JPH09502346A - Use of myelin oligodendrocyte glycoprotein and its peptide moieties in protocols associated with autoimmune disease - Google Patents

Abstract

  (57) [Summary] The present invention provides a nucleic acid molecule having a nucleotide sequence encoding human MOG, an autoantigen associated with demyelinating autoimmune disease. The present invention also provides recombinantly produced human MOG or antigenic fragments. The antigenic fragment of MOG that can be prepared synthetically represents the T-cell epitope of human MOG. Human MOG and fragments thereof are useful in diagnosing and treating autoimmune diseases. Also disclosed are methods of screening for autoimmune diseases and developing therapeutic agents useful in their treatment.

Description

Detailed Description of the Invention Myelin oligodendrocyte glycoprotein in a protocol associated with autoimmune disease Use of quality and its peptide moietiesTechnical field   The present invention relates to self-antigens and epitopes related thereto. More specifically The present invention provides myelin oligodendrocytes useful for the diagnosis, treatment, and prevention of autoimmune conditions. Glycoglycoprotein (MOG) and its peptide domain. Besides, autoimmune disease Also disclosed are methods of screening for patients and developing therapeutic agents useful in their treatment. Is done.Background technology   Autoimmune diseases represent a significant human health challenge and are not well understood. Not in. There are no obvious direct causes of microbial or viral factors. Therefore, the prevention, treatment, and diagnosis of such diseases is based on the etiology of the disease. There is a need. Its etiology usually involves endogenous metabolic intermediates, structural components, and cells. A complex series of reactions such as is involved. However, due to the nature of autoimmune conditions, At least one self-antigen is involved in triggering a series of events that The notion that it must bring about the symptoms is implied. For example of multiple sclerosis Such an autoimmune demyelinating disease is not an example. Multiple sclerosis has medium T lymphocytes It is an autoimmune disease that destroys central nervous system myelin. Multiple sclerosis affects western countries Is the most common cause of neurological disorders associated with illness.   A commonly used animal model for multiple sclerosis is the experimental allergic brain Myelitis (EAE), which is, for example, the use of whole brain homogenates. It is possible to induce in the guinea pig by giving. Demyelinating disorders of the central nervous system Affected EAE is induced by myelin basic protein (MBP) in mice And is already accepted as a mouse model of human multiple sclerosis. In the art, EAE is an MBP and a complete Freund. It is well known that it can be induced by immunization with an adjuvant. That Immunized animals present with the symptoms of EAE, which include paralysis and for a time For example, but not limited to death. MBP is related to human multiple sclerosis It is a linked autoantigen, and research into it is ongoing. However, this Continued research into other factors and other autoantigens that may contribute to disease (Immunology, 2d Ed. J. Kuby, (1994)   p. 451-457).   Myelin oligodendrocyte glial glycoprotein (MOG) The first clear indicator of self-antigen was Lebar, R .; et al. (J. Immun ol (1976) 116: 1439-1446). This study EAE Guinea Pig Serum IgG2 Antibodies Cause Serum Complement Dependent Demyelinating Activity The results of the identified studies were reported. Suitable antibodies are Central Nervous System (CNS) Mieri Reacted with a hypothetical autoantigen present in the homogenate of the protein. This self-antigen is CN It has been shown that S-myelin differs from the encephalitis-inducing basic protein (BP).   In subsequent papers, this known antigen, designated M2 there, is referred to as surface antigen. Have been previously identified, and CN of mouse, rabbit, rat, cow, and human It has been detected in S tissue as well as in guinea pigs. Lebar, R .; et a l. , J Exp Immunol (198 6) Yet another study, published as 66: 423-443, showed that M2 was 27 And two bands at 54 Kd, and these bands are glycoproteins There is a report. Monoclonal antibodies hypothesized to be M2-specific It is also reported in this paper.   1987 paper (Linington, Cand Lassman, H .;   J. Neuroimmunol (1987) 17: 61-69) , Where the role of M2 called MOG has been partially elucidated. In the rat In vivo demyelinating activity of serum was found to be associated with this anti-MOG antibody titer Was. The authors found that antibodies to MOG were in this case chronic relapsing EAE. Have been implicated in the pathogenicity of the model. Another by this group Studies have been conducted by Lassmann, H .; et al. Acta Neuropath ol (Berl) (1988) 75: 566-576, reported a year later. And the related phenomena in the EAE model have been further elucidated. This study Determine the association between anti-MOG antibodies and large numbers of T cells, and the nature of the observed symptoms. It is shown when setting. Kerleio de Rosbo, N .; et al. Further papers by J Neurochem (1990) 55: 583-587. In a monoclonal antibody against MOG in aggregating brain cell cultures. It has been shown to induce demyelination. Piddelsden, S .; et al . Clin Exp Immunol (1991) 83: 245-250, A study was conducted that the importance of complement activation was significant in the course of EAE.   Sun, J. et al. et al. J Immunol (1991) 146: 14. 90-1495 studied MS directly in patients, and B cells and And T cell responses to both MOGs were evaluated. This paper describes T cell response to MOG. The answer establishes that it is class II-restricted and that MOGs in multiple sclerosis It was confirmed to be an important antigen.   Purified mouse MOG showed a faint band of 53 Kd on SDS-page immunoblot. It was shown to run as a 26-28 Kd double band with thieu, J .; -M. And Amiguet, P .; Dev Neurosc i (1990) 12: 293-302. Amiguet, P. et al. J. Neurochem (1992) 58: 1676-16. 82 is a 25 Kd peptide with a single chemical and enzymatic deglycosylation of mouse MOG. It has been shown to bring petite. Therefore, this monomeric form of mouse MOG is 25 This is the amino acid sequence of kd. This article further adds to the first N-terminus of the mouse protein. It also discloses about 26 amino acids. Gardinier, M .; V. et al . J. Neurosci Res (1992) 33: 177-187 are some Rat MOG cDNA was isolated and the mouse MOG N-terminal peptide sequence was isolated. Their homology was confirmed by comparison with rows.   The rat cDNA obtained by Gardinier (supra) has 27 amino acids. Acid hypothetical signal peptide followed by the equivalent of 24,962 daltons It has an open reading frame encoding a mature 218-amino acid MOG peptide with a large abundance. Was. The N-terminal amino acid sequence obtained for this mouse protein is rat It was similar to that deduced from the cDNA.   The present invention is directed to recombinant materials for the production of human MOG proteins, as well as whole amino acids thereof. No acid sequence is provided. Using this information, the MOG protein Can determine useful peptides that represent a portion of the amino acid sequence of the MOG protein. Is possible, and they are diagnostic and therapeutic for demyelinating autoimmune disease in humans Useful for. Moreover, for screening for autoimmune diseases and its treatment Also disclosed are methods of developing the composition.Disclosure of the invention   The present invention relates to the entire amino acid sequence of human MOG protein (SEQ ID NO: 2), and its Recombinant material for the production of proteins and fragments thereof is provided. Knowledge of amino acid sequence See, those peptide moieties that are also useful in the diagnosis and treatment of autoimmune diseases Enable the design of.   Accordingly, in one aspect, the invention provides, optionally, recombinantly produced isolated And purified human MOG protein, and fragments thereof, which are demyelinating autologous It regulates the process of symptom development in autoimmune diseases. In another aspect, the invention features a MOG Recombinant material and method useful for producing protein or peptide portion thereof . In yet another aspect, the invention provides an agent for alleviating the effects of demyelinating autoimmune disease. Compositions and methods of their use.   In another aspect, the invention provides that conservative substitutions have already been made and are naturally occurring. Isolation and purification of T-cell epitopes of MOG proteins and peptides It relates to manufactured human MOG proteins and peptides.   In yet another aspect, the invention provides a screen for demyelinating autoimmune disease, comprising: Multiple sclerosis in rabbits and mammals, preferably humans, can be diagnosed, prevented, or treated. Development of methods for the identification of therapeutic compositions comprising a competent MOG or fragment thereof To show.Brief description of the drawing   FIG. 1 shows the entire nucleotide sequence of the DNA encoding the human MOG protein (SEQ ID NO: No. 1) and the deduced amino acid sequence (SEQ ID NO: 2) are shown.   FIG. 2 shows the peptides useful in the present invention in the form of amino acid sequence (SEQ ID NO: Nos. 4-9, 11, 15, 16 and 42-72).   FIG. 3 shows the defined positions on the peptide that bind to the DR4 MHC class II product. It is a table which shows the influence of each natural amino acid.   FIG. 4 shows 12 peptides that bind to the MHC class II product of DR4 (SEQ ID NO: IC about 19-32)₅₀3 is a table showing a comparison between the expected value and the measured value of FIG.   Figure 5a corresponds to SEQ ID NOs: 73-93 and is useful for the present invention (20 Is shown by the amino acid sequence.   Figure 5b shows human MOG1-121 containing at least one T-cell epitope. Is shown by the amino acid sequence.   FIG. 6 is a bar graph of the data from Example 3, where the X-axis is 4 Wells containing two different cell lines are shown, with seven peptides tested in separate legends , And the Y-axis represents counts per minute, in this case Data for 3H-thymi incorporated by each cell line in response to each individual peptide. Represented as gin (CPM).Mode for Carrying Out the Invention   The present invention encodes human MOG, an autoantigen for demyelinating autoimmune disease Nucleic acid sequences are provided. The present invention is further useful in modulating the autoimmune response A peptide representing a subunit of human MOG encoded by the nucleic acid molecule of the present invention I will provide a. Generally at least 12-1 These subunits, which contain as few as 3 amino acids, have the Cell epitope region.   The etiology of the onset of symptoms of autoimmune diseases such as multiple sclerosis is unclear. Though distant, certain events are thought to be important for the progression of this condition Can be Demyelinating autoimmune disease is associated with attack by the immune system on the myelin sheath Bring the equivalent of a short circuit in the nervous system. Attack by the immune system on T-cells More mediated. In this case it is a human MOG autoantigen that is part of myelin The response of T-cells to specific antigens is the uptake of antigen by antigen presenting cells and Subsequent proteolytic cleavage, as well as the class II major histocompatibility gene complex (M Presentation of antigens associated with HC-encoding proteins, which are recognized by T-cells. To make it possible). Therefore, the T-cell epitope region of the self-antigen is , A region displayed by class II MHC proteins to T-cell receptors . Related T-cells are by providing the T-cell epitope region of the autoantigen It is possible for multiple protocols to become non-responsive in an antigen-specific manner. This will be described in more detail below.   