CN109942671A - A kind of GPR1 antagonism polypeptide and its derivative and application - Google Patents
A kind of GPR1 antagonism polypeptide and its derivative and application Download PDFInfo
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- CN109942671A CN109942671A CN201711378017.0A CN201711378017A CN109942671A CN 109942671 A CN109942671 A CN 109942671A CN 201711378017 A CN201711378017 A CN 201711378017A CN 109942671 A CN109942671 A CN 109942671A
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Abstract
The invention discloses a kind of GPR1 antagonism polypeptide and its derivative and applications, more particularly to such as sequence SEQ ID No.1-7 and its derivative, the derivative of the binding peptide is on GPR1 binding peptide amino acid side groups, the aminoterminal of GPR1 antagonism polypeptide segment or c-terminus progress routinely modifys obtained product, or be to connect to be used for polypeptide or Protein Detection or the obtained product of the label of purifying on GPR1 antagonism polypeptide;The binding peptide and its derivative in vitro can be in conjunction with GPR1, by blocking the combination of chemerin and GPR1 that cAMP concentration is promoted to increase, inhibiting calcium (Ca caused by chemerin2+) in stream, provide effective treatment small-molecule drug for high expression GPR1 receptor diseases such as breast cancer etc., can be widely used in Med Biol field.
Description
Technical field
The present invention relates to biotechnologys and biomedicine field, specifically, the present invention is female reproduction disease target spot
GPR1 receptor antagonist polypeptide LRH7-G4 and its derivative and application.
Background technique
Breast cancer (Breast cancer) is to be only second to the mortality cancer of the 2nd high mortality of the whole world of lung cancer, it continues
Property destroys the life and health of the millions of women in the whole world and its family.According in the research of World Health Organization's international cancer
Heart recent statistics, global women with breast cancer new cases in 2012 account for whole female malignant morbidities up to 1,670,000
22.9%;460000 women because of breast cancer deaths, 13.7%, the Zhan Suoyou women die of Zhan Suoyou female malignant death
1.7%, suffering from cancer women for about 4 just has 1 to suffer from breast cancer.Female Breast Cancer in China age-standardized incidence is
21.6/10 ten thousand, occupy the 1st of female cancer morbidity;The death rate is 5.7/10 ten thousand, occupies the 6th of female cancer death.4%~
As metastatic breast cancer when 6% breast cancer diagnosis, and the early stage patient 30%~40% for receiving adjuvant treatment can develop to turn
Shifting property breast cancer, 5 years survival rates about 20% of patient.And perform the operation, the traditional treatments mode such as radiation and chemotherapy, the specificity of effect and
Specificity is bad, inevitably generates lethal effect to normal cell and tissue, brings great side effect to patient.
Therefore, the targeted drug for finding efficiently specificity, will be greatly improved the therapeutic effect of breast cancer!
Clinical research discovery, early-stage breast cancer often do not have typical sings and symptoms, are not easy to cause attention, often pass through
Physical examination or breast cancer screening could be found.Although breast cancer early diagnosis can for breast cancer treatment win preciousness when
Between, the therapeutic effect of breast cancer can be greatly improved, but the personnel ratios that China carries out early-stage breast cancer diagnosis at present are seldom.
Mammary cancer is transferred to lymph, is a kind of common metastasis symptom of breast cancer.In general, lesion on the outside of breast
2/3 is accounted for the chance of axillary lymphatic metastasis, the chance shifted by sternal is 1/3.On the inside of breast and the tumour of central portion,
The chance with outside breast cancer Lymph Node Metastasis respectively accounts for 1/2 inwardly, and breast cancer is easy to happen Lung metastases and Lymph Node Metastasis.Tumour is micro-
Environment is most important to the formation of tumour, determines the occurrence and development of tumour.It is that normal mammary stem cells cause at first
Cancer mutation is converted into breast carcinoma stem cell, generates the tumour of prognosis mala, and then these are swollen with metastatic poor prognosis
Tumor, under the influence of matrix fiber mother cell, a part of breast carcinoma stem cell is shifted, be transferred to brain, lung, liver with
And marrow.
Some researches show that overexpression is presented in Chemokine receptor CXCR4 in breast cancer tissue, and ligand matrices are thin
Born of the same parents' derivative factor -1 (CXCL12) is also high to be expressed in Metastasis in Breast Cancer position, in marrow, lymph node, lung and liver,
CXCR4/CXCL12 signal system plays an important role in distally other organ metastasis of going back to the nest of breast cancer, therefore
Become Bone of Breast Cancer and shift potential therapeutic targets, wherein CXCR4 antagonism polypeptide-CTCE-9908, comes into preclinical
Experimental stage can be good at the Bone tumour for inhibiting breast cancer in breast cancer animal model.Therefore, chemotactic factor (CF) is in breast cancer
It plays an important role, has using chemotactic factor (CF) as the targeted drug of target treatment breast cancer wide in occurrence and development and transfer
Market prospects and application value.
Breast cancer originates from each rank conduit of mammary gland and acinar epithelia, is gradually sent out by adenomatosis to atypical hyperplasia
Exhibition is carcinoma in situ, early invasive carcinoma to infiltrating cancer.The canceration that the conduit of different stage occurs, organization type are usually different.
95% or more is human malignant epithelial tumors in breast cancer, and sarcoma of breast is very rare.It is invaded for most common two kinds in histopathology
Lubricant nature breast cancer is respectively as follows: infiltrating duct carcinoma (also referred to as " plain edition, NOS ") and lobular carcinoma.Both breast cancer be by
What preceding wettability conduit and small leaf nodule were formed.The difference of infiltrating duct carcinoma and lobular carcinoma and other types of breast cancer
Mainly as caused by the morphological differences between cell.
Molecular Targeted Therapy for Breast Cancer refers to related for mammary gland carcinogenesis, the related signal path of development and its oncogene
Expression product is treated.Being remained high by Cancer Mortality is influenced, and lasting increase is presented in global anti-tumor drug market
The gesture of length, the sales volume of antitumor class drug in 2010 account for the 5.8% of international drugs sales volume, occupy the world up to 459.7 hundred million dollars
First, increased by 8% than 2009.Wherein, molecular targeted anti-tumor drug sales volume is 311.9 hundred million dollars, and growth rate reaches
23%.The anti-human epidermis of food and drug administration (Food and Drug Administration, FDA) approval in 1997
Molecular targeted therapy-Trastuzumab application of growth factor acceptor 2 (HER-2) has started breast cancer point
The new era of sub- targeted therapy.According to global best-selling drugs data statistics, global breast cancer medicines market scale is more than 100 within 2015
Hundred million dollars, it is Herceptin (Trastuzumab) that wherein sales volume is highest, and sales volume is 67.9 hundred million dollars, is increased compared with the same period
Long 4.2%.It is many study found that EGF-R ELISA (EGFR) is the key molecule for regulating and controlling breast cancer occurrence and development,
By activating downstream Ras/Raf/MEK/ERK and PI3K/AKT signal path, EGFR promotes the proliferation of breast cancer, migrates and invade
It attacks;In addition, epidermal growth factor acceptor 2 (HER-2) height is expressed in breast cancer cell, by forming homodimer or heterologous two
Aggressiveness, activation downstream PI3K/Akt and Ras/MAPK signal path promote breast cancer proliferation, angiogenesis, migration and invasion.Mesh
Before, mainly have for the molecular targeted agents of breast cancer treatment: for the Herceptin of Epidermal growth factor-recepor-2 treatment;
For the inhibitor everolimus in PI3K/AKT/mTOR access;For the Avastin of anti-angiogenic medicaments;For
The iniparib of BRCA1/2 mutation;And it is directed to CDK4/6 inhibitor palbociclib.It the appearance of these targeted drugs and answers
With new dawn is brought for patient with breast cancer, so that the treatment of breast cancer is become more accurate, dramatically reduce traditional treatment
Bring damages side effect!
