KR102621473B1 - Biomarker composition for diagnosing adult-onset still's disease - Google Patents

Abstract

The present application relates to a biomarker composition for diagnosing adult-onset Still's disease containing TLR2 protein.

Description

Biomarker composition for diagnosing adult-onset Still's disease {BIOMARKER COMPOSITION FOR DIAGNOSING ADULT-ONSET STILL'S DISEASE}

This application relates to a biomarker composition for diagnosing adult-onset Still's disease.

Still’s disease is a systemic form of juvenile rheumatoid arthritis. It is a disease whose cause has not yet been identified since it was first described by Still. It occurs in both children and adults. Adult-onset Still's disease, which develops in adults, has been reported all over the world since it was reported by Bywaters in 1971, and is known as a rare disease or a cause of unexplained fever.

Adult-onset Still's disease is generally reported to be a benign disease with a good prognosis, but fatal cases in which some patients have died from it have been reported, and if accompanied by hemophagocytosis syndrome, worsening liver function, infection, etc., the patient may die. It may reach a state of being. Domestic research has also reported a prognosis of death in approximately 10% of patients with the disease.

The diagnosis of Still's disease is mainly based on clinical findings, including high fever, joint pain or arthritis, characteristic skin lesions, lymphadenopathy, hepatomegaly, splenomegaly, serositis and sore throat, leukocytosis, increased blood needle rate, and antinuclear symptoms. Diagnosis is made through laboratory findings such as antibody negativity and rheumatoid factor negativity.

Most of the research being done on adult-onset Still's disease is a simple Enzyme-LinKed ImmunoSpecific Assay (ELISA) study or genetic study on inflammatory cytokines and acute reactor substances using the patient's serum, and is based on systematic biomarkers. There was no report about it. In addition, due to a lack of understanding of the pathogenic mechanism, treatment relies on experience and there is no consensus on this.

Therefore, there is a need for research on biomarkers that can be useful in diagnosing adult-onset Still's disease.

Korean Patent Publication No. 10-1806681, which is the background technology of this application, relates to a biomarker composition, diagnostic kit, and diagnostic method for diagnosing Still's disease, specifically, the expression level of CD11b or CD32 and the frequency ratio of granulocytes to lymphocytes. It is disclosed that Still's disease can be diagnosed in children and adults using as an indicator. However, there is no mention of a method for easily diagnosing adult-onset Still's disease using TLR2, or a diagnostic biomarker composition and kit.

The present application aims to solve the problems of the prior art described above and to provide a biomarker composition for diagnosing adult-type Still's disease.

Additionally, the purpose of the present application is to provide a kit for diagnosing adult-onset Still's disease containing an antibody that specifically binds to the TLR2 antigen protein or the TLR7 antigen protein.

Additionally, our purpose is to provide a method of providing information for diagnosing adult-onset Still's disease.

Additionally, the purpose of the present application is to provide a screening method for a treatment for adult-onset Still's disease.

However, the technical challenges sought to be achieved by the embodiments of the present application are not limited to the technical challenges described above, and other technical challenges may exist.

As a technical means for achieving the above-described technical problem, a first aspect of the present application provides a biomarker composition for diagnosing adult-onset Still's disease containing the TLR2 protein.

According to one embodiment of the present application, the adult-onset Still's disease may include, but is not limited to, arthritis.

According to one embodiment of the present application, the composition may additionally include TLR7 protein, but is not limited thereto.

A second aspect of the present application provides a kit for diagnosing adult-onset Still's disease comprising an antibody that specifically binds to the TLR2 antigen protein or the TLR7 antigen protein.

According to one embodiment of the present application, the antibody may be a monoclonal antibody or a polyclonal antibody, but is not limited thereto.

According to one embodiment of the present application, the kit may be used to diagnose adult-onset Still's disease by detecting TLR2 protein or TLR7 protein in a sample using an antigen-antibody binding reaction, but is not limited thereto.

According to one embodiment of the present application, the sample is from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. It may include those selected, but is not limited thereto.

According to one embodiment of the present application, the sample may be peripheral blood mononuclear cells (PBMC) isolated from an individual, but is not limited thereto.

According to one embodiment of the present application, the method for detecting the TLR2 protein or TLR7 protein includes Western blot, enzyme-linked immunosorbent assay (ELISA), dot blot assay, radioimmunoassay, radioimmunodiffusion assay, and Ouchterony immunoassay. A method selected from the group consisting of diffusion method, rocket immunoelectrophoresis, tissue immunostaining, immunoprecipitation assay, complement fixation assay, FLOW CYTOMETRY ANALYSIS (FACS), protein chip, sandwich assay, and combinations thereof. It may be performed using, but is not limited to this.

The third aspect of the present application includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease; Comparing the measured frequency with the frequency of a normal control sample; And information for diagnosing adult-onset Still's disease, including the step of diagnosing adult-onset Still's disease when the frequency of cells expressing TLR2 or TLR7 is increased in the sample of the individual suspected of having adult-onset Still's disease compared to the control group. Provides a method of provision.

According to one embodiment of the present application, the sample is from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. It may include those selected, but is not limited thereto.

According to one embodiment of the present application, the sample may be peripheral blood mononuclear cells (PBMC) isolated from an individual, but is not limited thereto.

The fourth aspect of the present application includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease; Treating the subject with a candidate substance for treating adult-onset Still's disease; and measuring the therapeutic effect of the candidate substance for the treatment of adult-onset Still's disease.