One embodiment of the nucleic acid sequence encoding human MOG is deduced from the amino acid sequence (sequence). It is shown in FIG. 1 (SEQ ID NO: 1) together with column number 2). 2 encoded mature proteins It contains 18 amino acids, and full-length protein (including signal peptide) is rat MOG 87% homology with protein. As described above, the predicted amino acid sequence of human MOG The utility is their peptide fragments that induce an immune response in mammals, as well as T- Design peptide fragments that are cellular epitopes, ie, for T-cell receptors More recognized Provides the opportunity to build those parts of the child. These peptides and fragments Beams are included within the scope of the present invention.   A vector containing a nucleic acid sequence encoding human MOG (PVL1393, Phar Mingen, CA) was transformed into host cells on September 8, 1994. Deposited to the Merchant Type Culture Collection And has received accession number 75554.   However, the scope of the present invention is encoded by the amino acid sequence set forth in FIG. Human MOG protein or the specific nucleic acid sequence displayed Absent. Naturally occurring variants, as well as for altering the nucleic acid sequence itself. The present invention also contemplates deliberate mutants designed to alter the encoded protein. Within the scope of which the details are described below. Regarding naturally occurring variants Does not affect DNA sequence polymorphism, especially the amino acid sequence of human MOG "Silent" suddenly affects sequence polymorphism and induces amino acid sequence changes Those responsible for the mutations are expected to be present in the human population. Code MOG One or more nucleotides of the sequence to be sequenced (up to about 1% of the nucleotides) These variants in are the result of natural allelic variants. Like this Any and all of the cleotide and resulting amino acid polymorphisms are within the scope of the invention. Contained within. Moreover, disclosed herein in terms of function and amino acid sequence. It is related to the MOG encoded by DNA but encoded by separate genes. There may be one or more “family members” of the MOG. Such family members are also human MOGs and the nucleotides that encode them. Distribution Included in the column definition.   Isolated and immunologically related to human MOG or fragments thereof The self-antigen protein or a fragment thereof (excluding those already identified) is the present invention. Included in the range. These are antibody cross-reactivity or T-cell cross-reactivity. Can be identified by Such a protein or a fragment thereof is the present invention Binding to an antibody specific to the protein or peptide of Stimulate T-cells specific for quality or peptide.   An "antigenic fragment" is an amino acid that has fewer amino acid residues than the complete protein. Acid sequence and is a sequence that induces an immune response in mammals, preferably humans. Fragment or peptide, and the immune response includes, for example, IgG and IgM antibodies Production of, or, for example, proliferation and / or lymphokine secretion and / or Or T-cell anergy and / or TH₁And TH₂Subset modification Like the T-cell response. Antigenic fragments containing T-cell epitopes Especially aimed. Peptides can be naturally occurring MOG sequences or conserved amino acids. It is possible to obtain from a peptide that has already been subjected to acid substitution. Each example It is shown in FIG. 2 (SEQ ID NOS: 4 to 9, 11, 15, 16 and 42 to 72).Nucleic acid preparation   A nucleic acid molecule containing a sequence encoding human MOG or an antigenic fragment thereof is a human brain. Or by reverse-transcribed mRNA present in other CNS tissues, as well as genomic DN Can be obtained from A and is most conveniently prepared using standard solid phase techniques It is possible. There are various methods of chemically synthesizing polydeoxynucleotides. It is known that Solid phase synthesis, which is fully automated in commercially available synthesizers such as (Eg, Itakura et a, incorporated herein by reference). l. U.S. Pat. No. 4,598,049; Caruthers et al. , U.S. Pat. No. 4,458,066; and Itakura, U.S. Pat. No. 4,4. 01,796 and 4,373,071). Nucleic acid molecule of the present invention Also includes RNA capable of being transcribed from the DNA prepared as described above.Preparation of human MOG and fragments thereof   The present invention also includes expression systems for the production of encoded proteins and traits in those systems. Transformed host cells are also provided. For example, E. coli (E. FIG.  col i ), Insect cells (baculovirus), yeast, or example For example, like Chinese hamster ovary cells (CHO). Includes mammalian cells. Appropriate host cells, as well as associated promoters, Expression vectors containing hancers and other expression regulators are available from Goeddel, G ene Expression Technology: Methods in   Enzymology 185, Academic Press, San D iego, California (1990). other Suitable host cells and expression vectors are known to those of skill in the art.   Expression in eukaryotic cells such as mammalian, yeast, or insect cells Is the partial or complete glycosylation of the recombinant protein and / or the appropriate chain It is possible to result in the formation of inter- or intrachain disulfide bonds. East S. Cerevisiae (S.  cerevisiaeFor expression in For example, pYepSec1 (B aldari. et al. , (1987) Embo J 6: 229-234. ), PMFa (Kurjan and Herskowitz, (1982) C. 30: 933-943), pJRY88 (Schultz et al. . , (1987) Gene 54: 113-123), and pYES2 (In Vitrogen Corporation, San Diego, CA) included. Vaccum available for expression of protein in cultured insect cells (SF9 cells) The Rovalius vector includes pAc series (Smith et al., (19 83) Mol Cell Biol 3: 2156-2165) and pVL si. Leeds (Lucklow, VA, and Summers, MD, (1 989) Virology 170: 31-39). Generally CO S cells (Gluzman, Y., (1981) Cell 23: 175-182. For the transient amplification / expression in mammalian cells, pCDM8 (Aruffo, A. and Seed, B.H. , (1987) Proc Natl Acad Sci USA 84: 8573-8577). Used, but CHO (dhfr^-  Chinese hamster ovary (Chi NeseHamsterOVary)) cells are stable amplification in mammalian cells / For expression, pMT2PC (Kaufman et al. (1987), EMBO.   J. 6: 187-195). Vector DN A is, for example, calcium phosphate or calcium chloride co-precipitated, DEAE-dex Normal techniques such as stran-mediated transfection or electroporation It can be incorporated into mammalian cells via surgery. Transforming host cells A suitable way to get ambrook et al. (Molecular Cloning: AL Laboratory Manual, 2nd Edition, Cold Sp ring Harbor Laboratory press (1989)), And can be found in reference books for other laboratories.   Those of skill in the art will use various methods of expression, but expression in prokaryotes may be fusion or Using any of the non-fusion inducible expression vectors E. coli (E. FIG.  coli) The most Is also implemented frequently. Fusion vectors usually contain a large number of N's to the expressed target gene. H₂Add terminal amino acids. These NH₂Terminal amino acids are often reporters Cited as a basis. Such reporter groups are usually: 1) the target recombinant protein And 2) act as a ligand in affinity purification. And serve the two purposes of assisting in the purification of the target recombinant protein. Often fusion proteolytic vectors have a proteolytic cleavage site for reporter group and target recombination. The target recombinant protein is separated from the reporter group by being introduced at the junction with the protein. And subsequent purification of the fusion protein is possible. Such enzymes and their equivalents Family recognition sequences include Factor Xa, thrombin, and enterokinase. Typical fusion expression vectors include pGEX (Amrad Corp., Melb). ourne, Australia), pMAL (New England Bi) olabs, Beverly, MA), and pRIT5 (Pharmaci) a company, Piscataway, NJ), which are glutathione S-tiger. Luciferase, maltose E binding protein, or protein A To the recombinant protein.   Inducible, non-fusion expression vectors include pTrc (Amann et al., (1 988) Gene 69: 301-315) and pET11d (Studio). r et al. , Gene Expression Technology; Methods in Enzymology 185, Academic P less, San Diego, California (1990) 60-89. ) Is included. Target gene expression is hybrid trp-lac in pTrc PET while relying on host RNA polymerase transcription from a fusion promoter Expression of the target gene inserted into 11d is the co-expressed viral RNA polymer. T7 gn10-lac0 fusion promoter mediated by Ralase (T7 gn1) Depends on the transcription from the promoter. This viral polymerase is lacUV5 pro From the endogenous g prophage harboring T7 gn1 under the transcriptional control of the motor to host strain B Supplied by L21 (DE3) or HMS174 (DE3).   E. coli (E. FIG.  coliOne approach to maximizing expression in Protein within a host bacterium that has an impaired ability to proteolytically cleave the protein. Expressing white matter (Gottesman, S., Gene Expre. session Technology: Methods in Enzymolo gy 185, Academic Press, San Diego, Cali fornia (1990) 119-128). Another method is for each amino acid E. coli (in which individual codons ofE. FIG.  coli) Preferential within protein Altering the coding sequence of that gene so that it is (Wada et al., (1992) Nuc Acids Res 20: 2111-2118). Such modifications of the nucleic acid sequences of the invention are standard. It could be done by quasi-DNA synthesis techniques.   Recombinant protein or peptide product is secreted during expression of the encoded gene And can be recovered from the medium. Alternatively, this protein Are retained in the cytoplasm, and the cells are harvested and lysed, and the protein It can be isolated and purified. Suitable media for cell culture are known to those of skill in the art. Have been. The proteins and peptides of the present invention are added to a cell culture medium, a host cell, or Techniques known in the art for purifying proteins and peptides from both. Can be purified using techniques such as ion exchange chromatography. -, Gel filtration chromatography, metal affinity chromatography, ultrafiltration, Electroporation and immunoaffinity purification with specific antibodies are included. The term "isolated And "purified" are used interchangeably herein and include recombinant DN Substantially free of cellular material or culture medium when produced by the A technique Peptides, proteins, protein fragments, and nucleic acid molecules, or chemically synthesized Peptide or protein substantially free of chemical precursors or other chemicals, It refers to white matter, protein fragments, and nucleic acid molecules. Therefore, the isolated peptides are Produced recombinantly or chemically and is substantially free of cellular material and culture medium. Free or substantially free of chemical precursors or other chemicals.Antigenic fragments and "antigenic" responses   Fragments of the proteins of the invention that induce the desired antigenic response (herein referred to as antigenic (Interchangeably referred to as a fragment or peptide) is, for example, part of the protein By screening the peptide corresponding to Can be obtained. These peptides use techniques known in the art Chemically synthesized, or produced recombinantly or through proteolysis can do. For example, make sure that the fragments of this protein do not overlap. Optionally split into pieces of desired length, or preferably overlap of desired length It can be divided into pieces. Examine each fragment to determine their antigenicity (Eg, the ability of the fragment to induce an immune response in a mammal). Disconnection of the protein If the strip is to be used for therapeutic purposes, for example, stimulation (ie growth or phosphorus). Can induce a T-cell response, such as (hocaine secretion), and / or T-cell response. Fragments capable of inducing cell anergy are particularly desirable.   