JP4437389B2 - New allergen derived from Japanese cedar pollen - Google Patents

Description

  The present invention relates to a novel allergen protein derived from cedar pollen, and diagnosis, prevention and treatment of allergy using the same.

  The morbidity rate and mortality rate of allergic diseases have been increasing worldwide over the past 10 years due to changes in diet and living environment. According to a private survey (present state and future prospects of new drug development, 1991 edition, Seed Planning Co., Ltd.), one in three people in Japan is typical of cedar pollinosis, atopic dermatitis, bronchial asthma, etc. It shows symptoms of IgE-dependent (type I) allergic diseases, and this data is supported by the Ministry of Health and Welfare Insurance Welfare Trend Survey (1991). Although allergic diseases are not directly related to life, they suddenly appear in the very young generation, and natural healing at an early stage cannot be expected. It is thought that it has a great influence on social activities.

  Japanese cedar pollinosis is said to affect 15-20% of the population and more in urban areas, but many patients suffer from this allergic symptom, especially in the spring when pollen is scattered. .

  The major allergens of cedar pollen are Cry j1 reported by Yasue et al., Having a molecular weight of 45,000 to 50,000 daltons and an isoelectric point of about 9.0 (for example, see Non-Patent Document 1). Two of Cry j2 reported by Sakaguchi et al. With a molecular weight of about 37,000 daltons and an isoelectric point of about 9.5 (see, for example, Non-Patent Document 2) are known. Reacts frequently with allergens.

  The most effective way to treat hay fever is to avoid contact with allergens, but in patients who are sensitized or developed with allergens that are free and present throughout the living environment, side effects such as antihistamines may also occur. The reality is that we have to rely on temporary solutions with symptomatic treatments. For this reason, unless you continue to use it, it will repeat the onset, and you will be burdened financially and physically, and if you stop using it, you may be worried about worsening symptoms due to rebound. Yes.

  On the other hand, attempts have been made on desensitization therapy in which allergens, which are allergic causative agents, are repeatedly administered to patients to cure them. There is a report that the symptoms improved in 90% or more of patients with desensitization treatment in ascidian asthma (for example, see Non-Patent Document 3). (For example, see Non-Patent Document 4). However, if there is a side effect such as anaphylactic shock if the antigen to be used is wrongly selected, an appropriate diagnosis for each patient is required.

  In the desensitization of Japanese cedar pollinosis, the main allergens Cry j1 and Cry j2 alone do not provide a sufficient therapeutic effect. For treatment, first, accurate diagnosis is important, but currently there are few diagnoses other than major allergens, and in recent years, detailed immunochemical characteristics of other allergen proteins have been desired. It is rare.

  As cedar pollen allergens other than Cry j1 and Cry j2 reported so far, CJP-6 (see, for example, Non-Patent Document 5) by Kawamoto et al. Showing high homology with isoflavone reductase, and SDS-poly. There are cedar pollen-derived allergens having a molecular weight measured by acrylamide gel electrophoresis of 57,000-67,000 daltons and an isoelectric point of 7.0-9.0 (see, for example, Patent Document 1). .

Yasueda, H. et al., J. Allergy Clin. Immunol. 71, 77-86, 1983 Sakaguti, M. et al., Allergy, 45, 309-312, 1990 Sigeta S. et al., Arerugi, 39 (3), 313-21, 1990 Bousquet J, et al., J. Allergy Clin. Immunol. 102, 558-62, 1998 Kawamoto S. et al., Clin. Exp. Allergy, 32 (7), 1064-70, 2002 JP 2001-151797 A

  In view of the prior art as described above, the present invention is intended to provide novel allergens other than Cry j1 and Cry j2 related to cedar pollinosis, diagnostic agents, preventive agents, and therapeutic agents for allergies using them. is there.

