From the Division of Nephrology, ¶ Department of Pediatrics, University Hospital St. Radboud, 6500 HB, Nijmegen, The Netherlands and the § Department of Biochemistry, Max Planck Institut für Entwicklungsbiologie, 72076 Tübingen, Germany
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ABSTRACT |
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We determined the specificity of two hamster monoclonal antibodies and a sheep polyclonal antiserum against heparan sulfate proteoglycan isolated from rat glomerular basement membrane. The antibodies were characterized by enzyme-linked immunosorbent assay on various basement membrane components and immunoprecipitation with heparan sulfate proteoglycan with or without heparitinase pre-treatment. These experiments showed that the antibodies specifically recognize approximately 150-, 105-, and 70-kDa core proteins of rat glomerular basement membrane heparan sulfate proteoglycan. Recently, we showed that agrin is a major heparan sulfate proteoglycan in the glomerular basement membrane (Groffen, A. J. A., Ruegg, M. A., Dijkman, H. B. P. M., Van der Velden, T. J., Buskens, C. A., van den Born, J., Assmann, K. J. M., Monnens, L. A. H., Veerkamp, J. H., and van den Heuvel, L. P. W. J. (1998) J. Histochem. Cytochem. 46, 19-27). Therefore, we tested whether our antibodies recognize agrin. To this end, we evaluated staining of Chinese hamster ovary cells transfected with constructs encoding full-length or the C-terminal half of rat agrin by analysis on a fluorescence-activated cell sorter. Both hamster monoclonals and the sheep antiserum clearly stained cells transfected with the construct encoding full-length agrin, whereas wild type cells and cells transfected with the construct encoding the C-terminal part of agrin were not recognized. A panel of previously characterized monoclonals, directed against C-terminal agrin, clearly stained cells transfected with either of the constructs but not wild type cells. This indicates that both hamster monoclonals and the sheep antiserum recognize epitopes on the N-terminal half of agrin. By immunohistochemistry on rat renal tissue, we compared distribution of N-terminal agrin with that of C-terminal agrin. The monoclonal antibodies against C-terminal agrin stained almost exclusively the glomerular basement membrane, whereas the anti-N-terminal agrin antibodies recognized all renal basement membranes, including tubular basement membranes. Based on these results, we hypothesize that full-length agrin is predominantly expressed in the glomerular basement membrane, whereas in most other renal basement membranes a truncated isoform of agrin is predominantly found that misses (part of) the C terminus, which might be due to alternative splicing and/or posttranslational processing. The possible significance of this finding is discussed.
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INTRODUCTION |
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Heparan sulfate proteoglycans
(HSPGs)1 are composed of a
core protein to which anionic heparan sulfate (HS) side chains are attached. Apart from its presence in basement membranes (BMs), HSPG is
found in other extracellular matrices and on many, if not all, cell
surfaces (1-3). The first extracellular matrix HSPG that was isolated
(from mouse Engelbreth-Holm-Swarm sarcoma), characterized, and cloned
was perlecan, named after its beads-on-a-string-like appearance in
rotary shadowing electron microscopy (4-6). Different isoforms of
perlecan have been found, which appear to be the result of alternative
splicing (7, 8). Agrin is another extracellular matrix HSPG that is not
related to perlecan (9, 10). Agrin was first isolated from the electric
organ of Torpedo (11) and was recently identified as an HSPG
(12). During formation of the neuromuscular junction, motor neurons
provide a number of signals that promote the differentiation of the
post-synaptic membrane. An early signal is the secretion of specific
isoforms of agrin and their incorporation into the basal lamina. Agrin initiates the clustering of nicotinic acetylcholine receptors and other
components of the muscle cell surface at the site of contact with axons
of motor neurons (13-16). The structure of the agrin molecule and the
functions of the various domains is extensively studied and presently
well understood (17). The C terminus of agrin contains several homology
regions with the G-domain of laminin and four epidermal growth
factor-like repeats (18). The binding site of agrin to -dystroglycan
is located on the C terminus as well. Agrin binds to
-dystroglycan
via its laminin G repeats (19). Furthermore, a heparin/HS binding site
is located on the C terminus and binding of heparin or HS prevents
clustering of the acetylcholine receptors, indicating that HSPGs
mediate this activity (20-22). Most alternative splicing sites have
been identified in the C terminus, three on rat agrin called x, y, and
z and two on chick and Torpedo agrin called A and B,
corresponding to rat y and z. This alternative splicing affects the
activity of agrin to cluster acetylcholine receptors. The most active
forms only occur in neural tissue, whereas the isoforms from non-neural
tissue are less active (14, 23-25). This suggests that splicing is
regulated in a tissue-specific manner. The N-terminus of agrin contains nine domains homologous to the Kazal family of protease inhibitors and
several laminin III homology regions (18). On the N-terminal half of
agrin, several attachment sites for HS side chains are found. Up until
now, only one alternative splicing site has been found in the
N-terminus. The insert on the N-terminal half is required for binding
to the extracellular matrix which is mediated by laminin (26-28).
