JP2009183176A - Il-1 type ii receptor gene deletion mutant mouse - Google Patents

Abstract

<P>PROBLEM TO BE SOLVED: To provide a gene deletion mutant animal that does not express an IL-1 type II receptor gene at all in order to elucidate the role of IL-1 type II receptor on signalization of IL-1 ligand. <P>SOLUTION: The IL-1 type II receptor gene deletion mutant mouse has deletion and/or insertion mutation on an IL-1 type II receptor gene locus on a mouse chromosome. The method for producing an antibody preparation for treating allergy and/or inflammation comprises a step of immunizing and sensitizing a mouse with a mouse IL-1 type II receptor protein to prepare a monoclonal antibody to the receptor protein. The method for screening an antiallergic agent or an anti-inflammatory agent candidate comprises a step of letting an IL-1 act on an IL-1 type II receptor or a cell expressing the receptor in the presence or absence of a test substance. <P>COPYRIGHT: (C)2009,JPO&INPIT

Description

  The present invention relates to an IL-1 type II receptor gene-deficient mutant mouse, a method for producing an antibody preparation for treating allergy and / or inflammation using the mutant mouse, and a method for screening an antiallergic drug or anti-inflammatory drug candidate And about.

IL-1 is a pro-inflammatory cytokine, and factors that down-regulate its production and / or activity are clinically important drug discovery targets. As explained in the review of Non-Patent Document 1 below, the IL-1 ligand family has three members: IL-1 alpha, IL-1 beta, and IL-1 receptor antagonist (IL-1Ra), It is known that IL-1 alpha and IL-1 beta function as agonists, and IL-1Ra is a specific antagonist. On the other hand, the IL-1 receptor family includes IL-1 type I receptor (IL-1R I), IL-1 type II receptor (IL-1R II), and IL-1 receptor accessory protein (IL-1RAcP). The IL-1 type I receptor is involved in IL-1 ligand signaling, but the IL-1 type II receptor has little intracellular domain and can bind to the IL-1 ligand. It is thought that no signal transduction occurs. The IL-1 type II receptor does not form a complex with the type I receptor, whereas the IL-1 receptor accessory protein forms a complex with both the IL-1 type I receptor and the IL-1 type II receptor. be able to.
Dinarello, C.I. H. , Blood, 87: 2095-2147 (1996).

The IL-1 type II receptor is traditionally a decoy receptor that regulates IL-1 signaling by competitively inhibiting the binding of the IL-1 type I receptor to the IL-1 ligand. Has been considered. In addition, when an IL-1 type II receptor binds to an IL-1 ligand, it also binds to an IL-1 receptor accessory protein to form a complex. Therefore, not only an IL-1 ligand but also an IL-1 receptor acceptor is formed. Solly protein has also been considered to competitively inhibit binding to IL-1 type I receptor (Non-patent Document 2). Furthermore, the extracellular domain of the type II receptor is cleaved by proteolytic enzymes and is present in the blood circulation as a soluble fragment. It is also known that the soluble fragment of this type II receptor has a 100-fold higher affinity for IL-1 alpha and beta and forms a stable soluble complex when associated with the soluble fragment of the receptor accessory protein. (Non-Patent Document 3).
Lang, D.D. et al. , J. et al. Immunol. 161: 6871-6877 (1998) Smith, D.D. E. et al. , Immunity, 18: 87-96 (2003)

  As shown in Table 1, the mouse IL-1 ligand and receptor family genes have been cloned one after another since the IL-1 alpha gene was cloned in 1984. The cloned genes have been produced in sequence by gene-deficient mice by homologous gene recombination methods to ES cells.

In Table 1, the inventors' group (Horai et al., 1998) of the present invention created gene-deficient mice for all of the IL-1 ligand family genes. That is, a mouse deficient in each of IL-1 alpha and IL-1 beta genes and a double deficient mouse were created, and a mouse deficient in IL-1Ra gene was also created (Non-patent Document 4).
Horai, R.A. et al. , J. et al. Exp. Med. 187: 1463-75 (1998)

  Mice deficient in the IL-1 receptor family gene have been created by other groups. That is, IL-1 type I receptor (IL-1R I) and IL-1 receptor accessory protein (IL-1RAcP) gene-deficient mice were created in 1997 and 1998, respectively. However, even though the IL-1 type II receptor gene was cloned in 1991, mice lacking the IL-1 type II receptor (IL-1R II) gene have reached the present from any laboratory in the world. There is no report that it was made until.