  In order to achieve the above object, the present inventors have extensively searched for spots that react frequently with IgE antibodies in sera of hay fever patients by proteomic analysis of cedar pollen crude antigen. As a result, it was found for the first time that a protein (CJP-16) having a molecular weight of about 25,000 to 40,000 daltons and an isoelectric point of about 4.0 to 5.0 has high allergenicity. Furthermore, the analysis by protein engineering and genetic engineering techniques has revealed its immunochemical characteristics, and the present invention has been completed.

That is, the present invention is as follows.
(1) a protein contained in cedar pollen, SDS-polyacrylamide gel electrophoresis the molecular weight as determined by method 25, and illustrates the 000～40,000 Dalton, measured by isoelectric 4.0 to 5 . 0 isoelectric point two indicates, characterized by comprising the amino acid sequence set forth in SEQ ID NO: 1, cedar pollen allergens.
(2) The cedar pollen crude antigen obtained by two or more methods selected from affinity purification using chitin, ion exchange chromatography, gel filtration chromatography, centrifugation, concentration, and dialysis. The cedar pollen allergen of (1) .

( 3 ) The cedar pollen allergen according to (1) or (2) above, which is a protein prepared by chemical synthesis.

(4) The cedar pollen allergen according to (1) or (2) above, which is a protein produced in a host cell transformed with a DNA comprising the nucleotide sequence set forth in SEQ ID NO: 1 .
( 5 ) The cedar pollen allergen according to (1) or (2) above, which is a protein prepared by a cell-free expression system .
(6) the (1) to (5) specifically reactive to monoclonal antibody to any one of cedar pollen allergens.

( 7 ) A diagnostic agent for hay fever patients using the cedar pollen allergen of any one of (1) to (5) .

  The novel cedar pollen allergen of the present invention can be used for diagnostics, preventives, and therapeutics for allergies, and allergen proteins and protein fragments thereof are Cry j1, Cry j2, and other cedars. By combining with pollen allergen, it can be used for diagnosis of cedar pollinosis or treatment for desensitization.

The present invention is described in detail below.
In the Japanese cedar pollen allergy, major antigens of Cry j1 and Cry j2 have been identified and studied in detail, but other allergens have not been sufficiently developed. Therefore, the present inventors developed a cedar pollen crude antigen by two-dimensional electrophoresis, and then specifically reacts with patient serum IgE by immunoblotting, aiming at a comprehensive analysis of allergens contained in cedar pollen. Searched for a spot. As a result, it was found that allergens that react with IgE also exist in the acidic region in addition to the basic regions Cry j1 and Cry j2. Thereafter, amino acid sequences of the obtained positive spots were performed using ESI Q-TOF MS, and homology search was performed. As a result, it was revealed that the positive spots showed high homology with class I chitinase derived from A. thaliana. Class I chi with amino acid structure in common with these
Tinase is known as one of causative antigens such as latex allergy. However, since there is no report that chitinase is an important allergen in Japanese cedar pollinosis, this protein was considered to be a novel Japanese cedar pollen allergen (CJP-16).

  Moreover, in order to isolate the cedar pollen allergen (CJP-16) gene of the present invention, a cedar cDNA was constructed using total RNA purified from cedar straw. A degenerate primer was designed from the conserved sequence of chitinase, and PCR was performed using cDNA as a template. Sequence analysis was performed on the amplified sequence, primers were further designed based on the obtained base sequence, and the full length gene of CJP-16 was obtained by the RACE method. The resulting sequence contained a start codon and a stop codon and its ORF was 846 bases. In addition, a sequence showing homology with the sequence obtained by analysis of ESI Q-TOF MS was also confirmed.

  Furthermore, the present inventors tried to purify the natural CJP-16 allergen from the cedar pollen crude antigen. Since CJP-16 allergen was present in the acidic region, it was applied to an SP-sepharose cation column, and the flow-through fraction was collected. In order to specifically obtain chitinase from this fraction, affinity purification using colloidal chitin was performed. As a result, CJP-16 protein having a molecular weight of about 30,000 daltons was obtained as measured by SDS-polyacrylamide gel electrophoresis.