Expression of agrin is not restricted to neurons. Agrin mRNA can be
detected in a wide range of different tissues (24), and the agrin
protein has been demonstrated to be a basal lamina component in many
tissues including kidney during early development (29). Recently, we
have shown the presence of agrin in the glomerular basement membrane
(glomerular BM) in adult human kidney (30).
In this study, we raised and characterized two hamster monoclonal antibodies (mAbs) and a sheep polyclonal antiserum against rat glomerular BM HSPG. The specificity of the mAbs is studied on Chinese hamster ovary (CHO) cells that are transfected with constructs coding for full-length agrin or the C-terminal half of agrin. These studies showed that these antibodies recognize epitopes on the N-terminal half of agrin. The staining on rat kidney tissue of these mAbs is compared with that of different mAbs against well-defined epitopes on the C terminus of agrin. These experiments suggest that most renal BMs except the glomerular BM express a truncated isoform of agrin that lacks (part of) the C-terminal half due to alternative splicing and/or posttranslational processing. We speculate on the possible involvement of the C terminus of agrin in glomerular function.
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MATERIALS AND METHODS |
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HSPG Purification
For immunization, rat glomerular HSPG was isolated from rat glomeruli (31). Proteoglycans were isolated by guanidine extraction, dialysis against urea, DEAE ion-exchange chromatography, chondroitinase ABC digestion (Sigma) and by fast protein liquid Q-Sepharose chromatography. For immunoprecipitation, HSPG was isolated from rat glomerular BM obtained by a detergent procedure (32), from which proteoglycans were isolated as described (31). All procedures were performed at 4 °C in the presence of 10 mM sodium EDTA, 1 mM phenylmethylsulfonyl fluoride, 5 mM benzamidine HCl, and 10 mM N-ethylmaleimide.
Antibody Production
Male Chinese hamsters were immunized with rat glomerular HSPG according to a previously described protocol (31). Hybridomas were screened in indirect immunofluorescence (IF) on rat kidney cryostat sections (see below) for a staining pattern comparable with the staining of previously described mAbs against human glomerular BM HSPG, which primarily stain the glomerular BM in a bright linear pattern and the tubular BMs to a lesser extent (33). Two hybridomas were found to meet these criteria, called MI-90 and MI-91, and were subcloned twice by limiting dilution so that all subclones displayed the same reactivity pattern. From these two clones, ascites production was elicited in nude mice.
A sheep was immunized intracutaneously with rat glomerular HSPG according to a previously described protocol (32), and after the last booster the sheep was bled and the serum (called GR-14) was collected.
Characterization of Antibodies
Enzyme-linked Immunosorbent Assay-- The reactivity of the antibodies with various BM components was determined in ELISA as described (34). Rat glomerular BM HSPG, human glomerular BM HSPG (isolated as described, Ref. 32), rat L2-laminin, mouse fibronectin, mouse collagen type IV (all from Sigma; all at 1 µg/well), and HS from bovine kidney (Seikagaku Kogyo, Tokyo, Japan; 5 µg/well) were coated in PBS. Primary antibodies MI-90 and MI-91 were diluted 1:100, and GR-14 was diluted 1:1000. The following peroxidase-conjugated secondary antibodies in a dilution of 1:500 were used: rabbit anti-hamster IgG (Nordic, Tilburg, The Netherlands) for mAb MI-90, goat anti-hamster IgG (Cappel-Organon Teknika, Turnhout, Belgium) for mAb MI-91, and rabbit anti-sheep Ig (Cappel) for GR-14.