According to one embodiment of the present application, measuring the therapeutic effect includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual treated with the therapeutic candidate substance; Comparing the frequency of cells expressing the TLR2 or TLR7 measured in a sample of an individual treated with the therapeutic candidate with the frequency of cells expressing the TLR2 or TLR7 measured before the step of treating the therapeutic candidate; And when the frequency of cells expressing the TLR2 or TLR7 measured in a sample of an individual treated with the therapeutic candidate decreases compared to the frequency of cells expressing the TLR2 or TLR7 measured before the step of processing the therapeutic candidate. This may include, but is not limited to, a step of considering the therapeutic candidate as a treatment for adult-onset Still's disease.

According to one embodiment of the present application, the sample is from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. It may include those selected, but is not limited thereto.

According to one embodiment of the present application, the sample may be peripheral blood mononuclear cells (PBMC) isolated from an individual, but is not limited thereto.

The above-described means of solving the problem are merely illustrative and should not be construed as intended to limit the present application. In addition to the exemplary embodiments described above, additional embodiments may be present in the drawings and detailed description of the invention.

According to the above-described problem solving means of the present application, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can accurately and quickly diagnose adult-onset Still's disease, which is difficult to diagnose.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can accurately and quickly diagnose adult-onset Still's disease with arthritis.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can easily diagnose adult-onset Still's disease using non-invasive biological samples without using biopsy or imaging technology, so it can be convenient and economical. .

In addition, the biomarker composition for diagnosing adult-type Still's disease according to the present application can be useful for disease onset, disease progression, disease diagnosis, and prognosis prediction, so it explains the etiology of the disease and reflects the activity of the disease. Disease-specific biomarkers can be provided.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present invention can be useful for initial diagnosis, determination of severity, reflection of disease activity, evaluation of treatment efficacy, confirmation of efficacy of drugs, and determination of the presence or absence of other accompanying diseases such as infectious diseases. Therefore, there is an advantage in increasing the treatment efficiency of adult-type Still's disease treatment.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can be usefully used to distinguish adult-onset Still's disease from other similar lesions (mimickers).

In addition, the screening method for a treatment for adult-onset Still's disease according to the present application can simply and quickly screen the therapeutic effects of various candidate substances for adult-onset Still's disease, and can be usefully used in the development of a treatment for adult-onset Still's disease.

However, the effects that can be obtained herein are not limited to the effects described above, and other effects may exist.

Figure 1 is a table showing clinical characteristics of clinical test subjects.
Figure 2 is a table showing the results of measuring the frequency of cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 in total peripheral blood mononuclear cells.
Figure 3 is an image showing a representative example of a flow cytometry histogram of surface-stained cells presenting various TLR markers in whole peripheral blood mononuclear cells of one AOSD patient.
Figure 4 is a table showing the correlation between the frequency of stained cells representing various TLR markers and disease activity markers or systemic scores in AOSD patients.
Figure 5 is a table showing the expression levels of various TLRs according to clinical symptoms in AOSD patients.
Figure 6 is a table showing the results of skin biopsy of AOSD patients.
Figure 7 is a table showing the results of TLR1, TLR2, TLR4, TLR7, and TLR9 immunohistochemical staining performed in AOSD patients, eczema patients, psoriasis patients, and controls.
Figure 8: Inflammatory cell grade (CD4/CD8/CD68 staining) in the skin of AOSD patients; and the average percentage of inflammatory cells expressing CXCL9, CXCL10, CXCL11, CXCR3, CXCL12 and CXCR4; and the average percentage of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7 and TLR9.
Figure 9 is a graph showing the results of evaluating the correlation between TLR markers in the skin of AOSD patients.
Figure 10 is a table showing the results of lymph node biopsy in AOSD patients.
Figure 11 shows the results of TLR1, TLR2, TLR4, TLR7, and TLR9 immunohistochemical staining performed in AOSD patients, T-cell lymphoma patients, histiocytic necrotic lymphadenitis patients, tuberculous lymphadenitis patients, non-specific reactive hyperplasia patients, and controls. It's a table.
Figure 12: Inflammatory cell grade (CD4/CD8 staining) in the skin of AOSD patients; and the average percentage of inflammatory cells expressing CXCL10, CXCL13, CXCR3, and S100A8/A9; and the average percentage of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9.

Below, with reference to the attached drawings, embodiments of the present application will be described in detail so that those skilled in the art can easily implement them.

However, the present application may be implemented in various different forms and is not limited to the embodiments described herein. In order to clearly explain the present application in the drawings, parts that are not related to the description are omitted, and similar reference numerals are assigned to similar parts throughout the specification.

Throughout this specification, when a part is said to be “connected” to another part, this includes not only the case where it is “directly connected,” but also the case where it is “electrically connected” with another element in between. do.

Throughout this specification, when a member is said to be located “on”, “above”, “at the top”, “below”, “at the bottom”, or “at the bottom” of another member, this means that a member is located on another member. This includes not only cases where they are in contact, but also cases where another member exists between two members.

Throughout the specification of the present application, when a part is said to “include” a certain element, this means that it may further include other elements rather than excluding other elements, unless specifically stated to the contrary.

Throughout the specification of the present application, when a part “includes” a certain element, this means that it may further include other elements rather than excluding other elements, unless specifically stated to the contrary.

As used herein, the terms "about", "substantially", etc. are used to mean at or close to the numerical value when the synthetic and material tolerances inherent in the stated meaning are presented, and to aid the understanding of the present application. It is used to prevent unscrupulous infringers from unfairly exploiting disclosures in which precise or absolute figures are mentioned. Additionally, throughout the specification herein, “a step of” or “a step of” does not mean “a step for.”

