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Previous Article | Next Article
The Journal of Neuroscience, January 1, 2000, 20(1):187-195
Ninjurin2, a Novel Homophilic Adhesion Molecule, Is Expressed in Mature Sensory and Enteric Neurons and Promotes Neurite Outgrowth
Toshiyuki Araki and Jeffrey Milbrandt Division of Laboratory Medicine, Department of Pathology and Medicine, Washington University School of Medicine, St. Louis, Missouri 63110
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
A large number of cell adhesion molecules mediate cell-to-cell and cell-to-extracellular matrix interaction during development, differentiation and regeneration of the peripheral nervous system. Here, we report the identification of a novel cell surface adhesion molecule, ninjurin2 (for nerve injury induced protein 2). Ninjurin2 is a homolog of a homophilic cellular adhesion molecule, ninjurin1, that was previously isolated as a gene induced in Schwann cells after nerve injury. Ninjurin1 and 2 share conserved hydrophobic regions for their transmembrane domains; however, they do not contain comparable adhesion motifs nor do they interact with each other. In the peripheral nervous system, ninjurin2 is expressed constitutively in mature sensory and enteric neurons but not in glial cells or in autonomic ganglia. Ninjurin2 is upregulated in Schwann cells surrounding the distal segment of injured nerve with a time course similar to that of ninjurin1, neural CAM, and L1. Ninjurin2 promotes neurite outgrowth from primary cultured dorsal root ganglion neurons, presumably via homophilic cellular interactions. Ninjurin2 is also highly expressed in hematopoietic and lymphatic tissues. Finally, the ninjurin2 gene is located on human chromosome 12p13 in which several disorders of unknown etiology have been mapped, including inflammatory bowel disease and acrocallosal syndrome.
Key words: cell adhesion; postmitotic; peripheral nervous system; hematopoietic and lymphatic organs; chromosome 12p13; inflammatory bowel disease; acrocallosal syndrome
INTRODUCTION
Cell surface adhesion molecules play an important role in the peripheral nervous system (PNS) (Colello and Pott, 1997
; Fu and Gordon, 1997
During efforts to identify genes upregulated in Schwann cells after sciatic nerve axotomy, we identified a novel cell adhesion molecule, which we termed ninjurin1 (for nerve injury induced protein 1) (Araki and Milbrandt, 1996
Here, we report the identification of a new molecule bearing significant homology to ninjurin1, which we named ninjurin2. Ninjurin2 is also a cell surface adhesion molecule, but it does not share the adhesion motif sequence with ninjurin1. Expression of ninjurin2 is constitutive and abundant in almost all the sensory ganglion neurons and enteric neurons but weak in peripheral glial cells and neurons in autonomic system. A developmental profile of ninjurin2 expression in DRG and enteric ganglia indicated that ninjurin2 expression is dramatically elevated in differentiated postmitotic neurons. In the CNS, ninjurin2 expression is observed in radial glial cells but not in neurons. Ninjurin2 is upregulated in Schwann cells in the distal nerve segment after peripheral nerve injury, and it promotes neurite outgrowth from DRG neurons via ninjurin2-mediated homophilic cellular interaction.
MATERIALS AND METHODS
Cloning and sequence analysis. All sequencing analysis was performed on an Applied Biosystems (Foster City, CA) 373DNA sequencer using Taq DyeDeoxy Terminator cycle sequencing kits (Applied Biosystems). Sequence editing, mapping, alignment, and contig generation were performed using the DNAstar software package. Expressed sequence tags (ESTs) were obtained from the Washington University-Merck EST project and sequenced completely. Based on the identified human ninjurin2 cDNA sequence, primers for mouse ninjurin2 (5'-ATGCTGGACGTGGCGCTCTTTATG-3' and 5'-TATGAAGACCAAGATGGTGGCAGCATT-3') were synthesized, and partial mouse ninjurin2 sequence was amplified by PCR. Rapid amplification of cDNA ends (RACE) PCR was performed using Klentaq-LA (Barnes, 1994
For the ninjurin2 expression construct (pNINJ2), the coding region of the human ninjurin2 cDNA was amplified by Klentaq-LA from the brain marathon RACE cDNA library, using primers 5'-GTCGAGATCTACCATGGAATCAGCAAGAGAA-3' and 5'-CTAAAAGCTTAGAGAGGATTCCTTGAGGC-3'. The product was cloned into pCB6 expression vector (Brewer, 1994
Analysis of RNA expression. The human RNA master blot (Clontech) containing normalized samples of poly(A+) RNA was used according to the manufacturer's instructions. The blot was probed with random hexamer-primed 32P-labeled cDNA probe (nucleotides 90-888 of human ninjurin2), and the signals were visualized with a PhosphorImager (Molecular Dynamics, Sunnyvale, CA). Human embryonic RNAs on the blot were pooled from fetal tissues of 10-30 weeks of gestation.
