CN111068040B - Application of inhibitor SC-4-SC-15 of Cyr61/CCN1 protein epitope polypeptide - Google Patents
Application of inhibitor SC-4-SC-15 of Cyr61/CCN1 protein epitope polypeptide Download PDFInfo
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Abstract
The invention discloses a Cyr61/CCN1 protein epitope polypeptide and application thereof in preparing a medicament for detecting or treating rheumatoid arthritis synovial cell hyperplasia, psoriasis epidermal cell hyperplasia and inflammatory diseases, wherein the amino acid sequence of the polypeptide is shown as SEQ ID NO.1 and SEQ ID NO. 2. The invention also discloses a specific anti-Cyr 61/CCN1 monoclonal antibody combined with the Cyr61/CCN1 protein epitope polypeptide and a Cyr61/CCN1 protein epitope polypeptide inhibitor. The Cyr61/CCN1 protein epitope polypeptide and related new drugs thereof have wide application prospects.
Description
The application is a divisional application of Chinese invention patent application with the application number of 201410152740.7 (the divisional application has the application number of 201610897943.8, the name of "Cyr61/CCN1 protein epitope polypeptide and inhibitor and monoclonal antibody thereof and application thereof"), the name of "Cyr61/CCN1 protein epitope polypeptide and inhibitor and monoclonal antibody thereof and application thereof", the filing application requires the priority of Chinese invention patent application with the application date of 2014 02, 08, the application number of 201410045817.0, the name of "Cyr61/CCN1 protein epitope polypeptide and inhibitor and monoclonal antibody thereof and application thereof".
Technical Field
The invention belongs to the field of medicines, and relates to Cyr61/CCN1 protein epitope polypeptide and application thereof in preparation of medicines for detecting or treating Rheumatoid Arthritis (RA) synovial cell (FLS) hyperplasia, psoriasis epidermal cell hyperplasia and inflammatory diseases.
Background
Cyr61 (cysteine-rich 61), also known as CCN1, is a secreted protein of 381 amino acid residues in relative molecular mass of 42kDa, and the earliest cloned Cyr61/CCN1 was discovered by Lau et al in 1985 when stimulating mouse BALB/c 3T3 fibroblasts with serum or platelet-derived growth factor (PDGF), and was named Cyr61/CCN1 because of the rich cysteine (containing 10% cysteine residues). Cyr61/CCN1 has obvious mitogenic activity and chemotaxis, can induce fibroblast and epidermal cell to proliferate and secrete extracellular matrix, participate in regulating cell proliferation, differentiation and embryonic development and formation, and is a basic protein for life activities.
In the binding reaction of antigen and antibody, the site where the antibody is involved in binding is called para (paratope) of the antibody, and the site where the antigen (Cyr 61/CCN1 protein) is involved in binding is called epitope (epitope) of the antigen. Epitopes are the basis for protein antigenicity. The determination of the antigen epitope (small molecule peptide segment) has important significance for determining the action site of the protein, namely the small molecule peptide segment, further designing and adopting the small molecule peptide segment to simulate the action of the protein, or designing a small molecule compound capable of simulating the peptide segment to replace the action of the protein or peptide molecule, or designing the small molecule compound to block the action of the protein, and the determination is also one of the development and preparation methods of novel medicaments which are popular internationally at present.
Disclosure of Invention
The invention provides Cyr61/CCN1 protein epitope polypeptide, the amino acid sequence of which is shown as SEQ ID NO.1 and is GLECNFG.
The invention also provides Cyr61/CCN1 protein epitope polypeptide which is a cyclic peptide segment shown as SEQ ID NO.2, namely, a cysteine is added at the N end of the peptide segment of SEQ ID NO.1, thereby forming a cyclic peptide segment 'C-G LECNF G' shown as SEQ ID NO. 2.
The Cyr61/CCN1 protein epitope polypeptide is positioned at 75-81 th amino acid of Cyr61/CCN1 protein, can be combined with specific anti-Cyr 61/CCN1 monoclonal antibody 093G9 (KD is 10-7) and neutralize the functions of Cyr61/CCN1 in vitro and in vivo, and can be artificially synthesized into a cyclic peptide segment 'C-G LECNF G' when a C is added at the N end.
In the invention, the Cyr61/CCN1 protein epitope polypeptide can be prepared by hydrolyzing protease, and the Cyr61/CCN1 protein epitope polypeptide can also be prepared by synthesizing by a conventional solid phase polypeptide synthesis method or a genetic engineering technology.
