CN108663528A - A kind of excellent effect lead chelating type immune complex and preparation method thereof - Google Patents
A kind of excellent effect lead chelating type immune complex and preparation method thereof Download PDFInfo
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- CN108663528A CN108663528A CN201810598903.2A CN201810598903A CN108663528A CN 108663528 A CN108663528 A CN 108663528A CN 201810598903 A CN201810598903 A CN 201810598903A CN 108663528 A CN108663528 A CN 108663528A
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- G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
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Abstract
The invention discloses a kind of excellent effect lead chelating type immune complex, which is following one kind:Lead ion is incorporated into the compound of immune complex formation;Or lead ion be incorporated into after carrier protein with and the antibody that specifically binds of the carrier protein be formed by compound;Or lead ion be incorporated into immunoglobulin after the compound to be formed is combined with carrier protein.The invention also discloses a kind of preparation methods of excellent effect lead chelating type immune complex, include the following steps:S1:Prepare chelating agent solution, S2:Formulation vehicle protein solution, S3:It is stirred overnight, S4:Dialysis treatment, S5:Lead ion, S6 is added:Devil liquor recovery processing;S7:It is specifically bound.The method of the present invention scope of application is wider, can be cost-effective, and improves dialysis rate, can shorten manufacturing cycle, also have the characteristics that energy conservation and environmental protection, avoids causing chemical contamination, therefore the present invention has the larger market competitiveness.
Description
Technical field
The present invention relates to a kind of chelate field, specially a kind of excellent effect lead chelating type immune complex and its preparation
Method.
Background technology
Chelate Mineral Floating Process, hydrometallurgy, metallic element extraction with detach, the catalyzing and synthesizing of substance, water
Softening, electroplating technology, medical industry, dyeing course etc. in be all widely used;Existing lead chelating type immune complex
Preparation method it is incomplete, the scope of application is ignored enough wide, it has not been convenient to the preparation process of object is completed in small-size laboratory,
And number of dialysing is excessive, can extend the manufacturing cycle of object to a certain extent, and there are no give up to the ion etc. in waste liquid
Object, which is done, clearly to be handled, and the wastes such as ion in waste liquid, which do not handle rear discharge up to standard, can cause chemical contamination.
Invention content
The purpose of the present invention is to provide a kind of excellent effect lead chelating type immune complexs and preparation method thereof, to solve
The problems mentioned above in the background art.
To achieve the above object, the present invention provides the following technical solutions:A kind of lead chelating type immune complex, lead chelating
Type immune complex is following one kind:
Lead ion is incorporated into the compound of immune complex formation;
Or lead ion be incorporated into after carrier protein with and the antibody that specifically binds of the carrier protein be formed by compound;
Or lead ion be incorporated into immunoglobulin after the compound to be formed is combined with carrier protein.
Preferably, zinc fingers, sulfydryl, cysteine are at least contained in the structure of the immune complex or carrier protein
One kind in residue, lead ion are mutually tied with immune complex or carrier protein with zinc fingers or sulfydryl or cysteine residues
It closes.
Preferably, the carrier protein is antibody protein, lipoprotein, hemoglobin, nuclear antigen, foreign sera antigen, disease
One kind among poison, bacterium, protozoon, worm or immunoglobulin.
Preferably, it is specifically bound again with energy and carrier protein after lead ion is combined by chelating agent with carrier protein anti-
Body combines, and the chelating agent is one kind in ITCBE, EDTA, polyphosphate, amino carboxylic acid, 1,3- diketone, hydroxycarboxylic acid.