Sciatic nerves were transected as described previously (Araki and Milbrandt, 1996
Immunohistochemical analysis. A mixture of three synthetic peptides (see Fig. 5) was conjugated to keyhole limpet hemocyanin by glutaraldehyde cross-linking. The conjugated protein was used to immunize rabbits following standard procedures. Anti-ninjurin2 antibodies were purified by chromatography over an affinity column in which the peptides were linked to EAH Sepharose 4B (Amersham Pharmacia Biotech, Uppsala, Sweden) per the manufacturer's instructions. Protein blot analysis was performed as described previously (Lee et al., 1995
Cell culture and transfection. CHO and Jurkat cells were cultured as described previously (Araki and Milbrandt, 1996
Peptide preparation. Three synthetic peptides with sequences corresponding to the indicated regions of human ninjurin2 (see Fig. 4C) were made and purified by HPLC. The purity and composition of the purified peptides were verified by mass spectrometry. The purified peptides were dissolved at 10 mg/ml in distilled water and stored at
70°C. A 30-residue synthetic peptide that was previously used for characterizing ninjurin1-mediated adhesion (P4 in Araki et al., 1997
Cell adhesion assays. Aggregation assays were performed using Jurkat cells stably transfected with pCB6 or pNINJ2 as described previously (Rothlein and Springer, 1986
For heterophilic adhesion analysis, ninjurin1-expressing Jurkat cells (N1 cells) or wild-type Jurkat cells were stained green with 1 µM 5-chloromethylfluorescein diacetate (CMFTA) (Molecular Probes, Eugene, OR), and ninjurin2-expressing cells (N2 cells) were stained red by 1 µM 5-(and6)-(((4-chloromethyl)benzoyl)amino)tetramethylrhodamine (CMTMR) as described in the manufacturer's instructions (Molecular Probes). The cells were resuspended to 1 × 106 cells/ml, and 2 ml of the mixed cell suspension were allowed to form aggregates in six-well culture plates for 2 hr. Quantitative analysis of heterophilic aggregation was performed as described previously with minor modifications (Murphy-Erdosh et al., 1995
RESULTS
Identification, sequence analysis, and genomic localization of ninjurin2
Ninjurin2 was identified by performing a basic local alignment search tool (BLAST version 2.0) (Altschul et al., 1990
The nucleotide sequence of the human ninjurin2 cDNA predicts an open reading frame of 142 amino acids, which is 73% identical to mouse ninjurin2. Human ninjurin2 protein is 55% identical to human ninjurin1 but has no significant homology to any other known proteins in the database. Ninjurin2 has two hydrophobic regions, both of which can form transmembrane domains (PSORT algorithm; Nakai and Kanehisa, 1992
To analyze the genomic locus of ninjurin2, we identified and sequenced a human ninjurin2 genomic clone. The ninjurin2 gene has three introns, and the location of all three of these introns is precisely conserved between ninjurin1 and ninjurin2 (Fig. 1). A BLAST search against the high throughput genome sequence database revealed that human ninjurin2 is located on chromosome 12, region p13. A search of the On-line Mendelian Inheritance in Men (OMIM) database showed that some human diseases of unknown pathogenesis have been linked to this region, including acrocallosal syndrome (polydactyly and loss of corpus callosum) and inflammatory bowel disease.
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Figure 1. Sequence analysis of ninjurin2. A, Alignment of human ninjurin1 and ninjurin2. Identical residues are boxed, and putative transmembrane domains are underlined. Arrowheads denote intron-exon junctions. Note that these sites are conserved between the ninjurin1 and 2 genes. B, Alignment of human and mouse ninjurin2 amino acid sequences. Identical residues are boxed, and putative transmembrane domains are underlined.
