From the Department of Clinical Chemistry and
Laboratory Medicine, and the ¶ Department of Anatomy, Faculty of
Medicine, Kyushu University 3-1-1, Maidashi, Higashi-ku, Fukuoka
812-8582, Japan
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ABSTRACT |
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The Hakata antigen is a novel, thermolabile
2-macroglycoprotein that reacts with sera from
patients suffering from systemic lupus erythematosus. In this study we
present the structure and the function of the Hakata antigen. We have
identified cDNA clones encoding the Hakata antigen and analyzed its
function. The cDNA included a possible open reading frame of 897 nucleotides, encoding 299 amino acids. The Hakata antigen consisted of
a collagen-like domain in the middle section and a fibrinogen-like
domain in the COOH terminus, both of which are homologous to human
ficolin-1 and opsonin P35, indicating that these three molecules form a distinct family. The molecular mass of the Hakata antigen expressed in
transfected cells was 35 kDa under reduced conditions, and it formed
ladder bands under nonreducing conditions compatible with the previous
result that the Hakata antigen exists in serum as homopolymers.
Purified Hakata antigen sustained lectin activity, showing affinity
with GalNAc, GlcNAc, D-fucose as mono/oligosaccharide, and
lipopolysaccharides from Salmonella typhimurium and
Salmonella minnesota. These results suggest that the Hakata
antigen, a new member of the ficolin/opsonin P35 family, plays a role
in the serum exerting lectin activity under physiological
conditions.
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INTRODUCTION |
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Inaba and Okochi (1) reported that sera from patients with
systemic lupus erythematosus
(SLE)1 contained an antibody
that reacted with normal sera. The antibody was shown to react against
a novel thermolabile 2-macroglycoprotein, designated the
"Hakata antigen" (2). A similar thermolabile substance had been
reported by Epstein and Tan (3), but it was not known whether the two
proteins are the same. The molecular mass of the Hakata antigen in
serum was 650 kDa as determined by gel filtration. The antigen was
thermolabile because it lost antigenicity upon heating to 56 °C for
1 min. The Hakata antigen was separated as a single band of 35 kDa by
SDS-PAGE under reducing conditions. However, under nonreducing
conditions it separated as ladder bands from 35 kDa to nearly the top
of the gel, suggesting that the Hakata antigen exists in serum as
homopolymers consisting of the 35 kDa subunit (2). All sera from 10,050 Japanese healthy blood donors, 99.99% of 751,352 Japanese patients'
sera, and 99.98% of 41,430 Swedish patients' sera contained the
Hakata antigen (4), thus implying that the Hakata antigen is a normal
serum protein. The reference range of the Hakata antigen was 7-23
µg/ml (2). The antibody against the Hakata antigen was possessed by
4.3% of 349 SLE patients and 0.3% of 703 patients with other autoimmune diseases (4). Among patients with other autoimmune diseases
who possessed the antibody against the Hakata antigen, one patient was
found among those with chronic glomerulonephritis and another in the
group with primary biliary cirrhosis.
In this study, we have cloned and characterized cDNA clones encoding the Hakata antigen revealing that the Hakata antigen is a novel serum protein that has Ca2+-independent lectin activity. The primary structure of the Hakata antigen is partially homologous to those of human ficolin-1 (5) and opsonin P35 (6), both of which contain collagen- and fibrinogen-like domains.
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MATERIALS AND METHODS |
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Purification of Human Hakata Antigen-- The Hakata antigen was purified according to Yae et al. (2) with minor modifications as follows. In brief, Hakata antigen in serum was affinity-purified on a CNBr-activated Sepharose 4B column conjugated with a monoclonal antibody (4H5) produced against the Hakata antigen that had been purified from the propositus SLE patient serum (2). Fractions of the Hakata antigen were passed through a Hi trap Protein G column (Amersham Pharmacia Biotech) equilibrated with Buffer A (20 mM Tris-HCl, pH 7.5, 0.5 M NaCl) and then applied to a Zn2+ column. Hakata antigen was eluted with 0-0.4 M glycine gradient in Buffer A. Hakata antigen-rich fractions were collected and dialyzed against Buffer A. The dialyzed Hakata fraction was applied to a lentil lectin-agarose column and eluted with Buffer A, containing 0.2 M methylmannoside. Purified Hakata antigen was dialyzed against Buffer A and its identity was confirmed by the reactivity with the autoantibody of the propositus SLE serum.