Among IL-1 related gene-deficient mice, IL-1Ra gene-deficient mice produced by the inventor's group spontaneously develop various autoimmune diseases including arthritis. It is used as a model animal (Non-patent Document 5). IL-1Ra is an antagonist of IL-1 ligand and inhibits stimulation of agonists IL-1alpha and IL-1beta. The IL-1 type II receptor is also a decoy receptor for IL-1 ligand and IL-1RAcP, and is thought to inhibit the stimulation of IL-1 alpha and IL-1 beta. Therefore, the IL-1 type II receptor gene (Il1r2 locus) ) -Deficient mice are expected to be useful disease model animals.
Horai, R.A. et al. , J. et al. Exp. Med. , 191: 313-320 (2000)

  In order to elucidate the role of IL-1 type II receptor in IL-1 ligand signaling, it is necessary to create a gene-deficient mutant animal in which the IL-1 type II receptor gene is not expressed at all. There is also a need to develop methods for analyzing the dynamics, complex formation and signaling of IL-1 ligands and receptors in such animals. Furthermore, it is also necessary to develop a screening method for substances having IL-1 signal transduction regulating activity from candidate substances that can complement the IL-1 type II receptor.

  The present invention provides an IL-1 type II receptor gene deletion mutant mouse having a deletion and / or insertion mutation at the IL-1 type II receptor locus on the mouse chromosome.

  In the mutant mutant mouse of the IL-1 type II receptor gene of the present invention, the mutation may express a green fluorescent protein instead of the full-length IL-1 type II receptor protein.

  The present invention includes a step of immunizing a mouse IL-1 type II receptor protein in the mouse of the present invention to produce a monoclonal antibody against the receptor protein, and immunization from a wild type mouse or a wild type mouse. And a method for producing an antibody preparation for treating allergy and / or inflammation, comprising the step of screening a monoclonal antibody that suppresses stimulation of the immune system by IL-1 by administration to cells.

  The present invention includes a step of allowing IL-1 to act on an IL-1 type II receptor or a cell expressing the receptor in the presence or absence of a test substance, IL-1 type II receptor and IL-1 A method for screening an antiallergic drug or anti-inflammatory drug candidate.

  In the present specification, a mutant mouse deficient in an IL-1 type II receptor gene refers to a mutant mouse that cannot normally produce a wild type IL-1 type II receptor. The IL-1 type II receptor locus is located on the first chromosome of mouse, a 9-exon linked mRNA is produced from a transcript of about 40.5 kb, and a polypeptide consisting of 410 amino acid residues Is translated.

  The deletion mutant of the present invention is encoded by at least a part of at least one exon of a wild type gene of IL-1 type II receptor, in addition to a mutant that does not produce any IL-1 type II receptor polypeptide. Where a polypeptide is produced, including variants that lack any or all of IL-1 ligand binding, association with IL-1 receptor accessory protein, and other functions. The variants of the present invention may have deletions and / or insertions in any part of any exon and / or intron of the IL-1 type II receptor locus. The mutant mouse of the present invention includes not only homozygous individuals in which both of the two first chromosomes contain the mutation, but also only one of the two first chromosomes contains the mutation and the other is a wild type. Some heterozygous individuals are also included.

  The mutant of the present invention may be produced by any method such as chemical, radiation and the like. A preferred method for producing the mutant of the present invention is described in detail, for example, in Manipulating the Mouse Embryo: A Laboratory Manual (3rd ed., Nagy, A. et al. Cold Spring Harbor Press NY, 2003). Mutation introduction into a target gene by homologous gene recombination method into a stem cell (ES cell).