When administered to individuals susceptible to demyelinating autoimmune disease, the isolated protein , Or a preferred antigenic fragment thereof, is the individual's B-cell response to its self-antigen. Answer, it is possible to modify the T-cell response, or both the B-cell and T-cell responses Or it can be shown to result in diminished symptoms. In this specification As cited, diminishing symptoms include treatment with the peptides or proteins of the invention. Includes any subsequent reduction of disease states of demyelinating traits. This reduction of symptoms is subjective Can be determined clinically or clinically.   Human T-cell stimulating activity is derived from the self-antigen and / or its self-antigen Culturing T-cells obtained from a subject having an autoimmune condition with the peptide, And whether T-cell proliferation occurs in response to self-antigens and / or peptides Is determined, for example, by measuring cellular uptake of tritiated thymidine It is possible to inspect by doing so. About the response to peptides by T-cells All stimulation indices are control CP It can be calculated as the maximum CPM in response to a peptide divided by M . A stimulation index (equal to or more than twice background level ( S. I. ) Is considered "positive". A positive result is used to identify the group of patients tested. Then the average stimulation index for each peptide is calculated. The preferred pellets of the present invention The peptide contains at least one T-cell epitope and is greater than 1.5 Alternatively, it has an average T-cell stimulation index equal to it. Significant number of patients tested > 1.5 in (ie at least 10% of the tested patients) or Peptides having an average T-cell stimulatory index equal to that are useful as therapeutic reagents Is assumed to be. Preferred peptides are at least 1.5, more preferably less It has an average T-cell stimulation index of at least 2.0-3.0.   Preferred peptides also affect a relatively high percentage of T-cells in some patients They can be identified by their ability. This rate depends on multiple phases from a patient. The same culture is prepared from a limited number of leukocytes and / or autoantigens and / or It is measured by making it using a peptide. The stimulation index ( The positive reactivity with the peptide is analyzed as specified by (described above). Pe Percentage of Ptide Reactive T-Cells Shows a Positive Stimulation Index Percentage of Cultures from Patients It is a tage.   Moreover, preferred peptides are at least about 100, more preferably at least A positive index (P.I.) of about 200, and most preferably at least about 300 Have. The positive index for a peptide is at least for such peptides. Also having a T-cell stimulation index of 1.5, more preferably at least 2.0 In a population of immune patients (eg, preferably at least 15 individuals, more preferred At least 30 individuals Body, or more individuals), average percent T-cell stimulation of individuals It is determined by multiplying by the chemical index. Therefore, the positive index is Intensity of T-cell response (SI) and to peptides in a population of autoimmune individuals Of the T-cell response of both.   The purpose of determining the correct T-cell epitopes, for example by means of subtle mapping techniques Has T-cell stimulatory activity, and is therefore a biological technique for T-cells. A peptide containing at least one T-cell epitope determined by Addition of amino acid residues at either the amino or carboxy terminus of tide Or modified by deletion, and a test is performed to T-target the modified peptide. Determine changes in cell responsiveness. Two if they share an overlapping region in the native protein sequence Or more peptides, as determined by T-cell biological techniques, If it is found to have T-cell stimulating activity, all of such peptides or It is possible to produce additional peptides containing certain moieties, and these Additional peptides can be tested by similar methods. After this technique Peptides are selected and these are produced recombinantly or synthetically. Pe Peptides are selected based on a variety of factors, which are Intensity of T-cell responses (eg, stimulatory index) and its distribution in the autoimmune patient population. Of the T-cell response to the peptides of Those of these selected peptides Physical and chemical properties (eg solubility, stability) have been investigated to determine these peptides. Whether the peptides are suitable for use in therapeutic compositions, or Decide whether you need the modifications described in the book. Selected peptide Is the ability of the selected modified peptide to stimulate human T-cells (eg, For example, proliferation and induction of lymphokine secretion) are determined.   The T-cell epitopes of the invention when administered to a subject in a therapeutic regimen -Containing peptides are capable of modifying that individual's response to self-antigens .   A preferred peptide of the present invention is at least one T-cell epitope of the full length protein. And thus the peptide is at least about 7, preferably at least Also comprises about 12-40, and more preferably 13-30 amino acid residues. this Have a tandemly repeated single epitope and / or more than one epitope. May include loops. For the purpose of therapeutic effect, the preferred therapeutic composition of the present invention. The article preferably comprises at least two T-cell epitopes. Moreover, the invention Therapeutic compositions containing one or more preferred isolated peptides are preferred. Or contains a sufficient percentage of the total protein of the T-cell epitope, The therapeutic regimen of administration of the composition thus results in amelioration of disease symptoms. Less than about 45 Of the present invention, and most preferably less than about 30 amino acid residues A light synthetically produced peptide is particularly desirable because it is a peptide of increased length. This is because it may cause a difficulty in synthesis. The peptide of the present invention has the Can also be produced recombinantly in the field and from 45 or longer amino acids It is preferred that the peptide is recombinantly produced.   Has T-cell stimulating activity, and therefore at least one T-cell epitaxy An isolated antigenic peptide fragment containing a taupe is particularly desirable. An epitope When referring to this epitope, this epitope is specifically referred to as immunoglobulin or histologically synthesized antibody. Receptors that are primordial and T-cell receptors Is the basic element or minimum unit of recognition by the Contains protein amino acids. Also use amino acid sequences similar to those of the epitope It is possible. T-cell epitope is the T-cell receptorbyBasis of recognition This element is the smallest unit, in which case this epitope is responsible for receptor recognition. Therefore, it contains amino acids in essential autoantigens. Similar to natural T-cell epitopes Similar amino acid sequences are also included within the scope of the invention. T-cell epitope It is thought to be involved in the initiation and perpetuation of the autoimmune response. These T-cell epi By being presented by the appropriate HLA molecule on the surface of antigen presenting cells An early event is initiated at the level of T helper cells, which results in the epitope To stimulate T-cell subpopulations using T-cell receptors appropriate for Can be These phenomena include T-cell proliferation, lymphokine secretion, local inflammatory response, anti-inflammatory It also recruits additional immune cells to the original / T-cell interaction site, as well as producing antibodies. It results in activation of the activating B-cell cascade.   Peptide or protein containing at least one T-cell epitope of self-antigen Exposure of the subject to the quality may result in tolerance, anergy, or so to the appropriate T-cell subpopulation. Otherwise, they would cause alterations, rendering them unresponsive to the self-antigen, Then it may not be involved in the intensification of the immune response. Besides, at least one Administration of proteins or peptides containing the T-cell epitopes of May alter lymphokine secretion properties compared to exposure to self antigens (eg, , Leading to a decrease in IL-4 and / or an increase in IL-2₁And T H₂Result in population modification). Moreover, exposure to such proteins or peptides Out Affects T-cell subpopulations that are normally involved in the response to self-antigens , Therefore, these T-cells may have sites (one or more) of normal exposure to self antigens. ) (Eg, CNS tissue) to treat the protein or peptides derived from it. Withdrawal to site (s) of therapeutic administration. T-cell subassembly This redistribution of groups improves or reduces the ability of the individual's immune system to positively self-antigen. It may stimulate the normal immune response at the normally exposed site leading to diminished symptoms. You.   T-cell epitope-containing peptides for particular diseases with which peptide One of ordinary skill in the art will attempt to work in many acceptable ways when determining Will In the present invention, the method chosen is not meant to be limiting. A work One mode of attempting work is to select, for example, a suitable T-subscription from a group of peptides. Cell epitope-identical by other methods by those skilled in the art, such as selecting peptides containing It is not intended to exclude other ways in which the results can be achieved. one Generally, in the present application, certain proteins will be identified as described in more detail herein. Purify and analyze, select peptides for testing, produce selected peptides , And the selected peptides for the characteristic properties of T-cell epitopes. inspect.Human MOG T-cell epitope region   Human MOG-derived pep that modulates a subject's response to MOG self-antigens Tids are also included within the invention. A likely candidate for such a peptide , Parents of candidates that bind the HLA DR protein as discussed above and / or Test for compatibility (The method for obtaining HLA DR protein is described in "HLA DR Purification and analysis of DR protein " Discussed in detail below) and its effect on T-cell proliferation. Can be inspected. Such peptides are for example B-cells and / Or produced as a peptide to be investigated for its ability to influence T-cell responses. Investigating the structure that should be produced and selecting the appropriate region (recombinant gene Via the current system, synthetically or otherwise), as well as these cells Identification by selecting a peptide containing an epitope recognized by Can be. One way to identify such peptides is to bind the human MOG protein. Divide the raw material into non-overlapping or overlapping peptides of desired length, and Of each peptide were synthesized, purified, and tested to ensure that each peptide Whether it also contains one T-cell epitope using any number of assays. Includes setting. Other methods use algorithms to predict these peptides. Rhythm is used. Other methods known to those skilled in the art can also be used. You. In the present application, certain of these peptides are referred to herein as The algorithm was selected in the manner discussed in detail.   