CN201852835U - ELISA (enzyme linked immunosorbent assay) kit of furaltadone metabolite - Google Patents
ELISA (enzyme linked immunosorbent assay) kit of furaltadone metabolite Download PDFInfo
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- CN201852835U CN201852835U CN 201020586590 CN201020586590U CN201852835U CN 201852835 U CN201852835 U CN 201852835U CN 201020586590 CN201020586590 CN 201020586590 CN 201020586590 U CN201020586590 U CN 201020586590U CN 201852835 U CN201852835 U CN 201852835U
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Abstract
The utility mode relates to an ELISA (enzyme linked immunosorbent assay) kit for detecting the furaltadone metabolite in an aquatic product. The kit comprises a 96-pore enzyme-labeled plate, enzyme-labeled secondary antibody, antibody working solution, standard substance solution, TMB (tetramethylbenzidine) substrate, stop solution, concentrated washing solution, concentrated composite solution, 2-nitrobenzaldehyde, a plate covering film, a valve bag, a specification and a quality inspection report. The use method of the kit comprises the steps of: precoating a coupling antigen on a micro-pore stripe of the enzyme-labeled plate by the indirect competitive ELISA method, wherein the residual furaltadone metabolite in a sample competes with the coupling antigen precoated on the micro-pore stripe for an antibody of the furaltadone metabolite; adding the enzyme-labeled secondary antibody; developing the color by the TMB substrate; and comparing the absorbance value of the sample with a standard curve, and multiplying by the corresponding diluting times to obtain the residual quantity of the furaltadone metabolite in the sample. Compared with an instrumental analysis technology, the ELISA kit has the characteristics that the operation is simple, the cost is low, the sensitivity is high, and the like.
Description
(1) technical field: the utility model relates to the detection kit of AMOZ residual quantity, particularly detect enzyme linked immunosorbent detection (ELISA) kit of AMOZ residual quantity in the aquatic products, ELISA (Enzyme Linked ImmunosorbnentAssay) is the abbreviation of enzyme-linked immunosorbent assay, and it is a kind of enzyme immune technology that grows up after immunofluorescence and radioimmunoassay technique.
(2) background technology: the itrofurans medicine once was widely used because of the dynamic (dynamical) characteristic of extraordinary antibacterial action and medicine is arranged, as the somatotrophic adjuvant of bird, aquatic products and pig.But finding in the process of experimental that for a long time itrofurans medicine and metabolin all can make animal used as test that canceration and gene mutation take place, just causing this type of drug withdrawal in treatment and feed, to use Just because of this.
Because the itrofurans medicine in vivo soon can be by metabolism, the metabolic product of combination then can retain long period of time in tissue, so the product often will analyze its metabolism when analyzing this type of medicine residual after, administrative authority is that means reach the residual purpose of detection itrofurans to detect metabolic product just.Furazolidone metabolite product A OZ; Furaltadone metabolic product AMOZ; Nitrofuran holder English metabolic product AHD; Nitrofurazone (nitrofurazone) metabolic product SEM.
The most popular method that is used for detecting AMOZ is LC-UV, LC-MS and LC-MS/MS, but it detects operation steps trouble of sample, and detection time is long, and disposable detection sample is few.
(3) utility model content: problem to be solved in the utility model provides a kind of AMOZ residue detection kit of small volume and less weight, it is easy and simple to handle, detect quick, accurate, highly sensitive, cost is low, good stability, the technology content that needs is not high, can carry out the mensuration of AMOZ residual quantity in a plurality of samples of one-time continuous, has reduced the needed time of test samples.
The technical solution of the utility model is: a kind of AMOZ ELISA detection kit, the ELISA Plate that comprises one 96 hole in box body and the box, a cover plate film, 15 bottles of reagent and the recessed bottle position of putting reagent, a valve bag, a instructions and a quality inspection report, it is characterized in that ELISA Plate is to adopt 96 hole agent plate as solid phase carrier, the check-out console that pre-bag is made by the AMOZ coupled antigen on the kit capillary strip, 15 bottles of reagent are respectively 7 bottles of standard solutions, ELIAS secondary antibody, the antibody working fluid, colour developing liquid A liquid, colour developing liquid B liquid, stop buffer, concentrated cleaning solution, concentrate redissolution liquid, the 2-nitrobenzaldehyde, totally 15 of recessed bottle positions.
ELISA Plate is made up of outer frame support and removable 12 enzymes mark reaction capillary strips of being placed on it, each dismantled and assembled enzyme mark reaction capillary strip has 8 reacting holes, put into the vacuum aluminium foil bag, box body is a carton box, recessed bottle position is made by plastic foam, with the plastics dura mater is the cover plate film, cover plate film size is consistent with ELISA Plate square section size, 15 bottles of bottle reagent are big or small with difference, the plastic bottle of different colours and vial splendid attire also are fixed in the recessed bottle position and ELISA Plate, the cover plate film, valve bag, instructions, the Quality Control report together is encapsulated in the carton box, so that carry and transport.15 bottles of reagent are respectively 7 bottles of 1ml standard solutions, 12ml ELIAS secondary antibody, 7ml antibody working fluid, 7ml colour developing liquid A liquid, 7ml colour developing liquid B liquid, 7ml stop buffer, 40ml concentrated cleaning solution, the concentrated liquid that redissolves of 50ml, 15.1mg 2-nitrobenzaldehyde.Reagent in each kit enough carries out 96 times and measures (comprising the standard analysis hole), both can carry out the detection of a plurality of samples of one-time continuous, also can take plate hole apart repeated detection.Put back in the aluminium foil bag with the valve bag sealing accuracy that like this can guarantee reagent box testing result with remaining.During detection, residual AMOZ in the sample will with the anti-AMOZ antibody of coupling AMOZ antigenic competition of pre-bag quilt on the ELISA Plate capillary strip, after adding ELIAS secondary antibody, develop the color with tmb substrate, in sample absorbance and the sample contain AMOZ residual quantity become negative correlation, multiply by its corresponding extension rate more again with typical curve, can draw the residual quantity of AMOZ in the sample, it is easy to operation.
Our experiments show that this kit has very high sensitivity: the lowest detection of fishes and shrimps sample is limited to 0.15 μ g/kg; The recovery of fishes and shrimps tissue is 75% ± 15%, is<0.1% with the cross reacting rate of the similar medicine of other AMOZs.With respect to other AMOZ method for detecting residue, the required instrument of this kit is less, only needs microplate reader, even matter device, vibrating machine, micro sample adding appliance, hydro-extractor etc., and generally all there is outfit in similar laboratory, and required cost is lower.
The beneficial effects of the utility model are: can be used for the residual detection of aquatic products AMOZ quick, easy, sensitive, exactly.
(4) description of drawings:
Fig. 1 is the lateral longitudinal sectional view (the long 8.55cm of being) of the utility model elisa plate;
Fig. 2 is the side drawing in side sectional elevation (the long 12.8cm of being) of the utility model elisa plate;
Fig. 3 is the vertical view of the utility model elisa plate;
Fig. 4 is the utility model cover plate membrane plane figure;
Fig. 5 is the utility model reagent bottle longitudinal profile planimetric map;
Fig. 6 is the vertical view of the utility model fixed foam mould;
Fig. 7 is the side view of the utility model box body and fixed foam mould.
Referring to accompanying drawing: enzyme mark reaction capillary strip (2) in advance coated AMOZ coupled antigen (3) is fixed on the outer frame support (1) of ELISA Plate, and enzyme mark reaction capillary strip (2) can be with requiring dismounting; Capping enzyme mark reaction capillary strip (2) when cover plate film (4) is put the insulating box internal reaction for ELISA Plate, the cross section in the same size of the size of cover plate film and agent plate; The translucent PE plastic bottle (5) of hyaline cap is used for encapsulation 40ml concentrated cleaning solution; The translucent PE plastic bottle (5) of blue cap is used for encapsulation 50ml and concentrates redissolution liquid; The white PE plastic bottle (7) of white cap (6) is used for encapsulation 7ml nitrite ion A liquid, the black PE plastic bottle (7) of red cap (6) is used for encapsulation 7ml nitrite ion B liquid, the white PE plastic bottle (7) of yellow cap (6) is used for encapsulation 7ml stop buffer, the white PE plastic bottle (8) of red cap is used for encapsulation 12ml ELIAS secondary antibody, the white PE plastic bottle (8) of green cap is used for encapsulation 7ml antibody working solution, the brown glass reagent bottle (9) of black caps is used for encapsulation 15.1mg 2-nitrobenzaldehyde, and the brown glass reagent bottle (9) of white cap is used for the standard solution of encapsulation 1ml/ bottle; Foamed plastics mould (10) has 15 bottle positions, placement location is followed successively by: 40ml concentrated cleaning solution bottle position (18), 50ml concentrates redissolution liquid (11), 7ml nitrite ion A liquid bottle position (14), 7ml nitrite ion B liquid bottle position (13), 7ml stop buffer bottle position (12), 7ml antibody working solution bottle position (16), 12ml ELIAS secondary antibody bottle position (15), the bottle position (17) of the standard solution of 7 kinds of various concentration of 1ml/ bottle and 15.1mg 2-nitrobenzaldehyde, box body (19) is carton box.
