CN110261611A - Application and its kit of the ZNF709 albumen as gastric cancer serum biomarker - Google Patents
Application and its kit of the ZNF709 albumen as gastric cancer serum biomarker Download PDFInfo
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- G01N33/574—Immunoassay; Biospecific binding assay; Materials therefor for cancer
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Abstract
Application and its kit, the kit the invention discloses a kind of ZNF709 albumen as gastric cancer serum biomarker include: the ZNF709 albumen being coated on ELISA Plate, the standard serum 1 of 0U/ml, the standard serum 2 of 100U/mL, enzyme marking reagent, enzyme substrate solution, confining liquid, sample diluting liquid, cleaning solution, terminate liquid.The immunoglobulin g antibody of anti-ZNF709 provided by the invention has high specific as gastric cancer serum biomarker;Kit detection is sensitive, safe, easy to operate, and the immunoglobulin g antibody that can be used to quantitative determine protein Z NF709 in human serum is horizontal, reflects the level of ZNF709 albumen, for diagnosing gastric cancer.
Description
Technical field
The present invention relates to bio-science fields, and in particular to a kind of ZNF709 albumen is as gastric cancer serum biomarker
Using and its kit.
Background technique
Gastric cancer is a kind of common malignant tumor of digestive tract, according to the statistics of the World Health Organization (WHO), the death of gastric cancer
Rate is in second, is only only second to lung cancer.According to the statistics of National Cancer Center and national tumour Register, gastric cancer is in China
Disease incidence is about 30/100000ths.For 2014, it is about 410,000 that gastric cancer number of cases is newly made a definite diagnosis in China, and mortality of gastric carcinoma
Case is 290,000 (death rate is 21/100000ths).Wherein the disease incidence of male's gastric cancer will be much higher than women, markization hair
Sick rate is about 2.4 times of women.Currently, gastric cancer overall 5 years survival rates in China's are 43.4%, but III and IV phase patients with gastric cancer
Five year survival rate there was only 28.01% and 8.42%.So improve the early diagnostic rate of gastric cancer, it will greatly improve patients with gastric cancer
Therapeutic effect.Biomarker can be used as the supplementary means of imageological examination, and being used in combination for the two can greatly improve
The early diagnostic rate of gastric cancer.
Ideal biomarker, which should meet, following characteristics: (1) high specific, i.e. marker are special in corresponding tissue
Anisotropic expression;(2) concentration of marker is related with tumor size, transfer, grade malignancy, can assist neoplasm staging and judgement
Prognosis;(3) half-life short, sensibility are high, can quickly reflect intracorporal physiological status, quickly increase under disease state, but
It is that concentration declines quickly after effectively treating;(4) it is easy to detect.
There are some gastric cancer biomarkers to apply in clinic at present: (1) carcinomebryonic antigen (Carcinoembryonic
Antigen, CEA), it is a kind of acid sugar Tang Bai with human embryos antigenic characteristic, is present in gastric cancer and other adenocarcinoma patients
Serum in, but, the dynamic observation that is mainly used for curing gastric cancer before and after smaller to the diagnostic significance of early carcinoma of stomach;(2) glycoprotein,
Such as CA125, CA19-9, CA50, CA724 and CA242, although these glycoprotein antigens have raising in the patients with gastric cancer of part
Phenomenon, but its sensibility only has 20~40%;(3) oncogene, such as DDC, c-myc, c-erb-2, p53 and nm23 are to stomach
The generation of cancer, transfer also have the certain significance, but are widely used in clinical being still restricted.In conclusion existing biomarker exists
Performance in diagnosing gastric cancer is all less desirable, therefore we need to find completely new gastric cancer biomarker.
Human protein ZNF709 (zinc finger 709) is by the ZNF709 gene on No. 19 chromosome 19p13.2
It is coded, contain 641 amino acid, molecular weight 74.65kDa altogether.It there are no at present raw using ZNF709 protein as gastric cancer
The report of object marker.