37 naturally occurring 13-mers (3 analogs of naturally occurring peptides 2) (with SEQ ID NOS: 4-9, 11, 15, 16, and 42-72). But the length of the amino acids is arbitrarily chosen. These peptides are optimal for MHC Selected according to an algorithm that predicts Russ II binding. Appropriate that peptide For the purpose of being able to bind to various T-cell receptors, it is a class II MHC It is essential that it be able to bind to proteins. Each N- and / or C-terminus From which 1-2 amino acids have been removed and still maintain MHC binding activity. To be It is possible. These peptides are represented by amino acid sequence and are shown in Figure 1 The display region within the mature amino acid sequence shown as positions 1-218 of column No. 2) is Represent. These subunit peptides bind to class II MHC proteins. Characterized by their ability and therefore effectively presented as T-cell epitopes Competence (Rothbard, et al., The EMBO Jour nal 7: 93-100, 1988). Of binding to class II MHC proteins The essential (but not necessarily sufficient) conditions for are eg glycine, alanine 4-amino acids from small amino acid residues such as, serine, threonine, or cysteine. Hydrophobic side chain residues separating the mino acids, preferably tyrosine, phenylalanine , Or the presence of tryptophan residues, and isoleucine, leucine The presence of valin, valine, or methionine residues is less desirable. Figure 2 (Sequence number No. 4-9, 11, 15, 16, and 42-72). Chid meets these minimum requirements. As further shown in FIG. 2, these peptides All of them bind to the MHC protein encoded by the given allele. Already tested for abilities. IC in the figure₅₀These, as indicated by the values Most of the peptides in DRB1 * 0101 and DRB1 * 1501 Binds tightly to both. The specificity of peptide binding is described belowInhibition I It is included in the item about. FIG. 2 is a typical example of an algorithm for selection. Are intended, and these are very useful. However this is all It does not include the presence of other potentially useful antigenic peptides. This is because it has the potential.   It was used as a reference to identify peptides as described in the previous section. The need for a four amino acid spacing between the hydrophobic residue and the small residue that is shown is demonstrated in the experiments below. Has already been demonstrated using a dynamic protocol: experiments of this design have Bind to nearly homologous positions in an orientation that interacts with the peptide backbone, and It is assumed that a conformation related to the tangent is applied. The experiment of this design is MHC Dividing the binding site of a class II molecule into individual subsites that specifically contribute to binding. And the overall free energy of binding is Is the total of the beneficial and harmful contacts that form in each pocket, and within each pocket We also assume that it is possible to observe interactions between peptides independently. I was The results of this experiment show these hypotheses, as well as the main chain interactions in the side chains. A model of binding free energy as a simple polynomial with individual conditions for I support. For peptides of general length, the main chain conditions are constant. On the other hand, the side chain contributions are due to their structure as well as the chemical pairing of complementary pockets at the binding site. Will vary depending on performance and size. The relative importance of the position of each side chain Peptides are common, although they may vary depending on the upset and isotype Binding can be observed as the sum of the individual and independent decreases.   Therefore, the results of Applicants' experiments show that the apparent parents of any sequence of common length are Compatibility is a database of relative effects of natural amino acids at each position of a model peptide. Predict within a factor of 2 or 3 of experimentally determined values based on be able to. Simplified peptide, AAYAAAKAAAAAAA (SEQ ID NO: 33) Synthesize all possible mono-substituted analogs at 11 central positions in Assay for binding to B1 * 0401 (formally referred to as DR4DW4) did. Each analog IC to be measured₅₀From the values, the ratio for the parental simplified peptide was calculated. this The ratios and measured values are shown in FIG. After that, using these ratios, Peptides known to bind to DRB1 * 0401 with a wide range of affinities Affinities of 12 unrelated native sequences (SEQ ID NOs: 19-32) corresponding to . The data shown in Figures 3 and 4 show that this model predicts a four amino acid spacing. It is proved that it is useful to do and is consistent with the experimental result. This model When used, the 13-mer candidate is likely to be a T-cell epitope-containing peptide. And then selected.Purification and analysis of HLA DR protein   For detergent solubilization and affinity purification of HLA-DR (human HMC protein) molecules The method used in Gorga (J. Biol. Chem. 262: 1608). 7-16094, 1987) and Bulow (Eur. J. Immunol). . 23: 69-76, 1993). Concise Describes the DRB1 * 0101 and DRB1 * 1501 alleles. CHO cells transfected with all genes (Marshall et al. l. J. Immunol. , 152: 4946-4957, 1994). 0% heat-inactivated fetal calf serum (FCS), 2 mM glutamine, and antibiotics Were grown in RPMI 1640 medium supplemented with. Collect cells and PBS Washed in 1%, lysed with 1% NP-40, and the supernatant was centrifuged by centrifugation. Separated from debris. The solubilized MHC class II protein was treated with sepharose (S epharose) using the monoclonal antibody LB3.1 conjugated to CL4B Affinity purified. Class II protein 1% octyl-β-D-glucopyranoside (octylglucoside), 50 m Elute with 1M phosphoric acid (pH 11.5) and immediately add 1M phosphoric acid (pH 6. It was neutralized with 0). The purified αβ heterodimer was purified from Bio-Gel A0.5. Isolated by size exclusion method using a 60 cm x 2.5 cm diameter column. this Fractions containing the heterodimer were collected from Amicon Centri-Prep ™ 30. The device was used to concentrate to a nominal concentration of 500 μg / ml.   The purity of this substance is as described above (Buelow et al., 1993), SDS-PAGE, high performance size exclusion chromatography (HPSEC), and Assayed by the Edman sequencing method. This HPSEC color Is a BIOSEP SEC-S3000 (300 x 7.5 mm) (Phenom E.g.) with 1.0% octyl glucoside and 1.0% acetoni. A flow rate of 0.800 ml / min using a PBS buffer system containing trill (approx. It was eluted in 25 minutes). Install a fluorescence detector to monitor the fluorescence of tryptophan Done (λ_ex= 282 nm, λ_em= 348 nm).Inhibition assay   The peptide binding assay was performed as previously described (Hill et al., 1). 994). Briefly, affinity-purified class II protein (10 nM) 1 in 96 well polypropylene plate (Coster) at pH 6.5 . Serial dilutions of test peptide in PBS containing 0% octyl glucoside And 16 hours with a fixed concentration of biotinylated HA 307-319 (2 nM) Incubated at 37 ° C. Double test of DR-peptide complex (50 μL) For, monochrome 96-well microtiter pre-precoated with null antibody LB3.1 Of each well and blocked with fetal bovine serum. Excess peptide is 0 . 02% Tween 20 and 0.05% NaN_ThreeWashing with PBS containing To remove. Europium-labeled streptavidin (Pharmaci) a) was added and incubated overnight. After washing, 0.1% Trit on X-100, 15 μM 2-naphthyltrifluoroacetone, and 50 0.1M acetate / phthalate containing pM tri-N-octylphosphine oxide A solution of a buffer solution (pH 3.2) was added to chelate the user from streptavidin. Ropium was dissociated. The resulting fluorescence, which is bound to biotinylated HA 30 7-319 proportional to the amount of fluorescent plate measuring instrument (DELPHIA LKB / (Pharmacia). This data is used to identify specific class II proteins Fit this data to the binding function to calculate the concentration of test peptide that binds to the protein. It was analyzed by₅₀Grade by value It is possible that lower values correspond to better binding peptides. .T-cell assay used to mimic MOG epitopes   The T-cell assay was performed to further identify the T-cell epitopes. Was. Peripheral blood lymphocytes were identified from human volunteer HLA-DR2-positive donors. Isolated using the technique outlined in the detailed example 2 Selected for inspection MOG peptides are: Met. Results of one such study of T-cell responses to human MOG peptides Will be explained in FIG. This result shows that MOG1-13 (SEQ ID NO: 42) is on the boundary line. It was described and indicated to be a T-cell epitope-containing peptide. That The above identical data indicates that at least one MOG 103-115 (SEQ ID NO: 55) It strongly suggested that it contained an epitope. Moreover, these results are overall Peptides below the 13-mer are T-cell epitope-containing peptides It does not rule out the possibility of being able to do it.   In addition, humans with multiple sclerosis Patient T-cell responses are discussed in Example 4, where MOG peptide (2 A mixture of 0 amino acids in length and shown in Figure 5a) has multiple sclerosis ( A small number of self-antigens responsible for multiple sclerosis It was found to contain at least one T-cell epitope. Besides these conclusions In the fruit, the peptides with less than 20-mers are T-cell epitope-containing peptides. We do not rule out the possibility of being able to become.   The structure of the protein or peptide of the present invention may be Or preventative efficiency, or stability (eg, ex vivo shelf life, and And resistance to proteolytic degradation in vivo). , Otherwise generally conservative substitutions and It can be modified by modification methods. For example, amino acid substitutions, deletions, or A modified protein or peptide whose amino acid sequence has already been changed by the addition of Produced to modify immunogenicity, or a component is added in advance for the same purpose. It is possible to produce what has been added. Figure 2 shows three such Minoic acids human MOG 70-82, A78 (SEQ ID NO: 8); human MOG74 -86, A78 (SEQ ID NO: 53); and human MOG88-100, K89, S. 98 (SEQ ID NO: 9) is shown.   Modification is in a manner such that the ability to recognize the appropriate T-cell subset is unchanged. Needs to be done in. In the art, which position of the amino acid side chain is in the APC A general understanding of what is oriented on the top surface and which is inward Have been. What is inward is a good candidate for modification, which is They are unlikely to affect binding to proper T-cell receptors This is because it is clear that   Certain embodiments of the invention include at least one T-cell epitope of the protein. , And shown in Figures 2, 5a, and / or 5b for T-cell receptor binding. Containing a region of a peptide of particular importance, or modifications thereof described above Modified form (possibly with unrelated amino acid sequences at the N- and / or C-termini) Has been stretched).   Another aspect of the invention is the inclusion of at least two T-cell epitopes as described above. Providing a peptide comprising. These T-cell epitopes can be homologous Or can be a different T-cell epitope suitable for human MOG You. This, as described in more detail above These T-cell epitopes are typically at least 7 amino acids, preferably 12 amino acids. -40 amino acids, and even more preferably 13-30 amino acids in length. Place If desired, the amino acid sequence of the T-cell epitope may be linked to a linker , It is possible to increase the sensitivity to processing by antigen presenting cells. Such a linker may be any non-epitope amino acid sequence, or other suitable It can be any binder or linking agent. At least two T-cells In a preferred peptide containing a pitope, these epitopes are native human MOGs. A conformation identical or different to the naturally occurring conformation of the epitope in the protein Align with. For example, T-cell epitope (s) may be contiguous or Can be aligned in non-adjacent conformations. Non-adjacent is an epitope A sequence of T-cell epitope (s) containing additional residues between Is determined. Moreover, these T-cell epitopes are arranged in a non-contiguous order. (E.g., its T-cell epitope (s) may be Order different from the order of amino acids in the resulting natural protein). The peptide of the present invention Is at least 10%, at least 20%, at least 30%, at least 40% , At least 60%, or more, of human MOG T-cell epitopes Can be included.   Preferred peptides include two or more of the T-cell epitopes discussed above. Including various combinations of the above. Two or more epitopes The preferred peptides containing the combination of 4-9, 11, 15, 16, and 42-72), in Figures 5a and 5b. Containing sequences selected from It is.   