Chemotactic factor (CF) and its receptor in the development process of breast cancer, not only with the foundation of tumor microenvironment and metastases
It is closely related, can be with the deterioration of mediate tumor cell, and promote the growth and proliferation of tumour cell.Research points out,
The chemotactic factor (CF)s such as CXCL8, CXCL12, CCL2, CCL5, CCL18, which have, promotees breast cancer effect, and other chemotactic factor (CF) is such as
XCL1, CXCL9, CXCL10, CXCL14, CCL16, CCL19 etc. may then have anti-breast cancer effect.Tumour associated fibroblast cell
(CAFs) and cancer cell can activate and secrete a large amount of CCL2, promote the self-renewing of tumor stem cell (CSC), and then strengthen swollen
Oncocyte to change, the repellence of radiotherapy and the transfer for promoting lesion.Positive rate of the CXCR4 in breast cancer is up to 60%,
CXCL12/CXCR4 effect network plays a significant role in the growth, transfer of a variety of solid tumors including breast cancer, hinders
Break this biological axis can inhibit angiogenesis and tumour diffusion, increase tumour cell to chemotherapy, the sensibility of radiotherapy.In 4T1
Mouse breast cancer model can inhibit angiogenesis and metastases with the oncolytic virus treatment for carrying CXCR4 antagonist.In TNBC
The expression (71%) of CXCR4 is higher than HER-2 positive breast cancer (44%) and Luminal type breast cancer (37%), CXCR4+TNBC
Patient tumors are big, Yi Fasheng liver, lung, brain metastes, poor prognosis.Chemotactic factor (CF) and its receptor antagonist or inhibitor have wide
Market prospects.Have statistics show about 30% small-molecule drug be with g protein coupled receptor for targeting.CXCR4 polypeptide is short of money
Anti-agent CTCE-9908 has been found to can inhibit the Lung metastases of Mouse Bone sarcoma and melanoma.CXCR1/CXCR2 antagonist-
Repertaxin can inhibit the growth and transfer of tumour in animal model, have been used for Advanced breast cancer patient clinical trial.
Therefore, effect of the research chemotactic factor (CF) in tumor development finds the novel targets of chemotactic factor (CF) treatment breast cancer, not only to explaination
Metastases have great significance, and have wide pharmaceutical market prospect.
The fat correlation research with breast cancer is seen earliest in the 1960s, case-control study proposes mammary gland earliest
The women of post menopausal obesity and high blood pressure is tended in the morbidity of cancer., it was also found that compared with the control group in animal experiment study,
Fat mice tumors grew speed obviously increases.World Cancer Research Foundation and american cancer research institute are demonstrate,proved with epidemiology
According to retrospective analysis is carried out, the result of study of animal model proves overweight and fat dramatically increases the risk to suffer from breast cancer.
Meta analysis shows that, the risk to suffer from breast cancer with BMI increase and increase, BMI > 30kg/m2The risk that suffers from breast cancer of patient
It is 1.3~2 times of normal person, obesity can dramatically increase the risk that women suffers from breast cancer.
Obesity promotes mammary gland carcinogenesis, the mechanism of development includes the following aspects: (1) estrogen.Obesity can increase
Add the synthesis of estrogen, reduces serum estradiol and sex hormone binding globulin (SHBG) is horizontal, serum estradiol is excessive, competition
Estrogen receptor on target organ causes Hypothalamus-Pituitary-Ovaries gonad index disorder, breaks mammoplasia and answers
Old balance promotes abnormality proliferation and the conversion of breast cancer cell;(2) chronic inflammation.It is activated in obese patient's adipose tissue
Macrophage can secrete a large amount of pro-inflammatory mediators, cause chronic inflammatory reaction, a large amount of inflammatory factors and internal various cells are tumour
Tumor microenvironment is formd, to promote the generation of breast cancer cell, development.When TG excessive concentration in blood, mammary gland blood vessel
Lipidosis leads to the generation of chronic inflammation, the inflammatory factor of inflammatory cell secretion and Stromal fibroblasts, lymphocyte, huge
Phagocyte, blood vessel and lymphatic network and extracellular matrix form tumor microenvironment, interfere the duplication and transcription of DNA, cause to dislike
Property tumour occur;(3) insulin and insulin-like growth factor-i (IGF-1).Easily there is insulin resistance in obesity, makes insulin
And the horizontal of IGF-1 increases, and facilitates the proliferation and revascularization of cancer cell.One research from swiss data library has collected
Receive within 2005 the data of 115 000 patients of insulin therapy, sweet smart pancreas islet is applied alone in discovery in next 2 year
Patient's pathogenesis of breast carcinoma risk of extract for treating is obviously relatively high (RR=1.99) using other insulin analogs.(4) fat cell
The factor.Obesity will affect the generation of Adipocyte Factor, reduce adiponectin, increase the level of leptin, PAI-1 etc., promote cell
Proliferation, anti-apoptotic and acceleration angiogenesis, to promote the proliferation and growth of cancer cell.Adiponectin can not only inhibit insulin
The Mitosis promoted is cooperateed with estrogen, can also reduce cancer by promoting Bax and p53 to promote the expression of apoptogene
The transfer of cell and wetting capacity.Leptin can be by activating JAK/STAT3, MAPK-ERK1/2 PI3K access, to promote
Into the growth of breast cancer;In addition, the expression that leptin can also generate element by induction of vascular promotes the generation of tumor-associated vessels, and
And leptin also can induce human epidermal growth factor receptor 2 ErbB-2) transcription, and participate in pancreas islet in triple negative breast cancer cell
The reaction of plain sample growth receptors 1 (IGF-1), activation EGF-R ELISA (EGFR) is to promote the invasion of cell and turn
It moves.Obesity is the risk factor of Postmenopausal Breast Cancer, fat in close relations and complicated, the great Liang Yan with mammary gland carcinogenesis, development
Study carefully and shows that obesity can produce certain negative regulation to the generation of breast cancer, development, diagnosis, tumour feature and prognosis.Therefore,
It can be the present by the further exploration and research of Adipocyte Factor and Breast Cancer to fat, adipose tissue and its secretion
The very important reference frame of corresponding measure offer for reducing breast cancer incidence and improving disease prognosis is provided afterwards.