  The allergenicity of the obtained natural CJP-16 was evaluated by ELISA. Analysis of the CJP-16-specific IgE antibody titer using hay fever patient serum showed a positive reaction in about 50% of the patient serum.

  Subsequently, since chitinase is known as one of the antigens causing latex allergy, the cross-reactivity of cedar pollen allergen CJP-16 was investigated using latex allergy patient serum. As a result, it was revealed that CJP-16 cross-reacted with latex allergy patient sera because it showed a positive reaction in all the patient sera analyzed (3 samples).

  Moreover, CJP-16 content in cedar pollen crude antigen (CJP) was investigated by ELISA inhibition assay. A 96-well plate was coated with the crude antigen CJP, and its inhibitory ability was examined by preincubating the patient pool serum with CJP-16, CJP and Rnase A. The amount of antigen showing a 50% inhibition rate was 321.4 for CJP-16. Since ng / ml and CJP were 7.72 ng / ml, it was estimated that the CJP-16 content in the cedar pollen crude antigen (CJP) was about 2.4%.

  The CJP-16 of the present invention can be obtained by incorporating cDNA encoding the entire protein or at least one fragment thereof into an expression vector, introducing it into Escherichia coli, yeast, insect or animal cells and culturing. It is. However, in expression systems using prokaryotic cells such as E. coli, it is better to use eukaryotic cells such as yeast for the expression of recombinant CJP-16 because appropriate modifications such as sugar chains are not performed. is there.

  The new cedar pollen allergen CJP-16 obtained in the present invention can be used as a diagnostic reagent for cedar pollinosis. In addition, it is possible to provide information on cross sensitization such as latex from the diagnosis result.

  Moreover, since the entire amino acid sequence of CJP-16 protein was clarified by the present invention, it became possible to identify the T cell epitope site of CJP-16 protein. Therefore, immunotherapy of cedar pollinosis using those T cell epitope peptides can be expected.

  Hyposensitization is one of the treatments for allergies, but side effects such as anaphylaxis are also considered, so in recent treatments, T cells are specifically recognized rather than administering allergens to patients. Peptide vaccines that administer peptides consisting only of the minimum region of allergens, that is, T cell epitopes, have attracted attention.

  So far, T cell epitopes of Cry j1 and Cry j2 which are main antigens have been reported (Japanese Patent Laid-Open No. 7-118295, Japanese Patent Laid-Open No. 8-47392). 10-259198).

  Since the method for identifying the T cell epitope of the allergen protein has already been established, the T cell epitope peptide of the CJP-16 protein can be easily obtained.

  The T cell epitope peptide of CJP-16 protein obtained in the present invention can be mixed with or combined with the T cell epitope peptide of Cry j1, Cry j2, and other cedar pollen allergens alone. It can be used for immunotherapy.

  Furthermore, the present invention can provide a monoclonal antibody and a polyclonal antibody that specifically react with the CJP-16 protein or a protein fragment thereof.

Hereinafter, the present invention will be described in more detail with reference to examples. In addition, this invention is not limited to the following Example.
<Example 1> Proteomic analysis of cedar pollen crude antigen Preparation of cedar pollen crude antigen 3.0 L of extraction buffer (20 mM PBS + 3 mM EDTA pH 7.6) was added to 80 g of Japanese cedar pollen (collected in Toyo-cho, Toyota-gun, Hiroshima). And stirred at 4 ° C. for 4 hours. Thereafter, ammonium sulfate was added to the supernatant obtained by centrifugation (7,000 rpm, 30 min) to a final concentration of 80% saturation, and the mixture was stirred overnight at 4 ° C. Next, the precipitate was collected by centrifugation (7,000 rpm, 30 min) and dialyzed overnight against milliQ water. Thereafter, the supernatant obtained by centrifugation (10,000 rpm, 30 min) was freeze-dried to obtain a cedar pollen crude antigen (CJP).