The protein or peptide of the present invention has the ability to induce T-cell unresponsiveness. And / or a strong response when administered in an immunogenic form Modified to bind to MHC proteins without the ability to induce a proliferative response It is possible to In this case, a critical consequence for T-cell receptor function is Compatible residues are known in the art (eg, substitution of each residue, and also the presence of T-cell reactivity). Or the determination of non-existence). T-cell receptor These residues found to be essential for interaction with Acids do not induce acids, although their presence makes T-cell reactivity more or less likely. Other residues known to exist, preferably similar amino acid residues (conservative substitutions) It can be modified by substituting with. Moreover, T-cell receptor These amino acid residues that are not essential for the interaction are -Binding to proper MHC, which may add or reduce cell reactivity. Can be modified by substituting with another amino acid that does not induce Noh.   Moreover, the peptides of the present invention are essential for their interaction with the MHC protein complex. The presence or absence of amino acids indicated by and whose presence causes T-cell activity to be increased or decreased. Others shown to induce but not similar amino acid residues, preferably similar amino acid residues It is possible to modify by substituting (conservative substitution). M with high affinity Peptides that bind HC confer T-cell immune passiveness in vivo at lower concentrations It is supposed to be done. Moreover, its interaction with the MHC protein complex Is not essential, the amino acid residue present on the bound peptide is Capture May induce or reverse T-cell responsiveness but not induce it. It can be modified by substituting it with a mino acid. To nonessential amino acids Preferred amino acid substitutions for are alanine, glutamic acid, or methyl. Substitutions with amino acids are included, but are not limited to.   Another example of protein or peptide modification is dimerization via disulfide bonds. Of cysteine residues for minimizing alanine, serine, threo Substitution with nin, leucine, or glutamic acid residues. In addition, the present invention It is possible to chemically modify the amino acid side chains of peptides. Other modifications are Cyclization of peptides.   For the purpose of enhancing stability and / or reactivity, the protein of the present invention or The peptide is modified to produce a protein that is derived from any naturally occurring allelic variant. Capable of incorporating one or more polymorphisms within the amino acid sequence of the self-antigen It is. In addition, D-amino acids, unnatural amino acids, or non-amino acid analogs To the modified protein or peptide within the scope of the present invention. It is possible to produce. In addition, the protein or peptide of the present invention is Sehon and co-workers (Wie et al., Supra). Modified with polyethylene glycol (PEG) to complex with PEG It is possible to produce proteins or peptides. Moreover, PEG is used in the present invention. Can be added during the chemical synthesis of the protein or peptide. Protein too Or modification of peptides or parts thereof involves reduction / alkylation (Tar). r: Methods of Protein Microcharacteri zation, J. E. FIG. Silver   ed. , Humana Press, Clifton NJ 155-194. (1986)); Acylation (Tarr, supra); Chemical cup into a suitable carrier. Ring (Michel and Shiigi, eds, SeleCted Methods in Cellular Immunology, WH Fr eeman, San Francisco, CA (1980), U.S. Pat. No. 4, 939, 239) or mild formalin treatment (Marsh (1971) , Int Arch of Allergy and Appl Immuno 41: 199-215).   Facilitates the purification of the protein or peptide of the present invention, and if possible In order to increase their solubility, the amino acid reporter Groups can be added. For example, hexahistidine can be used as an immobilized metal ion. Added to proteins or peptides for purification by affinity chromatography (Hochuli, E. et al., (1988). Bio / Technology 6: 1321-1325). Moreover, irrelevant To facilitate isolation of sequence-free proteins or peptides, specific And the protease and its reporter group and its protein or peptide. Can be incorporated between the sequences. An individual against a protein antigen For the purpose of successful desensitization, the solubility of a protein or peptide should be Whether by adding functional groups to the white matter or peptides, or of the protein It may be essential to increase by eliminating the hydrophobic region.   Possibly the appropriate antigen of the T-cell epitope within a peptide To aid in processing, standard protease-sensitive sites are Via a recombinant or synthetic method between regions containing at least one T-cell epitope It can be created by engineering. For example, charging like KK or RR A modified amino acid pair between regions within a peptide during the recombinant construction of that peptide It is possible to The resulting peptide is labeled with cathepsin and / or other peptides. It is possible to make it susceptible to cleavage by a lipsin-like enzyme, which A portion of the peptide containing one or more T-cell epitopes is made. So Moreover, such charged amino acid residues lead to increased solubility of certain peptides It is possible.   Site-directed mutagenesis of DNA encoding the peptide or protein of the present invention And the peptide or protein by methods known in the art. It is possible to modify the structure of. One such method is Polymerase chain using an oligonucleotide primer with a number of mutations Reaction (PCR) (Ho et al., (1989) Gene 77: 51-5. 9) or total synthesis of mutated genes (Hostostky, Z. et. al. , (1989) Biochem Biophys Res Comm 1 61: 1056-1063). Promote recombinant protein expression To apply the above-mentioned method, the codons present in the cDNA sequence of the present invention are Change to one that is preferentially utilized by the host cell in which the recombinant protein is expressed It is possible (Wada et al., Supra).   Diagnosing the demyelinating autoimmune response with the isolated protein and / or antigenic fragment It can be used for treatment and prevention methods. Therefore the book The invention provides isolated human MOGs (SEQ ID NOS: 1 and 2) or antigenic fragments thereof. , And a therapeutic composition comprising a pharmaceutically acceptable carrier or excipient. You. Moreover, this isolated protein and / or fragment may be used for screening for autoimmune diseases. Used for cleaning and for the development of candidates for therapeutic compositions. And it is possible.Pharmaceutical composition   Administration of the therapeutic compositions of the present invention uses known methods to ameliorate the disease. It is possible to carry out effective doses and durations. Single peptide or protein In addition to the composition containing white matter, each comprising at least one T-cell epitope of human MOG Mixture of at least two peptides (eg, at least two peptides) It is also possible to provide a physical mixture of tides), such a composition being a drug. Administration in the form of a therapeutic composition containing a pharmaceutically acceptable carrier or excipient Is possible. Furthermore, the therapeutic composition has at least two regions, each of which is Each region comprises at least one T-cell epitope of MOG). May be present in the human MOG. Can be aligned in a conformation different from that of One or more It is possible to administer a therapeutically effective amount of such a composition simultaneously or sequentially. is there.   Preferred compositions of peptides that can be administered simultaneously or sequentially and The preferred combination is for Figure 2 (SEQ ID NOs: 4-9, 11, 15, 16, and 42-72), 5a (SEQ ID NOs: 73-80, 82, 83), and 5b (human M The amino acid shown in the first 121 amino acids of the OG protein (SEQ ID NO: 2) No acid sequence, more preferably MOG1 ~ 13 (SEQ ID NO: 42) and MOG 103-115 (SEQ ID NO: 55). Including peptides.   The effective amount of the therapeutic composition depends on the degree of morbidity of the individual, the age, sex, and And weight, and the protein or protein that induces an antigenic response in the individual. It will vary depending on factors such as the capacity of the fragment. Adjust dosage regimen To provide the optimal therapeutic response. For example, the dose divided into several It may be given daily or the dose may be dictated by the therapeutic needs. It can be partially reduced when   Injection of the protein, peptide, or pharmaceutical composition thereof (subcutaneous, Intravenous, etc.), oral administration, sublingual administration, inhalation, transdermal application, or enteral administration Can be administered in a convenient manner such as Composition depending on route of administration Objects are protected from enzymes, acids, and other natural conditions that can cause inactivation. Can be included with the material.   For administration by injection, for example, about 1 μg to 3 mg per dose unit And preferably about 20 μg to 750 μg of protein or peptide is typical . Pharmaceutical compositions suitable for injectable use include sterile aqueous solutions (where water soluble) Or for dispersions and formulations according to prescriptions for sterile injectable solutions or dispersions There is a sterile powder of. In all cases, the composition must be sterile and Flows to the extent that easy syringability exists. It should be dynamic. The composition should be stable under the conditions of manufacture and storage. And should be protected against the mixed effects of microorganisms such as bacteria and fungi It is. This carrier is, for example, water, ethanol, a polyol (for example, glycero , Propylene glycol, and liquid polyethylene glycols, etc.) Can be a solvent or dispersible medium containing a suitable oil, as well as vegetable oils. Noh. Proper fluidity is achieved by the use of coatings such as lecithin , In the case of dispersion by maintaining the required particle size and by the use of surfactants. It can be maintained by using. Prevention of the action of microorganisms, for example, parabens (Parabenz), chlorobutanol, chlorobutanol Phenol, ascorbic acid, and thimerosal (timer) can be achieved with various antibiotics and fungicides such as You. In many cases, for example sugars, polyalcohols (eg mannitol, sorbite) It is preferable to include isotonic agents, such as tall, sodium chloride) in the composition. Will. Sustained absorption of injectable compositions delays absorption in the composition By including (eg, aluminum monostearate and gelatin) It can be achieved.   Sterile injectable solutions are listed above, with the active ingredient in the required amount in the appropriate solvent, as required. Uptake with one or a combination of ingredients, and then It can be prepared by performing filter sterilization. Generally a dispersion Is the active compound in sterile excipients containing basic dispersion medium, as well as listed above. It is prepared by incorporating the required other ingredients from the one. Sterilization In the case of sterile powders for the preparation of injectable solutions, the preferred method of preparation is suction drying. And freeze-dried, and the solution has been previously sterile filtered by these methods. Whichever Of the active ingredient (i.e. protein or pepti Powder) is produced.   