Ninjurin2 is located on the plasma membrane and mediates homophilic adhesion
To characterize the ninjurin2 protein and examine its cellular localization, we generated polyclonal antiserum against a mixture of three synthetic peptides derived from the ninjurin2 N terminus (amino acids 1-30, 15-45, and 31-60, as shown in Fig. 4C). Anti-ninjurin2 antibodies were then purified by immunoaffinity chromatography. These antibodies recognized a ~20 kDa protein expressed in CHO cells that were stably transfected with pNINJ2 but that was absent in either control CHO cells or CHO cells stably expressing ninjurin1 (Fig. 2).
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Figure 2. Protein blot analysis of ninjurin2. Proteins from lysates prepared from native CHO cells (lane 1), CHO cells stably transfected with a pNINJ1 expression construct (lane 2), and CHO cells stably transfected with pNINJ2 construct (lane 3) were electrophoresed on 12% SDS-polyacrylamide gels, transferred to nitrocellulose, and incubated with affinity-purified anti-ninjurin2 antibodies. Ninjurin2 was visualized by using enhanced chemiluminescence.
The high sequence homology with ninjurin1 in the putative transmembrane domain and immunocytochemical analysis of CHO cells stably expressing ninjurin2 suggested that ninjurin2 is located on the cytoplasmic membrane (Fig. 3B). To examine this possibility, we performed immunostaining of live CHO cells stably expressing ninjurin2 using conditions in which antibodies do not penetrate the cell membrane and are not internalized. Anti-ninjurin2 antibodies showed intense staining on the cell surface (Fig. 3C), whereas negative control
-actin antibodies showed no staining under similar conditions (data not shown). This clearly indicated that ninjurin2 is located on the plasma membrane and that the N-terminal region of ninjurin2 (to which the antibodies were raised) is located extracellularly.
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Figure 3. Ninjurin2 is localized on the plasma membrane. Immunocytochemical localization of ninjurin2 on wild-type CHO cells (A) and CHO cells transfected with pNINJ2 (B-D). Anti-ninjurin2 antibodies were applied to cells either after fixation with 4% paraformaldehyde (A, B) or before fixation (C). In D, anti-ninjurin2 antisera were blocked by incubation with the peptide immunogen and applied to cells as in B (see Materials and Methods). Scale bar, 40 µm.
The cell surface localization of ninjurin2 and its homology with the adhesion molecule ninjurin1 suggested that ninjurin2 might also be an adhesion molecule. To test whether ninjurin2 mediates cellular adhesion, we performed standard cell aggregation assays using Jurkat cells (Shimizu et al., 1990
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Figure 4. Ninjurin2 mediates homophilic cell adhesion. Native Jurkat cells (A) and Jurkat cells stably transfected with pNINJ2 (B) were resuspended at 1 × 106 cells/ml and allowed to aggregate at 37°C for 1 hr. Note the presence of large aggregates in B. C, List of peptides used in competition experiments and also as antigens to raise anti-ninjurin2 antisera. D, Aggregation assays were performed using ninjurin2 stably expressing Jurkat cells in the presence of each of the indicated peptides. The number of cells in aggregates was determined after 1 hr. The ratio of cells in aggregates to total cells was calculated and plotted versus peptide concentration. Data represents the mean ± SD of three independent experiments. E, F, Aggregation assays were performed with a mixture of N2 cells (stained with red-orange fluorescent dye) and either N1 cells (E) or wild-type cells (F) (stained with green fluorescent dye). Note that the green cells indicated by arrows and red-orange cells indicated by arrowheads individually form aggregates in E, and only red cells form aggregates in F as indicated by arrowheads. G, Quantitative analysis of aggregation assays using mixed cell populations. The aggregation assays were performed as in E and F, and red cells and green cells in each aggregate were counted. The graph represents the mean ± SD percentage of N2 cells in aggregates that consist predominantly of N2 cells.
The ability of ninjurin2 to associate heterophilically with ninjurin1 or other molecules expressed on wild-type Jurkat cells was also investigated, because many other homophilic adhesion molecules associate heterophilically with their family members. Aggregation assays were performed by mixing an equal number of Ninjurin1-expressing Jurkat cells (N1 cells) or wild-type cells (stained green) and N2 cells (stained red). For quantitative analysis, the number of green cells and red cells in each aggregate was counted. Aggregates formed in the N1-N2 mixture were either N1 cell-predominant or N2 cell-predominant (Fig. 4E), whereas mixed aggregates (containing N1 and N2 cells) were very rare. Only N2-predominant aggregates were observed in the N2 wild-type mixture (Fig. 4F). The percentage of N2 cells in N2 cell-predominant aggregates was calculated for each of the mixtures (Fig. 4G). The percentages of N2 cells were not significantly different, regardless of the cell type with which they were mixed, indicating that N2 cells do not interact with either wild-type or N1 cells. These results indicate that ninjurin2 does not show heterophilic association with ninjurin1 or surface molecules expressed on wild-type Jurkat cells.
