Neurexophilins Form a Conserved Family of Neuropeptide-Like Glycoproteins

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The Journal of Neuroscience, May 15, 1998, 18(10):3630-3638

Neurexophilins Form a Conserved Family of Neuropeptide-Like Glycoproteins
Markus Missler and Thomas C. Südhof
Howard Hughes Medical Institute and Department of Molecular Genetics, The University of Texas Southwestern Medical School, Dallas, Texas 75235

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Neurexophilin was discovered as a neuronal glycoprotein that is copurified with neurexin I $alpha$ during affinity chromatographyon immobilized $alpha$ -latrotoxin (Petrenko et al., 1996). We have nowinvestigated how neurexophilin interacts with neurexins, whetherit is post-translationally processed by site-specific cleavagesimilar to neuropeptides, and whether related neuropeptide-likeproteins are expressed in brain. Our data show that mammalianbrains contain four genes for neurexophilins the products of whichshare a common structure composed of five domains: an N-terminalsignal peptide, a variable N-terminal domain, a highly conservedcentral domain that is N-glycosylated, a short linker region,and a conserved C-terminal domain that is cysteine-rich. Whenexpressed in pheochromocytoma (PC12) cells with a replication-deficientadenovirus, neurexophilin 1 was rapidly N-glycosylated and thenslowly processed to a smaller mature form, probably by endoproteolyticcleavage. Similar expression experiments in other neuron-likecells and in fibroblastic cells revealed that N-glycosylationof neurexophilin 1 occurred in all cell types tested, whereasproteolytic processing was observed only in neuron-like cells.Finally, only recombinant neurexin I $alpha$ and III $alpha$ but not neurexinI $beta$ interacted with neurexophilin 1 and were preferentially boundto the processed mature form of neurexophilin. Together our datademonstrate that neurexophilins form a family of related glycoproteinsthat are proteolytically processed after synthesis and bind to $alpha$ -neurexins. The structure and characteristics of neurexophilinsindicate that they function as neuropeptides that may signal via $alpha$ -neurexins.

Key words: neurexins; $alpha$ -latrotoxin; synapse; gene duplication; proteolytic processing; neuropeptides; adenovirus expression

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Neurexins are neuronal membrane proteins with a domain structure similar to that of cell-surface receptors (for review, seeMissler and Südhof, 1998). Neurexins were discovered when neurexinI $alpha$ was purified on immobilized $alpha$ -latrotoxin as an affinity matrix(Ushkaryov et al., 1992). The binding of neurexin I $alpha$ to $alpha$ -latrotoxinsuggested that neurexin I $alpha$ is a receptor for this toxin. Thissuggestion was confirmed in studies with recombinant neurexinI $alpha$ and neurexin I $alpha$ knock-out mice, demonstrating that neurexinI $alpha$ functions as a high-affinity $alpha$ -latrotoxin receptor (Davletovet al., 1995; Geppert et al., 1998).

There are at least three genes for neurexins (Geppert et al., 1992; Ushkaryov et al., 1992, 1994; Ushkaryov and Südhof, 1993).Each gene has two independent promoters that direct transcriptionof longer $alpha$ -neurexins and shorter $beta$ -neurexins. The neurexin transcriptsare subject to extensive alternative splicing. The alternativesplicing may result in the synthesis of >1000 neurexin isoformsthat are differentially expressed in subpopulations of neurons(Ullrich et al., 1995). Although the domain structure of the neurexinssuggests a receptor function, their overall biological role isunknown. It seems likely that $alpha$ - and $beta$ -neurexins and some of theirvarious alternatively spliced forms perform distinct functions.The discovery of a family of ligands for $beta$ -neurexins called neuroliginssupports this hypothesis (Ichtchenko et al., 1995, 1996). Similarto neurexins, neuroligins are neuronal cell-surface proteins thatare type 1 membrane proteins. They bind only to $beta$ -neurexins andonly to one particular splice variant of $beta$ -neurexins. The bindingof neuroligins to $beta$ -neurexins causes cell adhesion, suggestinga mechanism for the formation of a novel intercellular junctionbetween neurons (Nguyen and Südhof, 1997). Intracellularly, $beta$ -neurexinsand neuroligins are associated with different PDZ-domain proteins;CASK binds to neurexins, and postsynaptic density (PSD)-95 bindsto neuroligins (Hata et al., 1996; Irie et al., 1997). Thus asubset of $beta$ -neurexins functions as cell adhesion molecules bybinding to neuroligins, thereby forming an intercellular junctionflanked by PDZ-domain proteins. Other neurexins, however, do notinteract with neuroligins, suggesting that they have other ligandsand different functions.