This protein or fragments thereof may be Can be administered and co-administered with enzyme inhibitors, or liposomes Can be administered in a suitable carrier such as. As a pharmaceutically acceptable excipient Include saline and aqueous buffer solutions. Adjuvant is used in its broadest sense And includes any immunostimulatory compound such as interferon . Adjuvants considered herein include resorcinols, nonionic salts. Surfactants such as polyoxyethylene oleyl ether and n-hexadecyl Polyethylene ether) is included. Enzyme inhibitors include pancreatic trypsin inhibition Agent, diisopropyl fluorophosphate (DEP), and trasilol included. Water-in-oil-in-water CGF emulsion, as well as ordinary liposome (Strejan et al., (1984) J. Neuroimmuno. l. 7:27) are included. For the purpose of inducing non-responsiveness of T-cells, this therapeutic The composition is administered in a non-immunogenic form (eg without adjuvant) Is preferred.   If the protein or peptide is adequately protected at the doses mentioned, this protein Alternatively, the peptide may be administered, for example, with an inert excipient or an assimilable edible carrier. Can be administered orally. Hard or soft this protein or other ingredients Encapsulating in gelatin capsules in shells, compressing into tablets, or individual It can also be incorporated directly into the body's diet. For oral therapeutic administration, Incorporation of the active ingredient with excipient administration, and ingestion tablets, buccal tablets , Lozenges, caps Used in the form of cell, elixir, suspension, syrup, and wafers Can be. Such compositions and preparations will contain an effective amount. Such drugs The amount of active compound in a pharmaceutically useful composition will be such that a suitable dosage will be obtained. Things. Preferred compositions or formulations according to the present invention have an oral dosage unit of about 1 It is prepared to contain between 0 μg and about 200 mg of active compound.   As used herein, the term "pharmaceutically acceptable carrier" refers to Some and all solvents, dispersion media, coatings, antibiotics and fungicides Agents, isotonic agents, absorption delaying agents and the like. This for pharmaceutically active substances The use of such media and reagents is well known to those of ordinary skill in the art. Any normal medium To the extent that a quality or reagent is incompatible with the active compound, it is excluded for therapeutic Its use in a composition is envisaged. The supplementary active compound is incorporated into the composition. It is also possible to include it.   Formulations of parenteral compositions in dosage unit form for ease of administration and uniformity of dosage. It is particularly advantageous to apply. Dosage unit form as used herein is intended for treatment Means a physically discrete unit suitable as a single dose for each mammalian subject; The unit cooperates with the required pharmaceutical carrier to produce the desired therapeutic effect. It contains a calculated, predetermined amount of the active compound. Specific dosage unit forms of the invention A description of (a) the unique properties of the active compound and the particular therapeutic effect to be achieved. , And (b) combining such active compounds for the treatment of individual susceptibility The limitations inherent in the art, of, and directly Depends on.   The invention relates to at least two, each containing at least one T-cell epitope. Of a peptide (eg, a physical mixture of at least two peptides) Also provide things. Such a composition may be administered to the pharmaceutics described previously herein. Administered to an individual in the form of a therapeutic composition with a pharmaceutically acceptable carrier or excipient. be able to. A therapeutically effective amount of one or more such compositions is Or it can be administered continuously.Diagnostic method   The protein or peptide of the present invention is used for the diagnosis and treatment of autoimmune diseases. It can be used in "purified" form for standardization of drugs. Isolation and purification Produced protein or peptide is an antiserum or monolayer for use in diagnosis. It is also useful for preparing clonal antibodies. For example, a mouse or a rabbit Immunize such animals with an immunogenic form of this isolated protein or peptide. It is possible, but if necessary, by coupling to a carrier , Or a protein or other protein by other techniques well known in the art. It is also possible to impart immunogenicity to the peptide and perform the previous immunization. This protein It is possible to administer the white matter or peptide in the presence of an adjuvant, The progress of immunization can be monitored by detecting the antibody titer in plasma or serum. And use a standard ELISA or other immunoassay as the antigen. It can be used with immunogens to assess antibody levels.   Antiserum is obtained after immunization and, if desired, polycloner Antibody can be isolated. Produce monoclonal antibodies To recover the antibody-producing cells (lymphocytes) from the immunized animal, The hybridoma is fused with an immortalized cell such as a myeloma cell by the somatic cell fusion method. Produce cells. The hybridoma cell is the protein of the present invention or its peptide. Can be immunochemically screened for production of antibodies that react with. Standardize reagents in standard assays using this antiserum or monoclonal antibody It is possible to   The protein, peptide or antibody of the present invention is used for the detection and diagnosis of autoimmune diseases. It can also be used for This means, for example, that blood obtained from an individual A liquid or blood product isolated antigenic peptide and its constituent components in blood (eg , Antibodies, HLA molecules, T-cells and B-cells) and their peptides (single or Or under suitable conditions for binding proteins, and This can be done by determining the extent to which such binding occurs. Departure Other autoimmune diseases that can use clear proteins, peptides, or antibodies Paper radioimmunoabsorption test (PRIST), enzyme-linked immunosorbent assay Yield assay (ELISA), radioimmunoassay (RIA), immunoradiometry Assay (IRMA), and luminescence immunoassay (LIA) You.Primers, probes, and other oligomers   The nucleotide sequence shown in Figure 1 (SEQ ID NO: 1) and its complement (SEQ ID NO: 1) Due to the availability of 2), various oligonucleosides useful in therapeutic and diagnostic situations Chid design is possible. Regulation of the expression of the gene encoding MOG is associated with autoimmune disease. Influences the progression of the disease; Monitor by monitoring expression -It is possible. Furthermore, based on the nucleotide sequence disclosed in FIG. 1 herein, The gomer is a standard assay for detecting DNA or RNA encoding MOG. It can be used for the Sei method.   Some oligomers "based on" the sequence disclosed in Figure 1 (SEQ ID NO: 1) Oligomers containing part of the sequence, oligomers complementary to the sequence or parts thereof -When a large amount of DNA is desired (eg, for genetic engineering), the sequence of An oligomer implying a primer for use in amplifying a portion, as well as M Affects triple helix formation with related parts of the OG gene double helix An oligomer designed based on the disclosed sequences is meant. PCR primer, single-stranded Oligomer capable of hybridizing to target, and triplex with DNA double helix Suitable design parameters for lixiformable oligomers are known in the art. Well-known in the field of surgery. Therefore, "based on" the DNA of Figure 1 (SEQ ID NO: 1) The rigomer has the same sequence as this part of DNA when passed through the conventional design parameters. , The same sequence as its complement or its part, or a different sequence 1 can have a sequence related to that disclosed in 1 (SEQ ID NO: 1).   A nucleotide sequence based on the nucleotide sequence shown in FIG. 1 (SEQ ID NO: 1) Can the oligomers have normal RNA or DNA multimers? , Or modified forms thereof commonly known in the art. Can be. For example, the phosphodiester linkages of those oligomers can be converted to Substitution with another linkage such as holothioate, and methylphosphonate. Can be. Moreover, another backbone formation for nucleotide bases has already been disclosed. And then Such modifications are included within the scope of the oligomers claimed herein.   The following examples are intended to illustrate, but not limit, the invention. Is not intended.                               Example 1                 CDNA encoding human MOG protein   In the first attempt to obtain human DNA encoding the MOG protein, human cDNA was used. The A library has been published by Gardinier et al (supra). Using 3'and 5'primers designed from rat MOG coding sequence It was subjected to polymerase chain reaction (PCR). This human MOG sequence is Of the human and rat sequences 5'and / or 3 It is hypothesized to be due to insufficient homology at the'-end.   Therefore, four rat middle oligonucleotides were designed. Two of them Is the upper strand of the gene (primers 94-111 and 166-183 (SEQ ID NO: No. 34), base 1 starts with ATG), and two of the genes are The lower strand (primers 538-555 (SEQ ID NO: 35) and 685-702) Was homologous to. Primers 166-183 (SEQ ID NO: 34) and 538-5 The combination of 55 (SEQ ID NO: 35) is about 4 from the human brain cDNA library. It was successful in carrying out amplification of fragments of the expected size of 00 bp. These plies The array of mars is:     a) 166-183: CAGAATCCGGGAAGAATGCCACG GC                             (SEQ ID NO: 34); and     b) 538-555: CAGCGGCCGCACGGAGTTTTT CCTCTCAG                         (SEQ ID NO: 35).   EcoThe RI site is present in the 166-183 primer (SEQ ID NO: 34);N ot The I site is present in the 538-555 primer (SEQ ID NO: 35).   The 400 bp PCR product was ligated into the expression vector pVL1393, pVL1393 (Pharmingen CA)EcoRI andNotDigesting with I The fragment obtained by digesting the amplified product with the same enzyme. Were connected. This insert contains a number of clones derived from the ligated plasmid. TheEcoRI andNot400 bp human MO digested with I and obtained Confirmed by sequencing the G fragment. The obtained insert fragment is 738b. Virtually 184 bp of 5'sequence and 2 based on the rat open reading frame The 01 bp 3'sequence is deleted.   The two primers are 400b from the upper and lower strands at positions 346-363. Design from p and show them below: and [In these sequences,EcoThe RI site is in the first strand, andNotI site is the second strand It exists inside.] The underlined region corresponds to the MOG sequence.   The upper and lower primers of human MOG346-363 (SEQ ID NO: 36 and 37) in combination with the 5'and 3'rat primers described above. And use each of them from the same human brain cDNA library as in the previous procedure. The 5'and 3'deleted ends of the gene were amplified. P corresponding to the 3'end of the gene A CR product was obtained but the corresponding 5'end did not occur.   The 3'fragment obtained has the expected 400 bp size, and this The fragment was cloned into pVL1393 and sequenced.   To obtain the 5'portion of this gene, it was pre-amplified and 8 x 10^Ten of human brain medulla obtained from Clontech with a titer of pfu / ml λ_gt10 libraries were screened according to the protocol described by the manufacturer. I learned. This library was run at 30,000 plaques / plate for 12 Plate on large plates and plaque nitrocellulose filters (2 replica filter / plate). Then 12 different Twelve filters removed from the plate were first cloned into human M Corresponds to the OG middle 400 bp fragment (positions 184-534)³²P-labeled professional Hybridized to the probe. Twenty-two strong positive plaques were obtained. Also Make a hole in the plug for each positive plaque from the original plate, and The phages were eluted from the agar by culturing with λ dilution buffer overnight. Then this test The tube was centrifuged and the supernatant removed.   