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제품 설명
Double-stranded RNA (dsRNA) ELISA kit
제품 번호
DEIA-BZ002P
제품 특징
Sample
vaccines and gene therapies
Species Reactivity
Universal
Detection Method
Sandwich-ELISA
Intended Use
This kit is used for quantitative detection of double stranded RNA (dsRNA) content in samples. The detected dsRNA is 40 bp or longer and is independent of its nucleic acid sequence.
Contents of Kit
No. | Components | Size | Storage Conditions |
1 | Microtiter Plate | 8×12 wells | 2-8°C |
2 | Detection Antibody (100×) | 120 μL | 2-8°C |
3 | HRP-Conjugated Antibody (100×) | 120 μL | 2-8°C |
4 | Sample Diluent | 30 mL | 2-8°C |
5 | Substrate Solution | 12 mL | 2-8°C |
6 | Stop Solution | 6 mL | 2-8°C |
7 | Wash Buffer (20×) | 40 mL | 2-8°C |
8 | Unmodified dsRNA Standard (5ng/μL) | 15μL | 2-8°C |
9 | pUTP-modified dsRNA Standard (5ng/μL) | 15μL | 2-8°C |
10 | N1-Me-pUTP-modified dsRNA Standard (5ng/μL) | 15μL | 2-8°C |
11 | 5-OMe-UTP-modified dsRNA Standard (5ng/μL) | 15μL | 2-8°C |
12 | STE buffer | 50mL | 2-8°C |
13 | Sealers | 4 sheets |
Storage
1. For unused kit: The whole kit could be stored at 2-8°C in shelf life. Strong light should be avoided for storage stability.
2. For used kit: Once the microplate is opened, please cover unused wells with plate sealer and return to the foil pouch containing the desiccant pack, zip-seal the foil pouch and return to 2-8°C as soon as possible after use. Other reagents should be returned to 2-8°C as soon as possible after use.
Precision
CV of Intra-Assay ≤10%,CV of Inter-Assay ≤10%
Sensitivity
Limit of Detection
Unmodified dsRNA Standard (5ng/μL): ≤0.001pg/μL
pUTP-modified dsRNA Standard (5ng/μL): ≤0.001pg/μL
N1-Me-pUTP-modified dsRNA Standard: ≤0.001pg/μL
5-OMe-UTP-modified dsRNA Standard (5ng/μL): ≤0.01pg/μL
Limit of Quantitation
Unmodified dsRNA Standard (5ng/μL): 0.0156pg/μL
pUTP-modified dsRNA Standard (5ng/μL): 0.0156pg/μL
N1-Me-pUTP-modified dsRNA Standard: 0.0312pg/μL
5-OMe-UTP-modified dsRNA Standard (5ng/μL): 0.0625pg/μL
General Description
mRNA has gained significant worldwide attention as a novel active ingredient in vaccines and gene therapies. The increasing demand for mRNA molecules has compelled mRNA manufacturers to quickly scale up production capacity while maintaining high mRNA quality. In vitro transcription by T7 polymerase is the standard procedure to synthesize mRNA. However, this procedure may introduce double-stranded RNA (dsRNA) contaminants from random priming of abortive transcripts, turn-around transcription, and antisense transcription. dsRNA immune activation results in the up-regulation of various pro-inflammatory cytokines, and cell death, which can lead to patient morbidity. Therefore, to improve the quality of mRNA translation, and minimize adverse effects, it is critical to carefully monitor in vitro-transcribed (IVT) mRNA products and confirm the removal of dsRNA after purification.
Standard Curve
Citations
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