After purification on immobilized $alpha$ -latrotoxin, part of neurexin I $alpha$ is isolated in a tight complex with a 29 kDa glycoproteincalled neurexophilin (Petrenko et al., 1993). cDNA cloning showedthat the primary translation product of neurexophilin is largerthan the neurexophilin protein bound to neurexin I $alpha$ in the eluatefrom the $alpha$ -latrotoxin affinity matrix (Petrenko et al., 1996).This suggested that neurexophilin may be physiologically processedby proteolytic cleavage or that it may have been partially degradedduring protein purification. The mouse genome contains two genesfor neurexophilin, but only one of these is transcribed (neurexophilin1). In contrast, mRNAs corresponding to the second gene neurexophilin2 were only found in bovine brain that, however, contained nodetectable mRNAs for neurexophilin 1 (Petrenko et al., 1996).Thus there may be a species-specific expression of the two genescharacterized up to now.

The structure of neurexophilin and its purification as a smaller protein in a complex with neurexin I $alpha$ suggested the hypothesisthat neurexophilin may be post-translationally cleaved from aprepropeptide similar to a neuropeptide (e.g., see Eipper andMains, 1980; Jacobs et al., 1981; Noda et al., 1982; Maisonpierreet al., 1990). The processed protein could then function as aligand for $alpha$ -neurexins. However, at present there is little directevidence of this hypothesis, and many questions remain. First,virtually all neuropeptides are part of protein families withseveral related members (e.g., see Wimalawansa, 1997). By contrast,neurexophilin has no sequence homology to other proteins, andonly a single neurexophilin gene was found to be expressed inmouse, rat, and bovine brain. Thus the question arises whetherneurexophilin is also part of a gene family. Second, neurexophilinwas purified in a complex with neurexin I $alpha$ , but its binding specificityis unclear. Does neurexophilin bind to all or only to a subsetof neurexins? Third, the neurexophilin complexed to neurexin I $alpha$ is shorter than the primary translation product of the cDNA. Isneurexophilin physiologically processed by proteolytic cleavage,or is the smaller protein purified in the complex with neurexinI $alpha$ on immobilized $alpha$ -latrotoxin the result of an artifact?

In the present paper, we have attempted to address these questions. We found that neurexophilins form a large gene family,that neurexophilin 1 specifically binds to $alpha$ -neurexins, and thatneurexophilin 1 is physiologically processed in neuronal but notin fibroblastic cells, indicating cell-specific proteolytic cleavage.Our results support the notion that neurexophilins represent afamily of signaling molecules that resemble neuropeptides andthat act by binding to $alpha$ -neurexins and possibly other receptors.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Molecular cloning. GenBank was searched using the BLAST programs of the NCBI (Altschul et al., 1997). Using the amino acidsequence of neurexophilin (Petrenko et al., 1996), we identifiedfour classes of homologs in the human expressed sequence tag (EST)data bank, two of which represent the human homologs of the previouslycloned mouse genes. The corresponding clones were obtained fromthe IMAGE consortium (clones 381246, 309825, 381764, and 704436),mapped with restriction endonucleases, and sequenced. The followingrestriction fragments were used as probes to screen rat brainand intestinal $lambda$ ZAP cDNA libraries (Stratagene, La Jolla, CA):0.62 kb NotI/BglII fragment from clone 381764, 0.6 kb SfiI fragmentfrom clone 309825, and 0.42 kb EcoRI/NheI fragment from clone704436. $lambda$ ZAP clones were plaque-purified and sequenced after invivo excision and subcloning into pBluescript II and M13 vectorsusing standard procedures (Sambrook et al., 1989). We isolatedthree distinct full-length neurexophilin 3 cDNA clones extendingup to 480 bp into the 5'-untranslated region and four distinctclones representing the C-terminal half of neurexophilin 3. Forneurexophilin 4, the library contained two distinct full-lengthclones that include up to 190 bp of 5'-untranslated region andan additional set of clones coding for all but the signal peptide.All neurexophilin sequences were submitted to GenBank (accessionnumbers: AF042713, AF042714, AF043467, AF043468, andAF043469).

Northern blots. Human, rat, and mouse multitissue RNA blots (obtained from Clontech, Cambridge, UK) were sequentially probedwith uniformly [ $alpha$ -³²P]dCTP-labeled fragments from neurexophilin 1-4 cDNAs. A 400 bpPstI/EcoRI fragment from the 5'-coding region of rat neurexophilin1 (Petrenko et al., 1996), a 620 bp NotI/BglII fragment from the5'-coding region of human neurexophilin 2 (EST clone 381764),a 530 bp EcoRI/BglII fragment from the 5'-region of rat neurexophilin3 (cDNA), and a 420 bp EcoRI/KpnI fragment from the 5'-regionof rat neurexophilin 4 (cDNA) were used as probes. Additionally,a 620 bp SfiI fragment from the 3'-region of human neurexophilin3 (EST clone 309825) and a 420 bp EcoRI/NheI fragment from the3'-region of human neurexophilin 4 (EST clone 704436) were usedto reprobe the human RNA blots to confirm the specificity of cross-specieshybridization signals. Prehybridizations and hybridizations wereperformed at 42°C overnight in 50% formamide plus 5× Denhardt'ssolution containing salmon sperm DNA at 0.1 mg/ml. Filters werewashed twice for 20 min at 61-63°C in 2× SSC and 0.5% SDS andwere exposed for 1-5 d. A second set of RNA blots was used forsome hybridizations with virtually identical results.