  In one embodiment of the invention, mutations have been introduced into the IL-1 type II receptor gene such that green fluorescent protein is produced. However, when a variant that does not produce any IL-1 type II receptor polypeptide or a polypeptide encoded by at least a part of at least one exon of the wild type gene of IL-1 type II receptor is produced. A sequence such as Cre, provided that it is a mutant lacking any or all of IL-1 ligand binding, association with IL-1 receptor accessory protein, and other functions Specific recombination sequences such as loxP recognized by specific recombinase are inserted, RNAi and other RNA and tRNA genes involved in gene expression control are inserted, green fluorescent protein and other fluorescent proteins, and Renilla Luciferase and other photoproteins derived from fireflies, etc., and alkaline phosphate Enzymes whose activity can be quantified or localized by enzymatic products such as oxidase, peroxidase and other enzyme reaction products, gene products that confer resistance to neomycin, hygromycin, zeocin, puromycin, blasticidin S and other drugs, and nutritional requirements Any protein is produced that includes, but is not limited to, a gene product that allows sex selection and a protein involved in another signaling mechanism that can be clearly distinguished from the signaling mechanism by the IL-1 ligand. It does not matter.

  In the mutation introduced in one embodiment of the present invention, the green fluorescent protein can be expressed using the expression control mechanism of the IL-1 type II receptor gene. When such a mutant mouse is used, the expression of the IL-1 type II receptor gene can be monitored using fluorescence emitted by the green fluorescent protein as an index. When the mutant mouse is used, a substance that up-regulates or down-regulates the IL-1 type II receptor gene can be screened from various drug discovery candidate substances in a high-throughput manner. A substance that affects the expression of an IL-1 type II receptor gene, comprising the step of administering and / or expressing a drug discovery candidate substance to an individual mouse or a cell thereof that is a mutant mutant of the IL-1 type II receptor gene of the present invention. The substance selected by the screening method can regulate the signal transduction mechanism by stimulating the IL-1 ligand through affecting the expression of the IL-1 type II receptor gene. Connected.

  In addition, by administering and / or expressing a drug discovery candidate substance to a mutant mutant mouse of the IL-1 type II receptor gene of the present invention or a cell thereof, the IL-1 type II receptor caused by the mutation of the present invention Active substances that compensate for dysfunction can be screened. By a method for screening a substance that affects the expression of an IL-1 type II receptor gene, comprising the step of administering and / or expressing a drug discovery candidate substance to an individual mutant mouse or a cell thereof that is defective in the IL-1 type II receptor gene The selected substance can regulate the signal transduction mechanism by stimulating the IL-1 ligand through affecting the complex formation of the IL-1 ligand, leading to the development of a novel immunomodulatory drug.

  For example, IL-6, procollagen, MCP (Monocyte Chemotactic Protein) -1, MIP (Macrophage Inflammatory Protein) -2, PGES (Prostaglandin E synthase), etc. are included in the downstream of signal transduction by stimulation of IL-1 ligand. However, there are genes that are not limited to these, and stimulation with IL-1 ligand leads to induction or enhancement of the expression of these genes. Therefore, in the development of the above-mentioned immunomodulatory drugs, signal transduction due to stimulation of IL-1 ligand includes IL-6, procollagen, MCP-1, MIP-2, PGES, etc., but is not limited to these gene expression levels Quantitative analysis can be performed based on the change of.

  In this specification, a drug discovery candidate substance is a substance that can be a new drug or a lead compound for its development, and may be either a natural substance or a synthetic substance, or a polymer or multimer of chemical substances of some unit structure. It may be a monomer or a substance having any chemical structure. The drug discovery candidate substance may be administered to a mouse individual or its cells using a drug delivery system according to the dissolution characteristics of the substance. When the drug discovery candidate substance is a virus particle or nucleic acid and has a function of inducing or inhibiting the expression of some gene in mouse cells, it is expressed by virus infection, electroporation, liposome method or other methods. There is a case to let you.

  It has been thought that IL-1 ligand binds to a membrane-bound IL-1 type II receptor or a soluble fragment thereof, thereby inhibiting signal transduction via the IL-1 type receptor. However, in the IL-1 type II receptor gene-deficient mutant mouse of the present invention, the result that stimulation by IL-1 was suppressed was obtained. This suggests that the IL-1 type II receptor performs a previously unknown function of promoting IL-1 stimulation in normal individuals. Therefore, a novel therapeutic agent for allergy and / or inflammation can be developed by searching for a substance that suppresses the IL-1 stimulation promoting function of the IL-1 type II receptor.