Immunoprecipitation and SDS-PAGE--
Rat glomerular BM HSPG was
labeled with 125I according to the chloramine T-method
(35). Part of the sample was treated with heparitinase (EC 4.2.2.8;
from Sigma) 1 unit/ml in 10 mM HEPES, pH 7.0, containing 2 mM CaCl2 for 6 h at 43 °C. Radiolabeled
HSPG was pre-absorbed with protein G-Sepharose CL-4B to remove eventual radiolabeled IgG. Normal hamster IgG and culture supernatants of mAbs
MI-90 and MI-91 were incubated with protein G-Sepharose, to which goat
anti-hamster IgG (Cappel) was immobilized. Normal mouse IgM (MOPC-104E;
Bionetics, Kensington, MD) and mouse anti-HS side chain mAb JM-403 (31,
36) were incubated with protein G-Sepharose to which goat anti-mouse
IgM (Cappel) was immobilized. Normal sheep IgG and sheep antiserum
GR-14 were directly coupled to protein G-Sepharose. After washing with
PBS-Tween, the immobilized antibodies were incubated overnight at
4 °C with radiolabeled rat glomerular BM HSPG (with or without
heparitinase pretreatment). After washing in PBS-Tween, sample buffer
containing 5% -mercaptoethanol was added, the sample was boiled for
3 min and centrifuged, and the supernatant was subjected to
polyacrylamide gel electrophoresis on a 7% homogenous gel. The gel was
dried and used for autoradiography for 3 days at
70 °C.
Agrin-transfected CHO Cells-- To investigate the reactivity of our antibodies with agrin, we used CHO-cells, stably transfected with constructs encoding full-length rat agrin or the C-terminal half of agrin (construct N1, amino acids 1137-1940) (17). The cells were cultured as described (17) and continuously selected for the presence of the construct by Geneticin (G418, 500 µg/ml; Life Technologies, Inc., Paisly, Scotland). Untransfected CHO cells were used as a negative control. On cytospins of CHO cells, indirect IF was performed with anti-HSPG mAbs MI-90, MI-91 antiserum GR-14, and anti-agrin mAb Agr-131 (17) (Table I) as described for the kidney cryostat sections (see below). For analysis by fluorescence-activated cell sorter (FACS), samples of 100 µl of cell suspension containing 5 × 106 cells were permeabilized and fixed with 1 ml of PermeaFix (Ortho Diagnostic, Beerse, The Netherlands) according to the instructions of the manufacturer. The cells were incubated with 100 µl of primary antibody (Table I) for 30 min at 0 °C. The cells were washed and incubated with fluorescein isothiocyanate-conjugated secondary antibody for 30 min at 0 °C. The cells were washed twice and kept in 1% paraformaldehyde until analysis on a Coulter Epics XL flow cytometer (Coulter Corp., Hialeah, FL). Mean fluorescence was determined on a scale between 0 and 1024, and values were corrected for staining by the secondary antibody alone.
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Indirect Immunofluorescence
Indirect IF was performed as described previously (34) on 2 µm cryostat sections of rat kidney. To evaluate the specificity of the hamster and sheep antibodies for the HSPG core protein, pretreatment of rat kidney cryostat sections was performed by incubating nonfixed sections with 0.25 units/ml heparitinase in 10 mM HEPES, pH 7.0, containing 2 mM CaCl2 for 30 min at 37 °C.
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RESULTS |
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Antibody Reactivity with Basement Membrane Components in ELISA-- The reactivity of hamster mAbs MI-90 and MI-91 and sheep antiserum GR-14 in ELISA with different BM components is shown in Fig. 1. For MI-90, a clear reactivity was observed with both rat glomerular BM HSPG and human glomerular BM HSPG. For MI-91, a reactivity was observed with rat glomerular BM HSPG, but not with human glomerular BM HSPG. Neither of the mAbs bound to rat L2-laminin, mouse fibronectin, mouse collagen IV, or HS. Antiserum GR-14 bound to rat glomerular BM HSPG, human glomerular BM HSPG, and to a lesser extent to rat L2-laminin, but not to the other BM components.
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Immunoprecipitation and SDS-PAGE-- After immunoprecipitation of intact, 125I-labeled rat glomerular BM HSPG with hamster mAbs MI-90, MI-91, and sheep antiserum GR-14, gel electrophoresis and autoradiography revealed a broad smear with a molecular mass larger than 220 kDa, which might have resulted from different core proteins and/or different extent of glycosylation (Fig. 2, lanes 2, 3, and 7). This is in agreement with previous findings (32). The same band is seen with the mouse anti-HS side chain mAb JM-403 (lane 5) (33). To assess the molecular mass of the HSPG core protein(s), HSPG was treated before immunoprecipitation with heparitinase to degrade the HS glycosaminoglycan side chains. This resulted in a major band of ~170 kDa and several bands with molecular masses of ~105 and 70 kDa, which were equal for MI-90, MI-91, and GR-14 (lanes 9, 10, and 14). mAb JM-403 directed against HS side chain, however, is negative after treatment with heparitinase, as expected (lane 12). Non-relevant hamster IgG (lanes 1 and 8), mouse IgM (lanes 4 and 11), and normal sheep IgG (lanes 6 and 13) with the same Ig concentration served as negative controls. These results indicate that the mAbs MI-90 and MI-91 and the sheep antiserum GR-14 are directed against the core protein(s) of an HSPG present in rat glomerular BM.
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Indirect Immunofluorescence on CHO Cells Transfected with Agrin Constructs-- To evaluate recognition of rat agrin by our antibodies, indirect IF was performed on CHO cells transfected with constructs encoding full-length agrin (37) or the C-terminal half of agrin (N1) (25). Binding of antibodies was evaluated either microscopically on cytospins or by FACS analysis. First, microscopical evaluation of cytospins showed that both hamster anti-HSPG mAbs MI-90 and MI-91 and sheep anti-HSPG GR-14 recognized full-length agrin as expressed by CHO cells transfected with full-length agrin (Fig. 3, A-C), whereas they did not bind to the C-terminal half of agrin as expressed by cells transfected with construct N1 (Fig. 3, E-G, Table II). Neither did they bind to wild type CHO cells. The positive control anti-agrin mAb Agr-131 bound to both full-length agrin and to the C-terminal half of agrin as expressed by cells transfected with full-length agrin or construct N1, respectively (Fig. 3, D and H, Table II) To confirm this crucial conclusion, we also performed fluorescence analysis by FACS and quantified mean fluorescence intensity. As shown in Table II, full-length agrin expressed by CHO cells is recognized by both hamster mAbs and the sheep antiserum. These antibodies, however, were negative on N1-transfected cells and on wild type CHO cells. Anti-agrin mAb Agr-131, however, recognized both full-length and C-terminal agrin. These results indicate that hamster mAbs MI-90 and MI-91 and the sheep antiserum GR-14 recognize epitopes on the N-terminal half of agrin.
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Distribution of Agrin in Rat Kidney-- In indirect IF, mAbs MI-90 and MI-91 stain most BMs in a linear way, the glomerular BM with the highest intensity (Fig. 4, A and B). This staining pattern closely resembles the staining of previously developed mAbs directed against human glomerular BM HSPG (38). Only mAb MI-91 weakly stained Bowman's capsule and BMs of smooth muscle cells in arteries and arterioles. Both mAbs stained BMs of endothelial cells in blood vessels but not the mesangial matrix and peritubular capillaries. (Fig. 4, A and B) mAb MI-90 also stained human kidney cryostat sections, and mAb MI-91 also stained mouse kidney cryostat sections. (Table III). The polyclonal antiserum GR-14 stained the glomerular BM, all tubular BMs, and BMs of endothelial cells in a bright linear way but not the mesangial matrix nor the peritubular capillaries. Bowman's capsule, and the smooth muscle cells in arteries and arterioles were stained weakly (Fig. 4C). This staining pattern is similar to that of a previously described polyclonal antibody directed to human glomerular BM HSPG (32). GR-14 also stained human and mouse kidney cryostat sections. (Table III) The staining pattern of MI-90, MI-91 and GR-14 could not be prevented by pre-treatment of the sections with heparitinase, indicating that the antibodies are directed against the core protein of HSPG. mAb JM-403 directed against the HS side chain, however, was negative after treatment with heparitinase, as expected. This confirms our data from the immunoprecipitation with heparitinase-pretreated glomerular BM HSPG (Fig. 2, lanes 8-14).