Two-dimensional electrophoresis of crude Japanese cedar pollen antigen Suspended with 200 mg of Japanese cedar pollen crude antigen (CJP) and suspended in 4 ml of PBS + 60 mg of dithiothreitol (DTT) and 2 ml of trichloroacetic acid prepared to 60% with PBS And then left on ice for 90 minutes. Thereafter, centrifugation (3,500 rpm, 15 min) was performed to collect the precipitate. The precipitate was suspended by adding 10 ml of cold acetone and washed. Further, after centrifugation (3,500 rpm, 20 min), the precipitate was dried by speed back. 1 ml of Lysis Buffer (8 M urea, 2 M thiourea, 2% CHAPS, 2% SB3-10, 1% DTT, 0.8% Ampholine) was added to the precipitate, suspended, and completely dissolved by ultrasonic crushing. Thereafter, centrifugation (18,000 rpm, 20 min) was performed, and the supernatant was used as a sample for two-dimensional electrophoresis.

  After the dry strips in the pI range 3-10 were swollen overnight in the lysis buffer, the CJP sample was applied to the strips and subjected to first-dimensional (isoelectric point) electrophoresis.

  A gladiendo gel having an acrylamide concentration of 9 to 18% was prepared, and a gel after isoelectric focusing was set thereon. After the low-melting point agarose was overlaid and solidified from the top of the gel, electrophoresis of the second dimension (molecular weight) was performed overnight at 80 V.

  After the second dimensional electrophoresis was completed, the protein was detected by silver staining of the gel. An example of the result is shown in FIG. In the cedar pollen crude antigen, many proteins were confirmed in addition to Cry j1 and Cry j2, which are the main antigens.

Western blotting The protein after two-dimensional electrophoresis was transferred to a membrane under the condition of 60 V for about 6 hours using a blotting kit (Hoefer DALT). Thereafter, the membrane was washed with PBST (0.1% Tween20 / PBS) and shaken overnight with a blocking solution (5% skim milk, 1% BSA / PBST). Thereafter, the plate was washed with PBST and incubated for 4 hours with shaking in patient serum diluted 10-fold with a blocking solution. After washing, anti-human IgE-biotin label (Biosource) diluted 2,500 times with blocking solution was added and incubated for 2 hours with shaking. After washing with PBST, it was incubated for 1 hour with streptavidin-HRP label (ZYMED) diluted 2,500 times with blocking solution. Thereafter, the plate was washed with PBST, incubated with ECL Westernblotting detection reagents (Amersham Pharmacia Biotech) for 5 minutes, and exposed to X-ray film to detect positive spots.

  As a result of analysis by Western blotting, it was found that there were many spots showing positive reaction other than Cry j1 and Cry j2 in the cedar pollen crude antigen. Of the 12 patients examined with serum IgE, spots with particularly strong positive reaction are shown by squares in FIG.

  Among them, an amino acid sequence of CJP-16 protein showing a reaction frequency of 50% or more was performed using ESI Q-TOF MS. As a result, a sequence of -Phe-Glu-Cys-Asp-Gly-Gly-Asn-Ala-Ala-Thr-Val-Ala-Ser-Arg- was obtained and homology search was performed. It became clear that it showed high homology with chitinase.