Purification of Human Hakata Antibody-- Anti-Hakata human IgG was obtained from serum of the propositus patient with SLE by 35% ammonium sulfate precipitation and DEAE-Sepharose ion-exchange chromatography as described previously (2).
Preparation of Monoclonal and Polyclonal Antibodies Against the Hakata Antigen-- Nonreduced, purified Hakata antigen (native form) and reduced, pyridylethylated Hakata antigen (denatured form) were used for preparation of antibodies. The antigen (200 µg) and complete Freund's adjuvant (Difco Laboratories) were injected into BALB/c mice. After 5 weeks, the mice were boostered with 200 µg of the antigen, and 3 days later spleens were removed and used for fusion with P3U1 cells. Hybridoma cells producing antibodies were screened using an enzyme-linked immunosorbent assay with the Hakata antigen. Two of the positive monoclonal antibodies (2H2, 4H5) were collected from ascites fluid of mice bearing the hybridoma cells and purified with ammonium sulfate precipitation followed by Protein G affinity column and a HPLC gel filtration column (Superdex 200, 10 × 300 mm; Amersham Pharmacia Biotech). 2H2 was an IgM isotype reacting with the denatured Hakata antigen, and 4H5 was an IgG1 isotype reacting preferentially with the native Hakata antigen.
Polyclonal antibodies were produced in rabbits by immunizing them with 1 mg of purified Hakata antigen in complete Freund's adjuvant, followed by four booster injections of the Hakata antigen at 2-week intervals. Antisera were collected 2 weeks after the last booster injection.Amino Acid Sequence Analysis of Hakata Antigen Fragmented by CNBr or Proteinases-- Purified Hakata antigen was reduced and pyridylethylated according to the procedure described previously (2, 7). The amino-terminal end of the Hakata antigen was blocked, and thereafter, partial amino acid sequences of the Hakata antigen were determined after fragmentation of the antigen with CNBr or proteinases; pyridylethylated Hakata antigen was fragmented by CNBr, chymotrypsin, lysyl endopeptidase, or Staphylococcus aureus V8 proteinase as described previously (7). Fragmented peptides were analyzed on a HPLC equipped with a reversed phase column (Cosmosil 5C18-AR-300, 4.6 × 250 mm; Chemco, Osaka, Japan), using a water/acetonitrile/propanol system containing 0.1% trifluoroacetic acid (8). Purified peptides fragmented from pyridylethylated Hakata antigen were sequenced on a gas phase sequencer (Applied Biosystems division, model 492, Urayasu, Chiba, Japan), and the phenylthiohydantoins were identified by an Applied Biosystems 120A phenylthiohydantoin analyzer on-line system.
cDNA Cloning of the Hakata Antigen--
To generate a
cDNA probe by PCR (9), several oligonucleotides were synthesized as
primers for the cDNA cloning of the Hakata antigen, based on
analysis of the amino acid sequences of the Hakata antigen. One pair,
the sense primer (a 22-mer designed from the peptide sequence LGEVDHYQ
in Fig. 1) and the antisense primer (a 21-mer designed from the peptide
sequence GRYAVSE in Fig. 1), was successfully used. PCR was performed
using a human lung gt11 cDNA library
(CLONTECH, Palo Alto, CA), and bands of the
expected size were subcloned to TA cloning vector and sequenced. One of
the PCR clones contained a unique sequence that encoded the partial
amino acid sequence of the Hakata antigen. Using the PCR product as a
probe (probe 1), a Hakata antigen cDNA clone lacking a portion of
the 3'-end (clone 11-9) was isolated from the lung
gt11 cDNA
library. By further screening using the cDNA clone as a probe
(probe 2), two positive clones, B-1 and D-1, were obtained (Fig.
2A). These positive clones were subcloned into pBluescript
II SK+ (TOYOBO Co., Osaka, Japan) and sequenced by dideoxy
method with a Thermo Sequenase kit (Amersham Pharmacia Biotech). By
overlapping the sequences of these clones, a stretch of Hakata antigen
cDNA was constructed. The 3'-end was determined by rapid
amplification of cDNA ends (3'-RACE) using a RACE PCR kit
(CLONTECH).
