Human lipoprotein lipase (LPL) ELISA kit

Instruction manual of human lipoprotein lipase (LPL) ELISA kit
Human lipoprotein lipase (LPL) ELISA kit is for research use only
Detection range: 3.1 ug / l-200 ug / l
Minimum detection limit: 0.78 ug / L
Intended application: ELISA method for quantitative determination of LPL content in human serum, plasma or other related fluids.
Specificity: This kit can detect recombinant or natural human LPL at the same time, and does not cross-react with other related proteins.
Experimental principle: This kit uses double antibody sandwich enzyme-labeled immunoassay to determine the level of LPL in the specimen. The microtiter plate is coated with purified antibody to make a solid phase antibody. LPL, biotinylated anti-human LPL antibody, and HRP-labeled avidin are added to the monoclonal antibody-coated microwells in turn. LPLB color development. LPL is converted into blue under the catalysis of peroxidase, and into the final yellow under the action of acid. The color depth is positively correlated with the LPL in the sample. The absorbance (OD value) was measured with a microplate reader at a wavelength of 450 nm, and the sample concentration was calculated.
The composition of human lipoprotein lipase (LPL) ELISA kit:
1. Enzyme-linked plate: one piece (96 wells)
2. Standard product (freeze-dried product): 2 bottles, each bottle is diluted with sample diluent to 1ml before use, and left to stand for more than 10 minutes after being capped, and then inverted / rubbed repeatedly to help dissolve, its concentration is 200 ug / L, after serial dilution, it is diluted to 200 ug / L, 100 ug / L, 50 ug / L, 25 ug / L, 12.5 ug / L, 6.2 ug / L, 3.1 ug / L, and its stock solution As the highest standard concentration directly, the sample dilution is directly used as the standard concentration of 0 ug / L, prepared within 15 minutes before use.
For example, to prepare a 100 ug / L standard: take 0.5ml 200 ug / L of the above standard and add it to an Eppendorf tube containing 0.5ml of sample diluent, mix well. The rest of the concentration can be deduced by analogy.
3. Sample diluent: 1 × 20ml / bottle.
4. Test dilution A: 1 × 10ml / bottle.
5. Test diluent B: 1 × 10ml / bottle.
6. Detection solution A: 1 × 120ul / bottle (1: 100) diluted with detection diluent A 1: 100 before use, prepared according to the pre-calculated total amount required for each experiment (100ul / well) before dilution , The actual preparation should be more 0.1-0.2ml. For example, 10 ul detection solution A plus 990 ul detection dilution A is prepared, mix gently, and prepare within one hour before use.
7. Detection solution B: 1 × 120ul / bottle (1: 100) is diluted 1: 100 with detection diluent B before use. The dilution method is the same as that of Test Solution A.
8. Substrate solution: 1 × 10ml / bottle.
9. Concentrated washing solution: 1 × 30ml / bottle, each bottle is diluted 25 times with distilled water.
10. Stop solution: 1 × 10ml / bottle (2N H2SO4).
Collection and preservation of specimens:
1. Plasma: EDTA or heparin can be used as an anticoagulant. Centrifuge the sample at 2-8 ° C 1000 xg for 15 minutes within 30 minutes after collection, or store the specimen at -20 ° C or -80 ° C, but avoid repeated freezing melt.
2. Serum: Whole blood specimens should be left at room temperature for 2 hours or overnight at 4 ° C and centrifuged at 1000 xg for 20 minutes. The supernatant can be taken for detection, or the specimens should be stored at -20 ° C or -80 ° C, but avoid repeated Freeze and thaw.
Note: The above specimens should be stored at 4 ℃ for less than 1 week, -20 ℃ or -80 ℃ should be sealed and stored, -20 ℃ should not exceed 3 months, -80 ℃ should not exceed 6 months; specimen hemolysis will affect the final As a result of the test, hemolytic specimens should not be tested; specimens with high blood lipids do not require special treatment and can be tested directly.
Steps:
Before starting the experiment, please prepare all the reagents in advance; when the reagents or samples are diluted, they should be mixed evenly. A standard curve should be made for each test. If the sample concentration is too high, the sample diluent should be used for dilution to make the sample meet the detection range of the kit. It is recommended that each laboratory conduct pre-experiment before operation to establish the optimal dilution factor.
1. Add sample: set blank hole, standard hole and sample hole to be tested respectively. Add 100ul of sample diluent to the blank well, and 100ul of the standard or the sample to be tested in the remaining well. Be careful not to have air bubbles. Add the sample to the bottom of the well of the microtiter plate. Do not touch the wall of the well. The target plate is covered with a cover or film and reacted at 37 ° C for 120 minutes.
To ensure the validity of the experimental results, please use a new standard solution for each experiment.
2. Discard the liquid and spin dry without washing. Add 100ul of detection solution A working solution (prepared within one hour before use) to each well, 37 ℃, 60 minutes.
3. After incubating for 60 minutes, discard the liquid in the hole, spin dry, wash the plate 3 times, soak for 1-2 minutes each time, 350ul / per hole, spin dry (you can also pat the liquid in the hole to pat dry).
4. Add 100ul of detection solution B working solution (same as the detection A working solution) to each well at 37 ℃ for 60 minutes.