<Example 2> Determination of base sequence and amino acid sequence of CJP-16 gene Purification of cedar total RNA Cedar meal (2 g) was pulverized in liquid nitrogen and 10 times (W / V) 2 × CTAB (cetyltrimethylammonium bromide). ) After dissolving in the solution, it was incubated at 65 ° C. for 10 minutes. An equal volume of chloroform / isoamyl alcohol (24: 1) was added and stirred, centrifuged at room temperature (15,000 rpm, 10 min), and the aqueous layer was collected. Again, add an equal volume of chloroform / isoamyl alcohol (24: 1), stir, centrifuge at room temperature (15,000 rpm, 10 min), collect the aqueous layer, add 3/4 volume of isopropanol at room temperature. Allowed to stand for 10 minutes. After centrifugation at 4 ° C. (15,000 rpm, 10 min), the precipitate was dissolved in TE buffer, and 1/4 volume of 10M lithium chloride solution was added and incubated on ice for 2 hours. After centrifugation at 1 ° C. (15,000 rpm, 10 min), the precipitate was dissolved in TE buffer, and an equal amount of TE saturated phenol (pH 9.0) was added and stirred. After centrifugation at room temperature (15,000 rpm, 10 min), the aqueous layer was collected, phenol / chloroform was added and stirred, and centrifuged at room temperature (15,000 rpm, 10 min). A 1 / 10-fold amount of 3M sodium acetate was added to the supernatant after centrifugation, and a 2-fold amount of cold ethanol (-20 ° C) was further added, and the mixture was allowed to stand at -80 ° C for 10 minutes. Centrifugation was performed at 4 ° C. (15,000 rpm, 10 min) to precipitate RNA, and the precipitate was washed with 70% ethanol. The precipitate was vacuum dried and then dissolved in an appropriate amount of TE buffer.

Preparation of cedar cDNA cDNA was synthesized from the obtained total RNA using 3 'RACE System for Rapid Amplification of cDNA Ends (# 18373-019 Invitrogen).
5 μl of total RNA (5 μg) solution, 1 μl of adapter primer, and 6 μl of DEPC-treated water were added, incubated (70 ° C., 10 min), and left on ice for 1 minute. Add 2 μl of 10 × PCR Buffer, 2 μl of MgCl ₂ (25 mM) solution, 1 μl of dNTP MI × (2.5 mM each) and 2 μl of DTT (0.1 M) to the reaction mixture, preincubate at 42 ° C for 5 minutes, and use SUPERSCRIPT 1 μl of II (Life Technologies, Inc. Rockville, MD) was added. After incubation (42 ° C., 50 min), the reaction was stopped (70 ° C., 15 min). The mixture was allowed to stand on ice, centrifuged, and the reaction mixture was collected, 1 μl of RNase H was added and incubated (37 ° C., 20 min), and stored at −80 ° C.

Determination of full-length gene sequence of CJP-16 Degenerate primer “5'- GARATHGCNGCNTTYTTYGC-3 ′” is designed based on amino acid sequence (EIAAFFAHV) highly conserved among several chitinases, and the prepared cDNA is used as a template. As a result, PCR reaction was performed. When sequence analysis was performed on the amplified sequence, the result shown in SEQ ID NO: 2 in the sequence listing was obtained. Based on the obtained base sequence (QGFGATI), the primer “5′-ATNGTNGCNCCRAANCCYTG-3 ′” was designed again and PCR was performed. As a result, the result shown in SEQ ID NO: 3 in the sequence listing was obtained. In these two results, a difference was observed in the 261st base sequence (SEQ ID NO: 2A, SEQ ID NO: 3T) and the 322nd base sequence (SEQ ID NO: 2G, SEQ ID NO: 3: C). Moreover, although the difference is seen also in the base sequence after 326 bases, homology with the base sequence of another plant chitinase increases by inserting 1 base in 326th, and also corresponds with the amino acid sequence of sequence number 2. From these facts, it was considered that the 326th base was deleted by PCR amplification reaction. Moreover, when this is considered, the sequence which shows homology with the partial amino acid sequence [FECDGGNAA] of CJP-16 revealed from the proteome analysis of the cedar pollen crude antigen exists in [MQCDGGNA] at the C-terminus. These facts suggested that there are at least two CJP-16 isoforms in the cedar cDNA.
Further, primers were designed from the conserved sequences in SEQ ID NO: 2 and SEQ ID NO: 3 and 5'-RACE was performed. Based on the 5′-side nucleotide sequence obtained, primers were further designed and 3′-RACE was performed to obtain a full-length gene of CJP-16. As a result, the base sequence of CJP-16 shown in SEQ ID NO: 1 was obtained. The resulting sequence contained a start codon and a stop codon and its ORF was 846 bases. In addition, since the sequence having homology with [FECDGGNAATVASR] obtained by TOF MS analysis is present in [247 MECDGGNAATVAST 260], it was shown that the obtained sequence was the full-length gene sequence of CJP-16. .