This DNA from individual poolsSstΛ containing II site_gt10 forward plies Mar: 5'-CTTTTGAGCAAGTTCAGCCTGGTTAAG-3 ' (SEQ ID NO: 38) orXhoΛ containing I site_gt1 0 reverse primer: 5'-ACCTCGAGGAGGGTGGCTTATGAG TATTTCTTCCAGGGTA-3 '(SEQ ID NO: 39), as well as human MO Upper or lower strand of G middle primer: 5'-GGTGCGGGGAAAG GTGACTCTCAGGATCCGGAAT-3 '(SEQ ID NO: 40), or Is 5'-ATTCCGGATCCTGAGAGTCACCTTTCCCGCAC Amplification was performed using C-3 '(SEQ ID NO: 41).   The latter two primers (SEQ ID NOS: 40 and 41) were used in the human MOG sequence. Exist in natureBamIt contains a HI site (underlined in the sequence).   Four different combinations of these primers: 1) Forward primer on the strand -/ Lower strand MOG middle primer; 2) lower strand reverse primer / lower Mid-prime of chain MOG; 3) Mid-primer of top MOG / below Reverse primer of strand; and 4) Middle primer of MOG of upper strand / upper strand Of the forward primer.   The first two combinations are the 5'end of the gene (BamUp to the HI site) , And the latter two provided the 3'end of the gene. Both 5'and 3'parts Both contain untranslated regions. Which of the two members of each combination is desired Is actually λ_gtOrientation of cDNA cloned within 10 Depends on.   The size of the fragments obtained varied from pool to pool. Also the 5 largest 5'fragments Preferably the 3'fragment of the SK polylinkerSstII andBamHI site IsBamHI andXhoSubcloned into the I site. Then each pool The three clones were sequenced and PC The presence of R errors was ruled out. This allows the entire coding region of the gene Sequences were provided, as well as 174 bp of 5'untranslated sequence.   Total DNA sequence recovered (SEQ ID NO: 1) and deduced amino acid sequence (sequence The number 2) is shown in FIG.   Human MOG encodes a 248 amino acid preprotein that is present in the rat protein. With 246 amino acids of 87% homology. The mature protein contains 218 amino acids , Which is numbered 1-218 in FIG. 1 (SEQ ID NO: 2). Mature protein Quality starts with the glycine shown at position 1 and from the MET start codon to position 1 From a presequence that extends to the alanine residue that occurs immediately before the indicated glycine Derived from a 248 amino acid preprotein by cleavage.   In addition, human MOG cDNA was cloned into E. coli (E. FIG.  coli) For expression in Cloned into pET H6 vector. Novagen (Madis on, WI) obtained from pET. H6 is a sequence encoding 6 histidines , Which allows for purification of any recombinant protein through a Ni ++ column. I have. Amino acids 1-121 of human MOG (the first 121 amino acids of SEQ ID NO: 2) Cleaved human MOG cDNA encoding acid (without leader sequence and The following oligonucleotides by PCR (without the membrane domain): Was amplified using. Then, a 363 bp PCR fragment was added to pET. H6 Non-iteration ofSstII andXhoIt was cloned between the I sites. After cloning The entire sequence of this cDNA was determined.                               Example 1A Expression of truncated human MOG in SF-9 insect cells and E. coli SF-9 expression   Amino acids 1-121 of human MOG (the first 121 amino acids of SEQ ID NO: 2) A PVL1393 transfer vector containing a truncated human MOG cDNA encoding aculogold linearized baculovirus DNA In SF-9 cells with (Pharmingen, San Diego, CA) Were co-transfected. The culture supernatant containing the recombinant virus was recovered after 4 days Was. The recombinant virus was plaque purified and subjected to 3 rounds of amplification to obtain high titers. Virus stock was obtained. After that, the AF-9 cells were added to the virus stock At a MOI of 2.0. Collect supernatant from infected cells 48 hours after infection And loaded onto a NiNTA agarose column. 2 this recombinant MOG protein Elute under non-denaturing conditions with 50 mM imidazole , 5% propionic acid and H₂Dialyzed against O and then lyophilized I let you. The protein concentration was assessed by BCA. Cooma with purified MOG protein 12.5% polyacrylamide stained with Coomassie blue Visualized on gel. E. coli (E. FIG.  coli) Expression   PET. Containing a truncated human MOG cDNA. The H6 vector was transformed to B L21 (DE3) cells (Novagen, Madison, WI. ). Several colonies in 2YT medium to an OD of 1.0 Were grown together. The bacterium was then induced with 1 mM IPTG overnight. Cells are harvested and 6M Guanidine / 100 mM T ris. Lysis was performed with HCl pH 8.0. This lysate is mixed at 20,000 rpm for 3 Centrifuge for 0 minutes and load the resulting supernatant onto a NiNTA agarose column. (Quiagen, Chatsworth, CA). This protein was added to 6M Guani Guanidine / 100 mM sodium phosphate, pH 4.5 Out, first for 5% propionic acid, then for H₂Dialysate against O, and After that, it was freeze-dried. Protein concentration was assessed by BCA. Purified MOG protein 12.5% polyacene stained with Coomassie blue Visualization was performed on a rilamide gel.                                Example 2 Human MOG expression in insect SF-9 to induce EAE in vivo   Recombination expressed in insect SF-9 into two groups of (PLJ x SJL) F1 mice 10 μg and 5 of N-terminal fragment of human MOG (-TM, recombinant, SF-9) 0 μg each was injected and this fragment wasExamples 1 and 1AObey Prepared. Cleaved MOG is amino acids 1-121 (hereafter MOG1 ~ 121), and this is in part a MOG. Solubility related to the solubility of amino acids 122-218 (SEQ ID NO: 2) of a protein Was chosen for. Completely Freund horsepower for MOG 1-121 Emulsified in tubant and injected subcutaneously into mice. MOG1-121 Note At the same time as the shot, 200 ng of pertussis toxin was also injected intravenously. 200 ng hundred I. cough toxin V. The injection was repeated 2 days later. Emulsions are MOG 1-121 (-T M, recombinant, SF-9) and 400 μg of H3 in CFA as described above. 7Ra (Difco Laboratories, Detroit, MI) It was prepared together. Starting on day 8 after the first immunization, the mice were examined for signs of paralysis. And observed daily and a daily assessment was made as an indicator of reduced EAE. Mice have the following criteria: 1, caudal paralysis; 2, partial hindpaw paralysis; 3, complete posterior Foot paralysis; 4, forelimb paralysis; 5, dying or dying, based on clinical signs I rate it.   The onset of symptoms began as early as 14 days for some mice. these The mice were observed for 31 days, and on the 31st day, the mice were sacrificed and the brain and spinal cord were collected. And histological examination was performed to confirm clinical findings. 50 μg rMOG 60% (60% of mice immunized with (-TM, recombinant, SF-9) ) And 10 μg of rMOG (-TM, recombinant, SF-9). Eighty percent (80%) of the mice had symptoms of EAE.   This method is repeated until E. coli (E. FIG.  coli) Recombinant human MO expressed in Recombinant N-terminal fragment of G1-121 (-TM, recombinant,E. FIG.  coli) Recombinant N-terminal fragment of recombinant human MOG1-121 expressed in worm SF-9 ( -TM, recombinant, SF-9) instead of. Although not yet established, Note that these results show similar findings.   Therefore, mice in which EAE is induced in this manner hold promise for the treatment of multiple sclerosis. Useful as an animal model for screening therapeutic agents There is a possibility. The following identifies therapeutic compositions for the treatment of multiple sclerosis Here is one way to do it:   Administration of human MOG in immunogenic form to mice induces EAE in said mice. Rub stage,   The mouse in which EAE was induced was treated before the onset of symptoms of EAE in the mouse. Or contains at least one antigenic fragment of human MOG after the onset of EAE symptoms Treating with a therapeutic composition, and   The therapeutic composition also initiates the symptoms of EAE in the EAE-induced mouse. Or the stage of deciding whether to prevent progression, including.                                Example 3                  T-cell response to human MOG peptide   If the peptide is a peptide synthesizer from Applied Biosystems, Use one of the robotics systems of Advanced Chemtech. , FastMOC ™ chemistry on commercially available Wang resin, And Fmoc-protected amino acids are utilized by Hill et al. (J.Imm unol. 52: 2890-2898, 1994). Synthesized. Hill, Buelow, Gorga, and Mar, cited above. The teachings of shall are incorporated herein by reference.   A T-cell assay was performed to further refine the identification of T-cell epitopes. . Peripheral blood lymphocytes from human volunteer HLA-DR2-positive donors to Fico Isolated with 11 Hypaque. 20 million lymphocytes, human AB blood In RPMI culture medium supplemented with 2 x 10 per le^Five96 well microtiter wells. Selected Added mixture of MOG peptides prepared at a final concentration of 50 μM for each peptide Was. The MOG peptides selected were naturally-occurring peptides and naturally-occurring peptides. Both are analogs of Cido and they are: Met. The culture is CO₂12 days in a 37 ° C incubator moistened with Incubate and intermittently human IL2 (20 U / ml) and IL4 (5 U / m) l) was supplemented. Remove the sample from each culture well, wash and add in advance Removed the peptides and added 4 wells of a new microtiter well. Re-seeded (for each sample, 2 wells contained the peptide mixture and 2 One well contains no peptide mixture). Irradiated and stored at low temperature Paspheres were added to antigen presenting cells. After an additional 3 days of incubation, 3H- Thymidine incorporation was measured. Add positive microtiter strains to the peptide wells Average uptake is greater than 1.5 times that of non-peptide wells or 1.5 Scored if equal to twice. Positive microtiter strain I Expanded with L2 and IL4 and then the next week, the peptide mix Were re-assayed by the same method with individual peptides except.   Peptides identified as peptides containing T-cell epitopes using this method Are MOG 1 to 13 (SEQ ID NO: 42) and MOG 103 to 115 (SEQ ID NO: 5) It was 5). FIG. 6 shows the results of the assay performed.                                Example 4 MOG 20-mer peptide and recombinant human MOG expressed in insect SF-9 Human MS patient T-cell response to N-terminal fragment (-TM, recombinant, SF-9)   Peptides (20 amino acids long) were applied to Applied Biosystems. Peptide Synthesizer or Advanced Chemtech Robotics FastM with commercially available Wang resin using either Hill ™ using OC ™ chemistry and Fmoc protected amino acids t al. (J. Immunol. 52: 2890-2898, 1994). Was synthesized as described above. Hill, Bulow, G cited above The teachings of orga and Marshall are incorporated herein by reference. . These peptides are 20-amino acid peptides of human MOG with 10-amino acid overlap. And is shown in Figure 5a.   After the method of Example 3, the T-cell response of a human patient suffering from multiple sclerosis is shown in FIG. a group of MOG dimeric peptides shown in a and expressed in insect SF-9 N-terminal fragment of recombinant human MOG1-121 (-TM, recombinant, SF-9) (This was the case in Example 2 where mice were given EAE Has been shown to induce). Of the MOG peptides tested One or more of at least for the self-antigen responsible for multiple sclerosis Suspected to contain one T-cell epitope.   Recombinant MOG1-121 (9 48 wells in 6) and a mixture of 10 MOG fragments (20 shown in Figure 5a). The cultures were initiated using both the (peptidic peptide) (48 wells in 96) separately. The cells were cultured according to the protocol of Example 3 except that From each culture well Remove sample, wash to remove pre-loaded peptides, and clean Reseeded in 6 wells of a microtiter dish. 6 microta Iterwell can then react with both rMOG and the peptide mixture. Found (2 wells from that culture started with rMOG and 4 wells from the sample were started with the peptide mixture). This result shows that MS patients One activated by MOG and contained in the MOG peptide mixture or It has been demonstrated to have T-cells that recognize multiple T-cell epitopes. Pe There are many wells that react with the peptide mixture but not with the recombinant MOG. I was The importance of these positive wells is less clear, but during the MOG MOG-reactive T-cells that recognize the E. coli epitope are easily processed in vitro It is thought that it is not done.