Cell culture and transfections. COS cells were cultured in DMEM with 10% fetal bovine serum (FBS) and transfected using DEAE-dextranwith chloroquine and a 2 min glycerol shock (Gorman, 1985). Humanembryonic kidney 293 cells and STO cells (stably transfected fibroblastsroutinely used in embryonic stem cell culture) were maintainedunder similar conditions and transfected by calcium phosphateprecipitation. The human neuroblastoma cell line SH-SY5Y was grownin 84% F12 medium supplemented with 15% FBS and 1% nonessentialamino acids. The human teratocarcinoma cell line NT2 (Ntera2/D1)cultures were differentiated into mature hNT cells that have someproperties of CNS neurons, using retinoic acid according to theprotocol of the supplier (Stratagene). Pheochromocytoma (PC12)cells were maintained in RPMI medium with 10% horse serum and5% FBS and were plated on collagen-coated dishes before adenovirusinfection experiments.

Recombinant adenovirus construction and infection studies. A 1.4 kb KpnI fragment containing the entire rat neurexophilin1 coding sequence was inserted into the multicloning site of theshuttle plasmid pAC-CMVpLqA. Replication-deficient adenovirusexpressing neurexophilin (AdNph1) or neurexin I $beta$ and neuroligin1 (as controls for antibody specificity) were made by homologousrecombination and were propagated essentially as described (Grahamand Prevec, 1991). The viral DNA used for cotransfection intoreplication-permissive 293 cells was from the 32 kb plasmid pJM17(virus type Ad5 with a deletion of the E1a region). Viral plaqueswere screened by Western and/or Southern blots. Positive plaqueswere amplified to high titer stocks and were purified throughcesium chloride gradients. Various cell lines were infected withserial dilutions of the different virus stocks to determine theoptimum expression conditions for a protein. In a typical experiment,subconfluent cell cultures were inoculated with different titersof AdNph1 in the respective growth medium, the medium was replacedwith virus-free medium after 8-24 hr, and cells were analyzedafter the indicated time periods.

Western blot analysis and deglycosylation of neurexophilin. Immunoblot analyses of cell extracts were performed with ECL detection.We tested the expression products of AdNph1 for glycosylationby denaturing infected PC12 cells with SDS and $beta$ -mercaptoethanol,digesting with recombinant PNGase F (New England Biolabs, Beverly,MA), and analyzing by SDS-PAGE and immunoblotting using anti-neurexophilinantibody F508 (Petrenko et al., 1996).

Binding of neurexophilin 1 to IgG fusion proteins of neurexins. Processed and unprocessed forms of neurexophilin 1 were solubilizedfrom infected PC12 cells using 2% 3-[(3-cholamidopropyl)dimethylammonio]-1-propane-sulfonate(CHAPS). PC12 cells were harvested, subjected to a hypo-osmolarshock (20 mM HEPES containing protease inhibitors for 10-15 minon ice), broken apart with a Dounce homogenizer (10-15 strokeson ice), and centrifuged to pellet insoluble material. Becauseinitial experiments showed that neurexophilin 1 is in the pelletfraction of this centrifugation step (data not shown), the pelletwas solubilized in 2% CHAPS in extraction buffer (40 mM Tris-HCl,pH 8.0, 0.15 M NaCl, and protease inhibitors). The supernatantof the solubilization step was used for binding experiments withdifferent neurexin-IgG fusion proteins immobilized on proteinA (Ushkaryov et al., 1994; Davletov et al., 1995; Ichtchenko etal., 1996). Binding experiments were performed in extraction buffercontaining 1% CHAPS and were analyzed by SDS-PAGE and immunoblotting.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cloning of neurexophilins: definition of a gene family

To identify neurexophilin homologs, we searched EST data banks with the neurexophilin sequence using the BLAST program. HumanEST clones corresponding to neurexophilins 1 and 2 were identifiedand sequenced, revealing that neurexophilins 1 and 2 are highlyconserved between rats, mice, and humans (>90% sequence identity;Fig. 1). The presence of human EST clones for both neurexophilin1 and 2 indicates that unlike in bovine and rodent tissues, bothneurexophilins are expressed in human tissues. In addition toEST clones for neurexophilins 1 and 2, we found human EST clonescoding for two novel neurexophilins, neurexophilins 3 and 4. Weused probes from these EST clones to screen a rat brain cDNA libraryand isolated clones containing the full coding region for bothnew neurexophilins. In addition, we rescreened the rat brain cDNAlibrary for neurexophilin 2 to confirm that this neurexophilinis absent in rats but again were unable to isolate positive clones.