(5) embodiment
One, the pre-treatment of sample
1. dosing
Dosing 1: derivatization reagent
In the reagent bottle that the 2-nitrobenzaldehyde is housed, add dissolve with methanol and be settled to 10ml (concentration is 10mM).
Dosing 2:0.1M dipotassium hydrogen phosphate solution
Taking by weighing 22.8g three hypophosphite monohydrate hydrogen dipotassiums adds deionized water dissolving and is settled to 1L.
Dosing 3:1M hydrochloric acid solution
Measuring the 8.3ml concentrated hydrochloric acid joins in the container that fills deionized water and is settled to 100ml.
Dosing 4:1M sodium hydroxide solution
Taking by weighing 4.0g NaOH adds deionized water dissolving and is settled to 100ml.
Dosing 5: redissolution working fluid
With deionized water the 2 * concentrated liquid that redissolves is diluted the redissolution that (1 part 2 * the concentrated liquid+1 part deionized water that redissolves) is used to extract sample by 1: 1 volume ratio, the working fluid that redissolves can be preserved one month at 4 ℃ of environment.
Dosing 6: cleansing solution working fluid
With deionized water 20 * concentrated cleaning solution is diluted the washing that (1 part of 20 * concentrated cleaning solution+19 part deionized water) is used for ELISA Plate by 1: 19 volume ratio, the washing working fluid can be preserved one month at 4 ℃ of environment.
2. aquatic products (fishes and shrimps etc.) tissue pre-treating method:
With homogenizer homogeneous sample; Take by weighing the tissue samples behind 1.0 ± 0.05g homogeneous, add deionized water, 0.5ml 1M hydrochloric acid solution and the 100 μ l derivatization reagents of 4ml, with the oscillator 2min that fully vibrates; At 37 ℃ of night incubation (approximately 16h); Add 5ml 0.1M dipotassium hydrogen phosphate solution, 0.4ml 1M sodium hydroxide solution and 5ml ethyl acetate, with oscillator thermal agitation 30s; More than the 3000g, the centrifugal 10min of room temperature (20-25 ℃/68-77) gets 2.5ml ethyl acetate to the glass test tube of 10ml drying, flow down to dry up in 50~60 ℃ of nitrogen and add 1ml normal hexane (or normal heptane), with vortex instrument whirling motion 30s, add 1ml redissolution working fluid again, with the abundant mixing of vortex instrument whirling motion 1min; More than the 3000g, (20-25 ℃/68-77F) centrifugal 10min of room temperature; Remove upper organic phase, take off layer water 50 μ l and be used for analyzing.
Two, use the operation steps of kit:
1, required reagent is taken out from cold storage environment, place room temperature (20-25 ℃) more than the balance 30min, note to shake up before every kind of liquid reagent uses.
2, take out the microwell plate that needs quantity, no microwell plate is put into valve bag, be stored in 2-8 ℃.
3, the washing working fluid also need be risen again before use.
4, numbering: the corresponding micropore of sample and standard items is numbered according to the order of sequence, and it is parallel that each sample and standard items are done 2 holes, and the position at record standard hole and sample aperture place.
5, add standard solution/sample solution and antibody working fluid: add standard solution/sample solution 50 μ l in the micropore of correspondence, add antibody working fluid 50 μ l/ holes then, the mixing that vibrates gently is with reacting 30min in the rearmounted 25 ℃ of lucifuge environment of cover plate membrane cover plate.
6, wash plate: carefully open the cover plate film, liquid in the hole is dried, with washing working fluid 250 μ l/ holes, fully wash 4-5 time, each 10s at interval pats dry (bubble that is not eliminated after patting dry can be poked with original rifle head) with thieving paper.
7, add ELIAS secondary antibody: add ELIAS secondary antibody 100 μ l/ holes, the mixing that vibrates gently with reacting 30min in the rearmounted 25 ℃ of lucifuge environment of cover plate membrane cover plate, takes out and repeats to wash plate step 6.