Throughout this specification, the term "combination thereof" included in the Markushi format expression means a mixture or combination of one or more components selected from the group consisting of the components described in the Markushi format expression, It means including one or more selected from the group consisting of.

Throughout this specification, description of “A and/or B” means “A or B, or A and B.”

Hereinafter, the biomarker composition for diagnosing adult-onset Still's disease (AOSD) containing the TLR2 protein of the present application will be described in detail with reference to embodiments and examples and drawings. However, the present application is not limited to these embodiments, examples, and drawings.

As a technical means for achieving the above-described technical problem, a first aspect of the present application provides a biomarker composition for diagnosing adult-onset Still's disease containing the TLR2 protein.

Adult-onset Still's disease (AOSD) has been reported all over the world since it was reported by Bywaters in 1971, and is characterized by fever, arthritis, rash, joint pain or arthritis, and leukocytosis. It is an inflammatory disease that manifests as symptoms, and its pathogenesis has not been clearly identified.

The diagnosis of Still's disease is mainly based on clinical findings, including high fever, joint pain or arthritis, characteristic skin lesions, lymphadenopathy, hepatomegaly, splenomegaly, serositis and sore throat, leukocytosis, increased blood needle rate, and antinuclear symptoms. Diagnosis is made through laboratory findings such as antibody negativity and rheumatoid factor negativity.

Most of the research being done on adult-onset Still's disease is a simple Enzyme-LinKed ImmunoSpecific Assay (ELISA) study or genetic study on inflammatory cytokines and acute reactor substances using the patient's serum, and is based on systematic biomarkers. There was no report about it. In addition, due to a lack of understanding of the pathogenic mechanism, treatment relies on experience and there is no consensus on this.

Accordingly, there is a need for research on biomarkers that can easily diagnose adult-onset Still's disease in the early stages without using biopsy or imaging technology.

Biomarkers are molecular information based on single molecules or patterns of molecules derived from DNA, RNA, metabolites, proteins and protein fragments, and detect changes in the body caused by genetic or epigenetic changes in the body. It means an indicator that can be done. Proteomics are protein biomarkers that exist in the patient's serum and have important value as biomarkers due to their ease of detection.

According to the above-described problem solving means of the present application, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can accurately and quickly diagnose adult-onset Still's disease, which is difficult to diagnose.

According to one embodiment of the present application, the composition may additionally include TLR7 protein, but is not limited thereto.

Specifically, the biomarker composition for diagnosing adult-onset Still's disease according to the present application was discovered and verified by discovering the difference in the frequency of cells expressing TLR2 or TLR7 between normal people and patients with adult-onset Still's disease.

Specifically, in one embodiment of the present invention, when comparing peripheral blood mononuclear cells (PBMC) of patients with adult-onset Still's disease with normal controls, the frequency of cells expressing TLR2 and the frequency of cells expressing TLR7 were determined. It was confirmed that the frequency was higher (Example 2).

The TLR2 (or Toll-like receptor 2) refers to a protein encoded by the TLR2 gene in humans. TLR2 was also designated CD282 (cluster of differentiation 282). TLR2 is one of the Toll-like receptors and plays a role in the immune system. In particular, the sequence of the human TLR2 protein is provided in NCBI database entry NP_003255 (May 25, 2014).

The TLR2 (or Toll-like receptor 2) refers to a protein encoded by the TLR2 gene in humans. TLR2 is one of the Toll-like receptors and plays a role in the immune system. In particular, the sequence of the human TLR2 protein is provided in NCBI database entry NP_003255 (dated May 30, 2021).

The TLR7 (or Toll-like receptor 7) refers to a protein encoded by the TLR7 gene in humans. TLR7 is one of the Toll-like receptors and plays a role in the immune system. In particular, the sequence of the human TLR7 protein is provided in NCBI database entry NP_057646 (dated May 3, 2021).

The diagnosis refers to confirming the presence or characteristics of a pathological condition, determining the susceptibility of an object, that is, a test subject, to a specific disease or disorder, and determining whether an object currently has a specific disease or condition. To determine the prognosis (e.g., to determine the stage of progression or to determine the responsiveness of a disease to treatment) of a particular disease or subject with a condition, or to determine therametrics (e.g., to determine the efficacy of a treatment). Includes monitoring the status of an object to provide information about it.

For example, the above diagnosis may be interpreted as confirming the occurrence of adult-onset Still's disease, but is not limited thereto.

According to one embodiment of the present application, the adult-onset Still's disease may include, but is not limited to, arthritis.

Specifically, in one embodiment of the present invention, it was confirmed that the TLR2 frequency of total cells in patients with adult-onset Still's disease was correlated with the whole body score, LDH level, and ferritin level, and that TLR2 frequency was correlated with the whole body score, LDH level, and ferritin level in AOSD patients with arthritis. It was confirmed that the expression level was significantly high (Example 3).

Therefore, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can accurately and quickly diagnose adult-onset Still's disease with specific disease activity markers (whole body score, LDH level, and ferritin level) and specific clinical symptoms (arthritis). There is an advantage.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can easily diagnose adult-onset Still's disease using non-invasive biological samples without using biopsy or imaging technology, so it can be convenient and economical. .