A kind of preparation method of lead chelating type immune complex as described in claim 1, includes the following steps:
S1:First chelating agent solution is prepared and is completed, then chelating agent is dissolved in solvent, you can obtains chelating agent solution;
S2:Appropriate carrier protein is taken, carrier protein is added in borate buffer solution, you can it is molten that carrier protein is made
Liquid;
S3:Chelating agent solution obtained is added in carrier protein solution, is placed in water bath with thermostatic control and stirs evenly,
Water bath with thermostatic control 4-30h, you can obtain mixed liquor;
S4:It fetches bag filter and EDTA-NaHCO3 solution is added in bag filter and boil, bag filter is fixed on water tank
Middle part, and enough ddH2O are added in water tank, the volume ratio of solution is 90-95 in the volume and bag filter of the ddH2O:1,
It repeats the step 3-4 times, the mixing in S3 is fitted into bag filter, bag filter is placed in constant temperature water tank, in constant temperature water tank
It is added enough ddH2O, the volume ratio of solution is 90-95 in the volume and bag filter of the ddH2O:1, it, will after dialysed overnight
Liquid in bag filter is collected.
S5:PH to 7.0 is adjusted dilute hydrochloric acid solution is added from the liquid collected in bag filter, it is molten to be slowly dropped into lead ion
Liquid, when instillation, do not stop to shake, and instill and complete to be placed in water bath with thermostatic control and stir evenly, water bath with thermostatic control 4-30h, then repeatedly S4
Once, liquid is collected, lead chelating type antigen is obtained.
S6:The waste liquid collected in solution and S5 in S4 outside bag filter is mixed, is added into mixed solution
The activated carbon for entering to have loaded nano-titanium dioxide is adsorbed, and repeats to add above-mentioned absorbent charcoal material, reuses atomic fluorescence
Method carries out quantitative analysis to processed solution, and when lead ion enrichment degree reaches 0.1mol/ml in solution, recycling lead ion is again
It utilizes.
S7:The antibody that can be specifically bound with carrier protein is added in above-mentioned lead chelating type antigen, lead is obtained after reaction
Chelating type immune complex.
The present invention also provides above-mentioned lead chelating type immune complexs to prepare detection lead chelating type CIC ELISA
Reagent or enzyme linked immunological kit in application.
The present invention also provides a kind of above-mentioned enzyme linked immunological kit of detection lead chelating type CIC ELISA, the examinations
Agent box includes the standard items of above-mentioned lead chelating type immune complex.
Preferably, mentioned reagent box further includes at least one following reagent:Albumen containing capture antigen antibody complex
Coating buffer, the coating buffer of antibody containing capture lead, enzyme labelled antibody.
A method of lead chelating type CIC ELISA is quantitatively detected, it is immune with the above-mentioned lead chelating type of known content
Compound is detected as standard items using a pair of sample of following methods:Enzyme-linked immunization, enzyme linked immunological and Atomic absorption
Spectrum combined techniques, enzyme linked immunological and inductivity coupled plasma mass spectrometry combined techniques, purification immune complex and atomic absorption spectrum
Combined techniques, purification immune complex and inductivity coupled plasma mass spectrometry combined techniques, electrophoresis and enzyme linked immunological or atomic absorption light
Spectrum or inductivity coupled plasma mass spectrometry combined techniques.
Compared with prior art, the beneficial effects of the invention are as follows:The method of the present invention scope of application is wider, can save into
This, and increase the differential water pressures inside and outside bag filter, dialysis rate is improved, manufacturing cycle can be shortened, also to the ion in waste liquid
Equal wastes are handled, and have the characteristics that energy conservation and environmental protection, avoid causing chemical contamination, therefore the present invention has larger market competing
Strive power.
Description of the drawings
Fig. 1 is the flow diagram of the present invention.
Specific implementation mode
The technical scheme in the embodiments of the invention will be clearly and completely described below, it is clear that described implementation
Example is only a part of the embodiment of the present invention, instead of all the embodiments.Based on the embodiments of the present invention, this field is common
The every other embodiment that technical staff is obtained without making creative work belongs to the model that the present invention protects
It encloses.
The present invention provides a kind of technical solution:A kind of lead chelating type immune complex, the lead chelating type immune complex are
Following one kind:
Lead ion is incorporated into the compound of immune complex formation;
Or lead ion be incorporated into after carrier protein with and the antibody that specifically binds of the carrier protein be formed by compound;
Or lead ion be incorporated into immunoglobulin after the compound to be formed is combined with carrier protein.