Transient Expression of the Hakata Antigen-- A transient expression plasmid for the Hakata antigen was constructed by subcloning the Hakata cDNA insert into the pCIneo (Promega Corp., Madison, WI). PLC (human liver cell line) cells were used for transient expression according to Östman et al. (10) with minor modifications. Briefly, cells were seeded into a 15-mm culture plate at a density of 5 × 105 cells/well, and 1 µg of plasmid was transfected by the lipofection method of TfxTM-50 (Promega Corp.) on the following day. After overnight incubation, cells were washed three times with a phosphate-buffered saline (10 mM sodium phosphate, pH 7.5, in 0.14 M NaCl) and incubated with Dulbecco's modified Eagle's medium supplemented without fetal calf serum for 3 more days with medium being changed everyday. The medium was then used for immunoprecipitation with the autoantibody of the propositus SLE serum.
Immunoprecipitation with Anti-Hakata Antigen Monoclonal Antibody
4H5 and Western Blot Analysis--
The medium was incubated with the
autoantibody of the propositus SLE serum for 1 h at 4 °C.
Immune complexes were bound to Protein G-Sepharose (Amersham Pharmacia
Biotech) for 1 h at 4 °C, washed three times with Tris-buffered
saline (TBS: 10 mM Tris-Cl, pH 7.2, 150 mM
NaCl) containing 1% Triton X-100, 0.1% SDS, and 1% Trasylol. The
immune complexes were eluted by boiling for 5 min in SDS-PAGE sample
buffer (100 mM Tris-Cl, pH 6.5, 0.01% bromphenol blue,
36% glycerol, 4% SDS) in the presence or absence of 10 mM -mercaptoethanol and analyzed by SDS-PAGE (10% acrylamide). After electrophoresis, the samples were transferred to polyvinylidene fluoride membrane (Millipore Corp., Bedford, MA) and probed with the
rabbit polyclonal anti-Hakata antigen antibodies. After washing with
TBS, the membrane was incubated with alkaline phosphatase-labeled anti-rabbit IgG and detected with an ECL chemiluminescent kit (Tropix
Inc., Bedford, MA).
Hemagglutinating Activity-- Fresh erythrocytes from human and sheep were washed and resuspended in TBS to yield a hematocrit of 10%. The erythrocyte suspensions were treated with trypsin (1 mg/ml) for 30 min at 37 °C and washed extensively with TBS. Hemagglutinating activity was determined in microtiter 96-well plates (U-shaped). Each well contained 25 µl of the cell suspension and 25 µl of serial dilutions of the Hakata antigen (highest concentration of Hakata antigen, 250 µg/ml) in TBS with or without 20 mM CaCl2 at a hematocrit of 1.0%. The inhibitory activity of lipopolysaccharides (LPSs) and mono/oligosaccharides was tested by adding the corresponding LPS and mono/oligosaccharide with serial dilutions from 0.5 M in a similar system of a 50 µl final volume, with 20 µg/ml Hakata antigen. LPS-sensitized erythrocytes were prepared by incubating the cells with 100 µg/ml LPS at 37 °C for 1 h. Hemagglutination was estimated visually after incubation at room temperature for 1 h.
Binding Activity with Mono/oligosaccharide-conjugated Column-- After 30 µg/ml purified Hakata antigen was applied to 1 ml of mono/oligosaccharide-conjugated Sepharose columns (EY Laboratories, Inc., San Mateo, CA) equilibrated with Buffer A, the columns were washed with 5 volumes of Buffer A. The bound Hakata antigen was eluted from the washed column by 0.1 M mono/oligosaccharide, 0.5 M mono/oligosaccharide, and 0.1 M glycine (pH 3.5), and then each fraction was applied to Western blotting of the Hakata antigen.
Electron Microscopy-- Hakata antigen was diluted to 20 µg/ml in TBS containing 50% glycerol. Rotary shadowed specimens were prepared by quickly spraying the diluted antigen onto freshly cleaved mica discs and shadowing with a carbon platinum at an angle of 3°. All of the specimens were examined with a Jeol 2000 EX electron microscope operated at 100 kV.