In addition, the biomarker composition for diagnosing adult-type Still's disease according to the present application can be useful for disease onset, disease progression, disease diagnosis, and prognosis prediction, so it explains the etiology of the disease and reflects the activity of the disease. Disease-specific biomarkers can be provided.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present invention can be useful for initial diagnosis, determination of severity, reflection of disease activity, evaluation of treatment efficacy, confirmation of efficacy of drugs, and determination of the presence or absence of other accompanying diseases such as infectious diseases. Therefore, there is an advantage in increasing the treatment efficiency of adult-type Still's disease treatment.

In addition, the biomarker composition for diagnosing adult-onset Still's disease according to the present application can be usefully used to distinguish adult-onset Still's disease from other similar lesions (mimickers).

Specifically, in one embodiment of the present invention, as a result of immunohistochemical staining of skin lesions and lymph node (LN) samples from AOSD patients, the average percentage of inflammatory cells expressing TLR2 or TLR7 is a feature that distinguishes them from other similar lesions (mimickers). It was confirmed that it had (Example 4 and Example 5).

A second aspect of the present application provides a kit for diagnosing adult-onset Still's disease comprising an antibody that specifically binds to the TLR2 antigen protein or the TLR7 antigen protein.

Regarding the kit for diagnosing adult-onset Still's disease of the second aspect of the present application, detailed description of parts overlapping with the first aspect of the present application has been omitted. However, even if the description is omitted, the contents described in the first aspect of the present application are the same as those of the present application. The same can be applied to the second aspect.

The antigen refers to an antibody and a protein-based immunogen capable of performing antigen-antibody binding. These antigens can be synthesized, isolated and purified through genetic recombination methods using conventional methods.

According to one embodiment of the present application, the antibody may be a monoclonal antibody (monoclonal antibody) or a polyclonal antibody (polyclonal antibody), but is not limited thereto.

The monoclonal antibody can be produced by techniques for producing immortalized cell lines by fusion known to those skilled in the art. For example, mice are immunized with the protein expressed by the above gene, or a peptide is synthesized and combined with bovine serum albumin to immunize mice. Immortalized hybridomas are created by fusing antigen-producing B lymphocytes isolated from mice with human or mouse myeloma, and the hybridoma cells are used for indirect enzyme-linked immunosorbent assay (enzyme-linked immunosorbent assay). Monoclonal antibodies can be produced by checking the production of monoclonal antibodies using linked immunoabsorbent assays (ELISA), selecting positive clones, culturing them, and then separating and purifying the antibodies or injecting them into the abdominal cavity of rats and collecting ascites. there is.

The monoclonal antibody is generally quantified by color development using secondary antibodies and their substrates coupled with enzymes such as alkaline phosphatase (AP) or horseradish peroxidase (HRP). Analysis can be performed, or quantitative analysis can be performed directly using a monoclonal antibody against the protein coupled to AP or HRP enzyme. Additionally, antibodies with various fluorescent labels, including fluorescein isothiocyanate (FITC) and phycoerythrin (PE), can be used.

The polyclonal antibody can be produced by injecting TLR2 or TLR7 protein or a fragment thereof as an immunogen into an external host according to a method known to those skilled in the art. External hosts include mammals such as mice, rats, sheep or rabbits. Immunogens are injected intramuscularly, intraperitoneally, or subcutaneously, and are generally administered with an adjuvant to increase antigenicity. Serum is collected regularly from external hosts, and sera showing improved titer and specificity for antigens are collected or antibodies are separated and purified therefrom.

According to one embodiment of the present application, the kit may be used to diagnose adult-onset Still's disease by detecting TLR2 protein or TLR7 protein in a sample using an antigen-antibody binding reaction, but is not limited thereto.

Specifically, the kit can be used to diagnose the onset of adult-onset Still's disease by measuring the level of TLR2 protein or TLR7 protein in a sample derived from an individual with adult-onset Still's disease.

The kit uses an antigen-antibody binding reaction to analyze the final signal strength of the sample through an antigen-antibody complex detection process, and if it is higher than the signal of the normal control sample, it is used to diagnose Sjögren's syndrome or to determine the course of treatment. can do.

The kit may further include one selected from antigens, antibodies, aptamers, and one or more other component compositions, solutions, devices, and combinations thereof suitable for analysis methods for measuring the level of the TLR2 protein or TLR7 protein. However, it is not limited to this.

For example, for the detection of the antigen-antibody complex, the kit may label the antigen with a labeling substance described later, or use a detection antibody or secondary antibody, and may additionally include a buffer solution, a chromogenic substrate solution, etc. , but is not limited to this.

For example, the detection antibody specifically binds to human IgG or IgA, and the detection antibody may be labeled with a substance that can be detected visually or using various image detection equipment, but is not limited thereto.

For example, the antigen or the detection antibody may be a labeling agent such as peroxidase such as horseradish peroxidase, alkaline phosphatase, glucose oxidase, and beta-galactosidase. beta-galactosidase, urease, catalase, asparginase, ribonuclease, malate dehydrogenase, staphylococcal nuclease staphylococcal nuclease, triose phospate isomerase, glucose-6-phosphate dehydrogenase, glucoamylase or acetylcholine esterase ) may be labeled with an enzyme that catalyzes a chemical reaction in the presence of a specific substrate, producing a detectable color reaction or emitting light, but is not limited thereto.

For example, the antigen or the detection antibody is viroluminescence, chemiluminescence, electroluminescence, electrochemilluminescence or photoluminescence, which emits light of a different wavelength from the irradiated light by irradiation of light. Chromophores used in nessens include, for example, green fluorescent protein as a protein or fluorescein isothiocyanate, rhodamine, phycoerythrin, and phycocyanin (as an organic compound). It may include, but is not limited to, phycocyanin, allophycocyanin, or fluorecamine.

