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品牌ELISA试剂盒供应——上海研域
品牌ELISA试剂盒供应——上海研域
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阅读:248发布时间:2013-08-05
品牌ELISA试剂盒供应——上海研域
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人 (Human) III型前胶原 (PC-III)试剂盒
PRINCIPLE OF THE METHOD
The PC-III kit is a solid phase phase sandwich enzyme linked immuno sorbent assay(ELISA). Samples , including standards of known PC-III concentrations and unknowns are pipetted into these wells. During the first incubation, the PC-III antigen and a biotinylated monoclonal antibody specific for PC-III are simultaneously incubated. After washing, the enzyme(streptavidin-peroxydase)is added. After incubation and washing to remove all the unbound enzyme, a substrate solution which is acting on the bound enzyme is added to induce a coloured reaction product. The intensity of this coloured product is directly proportional to the concentration of PC-III present in the samples.
REAGENTS PROVIDED AND RECONSTTTUTION
| REAGENTS(Store at 2-8℃) | 1×96 WELLS | 0.5×96 WELLS | RECONSTTTUTION |
| 96/48-wells microtiter plates | 1 | 0.5 | Ready-to-use |
| Plastiv cover | 2 | 1 | Ready-to-use |
| Standard: 160ng/ml | 1Vials (0.6ml) | 0.5Vials (0.3ml) | See reagents preparation on page 3 |
| Blank control | 1Vials (1.0ml) | 1Vials (0.5ml) | Ready-to-use |
| Standard Diluent | 1Vials (4.0ml) | 1Vials (2.0ml) | Ready-to-use |
| Biotinylated anti-PC-III | 1Vials (6.0ml) | 1Vials (3.0ml) | Ready-to-use |
| Streptavidin-HRP | 1Vials (8.0ml) | 1Vials (4.0ml) | Ready-to-use |
| Washing Buffer | 1Vials (20ml) | 1Vials (10ml) | 50× concentrate |
| Substrate A | 1Vials (6.0ml) | 1Vials (3.0ml) | Ready-to-use |
| Substrate B | 1Vials (6.0ml) | 1Vials (3.0ml) | Ready-to-use |
| Stopping Solution | 1Vials (6.0ml) | 1Vials (3.0ml) | Ready-to-use |
| Sample Diluent | 1Vials (12ml) | 1Vials (6.0ml) | Ready-to-use |
SPECIMEN COLLECTION\ PROCESSING AND STORAGE
Serum---Avoid any inintentional stimulation of the cells by the procedure. Use pyrogen\endotoxin free collecting tubes. Serum should be removed rapidly and carefully from the red cells after clothing. For that, after clothing, centrifuge at approximay 1000×g for 10 min and remove serum.
Plasma---EDTA\ citrate and heparin plasma can be assayed. Spin samples at 1000×g for 30 min remove particulates. Harvest plasma.
Cell culture supernatants---Remove particulates and aggregates by spinning at approximay 1000×g for 10 min.
Storage---If not analyzed shortly after collection, samples should be aliquoted(250-500ul) to avoid freeze-thaw cycles and stored frozen at -70℃. Avoid multiple freeze-thaw cycles of frozen specimens. When possible, avoid use of badly hemolyzed or lipemic sera. If large amounts of particles are present, this should be removed prior to assay by centrifugation or filtration.
Recommendation---Do not thaw by heating at 37℃ or 56℃. Thaw at room temperature and make sure that sample is compley thawed and homogenous before assaying.
PREPARATION OF REAGENTS
Standards: Standard have to be reconstituled with the volume of standard buffer diluent indicated on the vial. This reconstitution produces a stock solution of 160ng/ml PC-III. Allow standard to stand for 5
minutes with gentle swirling prior to making dilutions. Serial dilutions of standard must be made before each assys and cannot be stored.
| 160 ng/ml | (6 Standard) | Original density 50ul。 |
| 80 ng/ml | (5 Standard) | 100ul 6 Standard +100ul diludent |
| 40 ng/ml | (4 Standard) | 100ul 5 Standard +100ul diludent |
| 20 ng/ml | (3 Standard) | 100ul 4 Standard +100ul diludent |
| 10 ng/ml | (2 Standard) | 100ul 3 Standard +100ul diludent |
| 5.0 ng/ml | (1 Standard) | 100ul 2 Standard +100ul diludent |
| 0 ng/ml | Blank Control | 50ul。 |
ASSAY METHOD
Before use, mix all reagents thoroughly without making foam.
Determine the number of microwell strips required to test the desired number of samples,plus appropriate number of wells needed for running blanks standards. Each sample, standard and blank should be assayed in duplicate. Remove sufficient microwell strips from the pouch.
Add 50ul of standard diluent to standard wells B1,B2, C1,C2, D1,D2, E1, E2, F1,F2. Reconstitute standard vial with the appropriate volume as described in the chapter reagents preparation. Preparation. Pipet 100ul of standard into wells A1 and A2 (see plate scheme below). Transfer 50ul from A1 and A2 to B1 and B2 wells. Mix the contents by repeated aspirations and ejections. Take care not to scratch the inner surface of microwells. Repat this procedure from the wells B1,B2 to wells C1,C2 and from wells C1,C2 to D1,D2 and so on creating two parallel rows of PC-III standard dilutions ranging,Add 50ul of standard diluent to the bland wells.
Dilute samples 1:1 distribing 50ul of sample into 50ul of dilluent ,Add 50ul of diluted sample to wells..
Add 50ul of diluted biotinylated anti-PC-III to all wells.
Cover with a plate vover and incubate for 1 hour at 37℃.
Remove the cover and wash the plate as follows: ⑴ aspirate the liquid from each well, ⑵ dispensse 0.3ml of washing solution into each well. ⑶ Aspirate again the contet of each well after 0.5 minute. ⑷ Repeat steps ⑵ and ⑶ three times.
Distribute 60ul of streptavidin-HRP solution to all wells, including blank wells.
Cover and incubate 30 min at 37℃.
Remove the cover and empty wells, Wash microwell strips according to step, Proceed immediay to the next step.
Add 50ul Substrate A and Substrate B to each well。Incubate for 10 min at 37℃。
The enzyme-substrate reaction is stopped by quickly pipetting 50ul of H2SO4. stop reagent into each well, including the blank wells, to compley and uniformly inactivate the enzyme. Results must be red immediay after the addition of H2SO4.
Read absorbance of each well on a spectrophotometer using 450nm as the primary wavelength and optionally 620nm (610nm to 650nm is acceptable ) as the reference wavelength.
SUGGESTED PLATE SCHEME
| | Standard concentrations(ng/ml) | | ||||||||||
| A | 160 | 160 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| B | 80 | 80 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| C | 40 | 40 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| D | 20 | 20 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| E | 10 | 10 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| F | 5.0 | 5.0 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| G | 0 | 0 | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
| H | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample | sample |
CALCULATION OF RESULTS
The minimum detectable concentration in this assay is estimated to be 1.0ng/ml
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