LCAT ELISA. For Research Use Only. Not For Use In Diagnostic Procedures.

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LCAT ELISA For the quantitative determination of Lecithin-Cholesterol Acyltransferase (LCAT) in human serum and plasma. For Research Use Only. Not For Use In Diagnostic Procedures. Catalog Number: 47-LCAHU-E01 Size: 96 wells Version: 775502-003 ALPCO November 28, 2017 Page 1 of 5

1. Intended Use The LCAT ELISA kit is intended for the quantitative determination of lecithin-cholesterol acyltransferase (LCAT) in human serum and plasma by utilizing a two-step sandwich method of enzyme-linked immunosorbent assay (ELISA). For Research Use Only. Not For Use In Diagnostic Procedures. 2. Principle of the Assay Test wells are coated with anti-lcat monoclonal antibody (MoAb (36486)), which binds with LCAT in the sample. After the first incubation and washes to remove all of the unbound material, horseradish peroxidase (HRP)-labeled anti-lcat MoAb (36487) is added. The enzyme labeled MoAb (36487) binds with LCAT immobilized on the well by the coated MoAb (36486). After the second incubation and subsequent washes, the antibody / LCAT / enzyme complex is incubated with a substrate solution and terminated with a stop solution. The intensity of color that develops in the enzyme reaction is measured by using a microplate reader. The absorbance is proportional to the concentration of LCAT in the sample. 3. Procedural Notes 1. For research use only. 2. A standard curve must be run with each assay. 3. Read absorbences just after completion of the assay. 4. The human plasma used in the calibrator has been tested and found to be negative for hepatitis B surface antigen (HBsAg), antibodies to hepatitis C virus (HCV), and antibodies to human immunodeficiency virus (HIV-1 and HIV-2). Because no known test method can offer complete assurance that infectious agents are absent, handle reagents and samples as if they are capable of transmitting infectious disease. Observe universal precautions. 5. Stop reagent (7.7% H2SO4) is poisonous and can cause severe burns. Do not ingest. Avoid contact with skin, eyes, and clothing. If contact occurs, immediately wash the area thoroughly with water. 6. All residual wash buffers must be drained from the wells by aspiration or by decantation followed by tapping the plate forcefully on absorbent paper. 4. Materials 4.1. Materials Provided No. Reagent Composition Amount 1 LCAT-MoAb coated wells Anti-LCAT MoAb (36486) coated 96-well plate 1 plate 2 Dilution buffer (a) Citrate buffer (ph 5.0) 1 x 100 ml 3 Dilution buffer (b) Phosphate buffer (ph 7.2) 1 x 6 ml 4 HRP-labeled MoAb concentrate (7X) Horse radish peroxidase (HRP)-labeled anti-lcat MoAb (36487) 1 x 1 ml (for 7 ml) Page 2 of 5

5 6 Wash buffer concentrate (10X) Substrate (lyophilized) 7 Substrate buffer Phosphate buffer (ph 7.2) o-phenylenediamine H2O2 in citrate buffer (ph 5.0) 1 x 100 ml (for 1,000 ml) 2 vials (for 6 ml/vial) 1 x 15 ml 8 Stop Solution 7.7% H2SO4 1 x 10 ml 9 Calibrator (lyophilized) Human plasma 1 vial (for 1 ml) 4.2. Materials Required by not Provided Microplate reader capable of measurement at 492 nm. 8-channel pipette capable of delivering 50-200 μl. 1-channel pipette capable of delivering 20-1,000 μl. Deionized or distilled water. Plastic test tube. Graduated cylinder (1000 ml). Absorbent paper towels. Graph paper (log-log or semi-log). 96-well plate dust cover or lid (plastic wrap can be used as an alternative cover). Microplate shaker with horizontal, circular movement, if available. Plate washer, automated or manual, if available. 5. Preparation and Storage of Reagents Unprepared reagents are stable for 2 years when stored at 2-10ºC. 1. Working wash buffer: Dilute the wash buffer concentrate (5) with 900 ml of distilled water. The resulting working wash buffer is stable for 1 month at 2-10ºC. 2. Working anti-lcat MoAb HRP conjugate: Dilute the HRP-labeled MoAb concentrate with 6 ml of the dilution buffer (b). The resulting working anti-lcat MoAb HRP conjugate is stable for two weeks at 2-10ºC. 3. Working substrate solution: Just prior to use, reconstitute the substrate (lyophilized) (6) by adding 6 ml of the substrate buffer (7) to the substrate vial. Since the substrate is light sensitive, it should not be exposed to excessive light. The resulting working substrate solution should be used within 1 hour after reconstitution. 4. Calibrator: Reconstitute the calibrator (lyophilized) (9) by adding 1.0 ml of the dilution buffer (a) to the calibrator vial. The content of LCAT is indicated on the label. The stock solution is stable for 2 weeks at 2-10ºC. Prepare the serial calibrator dilutions immediately prior to use to obtain a calibration curve in the following manner: Page 3 of 5