Homology search for CJP-16 gene and protein
The homology of the obtained CJP-16 gene and protein was searched by FASTA and BLAST searches using the GenBank database. The result of investigating the homology between the amino acid sequence of CJP-16 and chitinase derived from other plants is shown in FIG. * Indicates a matched amino acid sequence. CJP-16 showed homology of 65.2% at the amino acid level with P.glauca chitinase protein, 62.4% at the DNA level, 59.1% at the amino acid level with V. venifera class IV endochitinase, and 60.1% at the DNA level. Moreover, it showed 54.4% amino acid level with A.thaliana class IV chitinase, 57.5% at DNA level, 49.3% at amino acid level with D.carota class IV chitinase, and 61.7% at DNA level. As described above, it was confirmed that CJP-16 retained high homology with other types of chitinases. Since all these chitinases were class IV chitinases, this CJP-16 was also considered to be a class IV chitinase.

  The results of a search for homology between chitinase and CJP-16 reported as allergens so far are shown in FIG. * Indicates a matched amino acid sequence. It showed 43.2% homology at the amino acid level and 47.6% at the DNA level with Hev b 11w, which is reported as a major allergen of latex allergy as a highly homologous allergen. In addition, avocado-derived Pers a 1 reported as an allergen in oral allergy syndrome showed 43.2% homology at the amino acid level and 48.7% at the DNA level. .

<Example 3> Purification of natural CJP-16 protein Production of colloidal chitin A suspension of 2 g of powdered chitin in 50 ml of distilled water and 50 ml of concentrated sulfuric acid were cooled on ice for 3 hours. Thereafter, concentrated sulfuric acid was added dropwise to the chitin / distilled water drop by drop on ice. After dropping, the mixture was filtered through glass wool and added to 90 ml of distilled water on ice. After the mixture was centrifuged (2000 g, 20 min, 4 ° C.), the precipitated colloidal chitin was washed with MilliQ water and PBS (2000 g, 20 min, 4 ° C.). After neutralizing the pH of the precipitate, it was stored at 4 ° C. until use.

Purification of CJP-16 protein 80 g of cedar pollen was dissolved in 3 L of PBS (pH 7.6 + EDTA) and stirred overnight at 4 ° C. After stirring, the mixture was centrifuged (7000 rpm, 35 min, 4 ° C.), the supernatant was pooled, ammonium sulfate was added to 80% saturation, and the mixture was stirred overnight at 4 ° C. Thereafter, the precipitate was collected by centrifugation (7000 rpm, 35 min, 4 ° C.), and the solution dissolved in acetate buffer (pH 5.0) was dialyzed against the acetate buffer (pH 5.0). After dialysis, centrifugation (10000 rpm, 15 min, 4 ° C) is performed, and the supernatant is filtered through 0.8 µm pore-size and then subjected to cation exchange chromatography (SP-Sepharose) to collect the flow-through fraction. did. The flow-through fraction was concentrated under reduced pressure to 100 to 200 ml using an evaporator, 5 g wet-weight colloidal chitin was added, and the mixture was stirred at 4 ° C. overnight. Thereafter, the mixture was further incubated on ice for 1 hour, and the precipitate was collected by centrifugation (2000 g, 30 min, 4 ° C.). The collected precipitate was washed with 0.1% Tween-20 / PBS, 3 ml of PBS was added to the obtained precipitate and incubated in a 60 ° C. hot water bath. Thereafter, the supernatant obtained by centrifugation (2000 g, 30 min, 25 ° C.) was lyophilized and dissolved in 1 ml of PBS to obtain purified CJP-16 protein (chitinase).