For example, the antigen or the detection antibody may be labeled with various radioisotope substances, but are not limited thereto.

For example, detection of the label may be performed by a scintillation counter if the label is a radioisotope, and if the label is a fluorescent substance, spectroscopy, a phosphoimaging device, or It can be performed by methods such as a fluorometer, and when labeled with an enzyme, it can be performed by measuring the coloring product that appears by conversion of the chromogenic substrate by the enzyme in the presence of an appropriate substrate, and comparing it with an appropriate standard or control. Through comparison, it can be detected by comparing the color of the coloring product that appears by the enzyme reaction, but is not limited to this.

For example, the coloring substrate solution may be ABTS (2,2'-azino-bis(3-ethylbenzothiazoline-6-sulfonic acid)), OPD (o-phenylenediamine), or TMB (tetramethyl benzidine). However, it is not limited to this.

Additionally, the kit may include, but is not limited to, reagents such as reagents necessary for performing negative and positive control reactions or buffers required for hybridization reactions. The optimal amount of reagent to be used in a particular reaction can be easily determined by a person skilled in the art after reading the contents of this specification. For example, the kit of the present invention may include the above-described components in a separate package or compartment, but is not limited thereto.

In addition, in the kit according to the present disclosure, the antigen is a microwell plate such as a 96 well microwell plate, beads or particles containing colloidal gold particles or colored latex particles, or cellulose, nitrocellulose, polyethersulfone, polyvinylidine, It may be attached to membranes such as fluoride, nylon, charged nylon, and polytetrafluoroethylene, but is not limited thereto. The method of attaching or coating may be a known method, for example, reference may be made to those described in the Examples herein.

According to one embodiment of the present application, the sample is from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. It may include those selected, but is not limited thereto.

Specifically, according to one embodiment of the present application, the sample may be peripheral blood mononuclear cells (PBMC) isolated from an individual, but is not limited thereto.

The subject refers to a person suspected of having adult-onset Still's disease, a person suffering from adult-onset Still's disease, or a person receiving treatment after being diagnosed with adult-onset Still's disease.

Specifically, the sample refers to a direct object isolated from the individual and measuring the expression level of the TLR2 protein or TLR7 protein. These samples are not particularly limited as long as the TLR2 protein or TLR7 protein can be detected, and refer to a substance or mixture of substances containing one or more detectable components, such as cells, tissues or body fluids derived from living organisms, especially humans. Examples include, but are not limited to, body fluids such as saliva and tears, whole blood, plasma, and serum.

For example, the sample may be blood, serum, or plasma of a patient with adult-onset Still's disease, specifically, peripheral blood mononuclear cells, but is not limited thereto.

According to one embodiment of the present application, the method for detecting the TLR2 protein or TLR7 protein includes Western blot, enzyme-linked immunosorbent assay (ELISA), dot blot assay, radioimmunoassay, radioimmunodiffusion assay, and Ouchterony immunoassay. A method selected from the group consisting of diffusion method, rocket immunoelectrophoresis, tissue immunostaining, immunoprecipitation assay, complement fixation assay, FLOW CYTOMETRY ANALYSIS (FACS), protein chip, sandwich assay, and combinations thereof. It may be performed using, but is not limited to this.

The detection includes quantitative and/or qualitative analysis, including detection of presence and absence, and measurement of concentration. Such methods are known in the art, and those skilled in the art will be able to select an appropriate method for the practice of the present application. .

For example, the method for detecting the TLR2 protein or TLR7 protein may be Western blot, enzyme-linked immunosorbent assay (ELISA), or dot blot assay, but is not limited thereto.

For example, the method involves binding antigen to a solid substrate, such as beads, membranes, slides, or microwell plates made of glass, plastic (e.g., polystyrene), polysaccharide, nylon, or nitrocellulose. After adding the sample, it is labeled with a label capable of direct or indirect detection, such as radioactive substances such as 3H or 125I, fluorescent substances, chemiluminescent substances, haptens, biotin, digoxigenin, etc., or has an effect on the substrate. It can be detected qualitatively or quantitatively through binding to antibodies conjugated with enzymes such as horseradish peroxidase, alkaline phosphatase, and malate dehydrogenase, which can develop color or emit light.

For example, the ELISA kit may further include a reagent capable of detecting bound antibodies, for example, a secondary detection antibody labeled with substances such as chromophores, enzymes, etc., and a substrate used for detection. However, it is not limited to this.

In addition, the kit according to the present application may additionally include instructions on how to use, and may additionally include, but is not limited to, a reagent capable of detecting antibodies specific to the control group or bound antibodies.

The third aspect of the present application includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease; Comparing the measured frequency with the frequency of a normal control sample; And information for diagnosing adult-onset Still's disease, including the step of diagnosing adult-onset Still's disease when the frequency of cells expressing TLR2 or TLR7 is increased in the sample of the individual suspected of having adult-onset Still's disease compared to the control group. Provides a method of provision.

Regarding the method of providing information for diagnosing adult-onset Still's disease in the third aspect of the present application, detailed description of parts overlapping with the first and second aspects of the present application has been omitted, but even if the description is omitted, the first aspect of the present application The contents described in the first and second aspects can be equally applied to the third aspect of the present application.