  One example of a substance that suppresses the IL-1 stimulation promoting function of the IL-1 type II receptor is an antibody against the IL-1 type II receptor. In the IL-1 type II receptor gene-deficient mutant mouse of the present invention, the immune response against the mouse IL-1 type II receptor is not suppressed, and therefore an antibody against the mouse IL-1 type II receptor protein can be prepared. For such antibodies, the monoclonal antibodies used in the present invention are described in Kohler and Milstein, Eur. J. et al. Immunol. 6: 511-519, 1976, and improved techniques thereof. These methods involve the preparation of immortal cell lines that can produce antibodies with the desired specificity. Such cell lines may be generated from spleen cells derived from the IL-1 type II receptor-deficient mice of the present invention immunized as described above. The spleen cells are immortalized by various methods, and an immortal cell line having antibody-producing ability is prepared. The spleen cells are immortalized by, for example, fusion of the immunized IL-1 type II receptor gene-deficient mutant mouse of the present invention with myeloma cells derived from the same or different animals. Various fusion techniques known to those skilled in the art may be used. For example, the spleen cells and myeloma cells are mixed with a nonionic surfactant for several minutes and then plated at a low concentration in a selective medium that supports the growth of hybrid cells but not the growth of myeloma cells. A preferred selection technique uses HAT (hypoxanthine, aminopterin, thymidine) selection. Hybrid colonies are observed after sufficient time, usually about 1 to 2 weeks. A single colony is selected and its culture supernatant is tested for binding activity against the polypeptide. Hybridomas with high reactivity and specificity are preferred. By repeating the cloning by the limiting dilution method, a hybridoma clone that stably produces a large amount of highly reactive and specific antibody is selected. Monoclonal antibodies may be isolated from the supernatants of colonies of cell lines derived from selected growing hybridoma clones. In addition, various techniques may be used to improve yield, such as injecting the hybridoma cell line into the peritoneal cavity of a suitable vertebrate host such as a mouse. Monoclonal antibodies may be recovered from the hybridoma cell ascites or blood. Contaminants may be removed from the antibody by conventional techniques such as chromatography, gel filtration, precipitation and extraction.

The antigen-binding fragment of the antibody used in the present invention includes an Fab fragment or F (ab ′) ₂ fragment obtained by degrading an intact polyclonal antibody or monoclonal antibody with the proteolytic enzyme papain or pepsin, respectively, as well as natural antibody molecules. Includes Fv fragments containing non-covalent heterodimers of V _H and V _L regions that contain an antigen binding site that retains much of the ability to recognize and bind antigen.

The recombinant antibodies used in the present invention may be prepared by expression cloning of antibody genes including transformation into a suitable bacterial host or transfection into a suitable mammalian cell host. The chimeric antibody used in the present invention is a fusion protein supported by the constant domain of the same or different antibody so that the antigen-binding site of the recombinant antibody of the present invention can specifically bind to the IL-1 type II receptor. is there. The chimeric antibody used in the present invention includes a short chain variable region antibody (scFv) comprising an antibody heavy chain variable region (V _H ) operably linked to an antibody light chain variable region (V _L ), a camelid ( A camelid heavy chain antibody (HCAb), or a heavy chain variable region domain (VHH) thereof, which is a class of IgG without light chain produced by animals of Camelidae, camels, dromedaries, llamas). The recombinant antibodies of the present invention can be prepared in large quantities using prokaryotic and eukaryotic derived gene expression systems.

  Examples are shown below, but these are intended to illustrate embodiments and are not intended to limit the scope of the present invention.

Structure of Targeting Vector 1 FIG. 1 is a schematic diagram showing the structure of targeting vector 1 and the structures of wild-type chromosomal DNA and homologous recombinant DNA corresponding thereto. E2 to E8 represent the positions of the second to eighth exons, respectively. Therefore, the IL-1 type II receptor gene is transcribed from left to right in the figure. As the targeting vector 1, a hygromycin resistance gene was used as a marker for selecting ES cells incorporating the targeting vector 1, the homologous region on the left side was 1.8 kb, and the homologous region on the right side was 11.2 kb. . The arrow of the hygromycin resistance gene indicates that the gene is transcribed from left to right. Further, as a marker for selecting a homologous recombinant, a diphtheria toxin gene is linked adjacent to the left homologous region. In targeting vector 1, the second exon to the fifth exon are deleted.