Expression of ninjurin2 mRNA and protein
To obtain further insight into the function of ninjurin2 in vivo, we examined mRNA expression in a variety of embryonic and adult organs on a human tissue mRNA blot. High expression of ninjurin2 mRNA was observed in a limited number of organs. In the adult, ninjurin2 mRNA expression was highest in the bone marrow, followed by peripheral leukocytes, lung, and lymph nodes (Fig. 5).
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Figure 5. Expression of ninjurin2 mRNA in human tissues. A human mRNA dot blot (Clontech) was probed with a 32P-labeled fragment of the human ninjurin2 cDNA. The hybridization signal intensity was quantified by using a PhosphorImager.
We further examined the expression of ninjurin2 in adult rat organs by immunohistochemistry. In addition to the organs expressing ninjurin2 identified by RNA blots, other tissues showed expression of ninjurin2 with restricted distribution patterns. In the kidney, ninjurin2 was detected specifically in the glomeruli (Fig. 6A). In the adrenal gland, ninjurin2 expression was observed only in the glomerular layer of the cortex (Fig. 6B). In the CNS, neuronal expression of ninjurin2 was very low; however, ninjurin2 was detected in radial glial cells during development and in adulthood (data not shown).
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Figure 6. Immunohistochemical analysis of ninjurin2 expression in adult rat. Affinity-purified antibodies were used to detect ninjurin2 expression by immunohistochemistry in kidney (A), adrenal (B), trigeminal ganglion (C), DRG (D), superior cervical ganglion (E), and enteric plexus (F). Arrows denote glomeruli in A and glomerular layer in the adrenal cortex in B. Arrows and arrowheads denote submucosal and myenteric plexus, respectively, in F. Scale bars, 100 µm.
Ninjurin2 is expressed in mature postmitotic sensory and enteric neurons
To determine whether ninjurin2 plays a role in the PNS, expression of ninjurin2 was examined in detail by immunohistochemistry. Expression of ninjurin2 was detected in most neurons of the sensory and enteric ganglia, but in contrast to ninjurin1 (Araki and Milbrandt, 1996
To explore the developmental regulation of ninjurin2 expression in the PNS, immunohistochemical analysis was performed on mouse DRG at E14, E19, and postnatal day 2 (P2) and in the mouse enteric ganglia at E17, P1, and P3. In the DRG, ninjurin2 expression was very weak at E14 (Fig. 7A), became apparent at E19 (Fig. 7B), and by P2, the intensity of staining was comparable with the adult level (Fig. 7C). An examination of the enteric ganglia revealed that ninjurin2 is not expressed at E17 (Fig. 7D), but weak ninjurin2 immunoreactivity was observed in neurons of the myenteric ganglia at P1 (Fig. 7E) and was more intense at P3 (Fig. 7F). In contrast, ninjurin2 expression was undetected in the submucosal plexus.
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Figure 7. Expression of ninjurin2 in sensory and enteric neurons during development. Immunohistochemistry was used to detect ninjurin2 in mouse DRG at E14 (A), E19 (B), and P3 (C) and in mouse enteric plexus at E17 (D), P1 (E), and P3 (F). Arrows denote the ganglia in each micrograph. Scale bars: A, D, E, 50 µm; B, C, F, 150 µm.