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RESULTS |
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Amino Acid Sequence Analysis of Fragmented Hakata Antigen-- The amino-terminal end of the Hakata antigen was blocked, and thereafter, partial amino acid sequences of pyridylethylated Hakata antigen were determined after fragmentation of the antigen with CNBr or proteinases. Fig. 1 shows the summary of amino acid sequences determined from the major fragmented peptides. The yield of individual peptides was 2-16% of the pyridylethylated Hakata antigen. Although it has been previously reported that the Hakata antigen contained five residues of hydroxyproline per molecule (2), peptide 1 in Fig. 1 contained six residues of hydroxyproline and also 11 GXY repeats in which X and Y residues were frequently proline and hydroxyproline residues, suggesting the collagen-like characteristics of the Hakata antigen.
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cDNA Cloning of the Hakata Antigen-- Based on the amino acid sequence of peptide 2 in Fig. 1, a pair of sense and antisense primers was designed, and PCR was performed to generate probe 1 (Fig. 2A) using a human lung cDNA library, as described under "Materials and Methods." Primary screening using probe 1 yielded a positive clone, 11-9, with the insert size of 1.3 kilobases that contained sequences of peptides 1, 2, 4, 5, and 6 as shown in Fig. 1. Because the clone 11-9 did not encode peptide 3 further attempts to obtain full-length clones were made using probe 2 (Fig. 2A) generated by a pair of primers corresponding to sequences of peptides 2 and 6, as shown in Fig. 1. Two additional positive clones, B-1 and D-1, were obtained that encoded the sequences of peptides 2, 3, 4, and 6 (Fig. 2A). The 3'-ends of these clones differed in that one lacked a poly(A) signal. The 3'-end was determined by 3'-rapid amplification of cDNA ends using liver and lung total RNA as templates. The 3'-untranslated sequence contained a polyadenylation signal, AATAAA, followed by a poly(A) tail (Fig. 2B). In the 5' part of the open reading frame, the initiation codon was determined considering protein sequences (Fig. 1) as well as Kozak's theory (11). The Hakata antigen cDNA sequence, made by combining the clones in Fig. 2A, yielded a 1592-base pair sequence with an ATG codon starting at position 544. The open reading frame was the position from 544 to 1440 encoding 299 amino acids (Fig. 2B).
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Primary Structure of the Hakata Antigen--
Fig. 2B
shows the complete nucleotide sequence and the deduced amino acid
sequence of the Hakata antigen. Underlined amino acid sequences
consisted of the sequences of peptides from purified Hakata antigen
(listed in Fig. 1). The peptides could be aligned in order of peptide
1, 5, 4, 6, 2, and 3 (Fig. 2A). The Hakata antigen is a
plasma protein (1, 2) and should have a hydrophobic signal sequence,
according to the rules of von Heijne (12). A hydrophobic stretch from
Met-1 to Gln-24 may be the signal sequence (Fig. 2). Cleavage at the
Gln-24/Glu-25 bond with a typical motif for the recognition of signal
peptidase (13) could yield a mature protein with 275 amino acids.
However, the secreted Hakata antigen was blocked at the
NH2-terminal end, and thus the NH2-terminal residue could not be confirmed by peptide sequencing. One potential N-glycosylation site was found at Asn-189 (Fig. 2). A
collagen-like domain, recognized beginning at Gly-48, contained 11 GXY repeats and six residues of hydroxyproline at positions
50, 53, 59, 65, 68, and 77 in the deduced sequence (Figs. 1 and 2).
Following a short neck region (amino acids 81-118), a fibrinogen-like
domain existed in the COOH terminus, which was homologous with human fibrinogen and
by 33 and 29%, respectively (Figs. 2 and
3). No calcium binding motif or C-type
lectin motif was found in the Hakata antigen sequence.
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Characterization of the Hakata Antigen in Transfected Cells-- To characterize the product of the Hakata antigen cDNA, the cDNA was subcloned into the pCIneo expression plasmid and expressed transiently in PLC cells. The Hakata antigen was secreted from the transfected cells to media. The Hakata antigen was immunoprecipitated from media with the autoantibody of the propositus SLE serum and analyzed by Western blot analysis (Fig. 4). Under nonreducing conditions the transfected Hakata antigen formed ladder bands, whereas the ladder bands migrated to a single band of 35-kDa on SDS-PAGE under reducing conditions (Fig. 4) as observed on the Hakata antigen purified from human serum (2). This indicated that the transfected Hakata antigen formed homopolymers of the 35 kDa subunits with disulfide bonds and that it was secreted into media as observed in serum.