Adipocyte Factor Chemerin
Adipocyte Factor Chemerin is also referred to as Tazarotene-induced gene 2 (TIG2) or retinol receptor response albumen 2.?
By after the clones such as Nagpal discovery, in 2003, Wittamer etc. passed through reverse phase height in the secondary ascites of oophoroma within 1997
Hydraulic fluid phase chromatography obtains its activated protein.163 amino acid of Chemerin amyloid protein precursor overall length have 6 cysteines
Residue forms 3 disulfide bond, removes several amino acid of N-terminal signal peptide and C-terminal, just has bioactivity, in blood
Chemerin activated form contains 134 amino acid (about 16kDa), and cecropin/cysteine proteinase suppression is belonged in structure
Preparation family, when be inflamed react when, chemerin can rapidly transform into activated form under several albumen enzyme effects.
Chemerin is mainly expressed in white adipose tissue, placenta and liver in the Various Tissues wide expression of human body, with 3 receptors
It combines: 1. g protein coupled receptor CMKLR1;2. g protein coupled receptor GPR1;③CCRL-2.After Chemerin combination GPR1,
On the one hand the calcium ion in GPR1 positive cell can be made to discharge, inhibits the aggregation of cAMP, makes map kinase phosphorylation;Other one
Aspect has facilitation to stream in intracellular calcium.On the one hand Chemerin is used as chemotactic factor (CF), chemotactic Dendritic Cells
And macrophage, it serves as a connection between adaptive immunity immune, chemotactic natural killer cell reaches inflammation part and participates in
Inflammatory reaction;On the other hand it as new Adipocyte Factor, is secreted and is generated by adipose tissue, adjust differentiation, the steatolysis of fat cell,
It can promote the biological effects such as insulin signaling pathway in fat cell.Chemerin is in fat and metabolic syndrome disease
Consequence is accounted in reason physiological mechanism.
GPR1 receptor
GPR1 is the immediate homologue of CMKLR1, with CMKLR1 it is shared be more than 40% sequence identity.It is a kind of
The g protein coupled receptor to play a crucial role in eukaryocyte usually stimulates glucose, lipid accumulation and by trophic signals
Pass to cAMP approach.Many signal transductions are mediated by G-protein → coupled receptor (GPCR) in eucaryote.G-protein β is even
Connection receptor is present in some eucaryotes, including yeast, double flagellates and animal.GPR1 is initially the G found in the mankind
G-protein linked receptor (GPCR), the receptor of chemerin is accredited as by experiment in vitro.Although not reporting Chemerin
Physiological function in conjunction with GPR1, but it is reported that GPR1 in mouse animal brown adipose tissue, white adipose tissue and skeletal muscle
Height is expressed, and GPR1 is mainly expressed in the vascular cell of white adipose tissue.It is struck in the GPR1 of feeding high fat diet
Except in mouse, it is found that its glucose intolerance ratio WT mouse is more serious.In addition, GPR1 knocks out small in pyruvic acid resistance test
The insulin level that mouse is able to suppress glucose α stimulation increases, and causes blood glucose rise.These results indicate that GPR1 is
The active acceptor of Chemerin, it is adjustable it is fat during the intracorporal balance of glucose.
Using Tango bioassay, measurement after increasing the treatment of Chemerin dosage CMKLR1 and GPR1 in HTLA cell
In activity.It was found that Chemerin activates CMKLR1 and GPR1 with similar effect, reach effect be 265.3 ± 182.2- and
185.6 ± 26.5- times of maximum the reaction (Emax) changed.In addition, Chemerin activation GPR1 ratio activation CMKLR1 (EC50,
54.6 ± 30.7nM) there is significant higher effect (EC50,18.2 ± 2.9nM), this proves that Chemerin has activated GPR1, together
When GPR1 be also highly sensitive Chemerin receptor.
GPR1 expression cell system passes through weak Ca2+Mobilize and ERK1/2 activation reacts to chemerin, but its due to swash
Dynamic agent in conjunction with and be effectively internalized by.Therefore, GPR1 may be as the Decoy receptors of chemerin, and so far, main thin
It is intracellular or there has been no the active descriptions mediated to GPR1 in vivo.And GPR1 is in central nervous system, skeletal muscle, skin and rouge
It is expressed in fat tissue, the activity of chemerin can be adjustable.
G protein coupled receptor superfamily (GPCRs) is played an important role in extracellular signal into transductive process intracellular, is adjusted
Control vital factor in these three carcinobiologies of cell movement, growth and genetic transcription-.In the past more than ten years,
The signal path of mediation has proven to the key regulatory person of protooncogenic signal, and is good drug target, at present
The drug 60% sold on the market is designed both for this receptor.And GPR1 does not still have at present as one of GPCRs member
Any drug is to treat clinical cancer directly against GPR1.Therefore, using GPR1 as target, the novel polypeptide medicine of anticancer is screened
Object and humanized antibody have important social effect and wide economic market.
Display technique of bacteriophage (Phage Display Technology) is the screening of a specific polypeptide or albumen
The polypeptide that target gene encodes can be showed in phage surface by technology, this technology in the form of fusion protein, and what is be demonstrated is more
Peptide or protein can keep relatively independent space structure and bioactivity, make a large amount of rondom polypeptides and its DNA encoding sequence it
Between establish direct connection so that the polypeptide ligand of various target molecules (such as antibody, enzyme and cell surface receptor) pass through it is external
Affine biopanning procedure is able to Rapid identification.Since asking display technique of bacteriophage generation, because of its high storage capacity, efficient and convenient and clever
The advantages such as screening living, phage antibody library technique are in progress very fast in recent decades, obtain in many fields of life science
To extensive use, the attention that is especially just increasingly being subject in the fields such as diagnosing tumor and tumour antibody medicine preparation.Polypeptide at present
The main function target spot of drug is g protein coupled receptor (GPCRs), has 39% polypeptide drugs to target GPCRs in clinical studies.
Polypeptide drugs have many advantages: (1) druggability is higher than general chemicals, and bioactivity is high, high specificity;(2) toxicity is anti-
It answers relatively weak, is not likely to produce accumulation in vivo;(3) compatibility fewer with the interaction of other drugs, with internal receptor
It is relatively good.Humanized monoclonal antibodies have high sensitivity, high specificity, efficiently, serum cross reaction is few or nothing, preparation cost
Low advantage.Polypeptide drugs and humanized antibody are screened using display technique of bacteriophage, the system of genotype and phenotype may be implemented
One, be it is a kind of prepare the technical method that antibody is efficient, practical, the technology using expression albumen and ligand affinity, will needed for
The albumen or polypeptide wanted screen, and the identification for being widely used in disease marker screens the screening with antibody drug and prepares it
In.