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Figure 1. Primary structure of neurexophilins from rat (R), mouse (M), bovine (B), and human (H). The amino acid sequences of the four neurexophilins (NPH1-NPH4) are aligned for maximal homology, with hyphens indicating gaps. Sequences are identified on the left and numbered on the right. Residues that are identical in all sequences are shown on a red background, and residues identical in at least two isoforms are shown on a blue background. The four conserved N-glycosylation sites in neurexophilins are identified by arrows, and the six cysteines present in all neurexophilins with identical spacing are marked by asterisks above the sequences. The putative signal sequence is shown in italics. The linker sequence in neurexophilin 4 between the N-glycosylation domain and the cysteine-rich domain contains seven imperfect GGxL repeats (residues 201-234). The human neurexophilin 1, 3, and 4 sequences were obtained from incomplete EST clones and are only partial. No rat neurexophilin 2 cDNA could be identified, leading to the absence of a rat neurexophilin 2 sequence; the mouse neurexophilin 2 sequence was deduced from the genomic sequence (Petrenko et al., 1996).

The translated amino acid sequences for all currently described neurexophilins, each with at least partial sequences fromtwo or more species, are aligned with each other in Figure 1.This alignment demonstrates that each neurexophilin is highlyconserved evolutionarily. Comparisons between different neurexophilinsreveal that they are closely related to each other in their C-terminalregions but diverge considerably in their N-terminal sequences.Thus neurexophilins form a family of at least four related evolutionarilyconserved proteins with divergent N terminals.

Domain structure of neurexophilins

The alignment of the neurexophilin sequences reveals a pattern of similarity and diversity that suggests a pronounced domainstructure. Five domains can be distinguished (Fig. 2): I, an N-terminalhydrophobic sequence with the properties of a signal peptide (Fig.1, italicized region); II, an N-terminal region that exhibitslittle sequence similarity between neurexophilins, although itis highly conserved evolutionarily for each individual neurexophilinand includes one conserved N-glycosylation consensus sequence;III, a central domain that represents the most conserved partof the neurexophilins and contains three N-glycosylation sites(Fig. 1, arrows); IV, a linker sequence that is only nine aminoacids in neurexophilins 1, 2, and 3 but 57 amino acids in neurexophilin4, with the 57 amino acid linker sequence of neurexophilin 4 primarilycomposed of an imperfect Gly-Gly-Xxx-Leu repeat; and V, a C-terminalconserved domain that contains six identically spaced cysteineresidues (Fig. 1, asterisks).

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Figure 2. Domain model of neurexophilins based on their primary structures. Five domains are proposed (identified by roman numerals): I, an N-terminal signal peptide; II, a variable N-terminal region that may be cleaved off during proteolytic processing; III, a highly conserved domain containing three N-glycosylation sites; IV, a linker sequence that varies in size and composition between different neurexophilins; and V, a conserved C-terminal domain with six cysteine residues that are identically spaced in all neurexophilins. The putative site of proteolytic cleavage is indicated by an arrow above the diagram, positions of N-glycosylation sequences are marked by branched lines, and the conserved cysteines are identified by letters C. The size range of the different domains in the neurexophilins and the sequence identities and homologies between neurexophilins in the domains are shown below the diagram. n.a., Not applicable.

Neurexophilins 1 and 2 are more homologous to each other than they are to neurexophilins 3 or 4 (Fig. 1). Neurexophilin 3is closer to neurexophilins 1 and 2 than to neurexophilin 4, andneurexophilin 4 is the most divergent neurexophilin. Many extracellulardomains, for example, Ig- and EGF-like domains, are composed ofsequences containing an even number of cysteine residues thatare spaced in a characteristic pattern and are disulfide bonded.Such domains can be defined by consensus sequences that are presentin many similar domains in a large number of proteins. With fourneurexophilins, a comparable consensus sequence can now be defined.However, we were unsuccessful in detecting any sequences in thedata banks that are related to the cysteine-rich or the centralconserved domain of neurexophilins except for a short sequencein Caenorhabditis elegans (accession number, U41995), suggestingthat the cysteine-rich domain of neurexophilins does not constitutea widely present extracellular motif.

Tissue-specific expression of neurexophilins

Cloning and analysis of EST data banks suggested that all four neurexophilins are expressed in humans, and neurexophilins1, 3, and 4 are expressed in rats and mice. To obtain a more accurateassessment of the expression patterns of different neurexophilinsin mouse, rat, and human tissues, we analyzed the tissue distributionof their mRNAs (Fig. 3). Although all neurexophilins were preferentiallyexpressed in brain, we observed a remarkable variability betweenspecies. This is surprising because the sequences of the individualneurexophilins are highly conserved evolutionarily.