FIG. 4 shows the purification process of the native CJP-16 protein. Using samples of crude cedar pollen antigen (FIG. 4 lane 2), flow-through fraction after cation exchange chromatography (FIG. 4 lane 3), and purified CJP-16 protein (FIG. 4 lane 4), SDS -PAGE (Laemmli method) was performed. After electrophoresis using a separation gel having a polyacrylamide concentration of 11.5%, the protein was stained with a staining solution (EtOH: AcOH: H ₂ O = 9: 2: 9 + 0.25% CBB R-250). Thereafter, destaining solution _{(EtOH: AcOH: H 2 O} = 25: 8: 65) except for the extra staining. A single band was confirmed at a molecular weight of about 30,000-35,000 Dalton (FIG. 4, lane 4), and the protein was considered to be CJP-16. Note that lane 1 in FIG. 4 is a molecular weight marker.

<Example 4> Allergenicity of natural CJP-16 protein (IgE binding ability)
The IgE binding ability of native CJP-16 protein was measured by ELISA. First, 50 μl of an antigen solution (250 ng / ml) diluted with 100 mM bicarbonate buffer (pH 9.3) was applied to the well of a microtiter plate. In addition, human IgE standard was first diluted to 1000 ng / ml, 50 μl of the double dilution series was added to each well, and left at room temperature for 2 hours. After washing with PBST, 300 μl of blocking buffer (PBS, 3% skim milk, 1% BSA) was applied and allowed to stand at 4 ° C. overnight. After washing, 50 μl of sera of cedar allergic patients and healthy subjects diluted 200-fold with the same buffer was applied and allowed to stand at 4 ° C. for 4 hours. After washing, 50 μl of anti-human IgE EPSILON CHAIN BIOTIN CONJUGATE (Biosource International, Inc.) diluted 1,000-fold with the same buffer was applied and allowed to stand at room temperature for 2 hours. After washing, 50 μl of alkaline phosphatase-labeled Streptavidin diluted 1,000-fold with the same buffer was applied, and left at room temperature for 1 hour. After thorough washing, 50 μl of AttoPhos ^™ was added, and the fluorescence intensity was measured with CytoFluor ^™ II (PerSeptive Biosyatems).

FIG. 5 shows the results of analysis of CJP-16-specific IgE antibody titer using 18 samples of cedar pollinosis patient serum (RAST Score ≧ 2) and 3 samples of healthy subject serum. As a reference, a value obtained by adding three times the standard deviation to the average value of three healthy subjects is indicated by a broken line. A specimen showing an IgE value equal to or higher than the broken line was evaluated as positive for the CJP-16 at a risk rate of 5% or less.
As a result, 9 samples out of 18 samples (No.2,4,5,7,8,9,12,13,14) (50%) were positive for IgE reaction against CJP-16. . These results are in good agreement with the results of evaluation of allergen reaction frequency by immunoblotting of two-dimensional electrophoresis (21 out of 40 reaction frequency (52.5%)), and purified CJP-16 protein has strong allergenicity. It was shown to have.

Inhibitory ability of CJP by native CJP-16 (ELISA inhibition assay)
An ELISA inhibition assay was performed for the purpose of investigating the content of CJP-16 in CJP. 50 μl of CJP solution (1 μg / ml) diluted with 100 mM bicarbonate buffer was applied and allowed to stand at room temperature for 2 hours. After washing, 300 μl of blocking buffer (3% skim milk, 1% BSA, 0.1% Tween 20 / PBS) was applied and allowed to stand at 4 ° C. overnight. In addition, patient pooled sera obtained by diluting antigen (CJP-16, CJP, RNase) with blocking buffer to a final concentration of 40 times to obtain various concentrations (1/10 dilution series of 10 μg-0.001 μg / ml) diluted with blocking buffer ( 11 specimens, RAST value ≧ 2) and preincubated overnight at 4 ° C. After washing the plate, the patient serum solution preincubated with the antigen was applied at 50 μl / well and allowed to stand at 4 ° C. for 4 hours. After washing, 50 μl of anti-human IgE EPSILON CHAIN BIOTIN CONJUGATE diluted 1,000-fold with Blocking buffer was applied, and allowed to stand at room temperature for 2 hours. After washing, 50 μl of alkaline phosphatase-labeled Streptavidin diluted 1,000-fold with the same buffer was applied, and left at room temperature for 1 hour. After thorough washing, 50 μl of AttoPhos ^™ was added and the fluorescence intensity was measured with CytoFluor ^™ II.