Summary of the invention
For overcome the deficiencies in the prior art and disadvantage, the primary purpose of the present invention is that providing one kind by phage display
The GPR1 antagonism polypeptide that library is screened, the antagonism polypeptide and Chemerin receptor GPR1 have specific high-affinity, can
The signal path of Chemerin/GPR1 is blocked by inhibiting the combination of Chemerin and GPR1, expresses GPR1 receptor in height
Disease targeted therapy in terms of have huge application value.
Another object of the present invention is to provide the derivative of above-mentioned GPR1 receptor antagonist polypeptide, which also can be with
GPR1 receptor has specific high-affinity, and the binding site of Specific competition Chemerin and GPR1, is able to suppress
Chemerin combination GPR1.
A further object of the present invention is to provide the applications of above-mentioned GPR1 antagonism polypeptide and its derivative.
In order to realize that above-mentioned task, the present invention take following technical solution:
GPR1 receptor antagonist polypeptide, which is characterized in that its amino acid sequence are as follows: Gly- (D) Phe-His-Tyr-Ser-
Leu-His-NH2SEQ ID No.1, i.e. LRH7-G4.
The screening technique of above-mentioned GPR1 antagonism polypeptide, this method utilize phage random peptide library, use GPR1 plasmid first
293T cell is transfected, the stable cell lines of permanent high expression GPR1 is obtained, is control adherent cell with wild type 293T cell, into
Row 5 takes turns full Cell depletion screening, and clone's single stranded DNA sequencing is extracted in the 50 positive bacteriophage amplifications of random picking.Analyze polypeptide
The essential characteristic of amino acid sequence, peptides homologous compare, the high polypeptide motif of the retrieval frequency of occurrences.BLAST retrieves protein
Database detects the higher protein of polypeptide motif homology, biological species of the discovery containing a large amount of polypeptides, and may combine
Cell surface receptor and ligand, be conducive to subsequent a large amount of extractions and purifying obtain polypeptide.
Hydrophilicity analysis shows that LRH7-G4 is hydrophilic polypeptides;
High performance liquid chromatography (HPLC) and the purity of mass spectrum (MS) detection LRH7-G4 synthesis have reached 99.85%.
The derivative that another aspect of the invention provides GPR1 receptor antagonist polypeptide of the present invention is GPR1 receptor
On antagonism polypeptide amino acid side groups, routinely modification obtains the progress of the aminoterminal of GPR1 receptor antagonist polypeptide fragment or c-terminus
Product, or be on GPR1 receptor antagonist polypeptide connection for polypeptide or Protein Detection or the obtained production of the label of purifying
Object;
Preferably, the routine is modified to amination, amidation, hydroxylating, carboxylated, carbonylation, alkylation, acetyl
Change, phosphorylation, sulphation, esterification, glycosylation, cyclisation, biotinylation, fluorophor modification, polyethylene glycol PEG modification or fixed
Change modification etc.;
Preferably, the label be His6, GST, EGFP, MBP, Nus, HA, IgG, FLAG, c-Myc or
ProfinityeXact。
Another aspect of the present invention provides the bioactive fragment or class of GPR1 receptor antagonist polypeptide of the present invention
Like object, as shown in SEQ ID No.2-7:
GFHYX1LH SEQ ID No.2, in which:
⑴X1For threonine, alanine, asparagine (T, A, N).
GFHYSX2H SEQ ID No.3, in which:
⑴X2For methionine (M);
The present invention also provides the derivative of the bioactive fragment of GPR1 receptor antagonist polypeptide or the like, the GPR1
On the amino acid side groups of the derivative of the bioactive fragment of receptor antagonist polypeptide or the like, aminoterminal or c-terminus into
Row routinely modifies obtained product, or is the upper connection of bioactive fragment of GPR1 receptor antagonist polypeptide or the like for more
The obtained product of label of peptide or protein detection or purifying;
Preferably, the routine is modified to amination, amidation, hydroxylating, carboxylated, carbonylation, alkylation, acetyl
Change, phosphorylation, sulphation, esterification, glycosylation, cyclisation, biotinylation, fluorophor modification, polyethylene glycol PEG modification or fixed
Change modification etc.;
Preferably, the label be His6, GST, EGFP, MBP, Nus, HA, IgG, FLAG, c-Myc or
ProfinityeXact。
In the inventive solutions, it is preferred that the GPR1 antagonism polypeptide LRH7-G4 and its derivative (SEQ
No.1~7 ID) it can be applied at least one of diseases such as preparation prevention and/or treatment breast cancer, fatty liver, diabetes
Drug;In terms of the GPR1 antagonism polypeptide and its derivative can be applied to preparation prevention and/or treatment female reproduction disease
Drug, existence form has: 1. containing 6 amino acid;2. being made of 7 amino acid.The GPR1 antagonism polypeptide spreads out
Biology is on GPR1 antagonism polypeptide amino acid side groups, the aminoterminal of GPR1 antagonism polypeptide segment or c-terminus carry out conventional repair
Obtained product is adornd, or is connection on GPR1 antagonism polypeptide for polypeptide or Protein Detection or the obtained production of the label of purifying
Object;The conventional modification is preferably amination, amidation, hydroxylating, carboxylated, carbonylation, alkylation, acetylation, phosphoric acid
Change, esterification, glycosylation, cyclisation, biotinylation, fluorophor modification, polyethylene glycol PEG modification or immobilization modification etc.;It is described
Label be preferably His6, GST, EGFP, MBP, Nus, HA, IgG, FLAG, c-Myc or ProfinityeXact etc.;
The GPR1 antagonism polypeptide and its derivative can derive from fungi, bacterium, bee, soft-shelled turtle, birds, insect, algae, beans
Class, beaver etc. are also possible to mammal or birds, such as primate (mankind);Rodent, including it is small
Mouse, rat, hamster, rabbit, horse, ox, canine, cat etc..
The derivative of the GPR1 antagonism polypeptide is preferred are as follows: second amino acid residue of above-mentioned GPR1 antagonism polypeptide is D
Configuration phenylalanine, end carry out amidation modification, as Gly- (D) Phe-His-Tyr-Ser-Leu-His-NH2。
The acquisition of the GPR1 antagonism polypeptide and its derivative is carried out using known method in the prior art, both may be used
To carry out chemical synthesis with polypeptide automatic synthesizer;By the way that short peptide sequence is derived nucleotide sequence, it is then cloned into carrier
Middle carry out biosynthesis;Largely it can also be extracted and be purified out of existing organism.
Specifically, GPR1 antagonism polypeptide LRH7-G4 and its derivative have following sequence:
1.GFHYX1LH (SEQ ID No.2), wherein:
⑴X1For threonine, alanine or asparagine (T, A, N).
2.GFHYSX2H (SEQ ID No.3), wherein:
⑴X2For methionine (M).
In addition, GPR1 antagonism polypeptide LRH7-G4 and its derivative also include the following polypeptide being naturally present in biology:
Another aspect of the present invention provides a kind of polynucleotide, encodes SEQ ID No.1-, and any one of 7 is described more
Peptide.