In the invention, the full-length sequence (GenBank: M _ 001554) of human Cyr61/CCN1 protein obtained by searching a gene library is shown as SEQ ID NO. 3:
wherein the sequence in the black box is a signal peptide of Cyr61/CCN1 protein.
The invention also provides a specific anti-Cyr 61/CCN1 monoclonal antibody, and the specific anti-Cyr 61/CCN1 monoclonal antibody can be combined with the Cyr61/CCN1 protein epitope polypeptide.
The invention also provides an inhibitor of the Cyr61/CCN1 protein epitope polypeptide, which can be combined with the Cyr61/CCN1 protein epitope polypeptide, can be combined with the GLECNFG ring structure and can block the mediated biological function.
The inhibitor of the Cyr61/CCN1 protein epitope polypeptide comprises a small molecular compound which can block the biological function of the Cyr61/CCN1 protein epitope polypeptide. Preferably, the small molecule compounds SC1-SC15 are shown in the embodiment of the invention. Specifically, a small molecular compound with the biological function of simulating and inhibiting the peptide fragment can be designed according to the conformational epitope of the peptide fragment of the Cyr61/CCN1 protein epitope polypeptide. The small molecular compound capable of blocking the polypeptide peptide segment has the effect of inhibiting the molecular pathobiology of Cyr61/CCN1, and has important application in further developing into a lead compound and preparing medicaments for resisting synovium hyperplasia and bone destruction, resisting Cyr61/CCN1 high-expression breast cancer cell proliferation, resisting epidermal cell hyperproliferation and resisting fibrosis (such as hepatic fibrosis). The inhibitor can be combined with a GLECNF6 ring structure and can block the mediated pathological effects (including causing inflammation, causing fibroblast proliferation, causing proliferation and metastasis of Cyr61/CCN1 high-expression breast cancer cells, causing proliferation and activation of epidermal cells and the like).
Previous studies of the present invention have shown that IL-17 is capable of upregulating Cyr61/CCN1 expression, whereas upregulating Cyr61/CCN1 expression promotes the hyperproliferation of synovial cells upon binding to the integrin receptor AvB5, which is indicated by synovial cells, and can promote the synthesis of metalloproteinase 3 and metalloproteinase 9 and thus be involved in cartilage and bone destruction. The research of the invention shows that Cyr61/CCN1 protein can directly promote synovial cells to produce IL-6, thereby participating in the generation and development of inflammation. Furthermore, the research of the invention shows that Cyr61/CCN1 can also promote the human epidermal cell proliferation and participate in the psoriasis. In the animal experiment of the invention, cyr61/CCN1 is also found to mediate the occurrence of sicca syndrome and proliferative inflammatory bowel disease. Experiments prove that the protein expression can be inhibited by neutralizing the anti-Cyr 61/CCN1 monoclonal antibody and the protein expression, so that the clinical symptoms and tissue damage and inflammation of arthritis in a CIA model can be relieved; inhibiting epidermal cell proliferation, relieving skin thickening and scale generation of psoriasis-like mice, and relieving inflammation and clinical symptoms of xerosis syndrome and proliferative enteropathy animal model.
The monoclonal antibody capable of binding Cyr61/CCN1 protein is prepared by the invention. These antibodies show differences in function due to the epitopes bound by these different monoclonal antibodies, i.e., different parts of the Cyr61/CCN1 protein.
The invention also provides application of the Cyr61/CCN1 protein epitope polypeptide in preparing medicaments for detecting and/or treating inflammatory diseases. Preferably, the inflammatory disease comprises rheumatic diseases, rheumatoid arthritis, psoriasis. Preferably, the inflammatory disease comprises sjogren's syndrome. Preferably, the inflammatory disease comprises a proliferative inflammatory bowel disease.
The invention also provides application of the Cyr61/CCN1 protein epitope polypeptide in preparing a medicament for resisting rheumatoid arthritis synovial cell hyperplasia. The embodiment of the invention shows that the monoclonal antibody 093G9 capable of specifically neutralizing the epitope can inhibit synovial cell proliferation of rheumatoid arthritis and animal models thereof, inhibit epidermal cell proliferation of psoriasis and animal models thereof, inhibit symptoms and inflammation of sjogren syndrome animal models, and inhibit inflammation and symptoms of proliferative inflammatory bowel disease animal models in vivo and in vitro.