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Lectin Activity of the Hakata Antigen-- The Hakata antigen agglutinated nontreated and trypsin-pretreated sheep erythrocytes at antigen concentrations of 125 and 15 µg/ml, respectively. However, the antigen did not agglutinate human erythrocytes at the antigen concentration of 250 µg/ml, no matter what cells were pretreated with trypsin (Fig. 5A). The agglutination activity was lost when the antigen was dissociated to monomer by reducing reagents (data not shown). The activity was resistant to heating at 56 °C for 10 min but not at 100 °C for 5 min. The agglutination activity was Ca2+-independent (data not shown).
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Binding Activity of the Hakata Antigen to Molecules Bound by Collectins and Ficolins-- We examined binding activity of the Hakata antigen to elastin, fibronectin, and zymosan, which had been reported to bind collectins and ficolins (14-16). The Hakata antigen did not bind to any of these proteins (data not shown).
Electron Microscopy of the Hakata Antigen-- Electron microscopy of rotary shadowed Hakata antigen is shown in Fig. 7. The rough image of the Hakata antigen resembled the electron micrographs of ficolin, having globular domains on the ends of thin rods (17). In the electron micrographs, we could visualize two configurations of octadecamer, Form 1 and Form 2, as indicated in Fig. 8. Interpretive drawings of the images are given in Fig. 8.
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DISCUSSION |
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The Hakata antigen is a novel, thermolabile
2-macroglycoprotein that reacts with sera from patients
suffering from SLE (1, 2). The Hakata antigen is a normal serum protein
with concentrations of 7-23 µg/ml. Transient Hakata antigen
deficiency was found in 15 patients suffering from autoimmune diseases
including SLE (4). The serum concentration of the Hakata antigen
correlated with those of albumin and cholinesterase among chronic liver
diseases, and the serum concentration decreased with increasing
severity of cirrhosis, suggesting that hepatocytes produce the Hakata
antigen (18).
The Hakata antigen was cloned and characterized. The amino acid
sequences determined from purified Hakata antigen were completely adjusted to the deduced amino acid sequence from cloned cDNA (Figs. 1 and 2). The cDNA included 1592 nucleotides with a possible open reading frame of 897 nucleotides (Fig. 2). The molecular mass of the
Hakata antigen in human serum was determined to be 35 kDa on SDS-PAGE
analysis under reduced conditions, but under nonreducing conditions it
was determined to be 650 and 520 kDa by Sepharose 4B gel filtration and
analytical ultracentrifugation, respectively (2), indicating that
Hakata antigen in serum is a homopolymer of the 35 kDa-subunit. The
transfected product of a cloned cDNA in PLC cells reacted with the
human anti-Hakata antibody obtained from serum of the propositus
patient with SLE (Fig. 3) and formed ladder bands from the gel top to
the position of 35 kDa molecular mass under nonreducing conditions,
whereas the ladder bands migrated to a single band of 35 kDa under
reducing conditions on SDS-PAGE (Fig. 3). This indicates that the
cloned cDNA codes the Hakata antigen a novel thermolabile
2-macroglycoprotein.
Collectins are a group of oligomeric
Ca2+-dependent (C-type) animal lectins
consisting of three domains: an NH2-terminal domain containing cysteine residues, a collagen-like domain containing Gly-X-Y triplet repeats, and a COOH-terminal domain
containing a carbohydrate recognition domain (19-22). Mannose-binding
protein, conglutinin, and pulmonary surfactant proteins (SP-A and SP-D) are included in the collectin group. Collectins bound to carbohydrates with the COOH-terminal domain in a
Ca2+-dependent manner (23-25). Human opsonin
P35 is also an oligomeric serum lectin containing a collagenous domain
similar to collectins. However, the COOH-terminal region of opsonin P35
contains a fibrinogen-like domain instead of a carbohydrate recognition
domain, although opsonin P35 has Ca2+-dependent
and GlcNAc-binding lectin activity (6). The overall sequence of opsonin
P35 is highly homologous to porcine ficolin and human ficolin-1, which
binds to transforming growth factor-1 and elastin (5, 6, 15, 26).