Further, it is residual that zinc fingers, sulfydryl, cysteine are at least contained in the structure of immune complex or carrier protein
One kind in base, lead ion are combined with immune complex or carrier protein with zinc fingers or sulfydryl or cysteine residues.
Further, it is residual that zinc fingers, sulfydryl, cysteine are at least contained in the structure of immune complex or carrier protein
One kind in base, lead ion are combined with immune complex or carrier protein with zinc fingers or sulfydryl or cysteine residues.
Further, carrier protein be antibody protein, lipoprotein, hemoglobin, nuclear antigen, foreign sera antigen, virus,
One kind among bacterium, protozoon, worm or immunoglobulin.
A kind of preparation method of lead chelating type immune complex as claimed in claim 1, include the following steps:
S1:First chelating agent solution is prepared and is completed, then chelating agent is dissolved in solvent, you can obtains chelating agent solution;
S2:Appropriate carrier protein is taken, carrier protein is added in borate buffer solution, you can it is molten that carrier protein is made
Liquid;
S3:Chelating agent solution obtained is added in carrier protein solution, is placed in water bath with thermostatic control and stirs evenly,
Water bath with thermostatic control is for 24 hours, you can obtains mixed liquor;
S4:It fetches bag filter and EDTA-NaHCO3 solution is added in bag filter and boil, bag filter is fixed on water tank
Middle part, and enough ddH2O are added in water tank, the volume ratio of solution is 91 in the volume and bag filter of the ddH2O:1, it repeats
Mixing in S3 is fitted into bag filter, bag filter is placed in constant temperature water tank by the step 2 time, and foot is added in constant temperature water tank
The volume ratio of solution is 91 in the volume and bag filter of the ddH2O of amount, the ddH2O:1, it, will be in bag filter after dialysed overnight
Liquid is collected.
S5:PH to 7.0 is adjusted dilute hydrochloric acid solution is added from the liquid collected in bag filter, it is molten to be slowly dropped into lead ion
Liquid, when instillation, do not stop to shake, and instill and complete to be placed in water bath with thermostatic control and stir evenly, water bath with thermostatic control for 24 hours, then repeatedly S4 mono-
It is secondary, liquid is collected, lead chelating type antigen is obtained.
S6:The waste liquid collected in solution and S5 in S4 outside bag filter is mixed, is added into mixed solution
The activated carbon for entering to have loaded nano-titanium dioxide is adsorbed, and repeats to add above-mentioned absorbent charcoal material, reuses atomic fluorescence
Method carries out quantitative analysis to processed solution, and when lead ion enrichment degree reaches 0.1mol/ml in solution, recycling lead ion is again
It utilizes.
S7:The antibody that can be specifically bound with carrier protein is added in above-mentioned lead chelating type antigen, lead is obtained after reaction
Chelating type immune complex.
The present invention also provides above-mentioned lead chelating type immune complexs to prepare detection lead chelating type CIC ELISA
Reagent or enzyme linked immunological kit in application.
The present invention also provides a kind of above-mentioned enzyme linked immunological kit of detection lead chelating type CIC ELISA, the examinations
Agent box includes the standard items of above-mentioned lead chelating type immune complex.
Mentioned reagent box further includes at least one following reagent:The coating of albumen containing capture antigen antibody complex
Liquid, the coating buffer containing the antibody for capturing lead, enzyme labelled antibody.
In the present invention, it is following several to realize that the kit of the object of the invention can be listed, but it is not limited to this.
A kind of kit for detecting lead chelating type CIC ELISA, including:It is multiple containing antigen-antibody can be captured
The coating buffer of the albumen of conjunction object, confining liquid, washing buffer, anti-antibody lead, enzyme labelled antibody, substrate, terminate liquid, dilution buffer
Liquid, positive control, negative control.
A kind of kit for detecting lead chelating type CIC ELISA, including:It is multiple containing antigen-antibody can be captured
The coating buffer of the albumen of conjunction object, confining liquid, washing buffer, eluent, positive control, negative control.