The invention also provides application of the Cyr61/CCN1 protein epitope polypeptide in preparing a medicament for inhibiting high expression of breast cancer cells. The embodiment of the invention shows that the monoclonal antibody 093G9 capable of specifically neutralizing the epitope of Cyr61/CCN1 protein can inhibit proliferation, migration and invasion of breast cancer cells with high expression of Cyr61/CCN1 protein in vivo and in vitro, and can inhibit the growth and lymphatic metastasis of the type of tumor in an animal model (in vivo).
The invention also provides application of the Cyr61/CCN1 protein epitope polypeptide in preparing anti-fibrosis drugs.
The invention also provides application of the Cyr61/CCN1 protein epitope polypeptide in preparing anti-psoriasis medicines. The embodiment of the invention shows that the monoclonal antibody 093G9 capable of specifically neutralizing the epitope can inhibit epidermal cell proliferation, skin thickening and scale generation of psoriasis-like mice in vivo and in vitro.
The invention also provides application of the inhibitor of the Cyr61/CCN1 protein epitope polypeptide in preparing a medicament for treating rheumatic diseases.
Functional analysis of the epitope located on Cyr61/CCN1 protein of the present invention showed that the cyclic peptide of the recognition peptide fragment of antibody 093G9 has the effect of stimulating the in vitro proliferation of the rheumatoid synovial cells, while the recognition epitope of control antibody 096B7 does not have such a property, as shown in FIG. 1.
The obtained antibody recognition epitope is artificially synthesized into peptide fragments, and the peptide fragments are added into cell culture to observe the biological characteristics of the peptide fragments. The result shows that certain peptide segments can inhibit the in vitro proliferation of synovial cells and Cyr61/CCN1 high-expression breast cancer cell strains, and the peptide segments have the function of simulating anti-Cyr 61/CCN1 monoclonal antibody. Therefore, the peptide fragments and the compound micromolecules capable of being combined with the peptide fragments have the function of inhibiting Cyr61/CCN1 protein and pharmaceutical potential.
The beneficial effect of the invention also includes the application of the Cyr61/CCN1 protein epitope polypeptide in researching and developing new drugs for treating rheumatoid arthritis, psoriasis, sicca syndrome and proliferative inflammatory bowel disease. The incidence of rheumatoid arthritis is as high as 0.4-1% in China; the morbidity of psoriasis in Chinese people is as high as 0.3-0.5%, and the morbidity of psoriasis in Caucasian people is higher (for example, the morbidity of the United states is 1-3%, and the morbidity of Norwegian is as high as 7%), so that the Cyr61/CCN1 protein epitope polypeptide and a new medicament developed according to the epitope have wide application prospects.
The significance of the epitope of the peptide fragment G LECNF G (114, cyclic peptide is 111) of the invention is as follows: according to "Trends Biochem Sci.2008October;33 (10): 461-473 "report sequence: amino acids 75-81 of IGFBP region of CCN family molecule sequence contain three conservative amino acids of G L C.
Of the above, 7 amino acids in the painted part are conserved sequences of the molecules of this family (CCN 1-6), but 093G9 binds only to Cyr61/CCN1. Although the G LECNF G is located only on Cyr61/CCN1 and is a specific recognition epitope of 093G9, the conserved sequence G-L-C is present in all CCN families. According to the experimental results of 093G9 binding not to the linear peptide G LECNF G, but only to the cyclic peptide C G LECNF G, it is suggested that although the conformational epitope formed by the cyclic peptide C-G-L-C may be located in the CCN family of molecules, G LECNF G is a specific epitope with pathogenic effect.
Biological significance of the epitopes of the invention include:
the cyclic peptide 111 can stimulate in vitro proliferation of synovial cells of RA patients and Cyr61/CCN1 high-expression breast cancer MDA-MB-231 cells, so that the peptide fragment is a specific pathogenic epitope of Cyr61/CCN1 molecules.
The monoclonal antibody 093G9 can specifically recognize an epitope in a peptide fragment (IGFBP) of Cyr61/CCN1, and the antibody 093G9 blocking the epitope has the effects of blocking the proliferation of Cyr61/CCN1 synoviocytes, high-expression breast cancer MDA-MB-231 cells and other fibroblasts.
According to the conformational epitope of the peptide fragment, a chemical small molecule (SC) which can simulate and inhibit the biological function of the peptide fragment can be designed. Wherein, the chemical small molecule (SC) capable of blocking the peptide segment has the function of inhibiting the molecular pathology and biology of Cyr61/CCN1. The compound has important application in further developing into a lead compound and preparing medicaments for resisting synovial membrane hyperplasia and bone destruction, resisting Cyr61/CCN1 high-expression breast cancer cell proliferation and resisting fibrosis (such as hepatic fibrosis).
As Cyr61/CCN1 protein is rich in cysteine and easy to form disulfide bonds, the expression is very difficult by adopting a genetic engineering method, and the peptide segment is easy to artificially synthesize, so that the protein can replace Cyr61/CCN1 molecular immunity to obtain antiserum for resisting the functional epitope or prepare a corresponding monoclonal antibody for further clinical detection and application in treatment.
The present invention is directed to protecting the sequence of polypeptide 111, the steric structure (including linear and cyclic structures) that may be generated by the sequence, and small molecule compounds that bind thereto and produce the same effects (e.g., promoting synovial cell proliferation, producing antibodies after immunization that can inhibit collagen-induced arthritis (CIA) mouse inflammation, etc.) or directly inhibit the function of these peptide fragments.
Drawings
FIG. 1 shows a schematic diagram of the mimic conformation and chemical structure of a polypeptide of the present invention, wherein (A) shows polypeptide 114 in a linear conformation; (B) polypeptide 111 in a cyclic conformation; (C) represents the chemical structure of the polypeptide 111.
FIG. 2 shows the results of an experiment in which the polypeptide of the present invention stimulates the proliferation of RA synovial cells in vitro.
FIG. 3 shows the results of an experiment in which the polypeptide of the present invention stimulates MDA-MB-231 cell proliferation.
FIG. 4 shows the inhibitory effect of the small molecule compound of the present invention on peptide fragment-stimulated synovial cell proliferation, wherein (A) shows that 15 chemical small molecules (SC 1-15) respectively inhibit the peptide fragment 111-stimulated synovial cell proliferation; (B) Shows that 15 chemical small molecules (SC 1-15) respectively have obvious inhibition on the synovial cell proliferation stimulated by Cyr61/CCN1 protein.
FIG. 5 shows the inhibitory effect of the small molecule compound of the present invention on the proliferation of the peptide-stimulated breast cancer cell line MDA-MB-231, wherein (A) shows that 15 chemical small molecules (SC 1-15) significantly inhibit the in vitro proliferation of the peptide-111-stimulated breast cancer cell line MDA-MB-231; (B) Shows that 15 chemical small molecules (SC 1-15) respectively inhibit the in vitro proliferation of a breast cancer cell strain MDA-MB-231 stimulated by Cyr61/CCN1 protein.
Detailed Description
The present invention will be described in further detail with reference to the following specific examples and drawings, and the present invention is not limited to the following examples. Variations and advantages that may occur to those skilled in the art may be incorporated into the invention without departing from the spirit and scope of the inventive concept, and the scope of the appended claims is intended to be protected. The procedures, conditions, reagents, experimental methods and the like for carrying out the present invention are general knowledge and common general knowledge in the art except for the contents specifically mentioned below, and the present invention is not particularly limited.
EXAMPLE 1 screening of epitope polypeptide of Cyr61/CCN1 protein of the present invention
In the invention, the immunoblotting method is adopted for screening: an improved traditional method for determining the epitope is adopted, namely a series of small peptide fragments of Cyr61/CCN1 are expressed in a segmented mode through genetic engineering, and then the 2 strains of antibodies are used for carrying out Western Blot (Western Blot) hybridization to screen binding epitopes, so that the peptide fragments capable of being combined with the 2 strains of Cyr61/CCN1 monoclonal antibodies are obtained.