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Figure 3. Tissue-specific expression of neurexophilins in rats, mice, and humans. RNA blots are hybridized with neurexophilin 1 (Nph 1; A, E, I), neurexophilin 2 (Nph 2; B, F, J), neurexophilin 3 (Nph 3; C, G, K), and neurexophilin 4 (Nph 4; D, H, L) probes. RNA blots from mouse (A-D), rat (E-H), and human (I-L) tissues contained total RNA from heart (H; lane 1), brain (B; lane 2), spleen (S; lane 3), lung (Lu; lane 4), liver (Li; lane 5), skeletal muscle (Sk; lane 6), kidney (K; lane 7), and testis (T; lane 8). A single multitissue RNA blot (obtained from Clontech) from each species was consecutively hybridized with probes for each neurexophilin. Rat probes were used for all hybridizations except for the blots for human neurexophilins 3 and 4 (K and L) that were hybridized with human probes. Arrowheads for D and H mark the position of the 28S RNA that cross-hybridizes with the glycine- and cysteine-rich rat neurexophilin 4 probe. Positions of molecular size markers are indicated on the left.

In mice and rats, neurexophilin 1 was expressed at high levels only in brain, whereas in humans, the strongest hybridizationsignals were detected in spleen (Fig. 3A,E,I) without a specificsignal in brain. Neurexophilin 2 was detected in humans in brainand kidney but in rodents only in mouse liver; no rat tissue testedwas positive (Fig. 3B,F,J). Neurexophilins 3 and 4 were most highlyexpressed in brain in all three species analyzed. However, therewere again major differences between species with regard to othertissues. In humans, neurexophilin 3 mRNA was almost brain-specific;in rats, low levels could be detected in several other tissues;and in mice, high levels were present in lung, kidney, and testis(Fig. 3C,G,K). Similarly, mRNA for neurexophilin 4 was detectedin mice only in brain, in rats also in kidney, and in humans inspleen and testis (Fig. 3D,H,L). Together these data show thatneurexophilins are preferentially expressed in brain but thatmRNAs for some neurexophilins are also present in non-neural tissuesin a species-specific pattern.

The tissue distribution of an mRNA is usually not simultaneously analyzed in multiple species. It is thus unknown whetherother genes, similar to neurexophilins, exhibit differences inexpression pattern between species. The variations in the expressionpatterns of different neurexophilin mRNAs indicate either thatneurexophilins have distinct, species-specific functions or, morelikely, that expression of a neurexophilin can occur in a tissuewithout necessarily providing a function.

Proteolytic processing of neurexophilin in PC12 cells

Previous studies showed that neurexophilin is purified on immobilized $alpha$ -latrotoxin in a tight complex with neurexin I $alpha$ . Inthis complex, neurexophilin is present as an N-glycosylated 29kDa protein that has a protein core of ~19 kDa (Petrenko et al.,1996). In contrast, the size of unglycosylated neurexophilin predictedfrom the cDNA sequence would be ~35 kDa (Fig. 1). This size discrepancyof 16 kDa could be explained by two hypotheses. (1) Neurexophilinmay be physiologically processed by site-specific proteolyticcleavage in the secretory pathway. In this case, the size of theprotein complexed to neurexin I $alpha$ corresponds to that of matureneurexophilin. (2) Neurexophilin may have been partially degradedduring purification of neurexin I $alpha$ on immobilized $alpha$ -latrotoxin.

The domain structure of neurexophilins with a highly variable N-terminal sequence resembles that of a prepropeptide (e.g.,see Eipper and Mains, 1980; Jacobs et al., 1981; Noda et al.,1982; Maisonpierre et al., 1990). This supports the notion thatneurexophilin is physiologically processed by proteolytic cleavage.To address this issue directly, we used an adenovirus expressionsystem to direct synthesis of neurexophilin 1 in PC12 cells, aneuron-like cell line. The size and glycosylation of neurexophilinin the infected cells was then analyzed as a function of time.We used an adenovirus expression system in these experiments becauseit is very difficult to transiently transfect neuron-like celllines with a high enough efficiency to allow analysis of expressedproteins. Permanent transfection of neuron-like cells, however,often leads to selection of dedifferentiated cells that have lostsome of the more interesting neuron-like properties. In this situation,protein expression with an adenovirus or similar system offersa unique advantage in that all cells in the dish will synthesizethe protein encoded by the recombinant virus.