5. After incubating for 60 minutes, discard the liquid in the well, spin dry, wash the plate 5 times, soak for 1-2 minutes each time, 350ul / per well, spin dry (you can also pat the liquid in the well to dry).
6. Add 90ul of substrate solution to each well in sequence, and develop color at 37 ° C in the dark (within 30 minutes, at this time, the first 3-4 wells of the standard product have a visible blue gradient, and the back 3-4 wells are not obvious. , You can terminate).
7. Add 50ul of stop solution to each well in sequence to stop the reaction. At this time, the blue color turns to yellow. The order of adding the stop solution should be the same as that of the substrate solution. In order to ensure the accuracy of the experimental results, the termination solution should be added as soon as possible after the substrate reaction time expires.
8. Measure the optical density (OD value) of each well in sequence using an enzyme-linked instrument at a wavelength of 450 nm. Test immediately after adding stop solution.
Note:
1. Leave one hole for each experiment as a blank zero adjustment hole (different from the blank hole), this hole does not add any reagents, just add the substrate solution and 2N H2SO4 at the end. Use this hole to adjust the OD value to zero when measuring.
2. Incubate in strict accordance with the prescribed time and temperature to ensure accurate results. All reagents must reach room temperature before use. Refrigerate the reagent immediately after use.
3. Incorrect plate washing can lead to inaccurate results. Before adding test solution B or substrate, make sure to absorb the liquid in the well as much as possible. In order to prevent the sample from evaporating, place the reaction plate in a closed box covered with a damp cloth during the test. The enzyme label plate is covered with a cover or film to avoid liquid evaporation; the next step should be performed as soon as possible after washing the plate to avoid the length of the enzyme label plate Time is dry.
4. Eliminate the remaining liquid and fingerprints on the bottom of the board, otherwise it will affect the OD value.
5. Avoid direct light irradiation during storage and incubation.
6. Store unused microplates or reagents at 2-8 ° C. Standard products, test solution A working fluid, and test solution B working fluid should be configured and used according to the required amount. Please accurately configure the standard product and working fluid, and try not to configure it in a small amount (such as when drawing test solution A, not less than 10ul at a time), To avoid concentration errors due to inaccurate dilution; the detection solutions A, B, and substrate solutions should be incubated at 37 ° C for 30 minutes before use; do not reuse the diluted standard and detection solution A Working fluid or detection solution B working fluid.
7. It is recommended to set a double-hole test when testing samples to ensure the accuracy of the test results.
Washing method:
1. Manual plate washing method: suck up (do not touch the wall) or shake off the liquid in the enzyme plate; put a few layers of absorbent paper on the experimental table, and force the enzyme plate down several times; take the recommended washing buffer Inject at least 0.3ml into the hole, soak for 1-2 minutes, and repeat this process several times as needed.
2. Automatic plate washing: If there is an automatic plate washing machine, it should be used in the formal experiment process after being used proficiently.
Calculation: Taking the concentration of the standard as the abscissa (logarithmic coordinate) and the OD value as the ordinate (ordinary coordinate), draw a standard curve on semi-logarithmic coordinate paper (recommended to use professional curve making software for analysis, such as curve expert 1.3), find the corresponding concentration from the standard curve according to the OD value of the sample, and then multiply it by the dilution factor; or calculate the regression equation of the standard curve using the concentration and OD value of the standard, and substitute the OD value of the sample into the equation to calculate The sample concentration, multiplied by the dilution factor, is the actual concentration of the sample.
Precautions:
1. The washing process is very important, inadequate washing is easy to cause false positives.
2. It is best to control the time of one sample addition within 5 minutes. If the number of specimens is large, it is recommended to use a multi-channel pipette to add samples.
3. Please make a standard curve at the same time of each measurement, it is best to make a complex hole.
4. If the content of the substance to be tested in the specimen is too high, please dilute it and then determine it. When calculating, please multiply by the dilution factor.
5. When preparing standard products and testing solution working fluid, please prepare with corresponding diluent, not to be confused.
6. Please keep the substrate away from light.
Explanation:
1. Avoid exposing the reagent to strong light during storage and incubation. All reagent bottle caps must be tightly closed to prevent evaporation and contamination. Reagents should be protected from microbial contamination, because the interference of proteolytic enzymes will lead to erroneous results.
2. Aspirate the reagents carefully and strictly observe the given incubation time and temperature. Please note that when drawing samples / standards, enzyme conjugates or substrates, if the time interval between the first well and the last well is too large, it will result in different "pre-incubation" time, which obviously Affect the accuracy and repeatability of the measured value. Moreover, insufficient washing will affect the test results.
3. Preservation of the kit: some reagents are stored at -20 ℃, and some reagents are stored at 2-8 ℃, depending on the label.
4. Salt will be precipitated from the concentrated washing liquid, which can be heated and dissolved in the water bath when diluted.
5. The well of the enzyme-linked plate just opened may contain a little water-like substance. This is a normal phenomenon and will not have any impact on the experimental results.
6. There may be inconsistencies between the Chinese and English instructions. Please refer to the English instructions.
7. All samples should be managed, and the samples and testing devices should be processed according to the prescribed procedures.
8. Validity: 6 months

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