─────────────────────────────────────────────────── ─── Continuation of front page (51) Int.Cl. ⁶ Identification code Internal reference number FI C07K 14/47 7804-4B C12N 1/21 C12N 1/21 9637-4B C12P 21/02 C C12P 21/02 9358 -4B 21/08 21/08 0276-2J G01N 33/53 V G01N 33/53 0276-2J 33/564 33/564 9284-4C A61K 39/395 D // A61K 39/395 9051-4C 37/02 ABB (C12N 1/21 C12R 1:19) (C12P 21/02 C12R 1:19) (C12P 21/02 C12R 1:91) (81) Designated country EP (AT, BE, CH, DE, DK, ES, FR , GB, GR, IE, IT, LU, MC, NL, PT, SE), OA (BF, BJ, CF, CG, CI, CM, GA, GN, ML, MR, NE, SN, TD, TG ), AT, AU, B, BG, BR, BY, CA, CH, CN, CZ, DE, DK, ES, FI, GB, HU, JP, KP, KR, KZ, LK, LU, LV, MG, MN, MW, NL , NO, NZ, PL, PT, RO, RU, SD, SE, SK, UA, US, UZ, VN (72) Inventor Sumilek, Dawn 95070 Saratoga Fredericksburg 12589, California, USA

Claims (1)

[Claims] 1. An isolated nucleic acid molecule comprising a nucleotide sequence encoding human myelin oligodendrocyte glycoprotein (MOG) or at least one antigenic fragment thereof. 2. 2. The nucleic acid molecule of claim 1, wherein said nucleotide sequence consists essentially of nucleotides encoding amino acids 1-218 (SEQ ID NO: 2) of Figure 1 or allelic variants thereof. 3. An oligomer comprising a nucleotide sequence based on the nucleotide sequence of Figure 1 (SEQ ID NO: 1). 4. An expression system which is a DNA molecule comprising a nucleotide sequence encoding human MOG or an antigenic fragment thereof and operably linked to a control sequence for expression in a compatible host. 5. The expression system of claim 4, wherein the nucleotide sequence encodes amino acids 1-218 (SEQ ID NO: 2) of Figure 1 or an antigenic fragment portion thereof. 6. A recombinant host cell modified to include the expression system of claim 4. 7. Isolated and purified human MOG or an antigenic fragment thereof. 8. a) culturing host cells modified to contain an expression system that directs expression of a nucleotide sequence encoding human MOG or a fragment thereof in a suitable medium to produce a culture containing human MOG or a fragment thereof. And b) a method of producing a human MOG or an antigenic fragment thereof, comprising the step of recovering the human MOG or a fragment thereof from the culture. 9. A peptide comprising at least one T-cell epitope of human MOG or a tandem copy thereof. 10. 10. The peptide of claim 9, wherein said peptide comprises any of the amino acid sequences shown in Figure 2 (SEQ ID NOS: 4-9, 11, 15, 16, and 42-72), Figures 5a and 5b. 11. A peptide that also comprises at least two T-cell epitopes of MOG in humans. 12. A modified form of human MOG or its antigenicity, wherein said modification comprises replacing one or more amino acids of said peptide or protein with a different amino acid which does not interfere with the biological activity of said peptide or protein. fragment. 13. A nucleic acid molecule comprising a nucleotide sequence encoding the peptide of any one of claims 9-12. 14． An expression system which is a DNA molecule comprising a nucleotide sequence encoding the peptide of any one of claims 9-12 and operably linked to a control sequence for expression in a compatible host. 15. A recombinant host cell modified to include the expression system of claim 14. 16. a) culturing a host cell modified to contain an expression system that directs the expression of the nucleotide sequence encoding the peptide in a suitable medium to produce a culture containing the peptide, and b) culturing the same. A method for producing a peptide according to any one of claims 9 to 12, comprising the step of recovering the peptide from a product. 17． The above-mentioned modification of the protein, fragment, or peptide is used to enhance the solubility of polyethylene glycol, protein, fragment, or peptide, to facilitate purification of the protein, fragment, or peptide, and a proteolytic cleavage site. A modified form of human MOG, or an antigenic fragment thereof, or a peptide of any of claims 9-12, comprising coupling to an additional moiety selected from the group consisting of: 18. Isolated human MOG, and / or at least one antigenic fragment thereof, and / or at least one peptide of claims 9-12 or 16, and a pharmaceutically acceptable carrier or A therapeutic composition comprising an excipient. 19. The human MOG is encoded by an amino acid sequence of positions 1-218 shown in FIG. 1 (SEQ ID NO: 2) or an allelic variant of the nucleotide sequence of FIG. 1 (SEQ ID NO: 1), or an antigenic fragment thereof. The therapeutic composition of claim 11 comprising: 20. 20. A method of treating a demyelinating autoimmune disease, comprising administering to a subject a therapeutically effective amount of the composition of claim 19. 21. A blood sample obtained from a subject to be examined is isolated from human MOG or an antigenic fragment thereof, or any of the peptides within claims 9 to 12 and 16, and a MOG of blood constituents or a MOG thereof. A method of diagnosing a demyelinating autoimmune disease comprising combining under appropriate conditions for binding to a fragment and determining the extent to which such binding occurs. 22. The extent to which binding occurs is determined by assessing T-cell function, T-cell proliferation, B-cell function, binding of its protein or its fragments to antibodies present in blood, or combinations thereof. The method of claim 21. 23. A monoclonal antibody or an immunoreactive fragment thereof which specifically reacts with human MOG or an antigenic fragment thereof, or the peptide of any one of claims 9 to 12 and 16. 24. Identifying hydrophobic amino acids contained in human MOG; intervening four amino acids N Characterizing an amino acid in the human MOG sequence that is separated from the hydrophobic amino acid by C, wherein the amino acid is a small amino acid selected from the group consisting of glycine, alanine, serine, threonine, and cysteine. Or whether it is a different amino acid, and identifying the hydrophobic and small amino acids as T-cell epitopes (wherein the small amino acid is 4 amino acids N from the hydrophobic amino acid). (Isolated by C), which comprises a T-cell epitope of human MOG. 25. The peptide comprises at least one T-cell epitope, wherein said peptide is MOG1-13 (SEQ ID NO: 42), MOG103-115 (SEQ ID NO: 55), MOG1-121 (first 121 amino acids of SEQ ID NO: 2), MOG1 to 20 (SEQ ID NO: 73), MOG11 to 30 (SEQ ID NO: 74), MOG21 to 40 (SEQ ID NO: 75), MOG31 to 50 (SEQ ID NO: 76), MOG41 to 60 (SEQ ID NO: 77), MOG51 to 70 (sequence) No. 78), MOG61-80 (SEQ ID NO: 79), MOG71-90 (SEQ ID NO: 80), MOG91-110 (SEQ ID NO: 82), and MOG101-120 (SEQ ID NO: 83). An isolated peptide of human MOG, which comprises the sequence of: 26. The mixture is MOG1-20 (SEQ ID NO: 73), MOG11-30 (SEQ ID NO: 74), MOG21-40 (SEQ ID NO: 75), MOG31-50 (SEQ ID NO: 76), MOG41-60 (SEQ ID NO: 77), MOG51-. 70 (SEQ ID NO: 78), MOG61-80 (SEQ ID NO: 79), MOG71-90 (SEQ ID NO: 80), MOG91-110 (SEQ ID NO: 82), and MOG101-120 (SEQ ID NO: 83), and A mixture of human MOG peptides, wherein the mixture comprises at least one T-cell epitope. 27. Administering human MOG to a mouse in an immunogenic form to induce EAE in said mouse, said EAE-induced mouse comprising at least one therapeutic composition comprising at least one antigenic fragment of human MOG. And treating the mice prior to or after the onset of EAE symptoms in the mouse, wherein the at least one therapeutic composition inhibits the onset or progression of EAE symptoms in the EAE-induced mice. A method for identifying a therapeutic composition for the treatment of multiple sclerosis, comprising: