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Comparable to LAL method - Endpoint fluorescent assay, comparable to other chromogenic quantitative LAL methods.
High specificity - Unlike LAL Assay, as Factor G is absent from the rFC test kit, false-positive results due to β-glucan activation are not expected to occur.
Accuracy - Traceability of endotoxin standards in the kit against USP Standard (Catalog No: 1235503).
Fast time to results - 1 hours.
High sensitivity - Sensitivity range from 0.005-5 EU/mL.
Extensive validation – Verification on multiplex biological products, kinds of microplate readers and various buffer systems, comprehensive validation of specificity, sensitivity, precision, accuracy, applicability, and other aspects according to the parameters listed in the EUROPEAN PHARMACOPOEIA 11.0 and USP chapter<<1225>>.
Sustainable resource - Get rid of dependence on animal derived reagents, reduce dependence on horseshoe crab resources and fishing pressure and realize long-term supply.
Good inter batch consistency - Batch consistency of products is guaranteed due to the use of genetic recombination technology for production.
Assay Type | FRET |
Analyte | Endotoxin |
Format | 96T |
Regulatory Status | RUO |
Sensitivity | 0.005 EU/mL |
Standard Curve Range | 0.005 EU/mL-5 EU/mL |
Assay Time | 1 hr |
Suitable Sample Type | For the quantitative determination of endotoxin from pharmaceutical products, biologicals for injection and some media for tissue cultures. |
Sample volume | 100 μL |
ID | Components | Size |
RES056-C01 | Bacterial Endotoxin Standard | 1 vial |
RES056-C02 | Recombinant Factor C Protein | 96 tests |
RES056-C03 | Fluorogenic Substrate | 96 tests |
RES056-C04 | Water for Bacterial Endotoxins Test | 50 mL |
Production process (Process control)
Raw materials
Water testing
Intermediate product testing
Final product (Release testing)
Parenteral drugs & Biological products
Infusion, injection or tranfusion cells
Cell culture media
Medical devices
It is for research use only.
Find the expiration date on the outside packaging and do not use reagents past their expiration date.
Take the logarithm of the concentration of the Endotoxin working standard solution as the abscissa, take the ΔRFU as the ordinate. Fitting the standard curve with linearly model, and the correlation coefficient R should be ≥ 0.98 (QC tested).
The rFC method was employed to detect endotoxin residues in β-glucan at concentrations of 10ug/mL and 1ug/mL. No non-specific signals were detected. In contrast, the dynamic chromogenic method used for β-glucan detection resulted in the detection of endotoxin and non-specific signals. This indicates that recombinant factor C does not react with β-glucan, demonstrating the good specificity of the rFC method.
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