For example, if the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease is significantly increased compared to the frequency of cells expressing TLR2 or TLR7 in a normal control sample, adult-onset Still's disease It can be determined that the disease has developed, and if there is no significant increase, it can be determined that the individual suspected of having adult-onset Still's disease has not developed adult-onset Still's disease, but is not limited to this.

According to one embodiment of the present application, the sample is from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. It may include what is selected, but is not limited thereto.

Specifically, according to one embodiment of the present application, the sample may be peripheral blood mononuclear cells (PBMC) isolated from an individual, but is not limited thereto.

The fourth aspect of the present application includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease; Treating the subject with a candidate substance for treating adult-onset Still's disease; and measuring the therapeutic effect of the candidate substance for the treatment of adult-onset Still's disease.

Regarding the screening method for the treatment of adult-onset Still's disease of the fourth aspect of the present application, detailed description of parts overlapping with the first to third aspects of the present application has been omitted. However, even if the description is omitted, the first aspect of the present application The contents described in the third aspect can be equally applied to the fourth aspect of the present application.

The screening method for a treatment for adult-onset Still's disease using the biomarker composition for diagnosing adult-onset Still's disease according to the present application is useful for developing a treatment for adult-onset Still's disease because it can simply and quickly screen the therapeutic effects of various candidate substances for adult-onset Still's disease. It can be utilized effectively.

According to one embodiment of the present application, measuring the therapeutic effect includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual treated with the therapeutic candidate substance; Comparing the frequency of cells expressing the TLR2 or TLR7 measured in a sample of an individual treated with the therapeutic candidate with the frequency of cells expressing the TLR2 or TLR7 measured before the step of treating the therapeutic candidate; And when the frequency of cells expressing the TLR2 or TLR7 measured in a sample of an individual treated with the therapeutic candidate decreases compared to the frequency of cells expressing the TLR2 or TLR7 measured before the step of processing the therapeutic candidate. This may include, but is not limited to, a step of considering the therapeutic candidate as a treatment for adult-onset Still's disease.

According to one embodiment of the present application, the sample is from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. It may include those selected, but is not limited thereto.

According to one embodiment of the present application, the sample may be peripheral blood mononuclear cells (PBMC) isolated from an individual, but is not limited thereto.

The present invention will be described in more detail through the following examples. However, the following examples are for illustrative purposes only and are not intended to limit the scope of the present application.

[Example 1] Experiment preparation

[Example 1-1] Subject selection

Figure 1 is a table showing clinical characteristics of clinical test subjects.

Specifically, 20 patients with adult-onset Still's disease (AOSD) and 15 healthy controls (HC) participated. Patients with AOSD were diagnosed according to Yamaguchi diagnostic criteria after excluding infections, other autoimmune diseases, and malignancies. HCs were healthy individuals with no history of autoimmune, rheumatic, or other malignant diseases.

[Example 1-2] Separation of peripheral blood mononuclear cells (PBMC)

PBMCs from each subject in Example 1-1 were isolated using BD Vacutainer CPT ^™ (BD Biosciences, Franklin Lakes, NJ).

[Example 2] Measurement of the frequency of cells expressing TLR2 or TLR7 in peripheral blood mononuclear cells

Figure 2 is a table showing the results of measuring the frequency of cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 in total peripheral blood mononuclear cells, and Figure 3 shows various TLR markers in total peripheral blood mononuclear cells of one AOSD patient. This image shows a representative example of a flow cytometry histogram of surface-stained cells.

Specifically, the frequencies of cells expressing various types of TLR were measured in the PBMCs isolated in Example 1-2.

More specifically, each ¹ Using flow cytometry (FACS), the number of cells to which antibodies were attached was counted, and the frequency of these cells in total cells (10,000) was analyzed.

Through this, it was confirmed that the average frequency of surface-stained cells expressing TLR2 in whole blood was significantly higher in the AOSD (1.27 ± 0.43) patient group than in the HC (0.98 ± 0.04, p < 0.001).

In addition, it was confirmed that the frequency of cells expressing TLR7 in whole blood was significantly higher in the AOSD (1.28 ± 0.29) patient group than in the HC (1.06 ± 0.86, p = 0.006).

Meanwhile, it was confirmed that there was no significant difference in the frequency of cells expressing TLR1, TLR4, or TLR9 between the AOSD group and HC.

This is because the frequency of cells expressing TLR2 and the frequency of cells expressing TLR7 is higher when PBMCs of patients with adult-onset Still's disease are compared with normal controls. By analyzing these, we can accurately and quickly diagnose adult-onset Still's disease, which is difficult to diagnose. This suggests that it can be diagnosed accurately.

[Example 3] Measurement of the frequency of cells expressing TLR2 or TLR7 according to disease activity markers or clinical manifestations in AOSD patients

Figure 4 is a table showing the correlation between the frequency of stained cells representing various TLR markers and disease activity markers or systemic scores in AOSD patients.

Through this, we found that TLR2 frequency in whole cells correlated with whole body score (r = 0.446, p = 0.049), LDH level (r = 0.728, p <0.001) and ferritin (r = 0.829, p <0.001) level. It was confirmed that TLR1 frequency was correlated with LDH (r = 0.716, p <0.001) and ferritin (r = 0.804, p <0.001).

Additionally, when we evaluated the correlation between each cell surface TLR marker in AOSD patients, we found that the frequency of TLR2 in PBMCs was higher than that of TLR4 (r = 0.838, p <0.001), TLR7 (r = 0.588, p <0.001), and TLR9 (r = 0.588, p <0.001). It was confirmed that there was a positive correlation with 0.932, p <0.001).

