Uni-medica provides a high-throughput and rapid solution for screening and detecting COVID-19 PCR reagent kit,COVID-19 ,SARS-CoV-2,Delta,Omicron,Influenza A,Influenza B,RSV Shenzhen Uni-medica Technology Co.,Ltd , https://www.unimedicadevice.com
Detection principle <br> The kit uses a double antibody sandwich enzyme-linked immunosorbent assay (ELISA). To the coated microwells of the pre-coated plant sweet potato virus 2 (SPLV2) capture antibody, a negative control, a positive control, a sample, an HRP-labeled detection antibody were sequentially added, and the cells were incubated and thoroughly washed. Using the substrate TMB to develop color, TMB is converted to blue under the catalysis of peroxidase and converted to the final yellow color by the action of an acid. The color depth is positively correlated with the plant sweet potato virus 2 (SPLV2) in the sample. The absorbance (OD value) was measured at 450 nm using a microplate reader to determine whether the sample contained plant sweet potato virus 2 (SPLV2).
Sample collection, processing and storage methods
1. Serum: Use a tube containing no pyrogen and endotoxin. Avoid any cell irritation during the procedure. After collecting the blood, centrifuge and centrifuge for 10 minutes at 3000 rpm to quickly and carefully separate the serum and red blood cells.
2. Plasma: EDTA, citrate or heparin anticoagulation. The supernatant was taken by centrifugation at 3000 rpm for 30 minutes.
3. Cell supernatant: Centrifuge at 3000 rpm for 10 minutes to remove particles and polymer.
4. Tissue homogenization: The tissue is mashed by adding appropriate amount of physiological saline. The supernatant was taken by centrifugation at 3000 rpm for 10 minutes.
5. Storage: If the sample is not detected in time after collection, please dispense it once, freeze it at -20 °C, avoid repeated freezing and thawing, thaw at room temperature and ensure that the sample is fully thawed evenly.
Bring your own items
Operational precautions
Kit composition name 96-well configuration 48 hole configuration Remarks Microporous ELISA plate 96 holes 48 holes no Negative control 0.3mL 0.3mL no Positive control 0.3mL 0.3mL no Sample diluent 6mL 3mL no Detection antibody-HRP 10mL 5mL no 20× washing buffer 25mL 15mL Dilute according to the instructions Substrate A 6mL 3mL no Substrate B 6mL 3mL no Stop solution 6mL 3mL no Sealing film 2 sheets 2 sheets no Instruction manual 1 copy 1 copy no Ziplock bag 1 1 no
Preparation of reagents 20× Wash buffer dilution: Distilled water was diluted 1:20, ie 1 part of 20× wash buffer plus 19 parts of distilled water.
Washing method
Steps
Result judgment
1. Test validity: the average value of the OD value of the positive control well is ≥ 1.00;
The average value of the OD value of the negative control well was ≤ 0.15.
2. Cut off calculation: critical value = negative control well average + 0.15
3. Negative judgment: sample OD value <Cut off value, sample is negative
4. Positive judgment: sample OD value > critical value (Cut off), sample is positive
Kit performance
Disclaimer
during medical observation and in suspected population. It includes:
· Disposable Virus Sampling Kits.
· Automatic Nucleic Acid Extraction system( Extractor & Kits).
· Real Time PCR Amplification System. This solution has been approved by the state drug administration and obtained NMPA
and CE certification. The kit has been verified by 600+ clinical samples and used in more
than 100 hospitals and Centers for Disease Control and Prevention.
Plant Sweet Potato Virus 2 ( SPLV2 ) ELISA Kit <br> User Manual