Isolation of homologous recombinant ES cells Transfection of targeting vector 1 was performed as follows. 20 μg of linearized targeting vector 1 per ⁷ × 1 × 10 ⁷ ES cells E14.1 strain was transfected by electroporation under conditions of 500 μF and 250 V for 1 week in ES cell medium supplemented with 140 μg / mL hygromycin After culturing, ES cells incorporating the targeting vector 1 were selected. In cells in which homologous recombination has not occurred between the chromosomal DNA and the DNA of the targeting vector 1 in the homologous region between the hygromycin resistance gene and the diphtheria toxin gene, the diphtheria toxin gene is expressed and the cell is killed. In many cases, the frequency of homologous recombination increases in colonies of ES cells resistant to hygromycin. Indeed, the inventors' group experience yields homologous recombinant clones with a frequency of 1-4% of the selected ES cells.

  1099 clones of hygromycin-resistant ES cells introduced with the targeting vector 1 were isolated and confirmed by Southern blotting to determine whether homologous recombination had occurred. None of the clones had undergone homologous recombination. It was.

Structure of Targeting Vector 2 FIG. 2 is a schematic diagram showing the structure of targeting vector 2 and the structures of wild-type chromosomal DNA and homologous recombinant DNA corresponding thereto. For the targeting vector 1, a hygromycin resistance gene was used as a marker for selecting ES cells incorporating the targeting vector 2, and the homologous region on the left side was 3.2 kb and the homologous region on the right side was 4.8 kb. . Further, as a marker for selecting a homologous recombinant, a diphtheria toxin gene is linked adjacent to the left homologous region. In targeting vector 2, the second exon and a part of the third exon are deleted.

Isolation of homologous recombinant ES cells Transfection of targeting vector 2 was performed in the same manner as targeting vector 1. 749 clones of hygromycin-resistant ES cells introduced with the targeting vector 2 were isolated and confirmed by Southern blotting whether homologous recombination had occurred. However, none of the clones had undergone homologous recombination. It was.

Structure of Targeting Vector 3 FIG. 3 is a schematic diagram showing the structure of targeting vector 3 and the structures of wild-type chromosomal DNA and homologous recombinant DNA corresponding thereto. As the targeting vector 3, a neomycin resistance gene was used as a marker for selecting ES cells incorporating the targeting vector 3. The homology region on the left side was 5.5 kb, and the homology region on the right side was 2.7 kb. Further, as a marker for selecting a homologous recombinant, a diphtheria toxin gene is linked adjacent to the right homologous region. In the targeting vector 3, a part of the second exon, the third exon and the fourth exon are deleted, and encoded such that green fluorescent protein (EGFP) is expressed instead of the IL-1 type II receptor protein.

Isolation of homologous recombinant ES cells Transfection of targeting vector 2 was performed in the same manner as targeting vectors 1 and 2, except that 300 μg / mL G418 was added to the ES cell medium instead of hygromycin. . 1150 clones of G418-resistant ES cells into which the targeting vector 3 was introduced were isolated, and it was confirmed by Southern blotting whether homologous recombination occurred. Here, genomic DNA digested with BamHI was separated by agarose gel electrophoresis and copied to a solid phase, and a KpnI-PstI fragment (about 360 bp) existing 3 ′ downstream of the fifth exon was used as a probe. The mutant can obtain a signal at about 7.0 kb with respect to the type of about 10.5 kb (FIG. 4). Of the 1150, only one 7A1 clone was a homologous recombinant.