A kind of kit for detecting lead chelating type CIC ELISA, including:It is multiple containing antigen-antibody can be captured
The coating buffer of the albumen of conjunction object, confining liquid, washing buffer, eluent, nitric acid, hydrogen peroxide, positive control, negative control.
A kind of kit for detecting lead chelating type CIC ELISA, including be used to extract needed for immune complex
Solution redissolves liquid, the coating buffer containing the antibody that can capture lead, confining liquid, washing buffer, enzyme labelled antibody, substrate, termination
Liquid, dilution buffer, standard items, negative control.
A kind of kit for detecting lead chelating type CIC ELISA:Including being used to extract needed for immune complex
Solution redissolves liquid, positive control, negative control.
In above-mentioned several kits, coating buffer be capture CIC ELISA albumen, as C1Q, CIF albumen,
Anti-C_3 antibody;Confining liquid is the bovine serum albumin(BSA) or skimmed milk power that mass concentration is 2%-4%;Eluent includes but not limited to
The Tris-HCl buffer solutions of papain;It is to include but not limited to redissolve liquid;Glue bed medium includes but not limited to agarose
Gel, polyacrylamide gel;Include but not limited to PEG solution, boric acid salt buffer for extracting solution needed for immune complex
Liquid;Substrate includes but not limited to TMB solution, ABTS solution;Sample-loading buffer includes but not limited to the Tris- containing bromophenol blue
HCl buffer solutions;Enzyme labelled antibody is the antibody marked containing enzymes such as horseradish peroxidase, alkaline phosphatases, as HRP enzyme marks are anti-
Body;Standard items include but not limited to the present invention lead chelating type CIC ELISA, other be chelated with the immune complex of lead;
Positive control include but not limited to lead chelating type CIC ELISA of the present invention, other be chelated with the immune complex of lead, the moon
Property control be dilution buffer.
Another object of the present invention is to provide a kind of method quantitatively detecting lead chelating type CIC ELISA, with
Know that the above-mentioned lead chelating type immune complex of content as standard items, is detected using a pair of sample of following methods:It is enzyme-linked
Immunization, enzyme linked immunological and atomic absorption spectrum combined techniques, enzyme linked immunological and inductivity coupled plasma mass spectrometry combined techniques, purification
Immune complex and atomic absorption spectrum combined techniques, purification immune complex and inductivity coupled plasma mass spectrometry combined techniques, electricity
Swimming and enzyme linked immunological or atomic absorption spectrum or inductivity coupled plasma mass spectrometry combined techniques.
In the present invention, the having of can listing of method with detection lead chelating type immune complex is following several, but not
It is limited to following several.
Unless otherwise indicated, the laboratory operating procedures being related to are the step of this field routine to the present invention, and reagent, material are such as
It is following cited, do not enumerate in the present invention come be commonly used in the art or can be obtained by mode purchased in market:
Dilution buffer is the 0.05M carbonate buffer solutions of pH9.6, preparation method example:Take 1.5g Na2CO3 and
The NaHCO3 dissolvings of 2.93g plus ddH2O are settled to 1000mL;
Washing buffer is the 0.15MPBS buffer solutions of pH7.4, preparation method example:Take KH2PO4,2.90g's of 0.2g
KCl, 0.5mLTween-20 of NaCl, 0.2g of Na2HPO412H2O, 8.0g, dissolving plus ddH2O are settled to 1000mL;
Confining liquid is bovine serum albumin solution, preparation method example:0.1g bovine serum albumin(BSA)s are taken, washing buffer is added
Liquid dilution is settled to 100mL;
Terminate liquid is 2MH2SO4, preparation method example:The ddH2O for taking 178.3mL is added along wall dense dropwise into ddH2O
H2SO4, it is stirring while adding, it is settled to 200mL;
The pH of substrate buffer solution is 5.0, the molar concentration of Na2HPO4 is 0.2M, the molar concentration of citric acid is 0.1M, often
The preparation method of the substrate buffer solution of 50mL is as follows:1.42gNa2HPO4,0.96g citric acid are taken, ddH2O then is added extremely
50mL to get;
Substrate is methyl biphenyl amine (TMB) solution, and methyl biphenyl amine (TMB) solution is by the group distribution according to following ratio
It makes:TMB:Substrate buffer solution:0.75%H2O2=0.5mL:10mL:32 μ L, wherein TMB are the methyl biphenyl amine second of 2g/L
Alcoholic solution;
The albumen that immune complex can be captured is the albumen that can be specifically bound with immune complex, including but not limited to
Such as C1Q, CIF albumen, anti-C_3 antibody;In following embodiment, can capture immune complex albumen it is specifically used be
C1qRecombinantProtein, article No. are " NOVUSH00000712-p01 ";
Substance with lead specific binding is the anti-PbmAb of mouse that article No. is " bar proud AP7019 ";In following implementation
With lead specific binding substance, anti-antibody lead be capture lead substance;
The antibody that can be specifically bound with human serum albumins is rabbit anti-human serum albumin antibodies, is commercially available.