According to the existing research result, cyr61/CCN1 protein is divided into small peptide segments with the length of about 25 amino acid segments, then primers are designed to clone the genes of the segments into escherichia coli, induction expression is carried out after correct expression sequencing, and the genes are transferred to nitrocellulose after PAGE electrophoresisOn the membrane, a mouse anti-human Cyr61/CCN1 specific monoclonal antibody 093G9 (CGMCC No) was then used.3351)And a mouse anti-human Cyr61/CCN1 specific monoclonal antibody 096B7 (CGMCC No).3299)Hybridization and color development were performed, and binding was observed. Binding is positive, otherwise negative. The binding epitopes of these two antibodies were thus determined. By the above method, the epitope to which the antibody 093G9 binds is selected to be located at amino acids 75 to 81 of Cyr61/CCN 1: cyr61/CCN1 75-81 GLECNFG. The position of this epitope in the sequence Cyr61/CCN1 (positions marked in bold):
example 2 Synthesis of Cyr61/CCN1 protein epitope Polypeptides
In the embodiment, the Cyr61/CCN1 protein epitope polypeptide is synthesized by Shanghai Qiangyao company. The basic principle is a full-automatic solid-phase synthesis method. The basic process is as follows: based on Fmoc chemical synthesis, the carboxyl of C-terminal amino acid of target polypeptide to be synthesized is connected with insoluble high molecular resin in a covalent bond mode, then the amino group of the amino acid is taken as the starting point of polypeptide synthesis and reacts with activated carboxyl of other amino acid to form peptide bond, and the process is repeated continuously to obtain the polypeptide. The synthesized polypeptide is purified by HPLC, and the purity is over 95 percent. According to the binding epitope obtained by screening, respectively synthesizing linear polypeptide and cyclic polypeptide, wherein the synthesized polypeptides are respectively: a linear polypeptide (No. 114) having the sequence GLECNFG; cyclic polypeptide (No. 111) having the sequence C GLECNFG.
Example 3 conformation and chemical Structure of Cyr61/CCN1 protein epitope polypeptide
And fitting the Cyr61/CCN1 protein epitope peptide fragment in a pure water solution by adopting Cassion molecular simulation computer software to obtain the most likely conformation formed in an in-vivo solution environment and obtain a molecular structure with a three-dimensional observation effect. The three-dimensional conformation of the Cyr61/CCN1 protein epitope polypeptide shown in figures 1 (a) and (b), wherein figure 1 (a) shows the polypeptide 114 as a linear conformation; FIG. 1 (b) shows polypeptide 111 in a circular conformation; FIG. 1 (c) shows the chemical structure of the polypeptide 111.
Example 4 Cyr61/CCN1 protein epitope Polypeptides stimulate synovial cells to proliferate in vitro
Culture and proliferation experiment of rheumatoid arthritis synovial cells
Clinical samples: all samples from the study were obtained from RA patients with clinical orthopedic knee replacement or synovectomy, and diagnosis in all cases met international diagnostic criteria. The patient synovial tissue was used for in vitro culture of cells. Clinical samples used in this study were informed of the patients.
Preparing synoviocytes and primary culture: obtaining synovial tissue aseptically, washing with PBS, and shearing into 1mm × 1mm × 1mm pieces with aseptic surgical scissors; digesting with collagenase I or collagenase II with 2-3 times of volume and 0.5mg/ml at 37 ℃ for 2 hours; after filtration through a 200 mesh gauze and centrifugation to remove the supernatant, the cells were resuspended in DMEM medium and plated in a petri dish at 37 ℃ and 5% CO 2 And (4) culturing. Then when FLS grows to be more than 80%, digesting and passaging. Observed under a microscope, the RA FLS of 3-5 generations grows rapidly, and the cell morphology tends to be long fusiform, is orderly arranged and is consistent in orientation. Detection by flow cytometry after labeling with specific lymphocyte differentiation antigens such as CD3, CD14, CD19, CD11C and the like, revealed that the above-mentioned molecules were expressed negatively (< 2% CD1Ib, < 2% CD14+, < 1% CD3+, and < 5% CD19 +), indicating that the cultured cells were homogeneous FLS with very little lymphocyte contamination.
Proliferation assay of synovial cells: taking FLS in logarithmic growth phase, digesting with 0.25% trypsin, and adjusting cell concentration to 1 × 10 4 Cells/ml, inoculated in 96-well cell culture plates, and added with the peptide fragments (final peptide fragment concentration: 2.5ug/ml,5.0ug/ml 10 ug/ml) at different concentrations. Cyr61/CCN1 intact protein was also used as a positive control (Proptech, inc., USA, san Diego). Culture medium controls were also provided. The peptide fragments or pure Cyr61/CCN1 protein were co-cultured with FLS, 1. Mu. Ci of 3H (per well) was added 16 hours before the end of the culture, the cells were collected, and proliferation was detected by beta-scintillation.