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DISCUSSION |
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In the present study, we characterized the N-terminal agrin specificity of two hamster mAbs MI-90 and MI-91 and a sheep polyclonal antiserum GR-14 raised against rat glomerular BM HSPG. Furthermore, we showed a differential agrin expression in renal BMs by comparing our antibodies with well-defined mAbs directed against the C terminus of agrin. The specificity of the antibodies was evaluated by means of ELISA on various BM components and by immunoprecipitation with isolated rat glomerular BM HSPG. In these experiments, it is shown that both hamster mAbs and the sheep antiserum recognize the core protein(s) of an HSPG present in rat glomerular BM with molecular masses of ~170, 105 and 70 kDa. The smaller molecules can be the result of proteolysis during purification; however, this is less likely since the whole purification procedure was performed at 4 °C in the presence of protease inhibitors. These molecular weights are in agreement with previous observations with human glomerular BM HSPG (32, 39). Both hamster mAbs and the sheep antiserum recognize epitopes on the N-terminal half of agrin as shown by immunofluorescence on CHO cells transfected with various constructs coding for full-length agrin or parts of the agrin molecule. This is in agreement with our recent observation that anti-agrin mAbs recognized glomerular BM HSPG (30). The conclusion that our antibodies recognize epitopes in the N-terminal half of agrin is based on the observation that they stain full-length agrin but not the C-terminal half of agrin. One could argue that our hamster mAbs and sheep antiserum need tertiary epitopes, which could not be present in the C-terminal half of agrin due to inadequate folding in the absence of the N terminus. Other observations, however, contradict this possibility. The mAbs directed against the C-terminal half of agrin are able to stain both full-length and C-terminal agrin, suggesting normal folding of the C terminus. Furthermore, the polyclonal antiserum GR-14 stains full-length agrin but not the C-terminal half of agrin, notwithstanding the ability of most polyclonal antibodies to recognize linear as well as tertiar epitopes. Moreover, the staining pattern of the hamster mAbs on rat kidney cryostat sections is different from that of the mAbs against the C-terminal half of agrin. These results strongly suggest that the hamster mAbs and the sheep antiserum recognize epitopes in the N-terminal half of agrin.
Polyclonal antiserum GR-14 demonstrated some cross-reactivity with rat L2-laminin. Two possibilities can explain this observation. The antiserum might recognize the laminin III homology regions which are present on the N-terminal half of agrin (18) and might therefore cross-react with laminin. Second, a low titer of anti-rat laminin antibodies may be present in the polyclonal antiserum due to minor contamination of the antigen with laminin. This is certainly possible, given the laminin-binding properties of agrin (28).