Summary of the invention
Application and its examination the purpose of the present invention is to provide a kind of ZNF709 albumen as gastric cancer serum biomarker
Agent box.Specificity using the serum mark analyte detection gastric cancer is 85%, sensibility 81%, and provided kit is one kind
Cancer diagnosis reagent box sensitive, safe, easy to operate can be used to the immune of protein Z NF709 in qualitative detection human serum
Thus Lysozyme antibody level reflects the level of ZNF709 albumen.
This kit using enzyme linked immunosorbent assay (ELISA) technology (Enzyme linked immunosorbent assay,
ELISA), horizontal using the immunoglobulin g antibody of protein Z NF709 in indirect method qualitative detection human serum.With the people of purifying
Solid phase antigen is made in protein Z NF709 coating microwell plate, then sequentially adds test serum and phase into the micropore of envelope antigen
Reagent, then two anti-bindings with HRP label are closed, ZNF709- antibody-ELIAS secondary antibody compound is formed, finally by thoroughly washing
Afterwards plus substrate TMB develops the color.TMB converts au bleu under the catalysis of HRP enzyme, and is converted to final yellow under the action of an acid,
The immunoglobulin g antibody level of its shade and protein Z NF709 in test sample is positively correlated.Finally use enzyme mark
Instrument measures absorbance value (OD value) as quantization testing result under 450nm wavelength.
The purpose of the present invention is what is be achieved through the following technical solutions:
In a first aspect, the application the present invention provides a kind of ZNF709 albumen as gastric cancer serum biomarker.
Preferably, the ZNF709 albumen is induced excessively from the saccharomyces cerevisiae being transformed via genetic engineering through galactolipin
Expression, then isolate and purify and obtain through agarose compatible medium glutathione.
Preferably, the ZNF709 albumen behaviour ZNF709 albumen.
Second aspect, the present invention provides a kind of gastric cancer serum biomarkers, including ZNF709 albumen.
The third aspect, the present invention provides a kind of gastric cancer serum marker detection kits, comprising: is coated on ELISA Plate
ZNF709 albumen, the standard serum 1 of 0U/ml, the standard serum 2 of 100U/mL, enzyme marking reagent, enzyme substrate solution, confining liquid,
Sample diluting liquid, cleaning solution, terminate liquid.
Preferably, the enzyme substrate solution is TMB application liquid, including color developing agent A and color developing agent B;
The color developing agent A is in terms of every 500mL, including following each component: sodium acetate 10.7-14.2g, citric acid 0.3-
1.9g, 30% hydrogen peroxide 0.2-0.6mL;
The color developing agent B is in terms of every 500mL, including following each component: TMB 200-650mg, DMSO 5-30mL, lemon
Sour 3.2-7.9g.
Preferably, in the preparation of the ZNF709 albumen being coated on ELISA Plate, the coating buffer used is 0.05M
Carbonate buffer solution;The carbonate buffer solution includes following components: sodium carbonate 1.59g/L, sodium bicarbonate 2.93g/L;It is described
The pH value of carbonate buffer solution is 7.4.
Preferably, the confining liquid is PBS buffering containing 0.5% bovine serum albumin(BSA), concentration is 0.01mol/L
Liquid specifically includes: bovine serum albumin BSA 5g/L, sodium chloride 8g/L, potassium chloride 0.2g/L, dipotassium hydrogen phosphate 0.2g/L, 12
Hypophosphite monohydrate hydrogen sodium 2.9g/L, pH value 7.4.
Preferably, the sample diluting liquid is the PBS buffer solution of 0.01mol/L, is specifically included: potassium chloride 0.2g/L, chlorine
Change sodium 8g/L, disodium hydrogen phosphate 0.2g/L, 12 hypophosphite monohydrate hydrogen sodium 2.9g/L, pH value 7.4.
Preferably, the cleaning solution is the PBST phosphate buffer of 0.01mol/L, is specifically included: potassium chloride 0.2g/L,
Sodium chloride 8g/L, dipotassium hydrogen phosphate 0.2g/L, 12 hypophosphite monohydrate hydrogen sodium 2.9g/L, Tween-20 0.5mL/L, pH value are
7.4;
The terminate liquid is 2mol/L sulfuric acid solution;
The enzyme marker is the immunoglobulin G antibody of horseradish peroxidase-labeled.