Type II collagen-induced mouse arthritis (CIA) model experiments:
the experiment for preventing the CIA mice from generating arthritis by peptide fragment immunization: the peptide fragment and CFA are completely mixed, DBA1 mice are immunized subcutaneously on the back for 3 times: for the first time: peptide + CFA, second and third: peptide + IFA (incomplete adjuvant), immunization dose: 100ug of peptide/mouse, 2-3 points of back immunization, 1 month interval each time, 7 days after the third immunization, tail blood collection, and ELISA for detecting whether antiserum is generated; meanwhile, CII100ug and the same amount of IFA are used for immunizing mice, and the morbidity, morbidity speed and inflammation intensity of the mice are observed.
Peptide fragment treatment or shock of CIA mice: namely, a CIA mouse model is prepared firstly, and the peptide segment is used for mucosal administration when the inflammation reaches 4 minutes. The method comprises the following steps: the peptide fragment is 2500ug/ml,10ul/mouse, and the final concentration is 25ug/mouse/day. Solvent was used as a negative control.
The peptide segments of the Cyr61/CCN1 protein epitope polypeptide are respectively added into synovial cells of a Fengguan primary culture, and the stimulating capability of the synovial cells to the proliferation of the synovial cells is detected after 48 hours, and the experimental result shows that the peptide segment 111 can obviously stimulate the proliferation of the synovial cells and is dose-dependent, as shown in figure 2. The experimental result shows that the peptide segment 111 positioned at 75-81 positions of Cyr61/CCN1 can form a ring conformation in aqueous solution to simulate the effect of Cyr61/CCN1 protein on stimulating the proliferation of synovial cells.
Example 5 Cyr61/CCN1 protein epitope polypeptide stimulates the in vitro proliferation of Cyr61/CCN1 high expression breast cancer cell strain (MDA-MB-231)
Will be 1 × 10 4 And (3) inoculating the MDA-MB-231 cells into a 96-well plate, adding peptide fragments with different concentrations (2.5 ug/ml, 5ug/ml and 10 ug/ml), adding 3H-TdR after 4 hours, continuously incubating for 16 hours, collecting the cells, and detecting a c.p.m. value by a Beta scintillator for judging the cell proliferation state. As shown in FIG. 3, peptide fragment 111 has a significant effect of stimulating cell proliferation.
Example 6 screening to obtain a Small Compound (SC 1-15) that binds to and inhibits the Activity of Cyclic peptide 111
Designing a chemical small molecule (SC) with the functions of simulating and inhibiting the biological function of the peptide fragment according to the conformational epitope (cyclic polypeptide C GLECNFG, number 111) of the peptide fragment, wherein the chemical small molecule (SC) capable of blocking the peptide fragment has the function of inhibiting the molecular pathobiology of Cyr61/CCN1. The compound has important application in further developing into a lead compound and preparing medicaments for resisting synovium hyperplasia and bone destruction, resisting Cyr61/CCN1 high-expression breast cancer cell proliferation and resisting fibrosis (such as hepatic fibrosis). The invention adopts a virtual screening method commonly used in the development of new drugs and screens out chemical molecules with possible therapeutic effect by a calculation method. At present, the method is widely applied to the virtual screening after the three-dimensional high-resolution structure of the target is obtained by the experiment of X-ray diffraction or Nuclear Magnetic Resonance (NMR) on the target of the drug or by the method of biological information structure prediction.
In this embodiment, the successful virtual drug screening includes: (1) a sufficiently large chemical space (chemical space), (2) an accurate scoring function (scoring function), and (3) a search algorithm (searching algorithm) with high efficiency. Chemical space, i.e., the chemical database used; in a broad sense, the chemical space includes the more likely conformation (conformation) of the ligand (ligand) and receptor; the scoring function is designed mainly by searching a Protein database (Protein database, http:// www. Pdb. Org) for a ligand-receptor combination (complex) with better resolution, applying energy calculation and a statistical method such as multivariate linear regression to establish an accurate mathematical function, and rapidly and effectively guessing whether an unknown ligand can be stably combined with a given receptor, even predicting the binding strength (binding affinity) or the binding free energy (binding free energy). The scoring function is based on the complex energy changes in translation (translation), rotation (rotation), or conformation changes of the ligand molecule relative to the receptor, and finds the binding mode with the best scoring value.
In this embodiment, on the basis of the research that the target cyclic polypeptide C GLECNFG (number 111) can effectively simulate the biological effect of Cyr61/CCN1 protein, lead compounds targeting cyclic peptide 111 with structural entities are obtained by screening, and these compounds with small molecular structures can bind to cyclic peptide 111 and inhibit the activity thereof. According to the chemical structure of the cyclic polypeptide 111, 15 small molecule compounds SC capable of binding with the cyclic polypeptide are screened by the method, and the structures and names of the compounds SC-1 to SC-15 are shown in the following table 1. The structure and the synthesis method of the small molecular compound SC are the prior art.