Another aspect of the present invention provides a kind of carrier, and it comprises nucleotide of the present invention, can pass through base
Because technological means and promoter sequence link.
Another aspect of the present invention provides a kind of host cell, has transfected carrier of the present invention.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative treat chemerin- in preparation
Purposes in GPR1 disease mediated drug.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative are situated between in treatment chemerin-GPR1
Lead the purposes in disease.
In the inventive solutions, the chemerin-GPR1 is disease mediated is selected from breast cancer, fatty liver, glycosuria
Disease, inflammatory reaction, polycystic ovary syndrome.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative inhibit chemerin to cause in preparation
CAMP concentration reduced drug in purposes.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative are inhibiting caused by chemerin
Purposes in the reduction of cAMP concentration.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative inhibit chemerin to cause in preparation
Calcium (Ca2+) effect of interior stream drug in purposes.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative are inhibiting calcium caused by chemerin
(Ca2+) in the active purposes of stream.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative inhibit chemerin to cause in preparation
Cell chemotaxis effect drug in purposes.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative are inhibiting thin caused by chemerin
Purposes in born of the same parents' chemotaxis.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative treat breast cancer, fat in preparation
Liver, diabetes, inflammatory reaction, polycystic ovary syndrome drug in purposes.
Another aspect of the present invention provides GPR1 receptor antagonist polypeptide of the present invention, GPR1 receptor antagonist polypeptide
Derivative, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative are in treatment breast cancer, fatty liver, sugar
Urinate disease, inflammatory reaction, the purposes in polycystic ovary syndrome.
Another aspect of the present invention provides a kind of pharmaceutical composition, wherein including GPR1 receptor antagonist of the present invention
Polypeptide, the derivative of GPR1 receptor antagonist polypeptide, the bioactive fragment or the like of GPR1 receptor antagonist polypeptide and its derivative
One of object is a variety of as active constituent.
The pharmaceutical composition can contain a kind of or a variety of pharmaceutically acceptable carriers;
Described kind pharmaceutically acceptable carrier be preferably diluent, excipient, filler, adhesive, wetting agent, collapse
Solve agent, sorbefacient, absorption carrier, surfactant or lubricant etc.;
A variety of shapes such as tablet, granula, capsule, oral solution or injection can be further made in the pharmaceutical composition
The drug of formula, various dosage forms can be prepared according to the conventional method of pharmaceutical field;
The invention also discloses the drugs in terms of a kind of prevention and/or treatment female reproduction disease or tumour, include this hair
The bioactivity of the bright GPR1 receptor antagonist polypeptide, the derivative of GPR1 receptor antagonist polypeptide, GPR1 receptor antagonist polypeptide
Segment or the like and its at least one of derivative.
The invention also discloses the drugs in terms of the disease of a kind of prevention and/or the high expression GPR1 receptor for the treatment of, include
GPR1 receptor antagonist polypeptide, the derivative of GPR1 receptor antagonist polypeptide, GPR1 receptor antagonist polypeptide bioactive fragment or class
Like at least one of object and its derivative.
In a specific experiment of the invention, the present invention can be effective using GPR1 antagonism polypeptide LRH7-G4 obtained
Alleviate chemerin to the inhibiting effect of cAMP signal path.Wherein, GPR1 antagonism polypeptide LRH7-G4 derivative (SEQ ID
No.1~7) there is phase same-action.
In another specific experiment of the invention, can effectively it be inhibited using GPR1 antagonism polypeptide LRH7-G4
Calcium (Ca caused by chemerin2+) effect of interior stream.Wherein, GPR1 antagonism polypeptide LRH7-G4 derivative (No.1~7 SEQ ID)
With phase same-action.
The present invention has the following advantages and effects with respect to the prior art:
(1) described the present invention provides a kind of GPR1 antagonism polypeptide LRH7-G4 and its derivative (No.1~7 SEQ ID)
Antagonism polypeptide and its derivative can specificity in conjunction with GPR1, and Specific competition Chemerin and GPR1 binding site,
It is able to suppress Chemerin/GPR1 signal path.It can be used as the biological species polypeptide drugs of Chemerin/GPR1 binding site,
Drug in terms of can be used for preparing prevention and/or treating the high disease for expressing GPR1 receptor, such as: breast cancer, fatty liver, glycosuria
Disease and inflammatory reaction, polycystic ovary syndrome.It can be widely used, and generate huge in Med Biol field
Social and economic effects.
Detailed description of the invention
Fig. 1: LRH7-G4 efficient liquid phase (HPLC) detection figure.
Fig. 2: LRH7-G4 mass spectrum (MS) detection figure.
Fig. 3: GPR1, chemerin and the hydrophobic profile comparative analysis of LRH7-G4 polypeptide.Wherein: the hydrophobic profile of A:GPR1
Figure;The hydrophobic profile diagram of B:chemerin;The hydrophobic profile diagram of C:LRH7-G4 polypeptide;D:GPR1, chemerin and LRH7-G4 are more
The hydrophobic profile of peptide compares figure.GPR1 profile is red, and chemerin profile is blue, and LRH7-G4 profile is green;
Fig. 4: LRH7-G4 alleviates chemerin to the inhibiting effect of cAMP signal path.Wherein, A, LRH7-G4 with
Effect of the Forsklin and Chemerin in 293T wild-type cell;B, LRH7-G4 are individually in 293T GPR1+/+In work
With;C, LRH7-G4 and Forsklin and Chemerin are in 293T GPR1+/+In effect;
Fig. 5: LRH7-G4 inhibits calcium (Ca caused by chemerin2+) effect of interior stream.
Specific embodiment
For a clearer understanding of the present invention, the present invention is further described referring now to the following example and attached drawing.Embodiment
It is only used for explaining without limiting the invention in any way.In embodiment, each Starting reagents material is commercially available, is not specified
The experimental method of actual conditions is conventional method and normal condition known to fields, or according to proposed by apparatus manufacturer
Condition.
Embodiment 1: elutriation, amplification, purifying, sequencing and the synthesis of GPR1 antagonism polypeptide LRH7-G4 are carried out.
The present embodiment is primarily to screening obtains the positive bacteriophage with GPR1 specific binding, then by biting the positive
Phage amplification, purifying extract phage single-chain DNA (ssDNA) and are sequenced, sequence obtained is analyzed and is compared, is finally closed
At the antagonism polypeptide LRH7-G4 of high-purity.