Dilution multiple proportions is w/v below.
Method one:ELISA method detection lead chelating type immune complex, is as follows:
1) albumen that can capture immune complex is coated on solid phase carrier:C1Q is diluted with dilution buffer
Albumen is added to 2500-20000 times in elisa plate micropore, and 4 DEG C of 16-18 hour overnight or 37 DEG C of water-baths 1-3 hours store
Refrigerator;
2) it closes:Dilution buffer is removed, washing buffer is used in combination to be washed, is waited after the completion of washing, adds confining liquid, 37
It DEG C places 1 hour, removes confining liquid, washing buffer is used in combination to be washed, after the completion of washing, elisa plate is placed 1 small in 37 DEG C
When;
3) add sample to be tested, and incubate:It is sampled from the circulatory system, makees sample to be tested;With the lead chelating type of known content
Immune complex makees standard items;10-40 times is diluted with dilution buffer, is added in micropore, 37 DEG C act on 1-2 hours;
4) substance of capture lead is added, and incubates:Sample to be tested is removed, washing buffer is used in combination to be washed, it is to be washed
After the completion of washing, addition is diluted with dilution buffer to be had the substance of affinity with lead or can react to form antigen antibody complex with lead
Anti- antibody lead be diluted to 60000-250000 times, 37 DEG C act on 1-2 hours, it is made to be reacted with the lead on immune complex;
5) enzyme conjugates incubates:Anti- antibody lead is removed, washing buffer is used in combination to be washed, is waited after the completion of washing, is added
With the diluted HRP enzyme labelled antibodies of dilution buffer, 37 DEG C act on 1-2 hours, it is made to be reacted with anti-antibody lead;
6) substrate incubates:Enzyme labelled antibody is removed, washing buffer is used in combination to be washed, is waited after the completion of washing, substrate is added,
37 DEG C are protected from light effect 30 minutes;
7) reaction is terminated:Terminate liquid is added dropwise to each micropore;
8) it is 405nm to take wavelength, and elisa plate is placed in microplate reader to the OD for reading sample to be tested group and standard items respectively
Value draws standard curve, acquires the content of sample to be tested.
In this method, when step 8) detects, microplate reader can not be used, qualitative inspection is directly carried out by the situation that develops the color yet.
This method utilizes enzyme linked immunosorbent assay (ELISA) (ELISA) principle, can be compound by the nospecific immunity in serum
Object extracts, and weight lead is partly chelated on the immune complex extracted, and the lead on this partial immunity compound can be with
It is captured by the substance for having affinity with lead or the specific antibody that the anti-lead to form antigen antibody complex can be reacted with lead, it
Can (antibody nonrecognition coating egg be captured by the antibody that the enzymes such as horseradish peroxidase, alkaline phosphatase mark again afterwards
In vain), the antibody in capture reads OD values under the action of color developing agent and terminate liquid under instrument, and exempts from without containing chelating lead
Epidemic disease compound will not then be captured by the specific antibody of anti-lead, will not be with the enzymes such as horseradish peroxidase, alkaline phosphatase
The antibody of label is captured, and lead (negative control group result is feminine gender) is not contained in agents useful for same yet, thus when read
When OD value results are shown as the positive, you can prove the lead for detecting to chelate on CIC ELISA.