Example 7 Effect of chemical Small molecules (SC) 1-15 binding to peptide fragment 111 in vitro inhibition of synovial cell proliferation stimulated by Cyclic peptide 111
Clinical samples, synovial cell preparations, and primary cultures were the same as those described in example 4.
Proliferation assay of synovial cells: taking FLS in logarithmic growth phase, digesting with 0.25% trypsin, and adjusting cell concentration to 1 × 10 4 Cells/ml were plated in 96 well cell culture plates and 10ug/ml of peptide fragment 111 and 2.5ug/ml of Cyr61/CCN1 protein (Proptech, san Diego, USA) were added. Then, 10. Mu.M of the small chemical molecules SC-1 to SC-15 selected by the method of example 6, as shown in Table 1 below, were added, and the mixture was co-cultured for 48 hours. 1 mu Ci of 3H (each well) is added 16 hours before the culture is finished, cells are collected, proliferation is detected by a beta liquid scintillation instrument, and the experimental result is shown in figure 4, wherein 15 chemical small molecules (SC-1 to SC-15) respectively have obvious inhibition effect on the proliferation of synovial cells stimulated by peptide fragment 111 (shown in figure 4A) and Cyr61/CCN1 protein (shown in figure 4B).
Example 8 Effect of small chemical molecules 1-15 binding to peptide fragment 111 in inhibiting proliferation of breast cancer cell line MDA-MB-231 stimulated by cyclopeptide 111 and Cyr61/CCN1 in vitro
Will be 1 × 10 4 Each MDA-MB-231 cell was seeded into a 96-well plate, and 10ug/ml of peptide fragment 111 and 2.5ug/ml of Cyr61/CCN1 protein (Proptech, inc., san Diego, USA) were added. Then 10 μ M of small chemical molecules SC-1 to SC-15 screened according to the method of example 6 are added, as detailed in table 1 below, 1 μ Ci of 3H (per well) is added after co-culture for 4 hours, incubation is continued for 16 hours, cells are collected, and a Beta scintillator detects c.p.m. value for judging the proliferation state of the cells. The experimental results are shown in FIG. 5, and the 15 chemical small molecules (SC 1-15) are coupled with the peptide fragment 111 (as shown in FIG. 5)A is shown in the figure) and Cyr61/CCN1 protein (shown in the figure 5B) has obvious inhibition effect on the in vitro proliferation of the breast cancer cell strain MDA-MB-231.
<110> Texas diagnostic System (Shanghai) Co., ltd
Application of SC-4-SC-15 inhibitor of Cyr61/CCN1 protein epitope polypeptide
<160> 3
<210> 1
<211> 7
<212> PRT
<213> race (Homo sapiens)
<400> 1
GLECNFG
<210> 2
<211> 8
<212> PRT
<213> race (Homo sapiens)
<400> 2
C-G LECNF G
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<211> 77
<212> PRT
<213> race (Homo sapiens)
<400> 3
MSSRI ARALA LVVTL LHLTR LALST CPAAC HCPLE APKCA PGVGL VRDGC GCCKV CAKQL NEDCS KTQPC DHTKG LECNF GASST ALKGI CRAQS EGRPC EYNSR IYQNG ESFQP NCKHQ CTCID GAVGC IPLCP QELSL PNLGC PNPRL VKVTG QCCEE WVCDE DSIKD PMEDQ DGLLG KELGF DASEV ELTRN NELIA VGKGS SLKRL PVFGM EPRIL YNPLQ GQKCI VQTTS WSQCS KTCGT GISTR VTNDN PECRL VKETR ICEVR PCGQP VYSSL KKGKK CSKTK KSPEP VRFTY AGCLS VKKYR PKYCG SCVDG RCCTP QLTRT VKMRF RCEDG ETFSK NVMMI QSCKC NYNCP HANEA AFPFY RLFND IHKFR D
Claims (2)
- The application of an inhibitor of Cyr61/CCN1 protein epitope polypeptide in preparing a medicament for resisting the proliferation of rheumatoid arthritis synovial cells is characterized in that the inhibitor of Cyr61/CCN1 protein epitope polypeptide comprises:。
- the application of an inhibitor of Cyr61/CCN1 protein epitope polypeptide in preparing a medicament for inhibiting proliferation of breast cancer cells is characterized in that the inhibitor of Cyr61/CCN1 protein epitope polypeptide comprises:。
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| CN2014100458170 | 2014-02-08 | ||