It is specific as follows:
1. establishing the 293T cell line of permanent high expression GPR1: 293T-GPR1+/+/LRH
1. the eugonic people's 293T cell to shine is chosen, in the day before transfection with 5 × 105A/hole, is inoculated in 6
In orifice plate, after culture to second day, cell fusion degree is 60%;
2. second day is transfected, as unit of a culture hole of 6 orifice plates, the opti-MEM culture medium with 200 μ L is dilute
3 μ g plasmids are released, 6 μ L liposome Lipofectamine2000 are separately diluted with the opti-MEM culture medium of 200 μ L, are gently mixed respectively
After even, it is placed at room temperature for 5 minutes;
3. two pipe dilutions are gently mixed, it is stored at room temperature after twenty minutes, is gently added 600 into mixed dilution
The opti-MEM culture medium of μ L;
4. cell to be transfected is gently rinsed once with PBS, culture hole is gently then added in the dilution mixed
In, it is placed in carbon dioxide incubator and cultivates;
5. transfection used medium to the greatest extent is abandoned in culture after 4~6 hours, 3mL complete medium is added into hole;
6. selecting the culture medium containing 1 μ g/mL puromycin (puromycin) to be screened after 48 hours;Not to cell
It obtains stablizing the 293T cell line for expressing GPR1 after occurring death again.
7. extracting total serum IgE with TRIzol, quantitative 2 μ g RNA carry out reverse transcription, and (Reverse Transcriptase kit is purchased from Promega public affairs
Department), and qPCR is carried out with specific primer sequences.
Specific primer sequences used are Hu-GPR1 primer sequence:
Fw 5’-AATGCCATCGTCATTTGGTT-3’(SEQ ID No.8)
Rv 5’-CAACTGGGCAGTGAAGGAAT-3’(SEQ ID No.9)
8. detecting the high expression level of GPR1 with comparing for pSM2c-Hu-scramble RNA has been transfected, and name
Are as follows: 293T-GPR1+/+/ LRH, it can screened for positive bacteriophage.
2. carrying out elutriation, amplification, purifying, sequencing and the synthesis of GPR1 antagonism polypeptide.
1. the preparation of ER2738 host's bacterium solution: aseptic operation first takes 200 μ l LB-Tet Liquid Cultures to be based on 1.5ml
It in sterile centrifugation tube, then is frozen from the glycerol of E.coli ER2738 and 0.2 μ l bacterium solution is taken to mix well in object therewith, all drawn
It is coated on LB-Tet plate, marks plate, be placed at room temperature for 3min, be subsequently placed in 37 DEG C of constant temperature incubation carton upside downs and be incubated overnight.
Next day observation, grow clone after sealed with sealed membrane, 4 DEG C be kept in dark place it is spare.With sterilizing pipette tips with asptic technique picking single bacterium
It falls, has been put into the 10ml sterile centrifugation tube added with 3ml LB-Tet fluid nutrient medium in advance, in 37 DEG C of constant-temperature table after label,
300rpm/min shaken cultivation is stayed overnight.Next day, bacterium amplification liquid are stored for future use in 4 DEG C.Take 10ml sterile centrifugation tube, sterile working
Be added 3ml LB-Tet fluid nutrient medium, the microbionation for taking 30 μ l to be incubated overnight wherein, 37 DEG C of constant-temperature table, 300rpm/min
2~3h of shaken cultivation, bacterium are in exponential phase of growth, visually observe (OD fog-like600~0.5).
2. the elutriation of GPR1 antagonistic peptide: height expression GPR1 cell is pressed 105A/culture dish is inoculated in coating poly in advance and relies
60 × 15mm of propylhomoserin2In culture dish, when routine culture to cell density 80%~90%, for eluriating (while with not expressing
The cell line of GPR1 is as blank control) every wheel eluent first takes 1 μ l to survey titre, and it is remaining to add it to 20ml LB culture
It is expanded in liquid, the titre after amplification is finally surveyed in repurity again, and amplified matter takes equal numbers magnitude to be used for down in 4 DEG C of short-term preservations
One wheel elutriation, remaining amplified matter are saved with 50% glycerol in -20 DEG C.
3. measuring the titre of bacteriophage: taking the 10ml centrifuge tube of 4 sterilizings, each bacteriophage dilution prepares 1 sterilizing
Centrifuge tube, micro-wave oven melt top agar (Agarose Top), and 3ml top agar is added in every pipe, and 45 DEG C of water-baths are spare.Each
Bacteriophage dilution prepares 1 piece of LB/IPTG/Xgal plate, 37 DEG C of pre- stand-by heats of constant incubator.By OD600~0.5
E.coli ER2738 Escherichia coli dispense according to 200 μ l/ pipe of bacteriophage dilution, and 4 DEG C save backup.Take 4 sterilizings
1.5ml centrifuge tube fills 100 μ l, 90 μ l, 90 μ l, 90 μ l LB-Tet culture mediums respectively, and bacteriophage to be measured is drawn 1 μ l and is entered
In 100 μ l LB-Tet culture mediums, by 10 times of gradient dilutions, it is respectively labeled as 10-1、10-2、10-3、10-4, each dilution is gently
Oscillation mixes, moment centrifugation.The bacteriophage for each dilution for taking 10 μ l to be titrated mixes with 200 μ l E.coli ER2738, gently
Light oscillation mixes, and moment centrifugation is incubated at room temperature 5min.Mixed bacteria liquid is rapidly added in top agar, quick oscillation mixes, and stands
The LB/IPTG/Xgal plate for pouring into preheating uniformly flattens it, the cooling 5min of room temperature, in 37 DEG C of constant incubators, is inverted
Plate incubated overnight.
4. the amplification and purifying of wash-out bacteriophage: the conical flask of 250ml is taken, in 1:100 ratio, by what is be incubated overnight
ER2738 host's bacterium solution is added into 20ml LB liquid medium, and 37 DEG C, the violent shaken cultivation 2h of 250rpm;It then will be wait expand
The phagocytosis body fluid of increasing is added in conical flask, and 37 DEG C, the violent shaken cultivation 4.5h of 250rpm;Culture is transferred to 50ml centrifuge tube
In, 4 DEG C of 10,000rpm are centrifuged 10min.Supernatant is transferred in another clean centrifuge tube, and 4 DEG C of 10,000rpm are centrifuged again
10min;It takes the 80% of supernatant to be transferred in another clean centrifuge tube, the PEG/NaCl of 1/4 volume is added, in 4 DEG C after being mixed by inversion
Precipitates overnight;Second day, 4 DEG C will be deposited in, 12,000rpm centrifugation 20min.With the careful Aspirate supernatant of clean pipette tips, then 4 DEG C
12,000rpm centrifugation 1min, remove residual supernatant;Then sediment is resuspended with 1ml TBS, gently blows and beats 100 times.Then will
Suspension is transferred in 2ml centrifuge tube, and 4 DEG C of 10,000rpm centrifugation 5min remove residual cells;Supernatant is added to the PEG/ of 1/4 volume
After NaCl, precipitated again in being incubated for 60min on ice;Centrifuge tube is taken out, 4 DEG C of 12,000rpm are centrifuged 20min, remove supernatant;With
Precipitating is resuspended in 200 μ l TBS, and 4 DEG C of 10,000rpm are centrifuged 1min.Supernatant is transferred in another centrifuge tube.4 DEG C of short-term preservations, can also
With with 50% glycerol in -20 DEG C of long-term preservations.The amplification of monoclonal phage, including (1) will be incubated overnight in 1:100 ratio
ER2738 host's bacterium solution be added into 2mL LB liquid medium, 37 DEG C, the violent shaken cultivation 2h of 250rpm;With sterilizing tooth
Label, choose the plate for being less than 100 plaques from fourth round titre plate, and picking separates good blue plaque, is added
Into culture tube, the violent shake culture 4.5h of 37 DEG C of 250r/min;Then culture is transferred in fresh centrifuge tube, 4 DEG C 10,
000rpm is centrifuged 30sec.Supernatant is transferred to in fresh tube, then same centrifugation is primary;Fresh centrifuge tube is transferred to by the 80% of supernatant
In, 4 DEG C of storages can also be with 50% glycerol in -20 DEG C of long-term preservations.
