammals. Proc Natl Acad Sci USA 90:6004-6008 .
[Abstract/Free Full Text] - Simon H-G, Tabin CJ (1993) Analysis of Hox-4.5 and Hox-3.6 expression during newt limb regeneration: differential regulation of paralogous Hox genes suggest different roles for members of different Hox clusters. Development 117:1397-1407 . [Abstract]
- Vainio S, Karavanova I, Jowett A, Thesleff I (1993) Identification of BMP-4 as a signal mediating secondary induction between epithelial and mesenchymal tissues during early tooth development. Cell 75:45-58 . [Web of Science][Medline]
- Wheeler EF, Bothwell M, Schecterson LC, von Bartheld CS (1994) Expression of BDNF and NT-3 mRNA in hair cells of the organ of Corti: quantitative analysis in developing rats. Hear Res 73:46-56 . [Web of Science][Medline]
- Whitehead MC, Morest DK (1985) The development of innervation patterns in the avian basilar papilla. Neuroscience 14:255-276 . [Web of Science][Medline]
- Winnier G, Blessing M, Labosky PA, Hogan BLM (1995) Bone morphogenetic protein-4 is required for mesoderm formation and patterning in the mouse. Genes Dev 9:2105-2116 .
[Abstract/Free Full Text] - Wu DK, Oh SH (1996) Sensory organ generation in the chick inner ear. J Neurosci 16:0000-0000.
- Ylikoski J, Pirvola U, Moshnyakov M, Palgi J, Arumae U, Saarma M (1993) Expression patterns of neurotrophin and their receptor mRNAs in the rat inner ear. Hear Res 65:69-78 . [Web of Science][Medline]
Copyright ©1996 Society for Neuroscience 0270-6474/1996/166463-13$05.00/0
This article has been cited by other articles:
F. Muller, H. Rohrer, and A. Vogel-Hopker
Bone morphogenetic proteins specify the retinal pigment epithelium in the chick embryo
Development, October 1, 2007; 134(19): 3483 - 3493.
[Abstract] [Full Text] [PDF]
N. Daudet, L. Ariza-McNaughton, and J. Lewis
Notch signalling is needed to maintain, but not to initiate, the formation of prosensory patches in the chick inner ear
Development, June 15, 2007; 134(12): 2369 - 2378.
[Abstract] [Full Text] [PDF]
S.-H. Cho and C. L. Cepko
Wnt2b/{beta}-catenin-mediated canonical Wnt signaling determines the peripheral fates of the chick eye
Development, August 15, 2006; 133(16): 3167 - 3177.
[Abstract] [Full Text] [PDF]
K. F. Barald and M. W. Kelley
From placode to polarization: new tunes in inner ear development
Development, September 1, 2004; 131(17): 4119 - 4130.
[Abstract] [Full Text] [PDF]
W. Chang, J. V. Brigande, D. M. Fekete, and D. K. Wu
The development of semicircular canals in the inner ear: role of FGFs in sensory cristae
Development, September 1, 2004; 131(17): 4201 - 4211.
[Abstract] [Full Text] [PDF]
H. Li, G. Roblin, H. Liu, and S. Heller
From The Cover: Generation of hair cells by stepwise differentiation of embryonic stem cells
PNAS, November 11, 2003; 100(23): 13495 - 13500.
[Abstract] [Full Text] [PDF]
W. Zheng, L. Huang, Z.-B. Wei, D. Silvius, B. Tang, and P.-X. Xu
The role of Six1 in mammalian auditory system development
Development, September 1, 2003; 130(17): 3989 - 4000.
[Abstract] [Full Text] [PDF]
R. D. Hawkins, S. Bashiardes, C. A. Helms, L. Hu, N. L. Saccone, M. E. Warchol, and M. Lovett
Gene expression differences in quiescent versus regenerating hair cells of avian sensory epithelia: implications for human hearing and balance disorders
Hum. Mol. Genet., June 1, 2003; 12(11): 1261 - 1272.
[Abstract] [Full Text] [PDF]
D. L. Thompson, L. M. Gerlach-Bank, K. F. Barald, and R. J. Koenig
Retinoic Acid Repression of Bone Morphogenetic Protein 4 in Inner Ear Development
Mol. Cell. Biol., April 1, 2003; 23(7): 2277 - 2286.