Neuronal proliferation in the myenteric ganglia is almost complete by P3, whereas in the submucosal plexus, neurons are generated later in development (by P14) (Pham et al., 1991
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Figure 8. Ninjurin2 is expressed in postmitotic neurons in enteric ganglia. A, B, Ninjurin2 immunoreactivity in enteric plexus in P3 mouse gut (A) was compared with neuron-specific enolase immunoreactivity on an adjacent section (B). Note that myenteric neurons denoted by arrows express ninjurin2, but submucosal neurons denoted by arrowheads in B, which differentiate later than myenteric neurons, lack ninjurin2 expression in A. Scale bar, 100 µm. C-F, BrdU and either ninjurin2 (C, D) or NSE (E, F) were visualized on the same section of mouse gut at P3. A mouse (P3) was injected with BrdU and killed 1 hr later for immunohistochemistry. Ninjurin2 (C) and NSE expression (E) were visualized by Cy3-conjugated secondary antibody, and proliferating cells were visualized by FITC-conjugated anti-BrdU immunohistochemistry (D, F). The ninjurin2-positive myenteric ganglia lack BrdU staining (arrows in C and D), whereas the NSE-positive cells in the submucosal ganglia indicated by arrows in E and F are BrdU-positive. Note that C and D represent the same section as do E and F. Scale bars, 50 µm.
Ninjurin2 is upregulated after nerve injury in Schwann cells
We were interested in characterizing the role of ninjurin2 after nerve injury, because the related ninjurin1 is highly induced in Schwann cells after nerve injury. To examine the expression of ninjurin2 after nerve injury, immunohistochemistry was performed to detect ninjurin2 in normal and injured nerves. In normal sciatic nerve, ninjurin2 expression was weak (Fig. 9A), but it was greatly upregulated 7 d after nerve transection in the distal segment of the injured nerve (Fig. 9B). The interdigitating pattern of ninjurin2 immunoreactivity in the injured nerve (Fig. 9D) closely resembled that observed for ninjurin1 (Fig. 9C), indicating that ninjurin2 is expressed by Schwann cells.
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Figure 9. Ninjurin2 is upregulated in Schwann cells after nerve injury. A-D, Immunohistochemistry was used to detect ninjurin2 on a longitudinal section of the normal sciatic nerve (A) or sciatic nerve segment distal to the site of injury (7 d after injury; B, low magnification; D, high magnification). In C, the section adjacent to D was stained with antibodies to ninjurin1. The very similar expression patterns in C and D indicate that ninjurin2 is expressed in Schwann cells in injured nerve. Scale bars: B, 100 µm; D, 50 µm. E, Total RNA (10 µg) was isolated from sciatic nerves distal to the site of transection at the indicated times after axotomy. The samples were electrophoresed, blotted, and hybridized with a 32P-labeled ninjurin2 cDNA probe. F, Ninjurin2 promotes neurite outgrowth from primary cultured DRG neurons. DRG neurons from E16 rat embryos were seeded onto a confluent monolayer of control CHO cells or CHO cells expressing ninjurin2. Six hours later, the cells were fixed, and neurites were visualized by immunostaining with neurofilament H antibodies. Neurite length was quantified by measuring neurites from ~50 neurons grown under each condition in three independent experiments. Data represent mean ± SD length.
To further characterize the regulation of ninjurin2 expression after nerve injury, we examined ninjurin2 mRNA levels for up to 8 weeks after nerve injury (Fig. 9E). A 1.0 kb ninjurin2 mRNA was detected at low levels in normal nerve but was highly upregulated after nerve injury and reached peak levels 7-14 d after injury. This time course of expression is similar to what has been observed for other nonmyelinating Schwann cell marker molecules, including ninjurin1 and p75 (Taniuchi et al., 1988
Ninjurin promotes neurite outgrowth from primary cultured DRG neurons
Upregulation of ninjurin2 in Schwann cells after nerve injury suggested that it may promote nerve regeneration by homophilic adhesive interactions as has been observed with other adhesion molecules (Seilheimer and Schachner, 1988
DISCUSSION
We have identified a novel member of the ninjurin family of adhesion molecules. Members of this family share high homology in the putative transmembrane domains, lack signal peptide sequences, and have the N-terminal hydrophilic region located extracellularly. The extracellular regions, especially the domains involved in adhesive interactions, are diverse. Although interactions between family members are commonly observed with other adhesion molecules (Brummendorf and Rathjen, 1996
The tissue distribution of ninjurin proteins indicates that they are involved in multiple functional systems in the body like most other known adhesion molecules. Ninjurin1 showed a wide distribution primarily among organs of epithelial origin, whereas ninjurin2 showed more restricted distribution; ninjurin2 was highly expressed in lymphatic and hematopoietic organs. In addition, the majority of human ninjuirn2 cDNA sequence in the dbEST database is derived from "germinal center B cells" libraries (data not shown). This suggests that ninjurin2 expression in the lymphatic cells is involved in B lymphocyte function, perhaps during maturation of B lymphocytes to the antibody-producing cells.