5. 13 bacteriophage ssDNA of agarose gel electrophoresis identification of M: gel shaped die horizontal being placed, the comb that will be chosen
Son is put well, and the space 1mm is stayed between comb bottom and mold;Weigh the conical flask that DNA electrophoresis is put into 250ml with agarose 1g
In, 1 × TAE of 100ml buffer is added, after mixing, flask is placed in micro-wave oven, heating is boiled, until agarose is completely molten
Solution;Electromagnetic oven is closed, conical flask is taken out, is set and is cooled to room temperature (holding flask can be resistant to) at room temperature, add bromine
Change 5 μ l of second ingot, after mixing, i.e., gel solution is poured into offset plate bed board.Plastic plate used in this experiment about needs glue 100ml;Room temperature
Under solidified completely to gel, take about 30 minutes, extract comb teeth, offset plate is put into electrophoresis tank;1 × TAE is added in electrophoresis tank
Buffer is advisable with being higher by gel surface 2mm;It is added in offset plate after sample is diluted with Loading buffer, pays attention to adding
Sample device suction nozzle should be placed in just in gel loading wells, not can pierce gel, also to prevent will be outside sample overfolw hole;Power on,
Voltage is adjusted to 50 volts, after electrophoresis 90min, gel slab is taken out, observes result in the UV lamp.
6. ssDNA sequencing and sequence analysis: the M13 bacteriophage ssDNA of extraction is sent to Shanghai Invitrogen biotechnology
Co., Ltd carries out DNA sequencing.Sequence analysis is carried out with Bioedit software after sequencing.By analysis result it is found that sample sequence
It is classified as Gly- (D) Phe-His-Tyr-Ser-Leu-His-NH2, wherein second phenylalanine is D configuration, with LRH7-G4 table
Show, last small peptide is synthesized by Shanghai Qiang Yao biotech firm.
Fig. 1 high performance liquid chromatography (HPLC) and the purity of Fig. 2 mass spectrum (MS) detection LRH7-G4 polypeptide are 99.85%, and
And molecular size range is consistent with predicted value.The hydrophobicity edge analysis of Fig. 3, it was demonstrated that LRH7-G4 polypeptide and chemerin have centainly
Similitude, similarity reaches 0.0122699 (PAM250).
Embodiment 2GPR1 antagonism polypeptide LRH7-G4 can effectively alleviate inhibition of the chemerin to cAMP signal path
Effect.
(1) cyclic adenosine monophosphate (cAMP) enzyme-linked immunosorbent assay:
1. plating cells: by 293T cell (the 293T GPR1 of wild type 293T cell and high expression GPR1+/+), respectively with
5ⅹ105A/hole is inoculated in 6 porocyte culture plates, and every hole culture volume is 1mL, is placed in after cultivating for 24 hours in incubator,
Overnight starvation, be added various concentration gradient (3 μM, 0.3 μM, 0.03 μM) LRH7-G4 polypeptide, Fosklin (25 μM) and
Chemerin (30nM) acts on 6h;
2. sample preparation: the cell pyrolysis liquid of 300 μ L is added in every hole, and 4 DEG C are placed 20 minutes, is scraped and is collected with cell scraper
Cell, after mixing of turning upside down, supernatant is collected in 12,000rpm centrifugations 10 minutes;
3. sample concentration measures: sample concentration is measured by BCA method;
4. cyclic adenosine monophosphate (cAMP) Enzyme-linked Immunosorbent Assay is tested:
A, reagent needed for preparing, 3 multiple holes of each preparation of samples;
The sample of 50 μ L or standard items addition are coated in 96 orifice plates of antibody by b;25 μ L are added in every hole again
CAMP peroxidase tracer conjugate;
C, every hole are added 50 μ L Anti-cAMP antibody, room temperature, are slowly incubated for 30 minutes on shaking table;
D is cleaned 5 times using eluent, and 100 μ L chemistry reflective agents are added in every hole, is incubated at room temperature 5 minutes;
E, microplate reader read plate record luminous value.
Fig. 4 shows that chemerin can reduce cell cAMP concentration when concentration is 30nM, but express in height
293T cell (the 293T GPR1 of GPR1+/+) in (3 μM, 0.3 μM, 0.03 μM) of LRH7-G4 of various concentration effects are added after, can
So that cAMP concentration significantly increases.And in wild type 293T cell, GPR1 receptor, therefore LRH7-G4 pairs are not expressed
Chemerin reduces the effect of cAMP concentration without obvious inhibiting effect.Likewise, in LRH7-G4 small peptide independent role group,
LRH7-G4 can not be such that cAMP concentration increases.In conclusion it can be concluded that LRH7-G4 can specificity by with GPR1
It acts on to further suppress chemerin to the reduction of cAMP concentration and act on.* P < 0.001 * * P < 0.05, * * P < 0.01, * with
Forskolin+chemerin group compares.
Embodiment 3GPR1 antagonism polypeptide LRH7-G4 can effectively inhibit calcium (Ca caused by chemerin2+) in stream make
With.
1. plating cells: by 293T cell (the 293T GPR1 of wild type 293T cell and high expression GPR1+/+), respectively with
5ⅹ103A/hole is inoculated in 96 porocyte culture plates, and every hole culture volume is 200 μ L, is placed in incubator and is cultivated for 24 hours
Afterwards, overnight starvation;
2. reagent configures: probenecid being incorporated in 1mL buffer solution, the probenecid that concentration is 250nM is configured to, shakes up
Afterwards, it is added in fluorescent reagent and prepares for use;
3. removing cell culture medium, various concentration gradient (30 μM, 3 μM, 0.3 μM, 0.03 μM, 0.003 μM) are added
LRH7-G4 polypeptide and chemerin (0.3nM) are acted on 30 minutes, and then the 100 above-mentioned fluorescent reagents of μ L are added in every hole;
4. 37 DEG C are placed 30 minutes, it is then placed at room temperature for 30 minutes;
5. measuring fluorescence light absorption value at exciting light 494nm and transmitting light 516nm.