Standard number: Calibrator material to add: Dilution buffer (a) to add: *Final dilution factor: 1 1 of stock calibrator 0 μl 1 2 1 of standard 1 1 2 3 1 of standard 2 1 4 4 1 of standard 3 1 8 5 1 of standard 4 1 16 6 1 of standard 5 1 32 7 0 μl 1 0 * The concentrations of calibrator can be obtained by dividing the concentration of the stock calibrator by the dilution factor. The stock concentration is found on the vial label. Plot these calculated results for your standard curve. 5. Other: Seal extra strips with plate tape sealer and store at 2-10ºC for future use. When stored at 2-10ºC, the dilution buffer (a), the substrate buffer, and the stop solution are stable until the expiration date on the label. 6. Sample Preparation Samples must be diluted to 1:100 with the dilution buffer (a) (sample 10 μl + the dilution buffer (a) 1,000 μl) before they are added to the plate. When the obtained absorbance exceeds the range of the calibration curve, dilute the sample with higher volume of the dilution buffer (a) and repeat the measurement. The dilution ratio should not be less than 1:20. 7. Assay Procedure 1. Add of samples and calibrators into respective wells. All standards and samples should be tested in duplicate. 2. Incubate the covered plate for 2 hours at room temperature. 3. Thoroughly remove solution from wells. Wash wells 3 times with 3 Working wash buffer. Thoroughly remove droplets. 4. Add of Working anti-lcat MoAb HRP conjugate Add to each test well. 5. Incubate the covered plate for 1 hour at room temperature. 6. Thoroughly remove solution from wells. Wash wells 3 times with 3 Working wash buffer. Thoroughly remove droplets. 7. Add of Working substrate solution to each test well. 8. Incubate the covered plate for 15 minutes at room temperature. 9. Add of Stop Solution to each test well. The incubation time of 15 minutes should be strictly kept for each test well. 10. Read the absorbance of each well at 492 nm. Page 4 of 5

8. Calculation of Results Calculate the Δ absorbance by subtracting the absorbance of the 0 μg/ml calibrator from those of other calibrators and unknown samples. Plot the Δ absorbance of the calibrators against the calibrator concentration on log-log or semi-log graph paper. Draw a smooth curve through these points to construct the calibration curve. Read the concentrations for the diluted unknown samples from the calibration curve. Do not correct for 1:100 sample dilution unless you have to further dilute samples to bring them within the range of the curve. If this is the case correct for only the dilution beyond 1:100. 9. References 1. Kobori K, Saito K, Ito S, et al. Atherosclerosis, supplements, 2001; 2: 74. 2. Kobori K, Saito K, Ito S, et al. J Lipid Res, 2002; 43: 325-334. 10. Summary of Assay Procedure Reagent Volume Procedure Samples or Calibrators Add sample to each test well. All standards should be tested twice. Incubate the covered plate for 2 hours at room temp. Thoroughly remove solution from wells. Working wash buffer 3 Wash wells 3 times. Thoroughly remove droplets. Working anti-lcat MoAb HRP conjugate Add to each test well. Incubate the covered plate for 1 hour at room temp. Thoroughly remove solution from wells. Working wash buffer 3 Wash well 3 times. Thoroughly remove droplets. Working substrate solution Stop reagent Add to each test well. Incubate the covered plate for 15 minutes at room temp. Add to each test well. (The incubation time of 15 minutes should be strictly kept for each test well.) Read the absorbance of each well at 492 nm. Page 5 of 5