8, colour developing: add substrate solution A liquid 50 μ l/ holes, add substrate solution B liquid 50 μ l/ holes again, the mixing that vibrates gently is with reacting 15min in the rearmounted 25 ℃ of lucifuge environment of cover plate membrane cover plate.
9, measure: add stop buffer 50 μ l/ holes, the mixing that vibrates is gently set microplate reader in the 450nm place, measures every hole OD value.
Three, the result judges
The result judges two kinds of methods, judges available the 1st kind of method roughly, quantitatively judges with the 2nd kind of method.Notice that the sample light absorption value becomes negative correlation with its contained AMOZ.
1, mean light absorbency value and the standard value with sample relatively can draw its concentration range (μ g/L).The absorbance of supposing sample 1 is 0.301, and the absorbance of sample 2 is 0.830, and the titer absorbance is respectively: 0 μ g/L is 2.018; 0.05 μ g/L is 1.475; 0.15 μ g/L is 1.030; 0.45 μ g/L is 0.472; 1.35 μ g/L is 0.187; 4.05 μ g/L is 0.079.Then the concentration range of sample 1 is that 0.45 μ g/L-1.35 μ g/L multiply by its corresponding extension rate again and can draw the residual concentration range of AMOZ in the sample; The concentration range of sample 2 is that 0.15 μ g/L-0.45 μ g/L multiply by its corresponding extension rate again and can draw the residual concentration range of AMOZ in the sample.
2, quantitative test
(1) calculating of percentage absorptance, the percentage absorptance that the percentage absorptance of standard items or sample equals standard items or sample equals the mean value (diplopore) of percentage absorbance of standard items or sample divided by the absorbance of first standard (0 standard), multiply by 100% again, promptly
Percentage absorbance (%)=B/B
0* 100%
The mean light absorbency value of B-standard solution or sample solution
B
0The mean light absorbency value of-0 μ g/L standard solution
(2) drafting of typical curve and calculating
With standard items percentage absorptance is ordinate, is horizontal ordinate with the semilog of AMOZ standard items concentration (μ g/L), the drawing standard curve map.In the percentage absorptance substitution typical curve with sample, read the pairing concentration of sample, multiply by the practical residue limit that its corresponding extension rate is AMOZ in the sample from typical curve.
If utilize kit specialty analysis software to calculate, accurate, the express-analysis of a large amount of samples of being more convenient for.
Four, measure preceding points for attention:
1, room temperature is lower than 20 ℃ or reagent and sample and does not get back to room temperature (20-25 ℃) and can cause the OD value of all standards on the low side.
2, in washing the plate process if the plate hole dry situation, it is non-linear then can typical curve to occur, the phenomenon that repeatability is bad.So should carry out next step operation immediately after washing plate and patting dry.
3, need it is shaken up before whenever adding a kind of reagent.
4, reaction terminating liquid is a 2M sulfuric acid, avoids contacting skin.
5, do not use the kit of date of expiration; Also do not use any reagent in the kit of the term of validity, the kit that used the term of validity of mixing can cause the reduction of sensitivity; The reagent in the different lot number kits is not used in exchange.
6, condition of storage
Preserve kit in 2-8 ℃, not freezing, put no microwell plate into valve bag and reseal.Therefore standard substance and colourless colour former will be avoided being directly exposed under the light to photaesthesia.
7, the rotten sign of reagent
Color development reagent has any color to show that colour former is rotten, should abandon it.When the absorbance of 0 standard (450/630nm) was worth less than 0.5 (A450nm<0.5), expression reagent may go bad.
8, after adding substrate solution A and substrate solution B liquid, the 10-15min that generally develops the color gets final product.If color is more shallow, can prolongs the reaction time to 20min (or longer), but must not surpass 30min.Otherwise, then shorten the reaction time.
9, this kit optimal reaction temperature is 25 ℃, too high or too low for temperaturely will cause detecting absorbance and sensitivity changes.
Claims (3)
1. AMOZ ELISA detection kit, the ELISA Plate that comprises one 96 hole in box body and the box, a cover plate film, 15 bottles of reagent and the recessed bottle position of putting reagent, a valve bag, a instructions and a quality inspection report, it is characterized in that: ELISA Plate is to adopt 96 hole agent plate as solid phase carrier, the check-out console that pre-bag is made by the AMOZ coupled antigen on the kit capillary strip, 15 bottles of reagent are respectively 7 bottles of standard solutions, ELIAS secondary antibody, the antibody working fluid, colour developing liquid A liquid, colour developing liquid B liquid, stop buffer, concentrated cleaning solution, concentrate redissolution liquid, the 2-nitrobenzaldehyde, totally 15 of recessed bottle positions.