Fourth aspect, the present invention provides a kind of immune balls based on aforementioned agents box measurement Proteins in Serum ZNF709
The method of protein G/antibody concentration, comprising the following steps:
(1) it is coated with: being added to hole enzyme mark after the human protein ZNF709 of purifying is diluted to 1 μ g/mL with coating buffer
It in plate, is coated with 2 hours, is washed out 3 times in 37 DEG C, dry;
(2) it closes: 200 μ L of confining liquid is added, is placed at room temperature for 2 hours, wash 3 times, drying;
(3) it is loaded: 0U/ml standard serum 1,100U/ml standard serum 2 and test serum sample is respectively pressed into 1:100 dilution
It is added in each antigen measuring orifice plate after to 100 μ L, shakes even rear capping or overlay film;
(4) incubate: ELISA Plate gets rid of liquid in clear opening after being placed in 37 DEG C of reactions 120 minutes, does not have to washing;
(5) enzyme label: every hole adds the 100 μ L of immunoglobulin G antibody of horseradish peroxidase-labeled, puts in 37 DEG C
It sets and gets rid of liquid in clear opening after sixty minutes, patted dry after board-washing 5 times.
(6) it develops the color: patting dry rear each hole drop and each 50 μ L of color developing agent A and color developing agent B is successively added, concussion is mixed, kept away in 37 DEG C
After light places colour developing 15 minutes, 50 μ L of terminate liquid is added, terminates reaction.
(7) optical density for sequentially measuring each hole in 450nm wavelength with enzyme-linked instrument, is then calculated to get egg in serum
The immunoglobulin g antibody concentration of white matter ZNF709.
Compared with prior art, the present invention have it is following the utility model has the advantages that
1. ZNF709 albumen provided by the invention has high specific as gastric cancer serum biomarker;
2. can be used to qualitative, quantitative the present invention provides a kind of commercial kit sensitive, safe, easy to operate and survey
The immunoglobulin g antibody for determining protein Z NF709 in human serum is horizontal, reflects the level of ZNF709 albumen, for stomach
Cancer diagnosis.
Specific embodiment
The present invention is described in detail combined with specific embodiments below.Following embodiment will be helpful to the technology of this field
Personnel further understand the present invention, but the invention is not limited in any way.It should be pointed out that the ordinary skill of this field
For personnel, without departing from the inventive concept of the premise, several changes and improvements can also be made.These belong to the present invention
Protection scope.
The present invention is described further in conjunction with the embodiments.
Embodiment 1
1. expression, purifying and identification ZNF709 albumen:
The acquisition of human protein ZNF709 is to utilize half from the saccharomyces cerevisiae being transformed by genetic engineering using conventional method
Lactose induces overexpression, then isolates and purifies gained through agarose compatible medium glutathione, and pass through Western-
Blotting identification.
2. the preparation of blood serum sample:
Whole blood sample is centrifuged 20 minutes after being placed at room temperature for 2 hours, and supernatant is taken to be dispensed, and is put in -80 DEG C of preservations.
Blood serum sample after defrosting just can be used for detecting after need to being centrifuged again.
The preparation method of the various buffers of 3.ELISA method and reagent:
(1) it is coated with buffer: 0.05M sodium carbonate-bicarbonate (pH 9.6)
(2) sample diluting liquid: the PBS solution of pH 7.4
(3) cleaning solution: the PBST solution of pH 7.4
(4) confining liquid: the PBS solution (pH 7.4) of 0.5%BSA
(5) enzyme substrate solution: color developing agent A and color developing agent B
(ready-to-use)
(ready-to-use)
(6) terminate liquid: 2mol/L sulfuric acid solution
(concentrated sulfuric acid is slowly dropped into distilled water by timing, and side edged mixes)
The immunoglobulin G antibody concentration and diagnosing gastric cancer of 4.ELISA method measurement Proteins in Serum ZNF709:
Specific steps are as follows:
(1) it is coated with: being added to 96 hole enzymes after the human protein ZNF709 of purifying is diluted to 1 μ g/mL with coating buffer
In target, it is coated in 37 DEG C 2 hours, is then washed 3 times using cleaning solution, drying.