  The result of ELISA inhibition assay is shown in FIG. Rnase A was used as a negative control. Since CJP-16 inhibited the reaction between CJP and patient serum IgE, it was shown that CJP-16 exists as an allergen in CJP. In addition, when the amount of antigen showing 50% inhibition rate is converted from the graph, it is 321.4 ng / ml for CJP-16 and 7.72 ng / ml for CJP, so the content of CJP-16 in CJP is about 2.4%. It was suggested.

Cross-reaction between natural CJP-16 and latex allergy patient sera Since CJP-16 protein has high homology with Hev b 11 which is a major antigen of latex allergy, CJP-16 is latex allergy patient serum IgE Cross-reactivity was investigated by ELISA. The results are shown in FIG. The total value of the value obtained by adding three times the standard deviation to the average value of the three healthy subjects is indicated by a broken line, and values above the broken line are defined as significant values. As a result, all of the analyzed latex allergy patient sera were positive for CJP-16. From these results, it was revealed that the CJP-16 has cross-reactivity with latex allergy patients.

SEQ ID NO: 2—Description of artificial sequence: cDNA prepared from the amino acid sequence of chitinase
SEQ ID NO: 3—Description of artificial sequence: cDNA prepared from amino acid sequence of chitinase

It is a figure which shows the two-dimensional electrophoresis of a cedar pollen crude antigen (CJP). It is a figure which shows the homology of a cedar pollen allergen CJP-16 and other plant origin chitinase. It is a figure which shows the homology of the cedar pollen allergen CJP-16 and other species chitinase which has allergenicity. It is the figure which analyzed the purification process of natural type CJP-16 allergen by SDS-PAGE. It is a figure which shows the result of having analyzed CJP-16 specific IgE antibody titer using 18 specimens (RAST Score> = 2) of a cedar pollinosis patient serum, and 3 healthy subject serums. It is a figure which shows the result of having analyzed the CJP binding inhibition ability of patient serum IgE by refined CJP-16 by ELISA inhibition. It is a figure which shows the result of having investigated the cross reaction of refinement | purification CJP-16 and latex allergy patient serum IgE by ELISA.

Claims (7)

In proteins contained in cedar pollen, SDS-polyacrylamide gel electrophoresis as determined by the molecular weight 25, it shows the 000～40,000 daltons, as determined by isoelectric focusing from 4.0 to 5. 0 isoelectric point two indicates, characterized by comprising the amino acid sequence set forth in SEQ ID NO: 1, cedar pollen allergens. The cedar pollen crude antigen was obtained by two or more methods selected from affinity purification using chitin, ion exchange chromatography, gel filtration chromatography, centrifugation, concentration, and dialysis. The cedar pollen allergen described. The cedar pollen allergen according to claim 1 or 2, which is a protein prepared by chemical synthesis . The cedar pollen allergen according to claim 1 or 2 , wherein the cedar pollen allergen is a protein produced in a host cell transformed with a DNA comprising the nucleotide sequence of SEQ ID NO: 1 . The cedar pollen allergen according to claim 1 or 2, which is a protein prepared by a cell-free expression system. A monoclonal antibody that specifically reacts with the cedar pollen allergen according to any one of claims 1 to 5. A diagnostic for hay fever patients using the cedar pollen allergen according to any one of claims 1 to 5.

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