Method two:ELISA method+AAS methods detect lead chelating type immune complex, are as follows:
1) albumen that can capture immune complex is coated on solid phase carrier:Coating protein is diluted with dilution buffer
It to 7000-13000 times, is added in elisa plate micropore, 4 DEG C of 16-18 hour overnight or 37 DEG C of water-baths 1-3 hours, storage refrigerator;
2) it closes:Dilution buffer is removed, washing buffer is used in combination to be washed, is waited after the completion of washing, adds confining liquid, 37
It DEG C places 1 hour, removes confining liquid, washing buffer is used in combination to be washed, after the completion of washing, elisa plate is placed 1 small in 37 DEG C
When;
3) add sample to be tested, and incubate:It is sampled from the circulatory system, makees sample to be tested;With the lead chelating type of known content
Immune complex makees standard items;10-40 times is diluted with dilution buffer, is added in micropore, 37 DEG C act on 1-2 hours;
4) it elutes:Sample to be tested is removed, washing buffer is used in combination to be washed, is waited after the completion of washing, eluent is added, in
It is acted on 1-2 hours at 37 DEG C;
5) it detects:It samples from ELISA micropores, is chelated in the lead on immune complex in Atomic Absorption Spectrometer detection,
Read respective value.
This method further combines atomic absorption spectrum (AAS) principle on the basis of enzyme linked immunological principle, utilizes original
Sub- absorption spectrometer detection chelating is in the lead on CIC ELISA, due to only containing immune complex in solution, and it is used
Without lead (negative control group result is feminine gender) in reagent, result will not be shone at interference, thus when read result is shown
For the positive when, you can prove the lead for detecting to chelate on CIC ELISA.
The method of the present invention scope of application is wider, can be cost-effective, and increases the differential water pressures inside and outside bag filter, improves
It dialyses rate, can shorten manufacturing cycle, also the wastes such as ion in waste liquid are handled, has the characteristics that energy conservation and environmental protection, keeps away
Exempt to cause chemical contamination, therefore the present invention has the larger market competitiveness.
It although an embodiment of the present invention has been shown and described, for the ordinary skill in the art, can be with
Understanding without departing from the principles and spirit of the present invention can carry out these embodiments a variety of variations, modification, replace
And modification, the scope of the present invention is defined by the appended.
Claims (9)
1. a kind of lead chelating type immune complex, which is characterized in that the lead chelating type immune complex is following one kind:
Lead ion is incorporated into the compound of immune complex formation;
Or lead ion be incorporated into after carrier protein with and the antibody that specifically binds of the carrier protein be formed by compound;
Or lead ion be incorporated into immunoglobulin after the compound to be formed is combined with carrier protein.
2. lead chelating type immune complex according to claim 1, it is characterised in that:The immune complex or carrier egg
At least containing one kind in zinc fingers, sulfydryl, cysteine residues, lead ion and immune complex or carrier in white structure
Albumen is combined with zinc fingers or sulfydryl or cysteine residues.
3. lead chelating type immune complex according to claim 2, it is characterised in that:The carrier protein is antibody egg
In vain, among lipoprotein, hemoglobin, nuclear antigen, foreign sera antigen, virus, bacterium, protozoon, worm or immunoglobulin
It is a kind of.
4. lead chelating type immune complex according to claim 1, it is characterised in that:The lead ion passes through chelating agent and load
Body protein is combined with the antibody of energy and carrier protein specific binding again after combining, and the chelating agent is ITCBE, EDTA, more phosphorus
One kind in hydrochlorate, amino carboxylic acid, 1,3- diketone, hydroxycarboxylic acid.