After infection, we followed the apparent size of neurexophilin as a function of time by SDS-PAGE and immunoblotting to testwhether it is processed after synthesis (Fig. 4). As a controlfor protein loads and for artifactual proteolysis, the same blotswere probed for synaptotagmin I, a synaptic vesicle protein thatis sensitive to proteolysis (Perin, 1991). In addition, cellswere also infected with virus encoding neurexin I $beta$ and neuroliginto control for adenovirus-induced changes unrelated to neurexophilin.No neurexophilin immunoreactivity was detected in noninfectedPC12 cells or in PC12 cells in the first hours after infection(Fig. 4, lanes 1-3). However, ~22 hr after infection, a proteinof 50 kDa that was immunoreactive with neurexophilin antibodiesbecame detectable; the size of this protein corresponded to thatof glycosylated full-length neurexophilin (Fig. 4, lanes 4-6).With a delay of ~4 additional hours, a second protein band reactivewith neurexophilin antibodies developed. This band had a sizeof ~29 kDa and comigrated with neurexophilin isolated in a complexwith neurexin I $alpha$ on immobilized $alpha$ -latrotoxin (Fig. 4, lanes 6-9;data not shown) (Petrenko et al., 1996). The lower band becamemore intense than the upper band with time, suggesting that mostof the full-length neurexophilin was converted to the smallerform (Fig. 4, lanes 10-12).

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Figure 4. Time-dependent proteolytic processing of neurexophilin 1. PC12 cells were infected with recombinant adenovirus encoding full-length neurexophilin 1 (AdNph1), and neurexophilin expression was analyzed as a function of time by SDS-PAGE and immunoblotting. To control for protein loads, we then reprobed the same blot for synaptotagmin I. Without adenovirus infection (lane 1), only synaptotagmin I but no neurexophilin can be detected. Full-length neurexophilin corresponding to the N-glycosylated form (Nph 1 [unprocessed]) is detected within 24 hr of infection (lanes 4-6), whereas the shorter, processed form of neurexophilin (Nph 1 [processed]) appears later (lanes 7-9) and becomes the dominant form only after 3 d (lanes 10-12). No processing is observed with neurexophilin expressed in COS cells (lane 13).

Together these results suggest that in PC12 cells, neurexophilin expressed with a recombinant adenovirus is first producedas an N-glycosylated full-length protein and then proteolyticallyprocessed to a mature peptide with a delay of ~4 hr. However,an alternative explanation for these data would be that afterthe 4 hr delay, full-length neurexophilin that is not glycosylatedis produced. Full-length nonglycosylated neurexophilin would havea size of ~35 kDa, and its size may not be distinguishable fromthat of neurexophilin purified in a complex with neurexin I $alpha$ .To eliminate this possibility, we investigated the N-glycosylationstatus of the different forms of neurexophilin using endoglycosidaseF (Fig. 5). Endoglycosidase F treatment caused a similar shiftin the apparent size of full-length neurexophilin and processedneurexophilin. Thus both the unprocessed and processed proteinswere N-glycosylated, and the smaller protein must be a productof proteolytic processing.

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Figure 5. N-glycosylation of neurexophilin 1 expressed in PC12 cells. PC12 cells infected with recombinant adenovirus encoding neurexophilin 1 (AdNph1) were lysed 2 d after infection, and lysates were treated with 1000 or 5000 units of endoglycosidase F (PNGaseF) or with control buffer. Samples were analyzed by SDS-PAGE and immunoblotting, demonstrating a similar shift of the unprocessed and processed forms of neurexophilin by endoglycosidase F treatment but not by control treatment. Numbers on the left indicate positions of molecular weight standards.

Cell-type specificity of proteolytic processing of neurexophilin

Inspection of the neurexophilin sequences revealed a conserved polybasic motif (KxKK) at the border between the N-terminalvariable and the central conserved domains (Fig. 1). Cleavageof neurexophilin at this motif would result in a processed formwith a size of ~19 kDa, suggesting that the boundary between variableand conserved domains in neurexophilin represents the site ofcleavage. Similar polybasic motifs in many proteins, for example,the insulin receptor or the surface receptor LRP (Bravo et al.,1994; Willnow et al., 1996), are recognized by ubiquitous processingproteases such as furin. In addition, many peptide hormones andneuropeptides are also processed at similar polybasic cleavagesites by specific processing enzymes that are restricted to afew specialized cell types (Thomas et al., 1986; Smeekens andSteiner, 1990; Rehemtulla and Kaufman, 1992). To investigate whetherthe processing of neurexophilin occurs by a ubiquitously presentcellular processing enzyme or by a specialized enzyme system restrictedto a limited number of cells, we studied the processing of neurexophilinin two additional neuron-like cell lines (hNT and SH-SY5Y cells)and two fibroblastic cell lines (STO and COS cells), with PC12cells as a positive control (Fig. 6). The processing of neurexophilin1 from a 50 kDa full-length glycosylated form to a 29 kDa formof identical size was observed in hNT and SH-SY5Y cells similarto that in PC12 cells (Fig. 6A,B). Fibroblastic STO and COS cells,however, were unable to process neurexophilin expressed eitherby the recombinant adenovirus or by transfection (Fig. 6C,D),although these cells do cleave polybasic motifs in LRP, for example(Willnow et al., 1996). Thus not all cells can process neurexophilin,suggesting that a special processing protease or accessory chaperoneis required.