(2) it closes: 200 μ L of confining liquid is added, is placed at room temperature for 2 hours, washed 3 times using cleaning solution, drying.
(3) it is loaded: by standard items (0U/ml standard serum 1,100U/ml standard serum 2;Directly to buy) and blood to be measured
Final proof product (obtained by the method for step 2) are added to step (1) after respectively diluting by 1:100 and (use sample diluting liquid) to 100 μ L and make
In 96 hole elisa Plates of standby coating human protein ZNF709, even rear capping or overlay film are shaken.Standard items and sample to be tested need to be
It is prepared in 15 minutes before use, it is disposable.
(4) incubate: ELISA Plate gets rid of liquid in clear opening after being placed in 37 DEG C of reactions 120 minutes, does not have to washing.
(5) enzyme label: every hole adds the 100 μ L of immunoglobulin G antibody of horseradish peroxidase-labeled, puts in 37 DEG C
It sets and gets rid of liquid in clear opening after sixty minutes, patted dry after board-washing 5 times.
(6) it develops the color: patting dry rear each hole drop and each 50 μ L of color developing agent A and color developing agent B is successively added, concussion is mixed, kept away in 37 DEG C
After light places colour developing 15 minutes, 50 μ L of terminate liquid is added, terminates reaction.
(7) result judgement:
I. the optical density (OD value) for sequentially measuring each hole in 450nm wavelength with enzyme-linked instrument, is then calculated by the following formula
Obtain the concentration (unit values of i.e. following formula) of the immunoglobulin g antibody of anti-ZNF709 in serum.
* A450 is the abbreviation of absorbance at 450nm.
* current ZNF709 antibody there is no the reference standard of the current international practice, therefore use when this test result calibration opposite
Unit.
Ii. in serum anti-ZNF709 value judgement:
Anti- ZNF709 value (U/mL) | Determine |
Greater than 5 | Gastric cancer |
2-5 | It is high-risk |
Less than 2 | Health |
Iii. quality controls
Each testing result has to comply with following standard:
The A450 of standard serum 1 :≤0.100
The A450 of standard serum 2: >=0.700
Above-mentioned standard is not met such as, then result is considered as in vain, it is necessary to detect again.
Iv. the explanation of inspection result
The ROC analysis of 50 Healthy Human Serums, 37 Serum Obtained From Advance Gastric Cancers, 14 high-risk patient serum is established above
Reference value.
5. specificity and sensitivity Detection: using 101 parts of blood serum samples (50 Healthy Human Serums, 37 blood in patients with gastric carcinoma
Clearly, 14 high-risk patient serum) specificity and sensitivity Detection have been carried out to the present invention.Spy of the present invention for the diagnosing gastric cancer that breaks
The opposite sex is 85%, sensibility 81%.
Specific embodiments of the present invention are described above.It is to be appreciated that the invention is not limited to above-mentioned
Particular implementation, those skilled in the art can make a variety of changes or modify within the scope of the claims, this not shadow
Ring substantive content of the invention.In the absence of conflict, the feature in embodiments herein and embodiment can any phase
Mutually combination.
Claims (10)
1. a kind of application of ZNF709 albumen as gastric cancer serum biomarker.
2. application according to claim 1, which is characterized in that the ZNF709 albumen was transformed from via genetic engineering
Saccharomyces cerevisiae induce overexpression through galactolipin, then isolate and purify and obtain through agarose compatible medium glutathione.
3. a kind of gastric cancer serum biomarker, which is characterized in that including ZNF709 albumen.
4. a kind of gastric cancer serum marker detection kit characterized by comprising the ZNF709 egg being coated on ELISA Plate
White, 0U/ml standard serum 1, the standard serum 2 of 100U/mL, enzyme marking reagent, enzyme substrate solution, confining liquid, sample diluting liquid,
Cleaning solution, terminate liquid.