Production of ES cell chimeric mouse A 7A1 clone having a mutation at the IL-1 type II receptor locus was prepared according to a conventional method using an agglutination chimera method. That is, an 8-cell embryo obtained by mating a BDF1 male mouse and a C57BL / 6J female mouse and 5-15 ES cells were contact-cultured overnight in M16 medium (Sigma) to obtain a chimeric blastocyst. After formation, chimeric mice were born by transplanting into the uterus of ICR female mice on the third day of pseudopregnancy treatment. Male chimeric mice showing a contribution ratio of 70% or more ES cells as judged by hair color were mated with female C57BL / 6J mice, and a germline transmission test was performed. For wild-colored offspring mice that are derived from ES cells, DNA is extracted from the tail, and whether or not the target locus (locus having a deletion and insertion by homologous recombination in the IL-1 type II receptor gene) is included in the PCR method And confirmed by Southern blotting. Mice having the target locus were backcrossed (8 generations in the C57BL / 6J system and BALB / cA system) and used for analysis.

Phenotype of IL-1 type II receptor gene-deficient mice IL-1 type II receptor gene-deficient mice are born according to Mendel's law in both C57BL / 6J and BALB / cA genetic backgrounds. There was no abnormality. Moreover, unlike IL-1Ra gene-deficient mice, autoimmune diseases such as rheumatoid arthritis and psoriasis-like dermatitis were not observed with aging. In addition, in IL-1 type II receptor gene-deficient mice, a phenotype indicating that the decoy receptor for IL-1 ligand has disappeared has not been recognized at present.

Contact-type hypersensitivity model by hapten application A contact-type hypersensitivity (CHS) model by application of hapten, which is known to be involved in exacerbation of IL-1 signal, was performed on IL-1 type II receptor gene-deficient mice. 2,4-Dinitrofluorobenzene (DNFB) or 2,4,6-trinitrochlorobenzene (TNCB) was used as a hapten for immunization. Two days after shaving, 50 μL of DNFB dissolved in 0.5% or TNCB dissolved in 3.0% was applied to the abdomen of the mouse. At this time, a mixed solution of olive oil (Wako): acetone (Nacalai) = 1: 4 was used as a solvent. Five days after immunization, 25 μL of 0.2% DNFB or 1.0% TNCB was applied to one pinna of the mouse, and inflammation was induced by applying only the solvent to the other pinna. 24 hours after the second hapten application, the left and right auricles of the mouse were cut with a punch having a diameter of 6 mm, and the weight difference was measured.

[Swelling of pinna (mg)] = [Weight of pinna to which hapten was applied (mg)]
-[Auricular piece weight (mg) coated with solvent].

  The result of CHS model allergic reaction by DNFB application is shown in FIG. 5A, and the result of CHS model allergic reaction by TNCB application is shown in FIG. 5B. As shown in FIG. 5A and FIG. 5B, in the IL-1 type II receptor gene-deficient mice, the onset of contact hypersensitivity due to hapten application was suppressed.

Confirmation of IL-1 type II receptor gene expression It was confirmed that the IL-1 type II receptor gene was expressed in wild type mice in the CHS model allergic reaction. The mouse auricle in which CHS was induced was homogenized in Sepazol RNAI Super (Nacalai), mixed with chloroform, and the aqueous phase from which RNA was extracted was collected. From this, RNA was purified using 100% isopropanol and 75% ethanol. This RNA was reverse transcribed using SuperScript (trademark) First-Strand Synthesis System for RT-PCR (Invitrogen) to obtain cDNA. Using this as a template, the expression level of IL-1R2 mRNA was examined using the RT-PCR method. Primer sequences used for PCR were IL-1R2 (Forward Primer; 5′-CTG GAA GGT GAA CCT GTG GT-3 ′ (SEQ ID NO: 1): Reverse Primer; 5′-CAT TTG CTC ACA GTG GGA TG-3 ′ (SEQ ID NO: 2)), Gapdh (Forward Primer; 5′-ACC ACA GTC CAT GCC ATC TCT GCC A-3 ′ (SEQ ID NO: 3): Reverse Primer; 5′-TCC ACC ACC CTG TTG CTG TAG TCG '(SEQ ID NO: 4)). Takara Ex Taq (Takara) was used as the thermostable DNA polymerase. The conditions for the PCR reaction were incubation at 94 ° C. for 2 minutes, followed by reaction for 35 cycles (94 ° C. for 15 seconds, 58 ° C. for 30 seconds, 72 ° C. for 30 seconds), followed by 10 minutes at 72 ° C. The test was performed under the condition of incubation for 1 minute.