Ninjurin2 expression in mature sensory and enteric neurons clearly distinguishes this molecule from ninjurin1 and other cell surface adhesion molecules. In mouse DRG, many neurons are generated between E10 and E13 in a neurotrophin-3-dependent manner (Farinas et al., 1996
Expression of ninjurin2 in the DRG neurons is not uniform; there are a very small number of neurons in which ninjurin2 immunoreactivity is weak or absent. Such neurons are more clearly observed after axonal injury when most DRG neurons increase ninjurin2 expression. Coimmunostaining of ninjurin1 and ninjurin2 showed that ninjurin1 is also not induced in neurons that lack ninjurin2 expression (data not shown). This result suggests that some DRG neurons are dependent on surface molecules other than ninjurins for axonal regeneration or other functions.
Although ninjurin1 and 2 are differentially expressed in the PNS, ninjurin2 is likely to play a role in nerve regeneration via homophilic interaction, just like ninjurin1. The time course of upregulation of ninjurin2 after nerve injury is similar to that of ninjurin1, and the level of neurite outgrowth enhancement in coculture experiments with DRG neurons and ninjurin2-expressing CHO cells was comparable with the ninjurin1-mediated effect (Araki and Milbrandt, 1996
In the human chromosome region 12p13 in which ninjurin2 is located, several diseases of unknown etiology have been mapped (Pfeiffer et al., 1992
FOOTNOTES Received July 26, 1999; revised Oct. 8, 1999; accepted Oct. 12, 1999.
This work was supported by grants from McDonnell Center for Cellular and Molecular Neurobiology and Uehara Memorial Foundation, and National Institute of Health Grant 5P01CA49712. We thank members of the laboratory for comments on this manuscript.
Correspondence should be addressed to Jeffrey Milbrandt, Division of Laboratory Medicine, Department of Pathology and Medicine, Washington University School of Medicine, 660 South Euclid Avenue, Box 8118, St. Louis, MO 63110. E-mail: jeff{at}milbrandt.wustl.edu.
REFERENCES
- Altschul SF, Gish W, Miller W, Myers EW, Lipman DJ (1990) Basic local alignment search tool. J Mol Biol 215:403-410[Web of Science][Medline].
- Araki T, Milbrandt J (1996) Ninjurin, a novel adhesion molecule, is induced by nerve injury and promotes axonal growth. Neuron 17:353-361[Web of Science][Medline].
- Araki T, Zimonjic DB, Popescu NC, Milbrandt J (1997) Mechanism of homophilic binding mediated by ninjurin, a novel widely expressed adhesion molecule. J Biol Chem 272:21373-21380
[Abstract/Free Full Text] .- Barnes WM (1994) PCR amplification of up to 35-kb DNA with high fidelity and high yield from lambda bacteriophage templates. Proc Natl Acad Sci USA 91:2216-2220
[Abstract/Free Full Text] .- Bixby JL, Lilien J, Reichardt LF (1988) Identification of the major proteins that promote neural process outgrowth on Schwann cells in vitro. J Cell Biol 107:353-361
[Abstract/Free Full Text] .- Brewer CB (1994) Cytomegalovirus plasmid vectors for permanent lines of polarized epithelial cells. Methods Cell Biol 43:233-245.
- Brummendorf T, Rathjen FG (1996) Structure/function relationships of axon-associated adhesion receptors of the immunoglobulin superfamily. Curr Opin Neurobiol 6:584-593[Web of Science][Medline].
- Bush TG, Savidge TC, Freeman TC, Cox HJ, Campbell EA, Mucke L, Johnson MH, Sofroniew MV (1998) Fulminant jejuno-ileitis following ablation of enteric glia in adult transgenic mice. Cell 93:189-201[Web of Science][Medline].
- Colello RJ, Pott U (1997) Signals that initiate myelination in the developing mammalian nervous system. Mol Neurobiol 15:83-100[Web of Science][Medline].
- Duerr RH, Barmada MM, Zhang L, Davis S, Preston RA, Chensny LJ, Brown JL, Ehrlich GD, Weeks DE, Aston CE (1998) Linkage and association between inflammatory bowel disease and a locus on chromosome 12. Am J Hum Genet 63:95-100[Web of Science][Medline].