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Figure 6. Proteolytic processing of neurexophilin 1 in different cell types. Cell lines of neuronal [hNT (A) and SH-SY5Y (B) cells] and non-neuronal [STO (C) and COS (D) cells] origin were infected with different concentrations (pfu, plaque-forming units) of recombinant adenovirus expressing neurexophilin 1. In addition, neurexophilin 1 was also expressed in the non-neuronal cells by transfection. The size of recombinant neurexophilin 1 produced in the various cell types was analyzed by SDS-PAGE and immunoblotting and compared with that produced in PC12 cells infected with the neurexophilin 1 adenovirus. Numbers on the left of each panel indicate positions of molecular weight markers; arrows on the right mark the migration of unprocessed (top) and processed (bottom) neurexophilin.

$alpha$ -Neurexins preferentially bind processed neurexophilin

Neurexophilin was discovered as a protein complexed to neurexin I $alpha$ (Petrenko et al., 1996). To investigate the binding specificityof neurexophilin to different neurexins and to evaluate the relativeability of processed and unprocessed neurexophilin to bind, wepurified IgG fusion proteins of $alpha$ - and $beta$ -neurexins from COS cellstransfected with the appropriate expression vectors (Ichtchenkoet al., 1995). IgG fusion proteins immobilized on protein A werethen incubated with lysates from PC12 cells infected with neurexophilinadenovirus. PC12 lysates were recovered early after infectionof the cells, at a time when most of the neurexophilin was notyet processed (Fig. 7, lane 1). In this manner, preferential bindingof processed over nonprocessed neurexophilin was easier to evaluate.Proteins bound to the immobilized fusion proteins were analyzedby SDS-PAGE and immunoblotting using neurexophilin antibodies.

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Figure 7. Binding of recombinant neurexophilin 1 to neurexin I $alpha$ . PC12 cells infected with recombinant adenovirus expressing neurexophilin 1 were incubated for 24 hr, the earliest time at which mature processed neurexophilin is detected (lane 1). Immobilized IgG fusion proteins of either neurexin I $beta$ (NxI $beta$ -1; lane 2), a short irrelevant sequence (control; lane 3), or rat and bovine neurexin I $alpha$ (NxI $alpha$ -1; lanes 4, 5) were incubated with lysates from infected PC12 cells, and bound proteins were analyzed by SDS-PAGE and immunoblotting for neurexophilin. Numbers on the left indicate positions of molecular weight markers. Note that both processed and unprocessed neurexophilin specifically binds only to neurexin I $alpha$ but that there is a relative enrichment of processed neurexophilin in the bound fraction.

Neurexin I $beta$ and control IgG fusion proteins were unable to bind either unprocessed or processed neurexophilin 1 (Fig. 7, lanes2, 3). Neurexin I $alpha$ and III $alpha$ fusion proteins, however, avidly boundrecombinant neurexophilin (Fig. 7, lanes 4, 5; data not shown).Although neurexin I $alpha$ bound both the unprocessed and processedforms of neurexophilin, the processed forms were highly enrichedin the bound fraction compared with the starting material (Fig.7, lanes 1 vs 4 and 5). These data suggest that only $alpha$ -neurexinsbind neurexophilin and that they preferentially bind processedover nonprocessed neurexophilin.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Neurexins are neuronal cell-surface proteins that are composed of three $alpha$ - and three $beta$ -neurexins (for review, see Misslerand Südhof, 1998). Neurexin I $alpha$ was initially discovered becauseit serves as a high-affinity receptor for $alpha$ -latrotoxin (Ushkaryovet al., 1992; Davletov et al., 1995). Although neurexin I $alpha$ isnot the only $alpha$ -latrotoxin receptor and is not essential for theexcitotoxic action of $alpha$ -latrotoxin, neurexin I $alpha$ potentiates toxinaction (Geppert et al., 1998). The $alpha$ -latrotoxin receptor activityof neurexin I $alpha$ suggests that this neurexin and maybe $alpha$ -neurexinsin general function as receptors for signaling molecules. By contrast,at least a subset of $beta$ -neurexins performs a role as a cell adhesionmolecule by binding to neuroligins (Ichtchenko et al., 1995, 1996).Binding of $beta$ -neurexins to neuroligins creates an intercellularjunction flanked by the PDZ domain proteins CASK and PSD-95 (Irieet al., 1997; Nguyen and Südhof, 1997).

