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Real Time Monkeypox PCR Test Kit With Positive / Negative Control

    Buy cheap Real Time Monkeypox PCR Test Kit With Positive / Negative Control from wholesalers
     
    Buy cheap Real Time Monkeypox PCR Test Kit With Positive / Negative Control from wholesalers
    • Buy cheap Real Time Monkeypox PCR Test Kit With Positive / Negative Control from wholesalers

    Real Time Monkeypox PCR Test Kit With Positive / Negative Control

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    Brand Name : LABNOVATION
    Price : Negotiation
    Supply Ability : 50000 Tests/Day
    Delivery Time : 7-10 working days
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    Real Time Monkeypox PCR Test Kit With Positive / Negative Control

    PCR Enzyme Real Time PCR Kit For Monkeypox Virus With Positive And Negative Control

    Real Time PCR Kit for Monkeypox Virus is based on real-time PCR technology. The kit can be used for detecting all DNA samples extracted from clinical samples such as nasal swabs, oropharyngeal swab, saliva, urine, lesion tissue, exudate, and blood, etc.
    This kit is used for in vitro qualitative nucleic acid detection of Monkeypox Virus in Human serum, lesion exudate samples and swab specimens. The test results of this kit are for clinical reference only and should not be used as the only standard for clinical diagnosis.


    Specification

    Product NameMonkeypox Virus Real Time PCR Kit
    Detection ChannelsFAM
    ICVIC
    Ct Value35
    Limit of Detection200 Copies/mL
    Storage-20℃±5℃
    TransportationUnder frozen condition
    Shelf Life12 Months
    Sample TypeNasal swabs, oropharyngeal swab, saliva, urine, lesion tissue, exudate, and blood, etc.
    Package24 Tests/Kit,48 Tests/Kit,96 Tests/Kit
    ComponentsPCR Reaction Buffer, PCR Enzyme Mixture, Positive control, Negative control



    APPLICABLE INSTRUMENT

    Real-Time PCR System: Molarray MA-6000, ABI 7500, ViiATM 7, QuantStudio 5, QuantStudio 6/7 pro, QuantStudio 6/7 flex, Agilent Mx3000P/3005P, Rotor-GeneTM 6000/Q, Bio-Rad CFX96 TouchTM/iQTM 5,Hongshi SLAN-96S/96P, AGS8830, AGS4800.


    COMPONENTS

    SpecificationsLQ-000301
    24T
    LQ-000302
    48T
    LQ-000303
    96T
    PCR Reaction Buffer336μL×1 tube672μL×1 tube672μL×2 tube
    PCR Enzyme Mixture30μL×1 tube50μL×1 tube100μL×1 tube
    Positive control50μL×1 tube100μL×1 tube200μL×1 tube
    Negative control50μL×1 tube100μL×1 tube200μL×1 tube
    Instruction for use (pcs)111

    Real Time Monkeypox PCR Test Kit With Positive / Negative Control


    PRODUCT PERFORMANCE INDEX
    1. Sensitivity: 200 copies/mL.
    2. Specificity: No cross reaction with Enterovirus (EV), Measles virus (MV), Rubella virus (RV), Varicella-zoster virus (VZV), Dengue virus (DenV), Human Parvovirus B19(HPVB19), Epstein-barr virus (EBv), human herpes virus 6(HHV-6), etc.
    3. Precision: CV ≤ 5%.


    PROCEDURES
    1. Sample preparations
    DNA extraction from clinical samples is conducted according to the corresponding requirements and procedures in the virus DNA extraction kit. The extracted
    DNA can be directly used for detection. If the sample is not detected immediately after extraction, it should be stored at -70°C for standby, avoiding repeated freeze-thaw cycles.
    2. Reaction system preparation
    (1) System preparation: Take out the reagent from the kit, and allow it to thaw completely at room temperature. Invert the mixture and centrifuge immediately. N test reactions (N = number of samples to be tested + positive control + negative control + 1) are prepared for reaction systems, respectively, as follows.

    ComponentsVolume for 1 reaction systemVolume for N reaction system
    PCR reaction buffer14μL14μLx N
    PCR Enzyme mixture1μL1μLx N
    Total volume15μL15μLx N

    (2) Reaction system distribution: Mix well the above reaction buffer, centrifuge, and dispense 15μL of aliquots into PCR tubes suitable for fluorescent PCR instrument. (Centrifuge the PCR tubes at 6,000rpm for 30s and transport to sample treatment zone.)
    3. Sample loading (Sample treatment zone)
    Add 10μL nucleic acid sample, negative control and positive control to the above PCR tubes respectively. Cap the tubes tightly and centrifuge at 6,000rpm for 10s and then transport to PCR amplification zone.
    * Precaution: Adding samples in the following order is
    recommended: negative control-> nucleic acid sample -> positive control.

    4. PCR amplification (PCR amplification zone)
    4.1 Put the caped PCR tubes into real-time PCR machine for amplification.
    4.2 Fluorescence PCR cycle condition setting

    ProgramTemperatureReaction durationNumber of cycles

    1

    50°C2 min1
    295°C2s1
    395°C1s41
    60°C13s/20s/35s

    Collect fluorescent signals at step 3:60℃; 35s for ABI 7500, 20s for SLAN-96S/96P, while 13s for other Real-Time PCR Systems. The total volume:25μL.
    4.3 Disposal after detection
    Dispose the PCR tubes in a sealed bag after reaction and treat the used tubes as medical wastes.

    5. Settings for result analysis
    Set the baseline at a region before the exponential amplification where the fluorescent signals of all the samples are relatively stable (no significant fluctuations in all the samples); set the starting point (cycle number) away from the signal fluctuations at the starting
    phase of fluorescence collection; set the end point (cycle number)1~3 cycles before the Ct of the first sample to enter exponential amplification. 4~15 cycles are recommended.
    Set the threshold right above the highest point of the negative control amplification curve (irregular noise curve).

    6. Quality control criteria
    Prior to evaluating the specimen results, the Positive Control and Negative Control should be interpreted using the interpretation table below, and the Positive Control and Negative Control curve must be performed correctly, otherwise the sample result is invalid.

    Channels/
    Controls
    Cycle threshold(Ct)value
    FAMVIC
    Positive controlCt > 40 or UNDETCt > 40 or UNDET
    Negative controlCt ≤ 35Ct ≤ 35


    7. Interpretation of Test Results
    FAM channels for Monkeypox Virus, detection result should be interpreted as below.
    a) Positive: Ct ≤ 38 and amplification curve is S-shaped.
    b) Suspected: 38 < Ct ≤ 40 and amplification curve is S-shaped, a second test is needed. Consider positive if Ct ≤ 40 and amplification curve is S-shaped for the second test. Considered negative if Ct > 40 or null Ct and Ct ≤ 35 in VIC channel for the second test.
    c) Negative: Ct > 40 or null Ct and Ct ≤ 35 in VIC channel.
    d) Re-test: Ct > 40 or null Ct and Ct > 35 in VIC channel.













































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