Product Details:
|
Specimen: | Serum | Storage: | 2-8℃ |
---|---|---|---|
EXP: | 24 Months | Size: | 96 Test/Kit |
Highlight: | Elisa LH Test Strip,ISO13485 Luteinizing Hormone Test Kit,Luteinizing Hormone LH Test Strip |
LH Elisa Kit Luteinizing Hormone
1. Intended use
Immunoassay for the in vitro quantitative determination of luteinizing hormone in human serum.
2. Summary
3. Test principle
Sandwich principle. Total duration of assay: 80 minutes.
• Sample, Anti-LH coated microwells and enzyme labeled Anti-LH are combined.
• During the incubation, LH presents in the sample is allowed to react
simultaneously with the two antibodies, resulting in the LH molecules being
sandwiched between the solid phase and enzyme-linked antibodies.
• After washing, a complex is generated between the solid phase, the LH within the sample and enzyme-linked antibodies by immunological reactions.
• Substrate solution is then added and catalyzed by this complex, resulting in a chromogenic reaction. The resulting chromogenic reaction is measured as absorbance.
• The absorbance is proportional to the amount of LH in the sample.
Reagents
Materials provided
• Coated Microplate, 8 x 12 strips, 96 wells, pre-coated with mouse monoclonal
Anti-LH.
• Calibrators, 6 vials, 1 ml each, ready to use; Concentrations: 0(A), 5(B), 20(C), 50(D), 100(E) and 200(F) mIU/mL.
• Enzyme Conjugate, 1 vial, 11 mL of HRP (horseradish peroxidase) labeled mouse monoclonal Anti-LH in Tris-NaCl buffer containing BSA (bovine serum albumin). Contains 0.1% ProClin300 preservative.
• Substrate, 1 vial, 11ml, ready to use, (tetramethylbenzidine) TMB.
• Stop Solution, 1 vial, 6.0 ml of 1 mol/L sulfuric acid.
• Wash Solution Concentrate, 1 vial, 25 mL (40X concentrated), PBS-Tween
wash solution.
• IFU, 1 copy.
• Plate Lid: 1 piece.
Materials required (but not provided)
• Microplate reader with 450nm and 620nm wavelength absorbent capability.
• Microplate washer.
• Incubator
4. Test procedure
• Use only the number of wells required and format the microplates’ wells for
each calibrator and sample to be assayed.
• Add 25 μL of calibrators or samples to each well.
• Add 100 μL of enzyme conjugate to each well.
• Shake the microplate gently for 30 seconds to mix.
• Cover the plate with a plate lid and incubate at 37 °C for 60 minutes.
• Discard the contents of the micro plate by decantation or aspiration. If
decanting, tap and blot the plate dry with absorbent paper.
• Add 350 μL of wash solution, decant (tap and blot) or aspirate. Repeat 4 additional times for a total of 5 washes. An automated microplate strip washer can be used. At the end of washing, invert the plate and tap out any residual wash solution onto absorbent paper.
• Add 100 μL of substrate to each well.
• Incubate at ambient temperature (18-25℃)in the dark for reaction for 20 minutes. Do not shake the plate after substate addition.
• Add 50 μl of stop solution to each well.
• Shake for 15-20 seconds to mix the liquid within the wells. It is important to
ensure that the blue color changes to yellow completely.
• Read the absorbance of each well at 450 nm (using 620 to 630 nm as the
reference wavelength to minimize well imperfections) in a micro plate reader.
Contact Person: Mr. Steven
Tel: +8618600464506