Fig. 5 is shown, in 293T cell (the 293T GPR1 of high expression GPR1+/+) in, chemerin is in activity
When 0.3nM, calcium (Ca can be promoted2+) stream signal path, increase calcium ion (Ca2+) concentration.And various concentration is being added
After LRH7-G4 small peptide, calcium ion (Ca can be significantly reduced2+) concentration, inhibit chemerin to calcium (Ca2+) stream signal path
Activation.But in the 293T cell that wild type does not express GPR1, chemerin is to calcium (Ca2+) signal path is flowed without activation work
With LRH7-G4 is to calcium (Ca2+) stream signal path is also without function and effect, by the experiment it can be concluded that chemerin can lead to
It crosses in conjunction with receptor GPR1 and activates calcium (Ca2+) stream signal path, and the inhibition that LRH7-G4 small peptide can be specific
Chemerin/GPR1 signal path reduces calcium ion (Ca2+) concentration.* P < 0.001 * * P < 0.05, * * P < 0.01, * with
Chemerin group compares.
SEQUENCE LISTING
<110>Shenzhen Xianjin Technology Academe
<120>a kind of GPR1 antagonism polypeptide and its derivative and application
<130> CP11701249C
<160> 9
<170> PatentIn version 3.3
<210> 1
<211> 7
<212> PRT
<213>artificial sequence
<400> 1
Gly Phe His Tyr Ser Leu His
1 5
<210> 2
<211> 7
<212> PRT
<213>artificial sequence
<220>
<221> MISC_FEATURE
<222> (5)..(5)
<223>threonine, alanine or asparagine
<400> 2
Gly Phe His Tyr Xaa Leu His
1 5
<210> 3
<211> 7
<212> PRT
<213>artificial sequence
<220>
<221> MISC_FEATURE
<222> (6)..(6)
<223>methionine
<400> 3
Gly Phe His Tyr Ser Xaa His
1 5
<210> 4
<211> 7
<212> PRT
<213>fungi, bacterium or bee
<400> 4
Gly Phe His Tyr Ser Leu His
1 5
<210> 5
<211> 7
<212> PRT
<213>fungi, bacterium, bee
<400> 5
Gly Phe His Tyr Ser Leu His
1 5
<210> 6
<211> 6
<212> PRT
<213>soft-shelled turtle, bacterium, fungi, birds, insect, algae, beans or beaver
<400> 6
Phe His Tyr Ser Leu His
1 5
<210> 7
<211> 6
<212> PRT
<213>soft-shelled turtle, bacterium, fungi, birds, insect, algae, beans or beaver
<400> 7
Phe His Tyr Ser Leu His
1 5
<210> 8
<211> 20
<212> DNA
<213>artificial sequence
<400> 8
aatgccatcg tcatttggtt 20
<210> 9
<211> 20
<212> DNA
<213>artificial sequence
<400> 9
caactgggca gtgaaggaat 20
Claims (11)
1. a kind of GPR1 antagonism polypeptide, which is characterized in that its amino acid residue sequence is Gly- (D) Phe-His-Tyr-Ser-
Leu-His-NH2 SEQ ID No.1。
2. a kind of bioactive fragment or the like of GPR1 antagonism polypeptide, as shown in SEQ ID No.2-7:
GFHYX1LH SEQ ID No.2, in which:
⑴X1For threonine, alanine or asparagine;
GFHYSX2H SEQ ID No.3, in which:
⑴X2For methionine (M);
3. the bioactive fragment of GPR1 antagonism polypeptide described in claim 1 or GPR1 antagonism polypeptide as claimed in claim 2
Or the like derivative, it is characterised in that:
The derivative is on the amino acid side groups of GPR1 antagonism polypeptide or its bioactive fragment analog living, ammonia
Obtained product is routinely modified in cardinal extremity or c-terminus progress, or is connection for polypeptide or Protein Detection or the label of purifying institute
Obtained product;
Preferably, the routine be modified to amination, amidation, hydroxylating, carboxylated, carbonylation, alkylation, acetylation,
Phosphorylation, esterification, glycosylation, cyclisation, biotinylation, fluorophor modification, polyethylene glycol PEG modification or immobilization modification;Institute
The label stated is His6, GST, EGFP, MBP, Nus, HA, IgG, FLAG, c-Myc or ProfinityeXact.
4. a kind of polynucleotide can encode any one of the SEQ ID No.1-7 polypeptide.
5. a kind of carrier, it comprises any bar polynucleotides described in claim 4, and by gene technology means with
Promoter sequence link.
6. a kind of host cell has transfected carrier described in claim 5.
7. GPR1 receptor antagonist polypeptide described in claim 1, bioactive fragment as claimed in claim 2 or the like and
Purposes of the derivative as claimed in claim 3 in treatment chemerin-GPR1 is disease mediated;
Preferably, the chemerin-GPR1 is disease mediated is selected from breast cancer, fatty liver, diabetes, inflammatory reaction, more capsule ovum
Nest syndrome.
8. GPR1 receptor antagonist polypeptide described in claim 1, bioactive fragment as claimed in claim 2 or the like and
Purposes in the reduced drug of cAMP concentration caused by derivative as claimed in claim 3 inhibits chemerin in preparation.
9. GPR1 receptor antagonist polypeptide described in claim 1, bioactive fragment as claimed in claim 2 or the like and
Calcium (Ca caused by derivative as claimed in claim 3 inhibits chemerin in preparation2+) effect of interior stream drug in purposes.
10. GPR1 receptor antagonist polypeptide described in claim 1, bioactive fragment as claimed in claim 2 or the like with
And the purposes in the drug of derivative as claimed in claim 3 cell chemotaxis effect caused by preparation inhibition chemerin.
11. a kind of pharmaceutical composition, wherein including GPR1 receptor antagonist polypeptide described in claim 1, as claimed in claim 2
Bioactive fragment or the like and one of derivative as claimed in claim 3 or a variety of, as active constituent;
Preferably, the pharmaceutical composition can contain a kind of or a variety of pharmaceutically acceptable carriers;
The pharmaceutically acceptable carrier be preferably diluent, excipient, filler, adhesive, wetting agent, disintegrating agent,
Sorbefacient, absorption carrier, surfactant or lubricant etc.;
The diversified forms such as tablet, granula, capsule, oral solution or injection can be further made in the pharmaceutical composition, respectively
The drug of kind dosage form can be prepared according to the conventional method of pharmaceutical field.
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Citations (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO1999063094A2 (en) * | 1998-06-01 | 1999-12-09 | Mount Sinai School Of Medicine Of New York University | Nucleotide and protein sequences of gpr1 and methods based thereon |
| CN105061560A (en) * | 2015-07-17 | 2015-11-18 | 暨南大学 | Nogo-A receptor binding peptide as well as derivative and application thereof |
-
2017
- 2017-12-19 CN CN201711378017.0A patent/CN109942671B/en active Active
Patent Citations (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO1999063094A2 (en) * | 1998-06-01 | 1999-12-09 | Mount Sinai School Of Medicine Of New York University | Nucleotide and protein sequences of gpr1 and methods based thereon |
| CN105061560A (en) * | 2015-07-17 | 2015-11-18 | 暨南大学 | Nogo-A receptor binding peptide as well as derivative and application thereof |
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