The Hakata antigen was homologous to human ficolin-1 and opsonin P35
and also contained three structural domains consisting of an
NH2-terminal domain, a collagen-like domain, and a
fibrinogen-like domain (Fig. 2), although the homology was not so high
as that between human ficolin-1 and opsonin P35 (Fig. 3). The Hakata
antigen shows 48% homology to human ficolin-1 and opsonin P35,
suggesting that the antigen should have lectin activity. Actually, the
antigen had lectin activity binding to GalNAc, GlcNAc,
D-fucose, and LPSs from S. typhimurium and
S. minnesota. The oligosaccharide chain of
S. typhimurium, which is completely lacking in the Ra
mutant, is composed of a trisaccharide repeating unit containing one
residue each of D-mannose, D-galactose, and
L-rhamnose, and a monosaccharide side chain, which is a
residue of a 3,6-dideoxy-D-xylohexose (abequose).
3,6-Dideoxy-D-xylohexose, whose structure is similar to
D-fucose, would be important for binding of the Hakata
antigen to the oligosaccharide chain of S. typhimurium. Unlike opsonin P35 (6), the lectin activity of the
Hakata antigen was Ca2+-independent, similar to ficolin
(17). Lectin activity of the Hakata antigen was retained by 56 °C up
to 10 min, although antigenicity of that is lost by heating for
56 °C for 1 min. The results indicate that Hakata antigen, human
ficolin-1, and opsonin P35 shared common features of domain structure,
polymerization tendency, images of electron micrographs, and lectin
activities, and the primary structures indicate that the Hakata antigen
forms a family with human ficolin-1 and opsonin P35.
Based on electronmicroscopy findings and on the analogy of the ficolin molecule (17), we propose that the Hakata antigen is an octadecamer consisting of an elementary trimer unit (Fig. 8). The elementary trimer unit has three fibrinogen-like globular domains connected to a collagen-like domain that terminate in a small, "triglobular" clustered NH2-terminal domain. Given that each monomer has an approximate molecular mass of 35 kDa, the trimer represents a molecular mass of 105 kDa. Because the Hakata antigen has a molecular mass of roughly 650 kDa in serum, we could visualize two sets composed of three units of each trimer coalescing to form an octadecameric structure (18 monomers) with two clusters of the amino-terminal ends remaining free (Form 1 in Fig. 8). Alternatively, we could also visualize the amino-terminal clusters of the octadecamer coalescing as depicted in Form 2 (Fig. 8). The dimensions of the octadecamer Form 1 are 40 nm in height with a width of 54 nm. Form 2, although having the same dimensions for height as in Form 1, has a reduced width of 33 nm because of the coalescing of the two amino-terminal clusters. Evidence that the interaction of the octadecamer with a molecular mass of 650 kDa was because of the sulfhydryl groups comes from the appearance of a single band corresponding to 35 kDa in SDS-PAGE under reducing conditions (Fig. 3) (2).
A histochemical study and the lower serum level in cirrhotic patients (18) indicated that the major production site in vivo was the liver. Although the fraction of SLE patients was small (4.3%), the Hakata antigen disappeared from the patients' sera, and the antibody against the Hakata antigen was produced (4). Furthermore, a dysfunctional mannose-binding protein allele was a risk factor for developing SLE (27). The physiological and pathological significance of ficolin/opsonin P35 and collectins remains to be determined.
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ACKNOWLEDGEMENT |
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We thank Dovie R. Wylie for critical review of this manuscript.
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FOOTNOTES |
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* This work was supported in part by grants-in-aid for scientific research from the Ministry of Education, Science, Sports and Culture of Japan.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.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) D88587.
Dr. Yae passed away in August 1996. This paper is dedicated to Dr.
Yae's collaborative efforts in scientific research in a career
spanning nearly a quarter of a century.
§ Present address: Dept. of Biochemical Genetics, Medical Research Inst., Tokyo Medical and Dental University, Tokyo, 113-0034, Japan.
Present address: The Fukuoka Red Cross Blood Center,
Chikushino, Fukuoka, 818-8588, Japan.
** Present address: National Nakatsu Hospital, Nakatsu, Oita, 871-0011, Japan.
To whom correspondence should be addressed. Tel.:
+81(92)642-5748; Fax: +81(92)642-5772; E-mail:
hamasaki{at}cclm.med.kyushu-u.ac.jp.
The abbreviations used are: SLE, systemic lupus erythematosus; TBS, Tris-buffered saline; LPS, lipopolysaccharide; PAGE, polyacrylamide gel electrophoresis; HPLC, high pressure liquid chromatography; PCR, polymerase chain reaction.
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REFERENCES |
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