5. a kind of preparation method of lead chelating type immune complex as described in claim 1, which is characterized in that including following step
Suddenly:
S1:First chelating agent solution is prepared and is completed, then chelating agent is dissolved in solvent, you can obtains chelating agent solution;
S2:Appropriate carrier protein is taken, carrier protein is added in borate buffer solution, you can carrier protein solution is made;
S3:Chelating agent solution obtained is added in carrier protein solution, is placed in water bath with thermostatic control and stirs evenly, constant temperature
Water-bath 4-30h, you can obtain mixed liquor;
S4:It fetches bag filter and EDTA-NaHCO3 solution is added in bag filter and boil, bag filter is fixed in water tank
Portion, and enough ddH2O are added in water tank, the volume ratio of solution is 90-95 in the volume and bag filter of the ddH2O:1, weight
Multiple step 3-4 times, the mixing in S3 is fitted into bag filter, bag filter is placed in constant temperature water tank, is added in constant temperature water tank
Enter enough ddH2O, the volume ratio of solution is 90-95 in the volume and bag filter of the ddH2O:1, it, will be saturating after dialysed overnight
The liquid analysed in bag is collected.
S5:PH to 7.0 is adjusted dilute hydrochloric acid solution is added from the liquid collected in bag filter, is slowly dropped into lead ion solution,
Do not stop to shake when instillation, instills and complete to be placed in water bath with thermostatic control and stir evenly, water bath with thermostatic control 4-30h, then repeatedly S4 mono-
It is secondary, liquid is collected, lead chelating type antigen is obtained.
S6:The waste liquid collected in solution and S5 in S4 outside bag filter is mixed, is added into mixed solution negative
The activated carbon for having carried nano-titanium dioxide is adsorbed, and repeats to add above-mentioned absorbent charcoal material, reuses atomic fluorescence method pair
Processed solution carries out quantitative analysis, and when lead ion enrichment degree reaches 0.1mol/ml in solution, recycling lead ion is sharp again
With.
S7:The antibody that can be specifically bound with carrier protein is added in above-mentioned lead chelating type antigen, lead chelating is obtained after reaction
Type immune complex.
6. lead chelating type immune complex as described in claim 1 chelates the reagent of CIC ELISA preparing detection lead
Or the application in enzyme linked immunological kit.
7. a kind of enzyme linked immunological kit of detection lead chelating CIC ELISA, it is characterised in that:The kit includes such as
The standard items of lead chelating type immune complex described in claim 1.
8. enzyme linked immunological kit as claimed in claim 6, which is characterized in that the kit further includes that at least one or less is tried
Agent:The coating buffer or the coating buffer containing the antibody for capturing lead, enzyme labelled antibody of albumen containing capture antigen antibody complex.
9. a kind of method of qualitative detection lead chelating type CIC ELISA, which is characterized in that wanted with the right of known content
It asks the lead chelating type immune complex described in 1 as standard items, is detected using a pair of sample of following methods:Enzyme linked immunological
Method, enzyme linked immunological and atomic absorption spectrum combined techniques, enzyme linked immunological and inductivity coupled plasma mass spectrometry combined techniques, purification are immune
Compound and atomic absorption spectrum combined techniques, purification immune complex and inductivity coupled plasma mass spectrometry combined techniques, electrophoresis and
Enzyme linked immunological or atomic absorption spectrum or inductivity coupled plasma mass spectrometry combined techniques.
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CN105044369A (en) * | 2015-07-14 | 2015-11-11 | 上海拜豪生物科技有限公司 | Lead-chelated immune complex and preparation method and application thereof |
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CN104987409A (en) * | 2015-07-14 | 2015-10-21 | 上海拜豪生物科技有限公司 | Lead-IgG chelate as well as preparation method and application thereof |
CN105044369A (en) * | 2015-07-14 | 2015-11-11 | 上海拜豪生物科技有限公司 | Lead-chelated immune complex and preparation method and application thereof |
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