Figure 5 is a table showing the expression levels of various TLRs according to clinical symptoms in AOSD patients.

Through this, it was confirmed that the TLR2 expression level was significantly high in AOSD patients with arthritis as a clinical symptom.

This suggests that the biomarker composition for diagnosing adult-onset Still's disease according to the present application can accurately and quickly diagnose adult-onset Still's disease with arthritis.

[Example 4] Histopathological evaluation of skin samples from AOSD patients

Figure 6 is a table showing the results of skin biopsy of AOSD patients.

Specifically, skin biopsy samples were obtained from 32 AOSD patients, 5 eczema patients, 5 psoriasis patients, and 5 normal controls (NC) for skin rash evaluation between 2000 and 2019. collected. Lymph node biopsy samples were collected from nine AOSD patients. Subsequently, H&E staining was performed on each sample, and three pathologists independently evaluated dermatopathological parameters.

Figure 7 is a table showing the results of TLR1, TLR2, TLR4, TLR7, and TLR9 immunohistochemical staining performed in AOSD patients, eczema patients, psoriasis patients, and controls.

Specifically, TLR1, TLR2, TLR4, TLR7, and TLR9 antibodies were used as primary antibodies, respectively, and immunohistochemical staining was performed using the Ventana Optiview DAB kit (Ventana Medical Systems Inc.). IHC results were graded according to the percentage of positive lymphoid cells and histiocytes.

Through this, the average percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 in skin lesions of AOSD patients were 81.9 ± 8.2, 34.8 ± 24.1, 52.3 ± 29.8, 19.3 ± 15.7, and 40.2 ± 27.9, respectively, compared to normal The mean percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 were 70.0 ± 18.4, 6.2 ± 3.6, 77.0 ± 11.0, 9.6 ± 6.6, and 5.4 ± 4.5, respectively, in skin lesions caused by eczema. The average percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 were 70.0 ± 16.0, 27.0 ± 30.9, 75.0 ± 10.0, 24.4 ± 31.2, and 17.6 ± 20.2, respectively. The average percentages of inflammatory cells expressing TLR4, TLR7, and TLR9 were found to be 72.0 ± 5.7, 27.2 ± 21.4, 64.0 ± 11.4, 19.3 ± 15.7, and 7.4 ± 9.9, respectively.

According to comparative analysis, it was confirmed that the proportion of inflammatory cells expressing TLR2 in skin lesions of AOSD patients was significantly greater than that in the control group (HC) (p = 0.002).

Figure 8: Inflammatory cell grade (CD4/CD8/CD68 staining) in the skin of AOSD patients; and a table showing the correlation between the average percentage of inflammatory cells expressing CXCL9, CXCL10, CXCL11, CXCR3, CXCL12, and CXCR4 and the average percentage of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9.

Through this, it was confirmed that the proportion of inflammatory cells expressing TLR2 in the skin of AOSD patients was positively correlated with the average percentage of inflammatory cells expressing CXCL10 (r = 0.467, p = 0.021).

Figure 9 is a graph showing the results of evaluating the correlation between TLR markers in the skin of AOSD patients.

Through this, it was confirmed that the frequency of TLR2 in the skin of AOSD patients was positively correlated with TLR4 (r = 0.370, p = 0.037) and TLR9 (r = 0.398, p = 0.024).

In summary, this suggests that the biomarker composition for diagnosing adult-onset Still's disease according to the present application can be usefully used to distinguish adult-onset Still's disease from other similar lesions (mimickers).

[Example 5] Immunohistochemical staining of lymph node (LN) samples from AOSD patients

Figure 10 is a table showing the results of lymph node biopsy in AOSD patients. Specifically, the results of TLR1, TLR2, TLR4, TLR7, and TLR9 immunohistochemical staining performed in AOSD patients, T-cell lymphoma patients, histiocytic necrotic lymphadenitis patients, tuberculous lymphadenitis patients, non-specific reactive hyperplasia patients, and control groups are shown. It's a ticket.

The lymph node biopsy samples were from 9 AOSD patients, T cell lymphoma patients, histiocytic necrotizing lymphadenitis (HNL, kikuchi disease) patients, tuberculous lymphadenitis (Tbc lymphadenitis) patients, and Collected from patients with nonspecific reactive hyperplasia. Next, H&E staining was performed on each sample, and three pathologists independently evaluated dermatopathological parameters.

TLR1, TLR2, TLR4, TLR7, and TLR9 antibodies were used as primary antibodies, respectively, and immunohistochemical staining was performed using the Ventana Optiview DAB kit (Ventana Medical Systems Inc.). IHC results were graded according to the percentage of positive lymphoid cells and histiocytes.

Through this, the average percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 in the lymph nodes of AOSD patients were 34.4 ± 17.9, 17.3 ± 16.6, 31.1 ± 13.6, 27.2 ± 20.0, and 18.3 ± 9.7, respectively, and reactive lymph nodes (Reactive Lymph Node, reactive LNs) The mean percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 in patients were 7.6 ± 7.6, 8.6 ± 4.7, 12.2 ± 7.2, 8.0 ± 2.7, and 2.6 ± 1.7, respectively; The mean percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 were 13.2 ± 13.2, 6.8 ± 5.7, 44.0 ± 26.0, 32.0 ± 4.5, and 11.2 ± 11.2, respectively, in the lymph nodes of patients with tuberculosis lymphoma and T-cell lymphoma. The mean percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 in patients were 9.2 ± 6.2, 20.0 ± 31.8, 4.4 ± 3.4, 8.2 ± 7.2, and 3.6 ± 4.0, respectively, in lymph nodes of patients with histiocytic necrotic lymphadenitis. The average percentages of inflammatory cells expressing TLR1, TLR2, TLR4, TLR7, and TLR9 were found to be 24.0 ± 12.9, 4.8 ± 3.0, 52.0 ± 17.5, 49.0 ± 12.5, and 21.0 ± 19.2, respectively.