[Abstract] [Full Text] [PDF]
B. H. Alsan and T. M. Schultheiss
Regulation of avian cardiogenesis by Fgf8 signaling
Development, March 6, 2003; 129(8): 1935 - 1943.
[Abstract] [Full Text] [PDF]
A. Vogel-Hopker and H. Rohrer
The specification of noradrenergic locus coeruleus (LC) neurones depends on bone morphogenetic proteins (BMPs)
Development, March 4, 2003; 129(4): 983 - 991.
[Abstract] [Full Text] [PDF]
J. Bryant, R. J Goodyear, and G. P Richardson
Sensory organ development in the inner ear: molecular and cellular mechanisms
Br. Med. Bull., October 1, 2002; 63(1): 39 - 57.
[Abstract] [Full Text] [PDF]
W. Wang, E. K. Chan, S. Baron, T. Van De Water, and T. Lufkin
Hmx2 homeobox gene control of murine vestibular morphogenesis
Development, December 15, 2001; 128(24): 5017 - 5029.
[Abstract] [Full Text] [PDF]
V. Vendrell, E. Carnicero, F. Giraldez, M. T. Alonso, and T. Schimmang
Induction of inner ear fate by FGF3
Development, May 15, 2000; 127(10): 2011 - 2019.
[Abstract] [PDF]
L. Gerlach, M. Hutson, J. Germiller, D Nguyen-Luu, J. Victor, and K. Barald
Addition of the BMP4 antagonist, noggin, disrupts avian inner ear development
Development, January 1, 2000; 127(1): 45 - 54.
[Abstract] [PDF]
S.-Z. Lin, B. J. Hoffer, P. Kaplan, Y. Wang, and C. Y. Hsu
Osteogenic Protein-1 Protects Against Cerebral Infarction Induced by MCA Ligation in Adult Rats • Editorial Comment
Stroke, January 1, 1999; 30(1): 126 - 133.
[Abstract] [Full Text] [PDF]
J. C. Lin and C. L. Cepko
Granule Cell Raphes and Parasagittal Domains of Purkinje Cells: Complementary Patterns in the Developing Chick Cerebellum
J. Neurosci., November 15, 1998; 18(22): 9342 - 9353.
[Abstract] [Full Text] [PDF]
J. T. Corwin
Identifying the genes of hearing, deafness, and dysequilibrium
PNAS, October 13, 1998; 95(21): 12080 - 12082.
[Full Text] [PDF]
H. Morsli, D. Choo, A. Ryan, R. Johnson, and D. K. Wu
Development of the Mouse Inner Ear and Origin of Its Sensory Organs
J. Neurosci., May 1, 1998; 18(9): 3327 - 3335.
[Abstract] [Full Text] [PDF]
C Haddon, Y. Jiang, L Smithers, and J Lewis
Delta-Notch signalling and the patterning of sensory cell differentiation in the zebrafish ear: evidence from the mind bomb mutant
Development, January 12, 1998; 125(23): 4637 - 4644.
[Abstract] [PDF]
M Xiang, W. Gao, T Hasson, and J. Shin
Requirement for Brn-3c in maturation and survival, but not in fate determination of inner ear hair cells
Development, January 10, 1998; 125(20): 3935 - 3946.
[Abstract] [PDF]
H Herbrand, S Guthrie, T Hadrys, S Hoffmann, H. Arnold, S Rinkwitz-Brandt, and E Bober
Two regulatory genes, cNkx5-1 and cPax2, show different responses to local signals during otic placode and vesicle formation in the chick embryo
Development, January 2, 1998; 125(4): 645 - 654.
[Abstract] [PDF]
T M Schultheiss, J B Burch, and A B Lassar
A role for bone morphogenetic proteins in the induction of cardiac myogenesis.
Genes & Dev., February 15, 1997; 11(4): 451 - 462.
[Abstract] [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 (88) Citing Articles via Google Scholar Google Scholar Articles by Oh, S.-H. Articles by Wu, D. K. Search for Related Content PubMed PubMed Citation Articles by Oh, S.-H. Articles by Wu, D. K.
ABSTRACT
|
|
|
|
 |
|