On rat kidney cryostat sections, the hamster mAbs stain all renal BMs in a bright, linear pattern but the glomerular BM with highest intensity. This staining pattern closely resembles that of previously developed mAbs directed against human glomerular BM HSPG (38). On the other hand, the mAbs directed against well-defined epitopes on the C terminus of agrin almost exclusively stain the glomerular BM. This indicates the existence of multiple isoforms of agrin in the kidney, namely a large agrin containing both C- and N terminus predominantly expressed in the glomerular BM. A shorter variant missing C-terminal regions is present predominantly in other renal BMs. One possible explanation for the generation of this shorter form is alternative splicing. While three alternative splicing sites have been identified on the C-terminal half of agrin, these cannot be responsible for our observation. Each of these sites allows the insertion of small peptide sequences and none of them codes for a new stop codon that could result in a truncated form of agrin (24-27). Furthermore, without the insertions on all the alternative splicing sites known (three sites on the C-terminal half and one on the N terminus), the molecular mass would be reduced by ~5.7 kDa. Therefore, alternative splicing alone cannot explain the molecular masses of 170 kDa and lower that we found for agrin. An alternative explanation for the presence of smaller isoforms is posttranslational processing of the agrin core protein. The predicted molecular mass of agrin is ~225 kDa (12, 18, 26). Smaller isoforms of agrin, however, have also been found. Nitkin et al. (40) describe agrin isoforms in the electric organ of Torpedo with molecular masses of 150, 135, 95, and 70 kDa. Godfrey (23) found agrin isoforms in Torpedo electric organ of 80 and 60 kDa and in adult chicken kidney, embryonic skeletal muscle, brain, and spinal cord of 90, 80, 72, and 60 kDa. In rat embryonic brain, spinal cord, and muscle, agrin isoforms of 200, 175, 135, and 115 kDa have been identified (18). In adult chick kidney, isoforms of 160 and 130 kDa are observed (41). Hagen et al. (9) have isolated HSPG isoforms from bovine tubular BM with core protein molecular masses of 145, 125, 88, and 83 kDa. From this HSPG, three tryptic peptides show homology to the N terminus of rat agrin, indicating that in tubular BM an HSPG isoform is present that is homologous to the N terminus of agrin (9, 26). An antiserum against this bovine tubular BM HSPG stained all renal BMs in a linear way, identical to our hamster and sheep antibodies. These data clearly show the existence of smaller agrin isoforms that presumably are the result of alternative splicing and/or posttranslational modification (possibly proteolytic processing).
Differential post-translational modification of agrin in glomeruli and tubuli implies that either a proteinase which is able to cleave agrin or a proteinase-inhibitor is differentially expressed in glomeruli and tubuli. Until now, however, no comparative studies on the differential expression of proteinases and/or proteinase-inhibitors in glomeruli and tubuli have been performed.
What might be the function of C-terminal agrin expression exclusively
in the glomerular BM? The glomerular BM is an important part of the
filtration barrier of the glomerular capillary wall. The HS side chains
of HSPG contribute to the net negative charge of the glomerular BM,
which is thought to be responsible for the charge-selective
permeability of the glomerular filtration barrier (42, 43). These HS
side chains, however, are attached to the N-terminal half of agrin and
are consequently not specific for the glomerular BM. The C-terminal
half of agrin contains a HS/heparin binding site and the binding
regions for the receptors muscle-specific kinase (MuSK) and
-dystroglycan. The HS/heparin binding site is only present in agrin
isoforms containing the insert at the y-position in rat or A-position
in chick and Torpedo, and this alternatively spliced isoform
is only present in neuronal tissue (44, 45), excluding a role for this
HS/heparin binding site in the glomerulus. The agrin receptor MuSK is
only expressed in skeletal muscle where it is essential for the
acetylcholine receptor clustering activity of agrin. This rules out a
possible involvement of MuSK in the glomerulus (46-48). The agrin
receptor
-dystroglycan was shown to play a role in epithelial
development in kidney (49). Although it has been isolated from adult
chick kidney, its presence in the glomerulus remains to be shown
(50).
In conclusion, the present study shows that in the glomerular BM predominantly a large agrin isoform is expressed, whereas in most other renal BMs predominantly a truncated agrin isoform is found that misses (part of) the C-terminal region.
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ACKNOWLEDGEMENTS |
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We thank Cor Jacobs and Sigrun Helms for excellent technical assistance.
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FOOTNOTES |
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* This study was supported by grants from the Dutch Kidney Foundation (Grants C93.1318 and C93.1309) and the Dutch Diabetes Foundation (Grant DFN 940-10-009).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Division of Nephrology
(545), University Hospital St. Radboud, P. O. Box 9101, 6500 HB
Nijmegen, The Netherlands. Tel.: 31-24-361-6539; Fax: 31-24-354-0022;
E-mail: C.Raats{at}nefro.azn.nl.
1 The abbreviations used are: HSPG, heparan sulfate proteoglycan; HS, heparan sulfate; BM, basement membrane; CHO, Chinese hamster ovary; mAb, monclonal antibody; PBS, phosphate-buffered saline; IF, immunofluorescence; ELISA, enzyme-linked immunosorbent assay; FACS fluorescence-activated cell sorter; PAGE, polyacrylamide gel electrophoresis; MuSK, muscle-specific kinase.
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REFERENCES |
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