5. gastric cancer serum marker detection kit according to claim 4, which is characterized in that the enzyme substrate solution is
TMB application liquid, including color developing agent A and color developing agent B;
The color developing agent A is in terms of every 500mL, including following each component: sodium acetate 10.7-14.2g, citric acid 0.3-1.9g,
30% hydrogen peroxide 0.2-0.6mL;
The color developing agent B is in terms of every 500mL, including following each component: TMB 200-650mg, DMSO 5-30mL, citric acid
3.2-7.9g。
6. gastric cancer serum marker detection kit according to claim 4, which is characterized in that described to be coated in ELISA Plate
On ZNF709 albumen preparation in, the coating buffer used is 0.05M carbonate buffer solution;The carbonate buffer solution packet
Include following components: sodium carbonate 1.59g/L, sodium bicarbonate 2.93g/L;The pH value of the carbonate buffer solution is 7.4.
7. gastric cancer serum marker detection kit according to claim 4, which is characterized in that the confining liquid be containing
0.5% bovine serum albumin(BSA), concentration be 0.01mol/L PBS buffer solution, specifically include: bovine serum albumin BSA 5g/L, chlorine
Change sodium 8g/L, potassium chloride 0.2g/L, dipotassium hydrogen phosphate 0.2g/L, 12 hypophosphite monohydrate hydrogen sodium 2.9g/L, pH value 7.4.
8. gastric cancer serum marker detection kit according to claim 4, which is characterized in that the sample diluting liquid is
The PBS buffer solution of 0.01mol/L, specifically includes: potassium chloride 0.2g/L, sodium chloride 8g/L, disodium hydrogen phosphate 0.2g/L, Shi Ershui
Close dibastic sodium phosphate 2.9g/L, pH value 7.4.
9. gastric cancer serum marker detection kit according to claim 4, which is characterized in that the cleaning solution is
The PBST phosphate buffer of 0.01mol/L, specifically includes: potassium chloride 0.2g/L, sodium chloride 8g/L, dipotassium hydrogen phosphate 0.2g/
L, 12 hypophosphite monohydrate hydrogen sodium 2.9g/L, Tween-20 0.5mL/L, pH value 7.4;
The terminate liquid is 2mol/L sulfuric acid solution;
The enzyme marker is the immunoglobulin G antibody of horseradish peroxidase-labeled.
10. a kind of immunoglobulin g antibody concentration based on kit measurement Proteins in Serum ZNF709 described in claim 4
Method, which comprises the following steps:
(1) it is coated with: being added in hole elisa Plates after the human protein ZNF709 of purifying is diluted to 1 μ g/mL with coating buffer,
It is coated with 2 hours, is washed out 3 times in 37 DEG C, dry;
(2) it closes: 200 μ L of confining liquid is added, is placed at room temperature for 2 hours, wash 3 times, drying;
(3) it is loaded: 0U/ml standard serum 1,100U/ml standard serum 2 and test serum sample is respectively diluted to 100 by 1:100
It is added to after μ L in each antigen measuring orifice plate, shakes even rear capping or overlay film;
(4) incubate: ELISA Plate gets rid of liquid in clear opening after being placed in 37 DEG C of reactions 120 minutes, does not have to washing;
(5) enzyme label: every hole adds the 100 μ L of immunoglobulin G antibody of horseradish peroxidase-labeled, places 60 in 37 DEG C
Liquid in clear opening is got rid of after minute, is patted dry after board-washing 5 times.
(6) it develops the color: patting dry rear each hole drop and each 50 μ L of color developing agent A and color developing agent B is successively added, concussion mixes, is protected from light and puts in 37 DEG C
After setting colour developing 15 minutes, 50 μ L of terminate liquid is added, terminates reaction.
(7) then the optical density for sequentially measuring each hole in 450nm wavelength with enzyme-linked instrument is calculated to get albumen anti-in serum
The immunoglobulin g antibody concentration of matter ZNF709.
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CN117487816A (en) * | 2023-11-03 | 2024-02-02 | 中山大学孙逸仙纪念医院 | Application of ZNF709 gene in preparing medicament for treating PBC |
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CN117487816A (en) * | 2023-11-03 | 2024-02-02 | 中山大学孙逸仙纪念医院 | Application of ZNF709 gene in preparing medicament for treating PBC |
CN117487816B (en) * | 2023-11-03 | 2024-06-04 | 中山大学孙逸仙纪念医院 | Application of ZNF709 gene in preparing medicament for treating PBC |
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