| CN201410152740.7A CN103923174B (en) | 2014-02-08 | 2014-04-16 | Cyr61/CCN1 protein antigenic epitope polypeptide, inhibitor and application thereof as well as monoclonal antibody |
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| CN201410152740.7A Division CN103923174B (en) | 2014-02-08 | 2014-04-16 | Cyr61/CCN1 protein antigenic epitope polypeptide, inhibitor and application thereof as well as monoclonal antibody |
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| CN201911091016.7A Active CN111012895B (en) | 2014-02-08 | 2014-04-16 | Application of inhibitor SC-3 of Cyr61/CCN1 protein epitope polypeptide |
| CN201911090995.4A Active CN111068040B (en) | 2014-02-08 | 2014-04-16 | Application of inhibitor SC-4-SC-15 of Cyr61/CCN1 protein epitope polypeptide |
| CN201610897943.8A Active CN106492188B (en) | 2014-02-08 | 2014-04-16 | Cyr61/CCN1 protein epitope polypeptide, inhibitor and monoclonal antibody thereof, and application thereof |
| CN201410152740.7A Active CN103923174B (en) | 2014-02-08 | 2014-04-16 | Cyr61/CCN1 protein antigenic epitope polypeptide, inhibitor and application thereof as well as monoclonal antibody |
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| CN201410152740.7A Active CN103923174B (en) | 2014-02-08 | 2014-04-16 | Cyr61/CCN1 protein antigenic epitope polypeptide, inhibitor and application thereof as well as monoclonal antibody |
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Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5326751A (en) * | 1992-06-26 | 1994-07-05 | Arizona Board Of Regents On Behalf Of The University Of Arizona | Enkephalin analogs |
| CN101492495A (en) * | 2009-02-24 | 2009-07-29 | 中国农业科学院哈尔滨兽医研究所 | A group of antigen epitope polypeptide and uses thereof |
| CN101709088A (en) * | 2009-12-04 | 2010-05-19 | 上海市免疫学研究所 | Monoclonal antibody for resisting Cyr61 protein and application thereof |
| WO2011054315A1 (en) * | 2009-11-06 | 2011-05-12 | 上海市免疫学研究所 | Use of cyr61 protein for preparing medicine |
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| IL121134A0 (en) * | 1997-06-22 | 1997-11-20 | Yeda Res & Dev | Peptides and antiallergic compositions comprising them |
| TW201102086A (en) * | 2009-06-04 | 2011-01-16 | Hoffmann La Roche | Antibodies against human CCN1 and uses thereof |
| WO2013049830A2 (en) * | 2011-09-30 | 2013-04-04 | The Washington University | Tip-1 and grp-78 binding peptides and method of identifying peptide receptors |
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- 2014-04-16 CN CN201911091007.8A patent/CN111150832B/en active Active
- 2014-04-16 CN CN201911091016.7A patent/CN111012895B/en active Active
- 2014-04-16 CN CN201911090995.4A patent/CN111068040B/en active Active
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Patent Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5326751A (en) * | 1992-06-26 | 1994-07-05 | Arizona Board Of Regents On Behalf Of The University Of Arizona | Enkephalin analogs |
| CN101492495A (en) * | 2009-02-24 | 2009-07-29 | 中国农业科学院哈尔滨兽医研究所 | A group of antigen epitope polypeptide and uses thereof |
| WO2011054315A1 (en) * | 2009-11-06 | 2011-05-12 | 上海市免疫学研究所 | Use of cyr61 protein for preparing medicine |
| CN101709088A (en) * | 2009-12-04 | 2010-05-19 | 上海市免疫学研究所 | Monoclonal antibody for resisting Cyr61 protein and application thereof |
Also Published As
| Publication number | Publication date |
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| CN111068040A (en) | 2020-04-28 |
| CN111150832A (en) | 2020-05-15 |
| CN111012895B (en) | 2023-03-07 |
| CN103923174B (en) | 2017-01-11 |
| CN111012895A (en) | 2020-04-17 |
| CN106492188A (en) | 2017-03-15 |
| CN103923174A (en) | 2014-07-16 |
| CN106492188B (en) | 2019-12-20 |
| CN111150832B (en) | 2023-03-07 |
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