According to comparative analysis, the proportion of inflammatory cells expressing TLR2 in the lymph nodes of AOSD patients was significantly greater than that in the lymph nodes (kikuchi) of lymphadenitis patients (p = 0.042), and TLR4 and TLR7 were found in the lymph nodes of AOSD patients. And the proportion of inflammatory cells expressing TLR9 was confirmed to be significantly higher than that in T cell lymphoma patients (p = 0.001) and reactive lymph node patients (p = 0.012).

In summary, this suggests that the biomarker composition for diagnosing adult-onset Still's disease according to the present application can be usefully used to distinguish adult-onset Still's disease from other similar lesions (mimickers).

The description of the present application described above is for illustrative purposes, and those skilled in the art will understand that the present application can be easily modified into other specific forms without changing its technical idea or essential features. Therefore, the embodiments described above should be understood in all respects as illustrative and not restrictive. For example, each component described as unitary may be implemented in a distributed manner, and similarly, components described as distributed may also be implemented in a combined form.

The scope of the present application is indicated by the claims described below rather than the detailed description above, and all changes or modified forms derived from the meaning and scope of the claims and their equivalent concepts should be construed as being included in the scope of the present application.

Claims (16)

Biomarker composition for diagnosing adult-onset Still's disease containing TLR2 protein.
According to paragraph 1,
A biomarker composition for diagnosing adult-onset Still's disease, wherein the adult-onset Still's disease includes the manifestation of arthritis.
According to paragraph 1,
A biomarker composition for diagnosing adult-onset Still's disease, wherein the composition further includes TLR7 protein.
A kit for diagnosing adult-type Still's disease containing an antibody that specifically binds to the TLR2 antigen protein or the TLR7 antigen protein.
According to claim 4,
A kit for diagnosing adult-type Still's disease, wherein the antibody is a monoclonal antibody or polyclonal antibody.
According to claim 4,
The kit is a kit for diagnosing adult-onset Still's disease by detecting TLR2 protein or TLR7 protein in a sample using an antigen-antibody binding reaction.
According to claim 6,
The sample includes one selected from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph fluid, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. , Adult-type Still’s disease diagnostic kit.
According to claim 6,
A kit for diagnosing adult-onset Still's disease, wherein the sample is peripheral blood mononuclear cells (PBMC) isolated from an individual.
According to claim 6,
Methods for detecting the TLR2 protein or TLR7 protein include Western blot, enzyme-linked immunosorbent assay (ELISA), dot blot assay, radioimmunoassay, radioimmunodiffusion method, Ouchteroni immunodiffusion method, rocket immunoelectrophoresis, It is performed using a method selected from the group consisting of tissue immunostaining, immunoprecipitation assay, complement fixation assay, FLOW CYTOMETRY ANALYSIS (FACS), protein chip, sandwich assay, and combinations thereof. , Adult-type Still’s disease diagnostic kit.
Measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease;
Comparing the measured frequency with the frequency of a normal control sample; and
Diagnosing adult-onset Still's disease when the frequency of cells expressing TLR2 or TLR7 increases in a sample of an individual suspected of having adult-onset Still's disease compared to the control group;
Method of providing information for diagnosis of adult-onset Still's disease, including.
According to claim 10,
The sample includes one selected from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph fluid, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. , Method of providing information for diagnosis of adult-onset Still's disease.
According to claim 10,
A method of providing information for diagnosing adult-onset Still's disease, wherein the sample is peripheral blood mononuclear cells (PBMC) isolated from an individual.
Measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual suspected of having adult-onset Still's disease;
Treating the subject with a candidate substance for treating adult-onset Still's disease; and
Measuring the therapeutic effect of the candidate substance for the treatment of adult-onset Still's disease;
A screening method for a treatment for adult-onset Still's disease comprising.
According to claim 13,
Measuring the therapeutic effect includes measuring the frequency of cells expressing TLR2 or TLR7 in a sample of an individual treated with the therapeutic candidate;
Comparing the frequency of cells expressing the TLR2 or TLR7 measured in a sample of an individual treated with the therapeutic candidate with the frequency of cells expressing the TLR2 or TLR7 measured before the step of treating the therapeutic candidate; and
When the frequency of cells expressing TLR2 or TLR7 measured in a sample of an individual treated with the therapeutic candidate decreases compared to the frequency of cells expressing TLR2 or TLR7 measured before the step of processing the therapeutic candidate, Considering the therapeutic candidate as a treatment for adult-type Still's disease;
A screening method for a treatment for adult-onset Still's disease, comprising:
According to claim 13,
The sample includes one selected from the group consisting of whole blood, serum, plasma, tissue, saliva, tears, urine, sputum, lymph fluid, cerebrospinal fluid, interstitial fluid, bone marrow fluid, ascites, and combinations thereof isolated from an individual. , Screening method for treatments for adult-onset Still's disease.
According to claim 13,
A screening method for a treatment for adult-onset Still's disease, wherein the sample is peripheral blood mononuclear cells (PBMC) isolated from an individual.