If neurexin I $alpha$ , as a receptor for $alpha$ -latrotoxin, functions as a signaling receptor, there must be endogenous ligands for neurexinI $alpha$ and other $alpha$ -neurexins. Previous studies established that a29 kDa protein called neurexophilin is purified from brain ina tight complex with neurexin I $alpha$ and may represent an endogenousligand for neurexin I $alpha$ (Petrenko et al., 1996). Only part of theneurexin I $alpha$ purified on immobilized $alpha$ -latrotoxin was complexedto neurexophilin, and neurexophilin was not required for $alpha$ -latrotoxinbinding (Davletov et al., 1995). Neurexophilin is a secreted glycoproteinthat is expressed in a small subset of neurons. Its structureand tight complex with neurexin I $alpha$ suggested the possibility thatneurexophilin may be a proteolytically processed novel neuropeptidethat represents an endogenous ligand for neurexins. We have nowinvestigated this possibility. The experiments reported in thecurrent paper establish four conclusions. (1) Neurexophilins forma gene family of at least four members that constitute secretedglycoproteins and exhibit a domain structure similar to that ofneuropeptides (Figs. 1, 2). (2) In all species studied, eitherneurexophilin 1 or 2 is expressed in brain together with neurexophilins3 and 4. In addition, neurexophilin mRNAs are transcribed in somenon-neuronal tissues in a highly species-specific pattern (Fig.3). (3) Neurexophilin 1 and probably also other neurexophilinsare N-glycosylated immediately after synthesis and proteolyticallyprocessed with a delay of ~4 hr. Proteolytic processing is notubiquitously performed but takes place only in neuron-like cells(Figs. 4-6). (4) Neurexophilin 1 specifically binds to neurexinI $alpha$ and III $alpha$ but not to $beta$ -neurexins, with the processed form beingpreferentially bound, suggesting that neurexophilins are ligandsfor $alpha$ -neurexins (Fig. 7).

Together with previous observations, these data provide evidence of the concept that neurexophilins constitute a novel classof neuropeptides with $alpha$ -neurexins as their receptors. This conceptis supported by the following findings. (1) The domain structureof neurexophilins is composed of variable N-terminal sequencesand conserved C-terminal sequences and thereby resembles the prepropeptidestructure of neuropeptides (e.g., see Eipper and Mains, 1980;Jacobs et al., 1981; Noda et al., 1982; Maisonpierre et al., 1990).(2) Neurexophilin 1 and possibly other neurexophilins are endoproteolyticallyprocessed after synthesis by cleavage at a defined position. (3)Neurexophilin purified from brain in a complex with neurexin I $alpha$ is exclusively present in the mature processed form (Petrenkoet al., 1996; data not shown). (4) The proteolytic cleavage ofnewly synthesized neurexophilin occurs only in neuron-like cellsand not in the non-neuronal cells tested. (5) Similar to otherneuropeptides, neurexophilins are N-glycosylated and have a conservedC-terminal glycine residue that may be amidated (Murthy et al.,1986). (6) Neurexophilins are primarily synthesized in brain butexhibit species-specific expression patterns in non-neural tissues,similar, for example, to the aberrant high-level expression ofNGF in the mouse salivary gland. (7) Neurexophilin 1 and possiblythe other neurexophilins are synthesized in only a subset of neurons(Petrenko et al., 1996). (8) In brain, neurexophilin binds tightlyto the extracellular domains of $alpha$ - but not $beta$ -neurexins. (9) Theprocessed form of neurexophilin preferentially binds to $alpha$ -neurexins.

If neurexophilins are neuropeptides, they could represent the endogenous ligands for $alpha$ -neurexins that may activate $alpha$ -neurexinsin a manner physiologically similar to the mechanism by which $alpha$ -latrotoxin activates neurexin I $alpha$ pathologically. Signal transductionmight be mediated by CASK, a PDZ domain protein that binds tothe cytoplasmic domain of neurexins (Hata et al., 1996). Becauseat least a subset of $beta$ -neurexins functions as cell adhesion proteins(Nguyen and Südhof, 1997), it seems likely that $alpha$ - and $beta$ -neurexinshave distinct functions in agreement with their different domainstructures. This suggests that neurexins generally perform dualfunctions as signaling receptors and cell adhesion molecules.

  FOOTNOTES

Received Jan. 26, 1998; revised Feb. 27, 1998; accepted Feb. 27, 1998.

This study was supported by National Institutes of Health Grant MH52804 and by a fellowship Grant from the Deutsche Forschungsgemeinschaftto M.M. We thank I. Leznicki, A. Roth, and E. Borowicz for excellenttechnical assistance and Drs. M. S. Brown and J. L. Goldsteinfor critical advice.
Correspondence should be addressed to Dr. Thomas C. Südhof, HHMI, Room Y5.322, 5323 Harry Hines Boulevard, Dallas TX 75235.

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Results
Discussion
References

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Copyright © 1998 Society for Neuroscience 0270-6474/98/18103630-09$05.00/0

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