  As shown in FIG. 6, as a result of IL-1 type II receptor gene expression analysis by RT-PCR method, in wild type mice, expression of IL-1 type II receptor gene was enhanced during the CHS model allergic reaction by DNFB application. However, no IL-1 type II receptor gene expression was detected in mice lacking the IL-1 type II receptor locus.

  The IL-1 type II receptor has been thought to suppress IL-1 stimulation as a decoy receptor. Thus, it was predicted that IL-1 type II receptor gene-deficient mice could not suppress IL-1 stimulation and thus allergic reactions were exacerbated. However, as shown in FIG. 6, in the CHS model allergic reaction, although the IL-1 type II receptor gene is not expressed at all, as shown in FIGS. 5A and 5B, in the IL-1 type II receptor gene-deficient mice, Allergic reactions were suppressed more than wild type mice. This is a result contrary to the conventional prediction.

IL-1 type II receptor gene-deficient mice as new IL-1 signal analysis tools Analysis using conventional gene-deficient mice reveals that IL-1 alpha signal is important for CHS exacerbation (Nakae et al., Int. Immunol. 13: 1471-1478 (2001)). Recently, in fibroblasts derived from scleroderma patients, pre-IL-1 alpha present in the nucleus is involved in induction of expression of IL-6 and the like. At this time, pre-IL-1 alpha is IL-1R2. It was reported that it functions as a transcription factor by forming a complex with (Kawaguchi, Y et al., Proc. Natl. Acad. Sci. USA, 103: 141514-1506 (2006)). . Therefore, CHS, which is an IL-1alpha-dependent / IL-1beta-independent allergy model, is involved in the exacerbation of a new concept, pre-IL-1alpha / IL-1 type II receptor signal. It was suggested that

  When IL-1 is searched by PubMed (http://www.ncbi.nlm.nih.gov/sites/entrez?db=PubMed), which is a medical / biological literature database published by NCBI, 2008 As of January of this year, 43,014 papers are hit, and this is a very high-profile molecule. In addition, biologics targeting the IL-1 system (eg, Anakinra) have also been put into practical use as therapeutic agents for immune diseases. From these facts, it is considered that the IL-1 type II receptor gene-deficient mouse is a valuable genetically modified mouse that is extremely useful and necessary as a signal analysis tool for IL-1.

The schematic diagram which shows the structure of the targeting vector 1, and the structure of homologous recombinant chromosomal DNA by this. The schematic diagram which shows the structure of the targeting vector 2, and the structure of homologous recombinant chromosomal DNA by this. The schematic diagram which shows the structure of the targeting vector 3, and the structure of homologous recombinant chromosomal DNA by this. The Southern blot figure which confirms the variation | mutation in the IL-1 type II receptor locus by the targeting vector 3. FIG. The bar graph which shows that the CHS model allergic reaction by DNFB application | coating is not seen in the pinna of an IL-1 type II receptor gene deletion mouse | mouth. The bar graph which shows that the CHS model allergic reaction by TNCB application is not seen in the pinna of the IL-1 type II receptor gene deficient mouse. Electropherogram of RT-PCR product showing IL-1 type II receptor gene expression in CHS inflammatory sites.

Claims (4)

  A deletion mutant mouse of an IL-1 type II receptor gene, characterized by having a deletion and / or insertion mutation at an IL-1 type II receptor locus on a mouse chromosome.   [2] The mutant mutant mouse of IL-1 type II receptor gene according to claim 1, wherein the mutation expresses green fluorescent protein instead of full-length IL-1 type II receptor protein.   A step of immunizing a mouse IL-1 type II receptor protein to the mouse according to claim 1 or 2 to produce a monoclonal antibody against said receptor protein; and said monoclonal antibody is derived from a wild type mouse or a wild type mouse. A method for producing an antibody preparation for treating allergy and / or inflammation, which comprises the step of screening a monoclonal antibody that is administered to immune cells and suppresses stimulation of the immune system by IL-1.   Allowing IL-1 to act on IL-1 type II receptor or a cell expressing the receptor in the presence or absence of a test substance, and binding of IL-1 type II receptor to IL-1 A method for screening an anti-allergic drug or anti-inflammatory drug candidate.