- Eichler ME, Rich KM (1989) Death of sensory ganglion neurons after acute withdrawal of nerve growth factor in dissociated cell cultures. Brain Res 482:340-346[Web of Science][Medline].
- Farinas I, Yoshida CK, Backus C, Reichardt LF (1996) Lack of neurotrophin-3 results in death of spinal sensory neurons and premature differentiation of their precursors. Neuron 17:1065-1078[Web of Science][Medline].
- Farinas I, Wilkinson G, Backus C, Reichardt L, Patapoutian A (1998) Characterization of neurotrophin and Trk receptor functions in developing sensory ganglia: direct NT-3 activation of TrkB neurons in vivo. Neuron 21:325-334[Web of Science][Medline].
- Fu SY, Gordon T (1997) The cellular and molecular basis of peripheral nerve regeneration. Mol Neurobiol 14:67-116[Web of Science][Medline].
- Gennarini G, Durbec P, Boned A, Rougon G, Goridis C (1991) Transfected F3/F11 Neuronal cell surface protein mediates intercellular adhesion and promotes neurite outgrowth. Neuron 6:595-606[Web of Science][Medline].
- Lee SL, Tourtellotte LC, Wesselschmidt RL, Milbrandt J (1995) Growth and differentiation proceeds normally in cells deficient in the immediate early gene NGFI-A. J Biol Chem 270:9971-9977
[Abstract/Free Full Text] .- Lemmon V, Farr KL, Lagenaur C (1989) L1-Mediated axon outgrowth occurs via a homophilic binding mechanism. Neuron 2:1597-1603[Web of Science][Medline].
- Murphy-Erdosh C, Yoshida CK, Paradies N, Reichardt LF (1995) The cadherin-binding specificities of B-cadherin and LCAM. J Cell Biol 129:1379-1390
[Abstract/Free Full Text] .- Nakai K, Kanehisa M (1992) A knowledge base for predicting protein localization sites in eukaryotic cells. Genomics 25:897-911.
- Panes L, Granger DN (1998) Leukocyte-endothelial cell interactions: molecular mechanisms and implications in gastrointestinal disease. Gastroenterology 114:1066-1090[Web of Science][Medline].
- Pfeiffer RA, Legat G, Trautmann U (1992) Acrocallosal syndrome in a child with de novo inverted tandem duplication of 12p11.2-p13.3. Ann Genet 35:41-46[Web of Science][Medline].
- Pham TD, Gershon MD, Rothman TP (1991) Time of origin of neurons in the murine enteric nervous system: sequence in relation to phenotype. J Comp Neurol 314:789-798[Web of Science][Medline].
- Rothlein R, Springer TA (1986) The requirement for lymphocyte function-associated antigen 1 in homotypic leukocyte adhesion stimulated by phorbol ester. J Exp Med 163:1132-1149
[Abstract/Free Full Text] .- Satsangi J, Parkes M, Louis E, Hashimoto L, Kato N, Welsh K, Terwilliger JD, Lathrop GM, Bell JI, Jewell DP (1996) Two stage genome-wide search in inflammatory bowel disease provides evidence for susceptibility loci on chromosomes 3, 7 and 12. Nat Genet 14:199-202[Web of Science][Medline].
- Scherer SS (1997) The biology and pathobiology of Schwann cells. Curr Opin Neurol 10:386-397[Web of Science][Medline].
- Seilheimer B, Schachner M (1988) Studies of adhesion molecules mediating interactions between cells of peripheral nervous system indicate a major role for L1 in mediating sensory neuron growth on schwann cells in culture. J Cell Biol 107:341-351
[Abstract/Free Full Text] .- Shimizu Y, Van Seventer GA, Horgan KJ, Shaw S (1990) Regulated expression and binding of three VLA (
- Taniuchi M, Clark HB, Schweitzer JB, Johnson Jr EM (1988) Expression of nerve growth factor receptors by Schwann cells of axotomized peripheral nerves: ultrastructural location, suppression by axonal contact and binding properties. J Neurosci 8:664-681[Abstract].
- Vits L, Camp GV, Coucke P, Fransen E, De Boulle K, Reyniers E, Korn B, Poustka A, Wilson G, Schrander-Stumpel C, Winter RM, Schwartz C, Willems PJ (1994) MASA syndrome is due to mutations in the neural cell adhesion gene L1CAM. Nat Genet 7:408-413[Web of Science][Medline].
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