2. kit according to claim 1 is characterized in that: box body is a carton box; The polystyrene ELISA Plate in 96 holes is put in the vacuum aluminium foil bag; The cover plate film is the plastics dura maters; Standard solution is with the Brown Glass Brown glass bottles and jars only of white cap, ELIAS secondary antibody is with the white PE plastic bottle of red cap, the antibody working fluid is with the white PE plastic bottle of green cap, the white PE plastic bottle of liquid A liquid with white cap develops the color, colour developing liquid B liquid is with the black PE plastic bottle of red cap, and stop buffer is with the white PE plastic bottle of yellow cap, the translucent PE plastic bottle of concentrated cleaning solution usefulness hyaline cap, concentrate the translucent PE plastic bottle of redissolution liquid, the 2-nitrobenzaldehyde Brown Glass Brown glass bottles and jars only of black caps with blue cap; Recessed bottle position is made by plastic foam.
3. kit according to claim 1 is characterized in that: ELISA Plate is made up of outer frame support and removable 12 enzymes mark reaction capillary strips of being placed on it, and each dismantled and assembled enzyme mark reacts capillary strip 8 reacting holes; Cover plate film size is consistent with ELISA Plate square section size; 7 bottles of standard solutions, the 1ml/ bottle; 1 bottle of ELIAS secondary antibody, 12ml; 1 bottle of antibody working fluid, 7ml; 1 bottle of colour developing liquid A liquid, 7ml; 1 bottle of colour developing liquid B liquid, 7ml; 1 bottle of stop buffer, 7ml; 1 bottle of concentrated cleaning solution, 40ml; Concentrate 1 bottle of redissolution liquid, 50ml; 1 bottle of 2-nitrobenzaldehyde, 15.1mg.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 201020586590 CN201852835U (en) | 2010-10-27 | 2010-10-27 | ELISA (enzyme linked immunosorbent assay) kit of furaltadone metabolite |
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| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 201020586590 CN201852835U (en) | 2010-10-27 | 2010-10-27 | ELISA (enzyme linked immunosorbent assay) kit of furaltadone metabolite |
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| CN201852835U true CN201852835U (en) | 2011-06-01 |
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| CN 201020586590 Expired - Fee Related CN201852835U (en) | 2010-10-27 | 2010-10-27 | ELISA (enzyme linked immunosorbent assay) kit of furaltadone metabolite |
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Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN103018449A (en) * | 2011-09-20 | 2013-04-03 | 北京勤邦生物技术有限公司 | Enzyme-linked immunoassay kit and method for furaltadone metabolite detection |
| CN103852581A (en) * | 2014-03-11 | 2014-06-11 | 河南工业大学 | 3,4-benzopyrene enzyme-linked immune detection kit |
| CN106770227A (en) * | 2016-11-30 | 2017-05-31 | 百奥森(江苏)食品安全科技有限公司 | The detection method and test strips of AMOZ in a kind of dairy products |
-
2010
- 2010-10-27 CN CN 201020586590 patent/CN201852835U/en not_active Expired - Fee Related
Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN103018449A (en) * | 2011-09-20 | 2013-04-03 | 北京勤邦生物技术有限公司 | Enzyme-linked immunoassay kit and method for furaltadone metabolite detection |
| CN103018449B (en) * | 2011-09-20 | 2016-02-24 | 北京勤邦生物技术有限公司 | Detect enzyme linked immunological kit and the method thereof of AMOZ |
| CN103852581A (en) * | 2014-03-11 | 2014-06-11 | 河南工业大学 | 3,4-benzopyrene enzyme-linked immune detection kit |
| CN106770227A (en) * | 2016-11-30 | 2017-05-31 | 百奥森(江苏)食品安全科技有限公司 | The detection method and test strips of AMOZ in a kind of dairy products |
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| Date | Code | Title | Description |
|---|---|---|---|
| C14 | Grant of patent or utility model | ||
| GR01 | Patent grant | ||
| C17 | Cessation of patent right | ||
| CF01 | Termination of patent right due to non-payment of annual fee |
Granted publication date: 20110601 Termination date: 20111027 |