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OxiSelect™ Cellular UV-Induced DNA Damage Staining Kit (CPD)

CA Reaktivität: Others Fluorometric Cell Samples
Produktnummer ABIN2344980
  • Reaktivität
    Others
    Nachweismethode
    Fluorometric
    Applikation
    Cellular Assay (CA)
    Marke
    OxiSelect™
    Proben
    Cell Samples
    Produktmerkmale
    OxiSelect™ Cellular UV-induced DNA Damage Staining Kit (CPD) is an immunofluorescence assay developed for rapid detection of CPDs in genomic DNA of cultured cells. Each kit provides sufficient reagents for up to 96 stainings in a 96-well plate. Figure 1: Structures of DNA lesions induced by UV Light
    Bestandteile
    1. Anti-CPD Antibody, 100X : One 100 μL vial.
    2. Secondary Antibody, FITC Conjugate, 100X : One 100 μL amber vial.
    3. Denaturation Solution A, 100X : One 200 μL vial.
    4. Denaturation Solution B, 100X : One 200 μL vial.
    5. Assay Diluent : One 50 mL bottle.
    6. 10X Wash Buffer : One 50 mL bottle.
    Benötigtes Material
    1. 96-well tissue culture plate
    2. Cell line of interest
    3. UV crosslinker, irradiator, or germicidal lamp
    4. DPBS containing magnesium and calcium
    5. 75 % Methanol/25 % Acetic Acid
    6. 70 % Ethanol
    7. 10 μL to 1000 μL adjustable single channel micropipettes with disposable tips
    8. 50 μL to 300 μL adjustable multichannel micropipette with disposable tips
    9. Fluorescence microscope with FITC filter
  • Applikationshinweise
    Optimal working dilution should be determined by the investigator.
    Kommentare

    • Measure CPD structures of DNA lesions induced by UV light
    • Detect structures by immunofluorescence staining under a fluorescence microscope

    Protokoll
    Cells are first seeded in a 96-well tissue culture plate. Wells are then UV irradiated to induce DNA damage. After fixation and denaturation, cells containing CPD damage are probed with an anti-CPD antibody, followed by a FITC conjugated secondary antibody. The unbound secondary antibody is removed during a wash step, and stained cells can then be visualized with a fluorescence microscope.
    Aufbereitung der Reagenzien

    1X Wash Buffer: Dilute the 10X Wash Buffer Concentrate to 1X with deionized water. Stir to homogeneity. Anti-CPD Antibody and Secondary Antibody, FITC Conjugate: Immediately before use dilute the Anti-CPD Antibody 1:100 and Secondary Antibody 1:100 with Assay Diluent. Do not store diluted solutions. Denaturation Solution A: Immediately before use dilute the Denaturation Solution A 1:100 with 70 % Ethanol. Do not store diluted solution. Denaturation Solution B: Immediately before use dilute the Denaturation Solution B 1:100 with DPBS (containing magnesium and calcium). Do not store diluted solution.

    Testdurchführung

    The following assay protocol is written for a 96-well format. Refer to the below table for the appropriate dispensing volumes of other plate formats. Note: using other plate formats will decrease the number of assays possible with this kit. Culture Dish 96-well 48-well 24-well 12-well 6-well DPBS during UV 100 200 400 800 1600 Irradiation (μL/well) 75 % Methanol/ 25 % Acetic Acid 100 200 400 800 1600 (μL/well) 70 % Ethanol (μL/well) 100 200 400 800 1600 Denaturation Solution A 100 200 400 800 1600 (μL/well) DPBS during Washing 200 400 800 1600 3200 (μL/well) Denaturation Solution B 100 200 400 800 1600 (μL/well) Assay Diluent Blocking 200 400 800 1600 3200 (μL/well) 1X Anti-CPD Antibody 100 200 400 800 1600 Solution (μL/well) 1X Secondary Antibody, FITC Conjugate Solution 100 200 400 800 1600 (μL/well) Wash Buffer (μL/well) 250 500 1000 2000 4000 Table

    1. Dispensing Volumes of Different Plate Formats. 4

      I. Cell Seeding 5

      1. Harvest and resuspend cells in culture medium at 2-4 x 10 cells/mL. Seed 100 μL in each well of a 96-well tissue culture plate and incubate overnight at 37 °C, 5 % CO2 (cells should be > 80 % confluent).

      II. UV Treatment, Fixation and Denaturation

      1. Carefully remove medium from the wells by tilting the plate and aspirating from the edge. Gently add 100 μL of DPBS (containing magnesium and calcium) to each well, taking care not to dislodge the cells.
      2. Perform UV irradiation to desired wells (removal of plate cover is recommended). Include wells without irradiation as a negative control. Samples should be performed in triplicate.
      3. Aspirate the wells and add 100 μL of 75 % Methanol/25 % Acetic Acid to each well. Incubate 30 minutes at room temperature.
      4. Aspirate the wells and add 100 μL of 70 % Ethanol to each well. Incubate 30 minutes at room temperature.
      5. Aspirate the wells and add 100 μL of Denaturation Solution A (see Preparation of Reagents) to each well. Incubate 5 minutes at room temperature.
      6. Gently wash 3 times with 200 μL DPBS (containing magnesium and calcium).
      7. Aspirate the wells and add 100 μL of Denaturation Solution B (see Preparation of Reagents) to each well. Incubate 10 minutes at room temperature.
      8. Aspirate the wells and add 200 μL of Assay Diluent to each well. Block the wells 30 minutes at room temperature.

      III. CPD Immunofluorescence Staining

      1. Aspirate the wells and add 100 μL of the diluted anti-CPD antibody (see Preparation of Reagents) to each well. Incubate at room temperature for 1 hour on an orbital shaker.
      2. Wash microwell strips 4 times with 250 μL 1X Wash Buffer per well with thorough aspiration between each wash. After the last wash, empty wells and tap microwell strips on absorbent pad or paper towel to remove excess 1X Wash Buffer.
      3. Add 100 μL of the diluted Secondary Antibody, FITC Conjugate (see Preparation of Reagents) to each well. Incubate at room temperature for 1 hour on an orbital shaker.
      4. Wash microwell strips 4 times according to step 2 above. Proceed immediately to the next step.
      5. Add 100 L of DPBS to each well.
      6. View staining with a fluorescence microscope using FITC filter. 5

    Beschränkungen
    Nur für Forschungszwecke einsetzbar
  • Lagerung
    4 °C
    Informationen zur Lagerung
    Store all kit components at 4°C until their expiration dates.
  • Hasegawa, Nakashima, Suzuki: "Nuclear DNA damage-triggered NLRP3 inflammasome activation promotes UVB-induced inflammatory responses in human keratinocytes." in: Biochemical and biophysical research communications, Vol. 477, Issue 3, pp. 329-35, (2016) (PubMed).

    Núñez-Lozano, Pimentel, Castro-Smirnov, Calvo, Míguez, de la Cueva-Méndez: "Biocompatible films with tailored spectral response for prevention of DNA damage in skin cells." in: Advanced healthcare materials, Vol. 4, Issue 13, pp. 1944-8, (2015) (PubMed).

  • Hintergrund
    Absorption of ultraviolet (UV) light produces two predominant types of DNA damage, cyclobutane pyrimidine dimers (CPD) and pyrimidine (6-4) pyrimidone photoproducts (6-4PP) (Figure 1). The result is a transition of C to T and CC to TT, which are the most frequent mutations of p53 in both human and mouse skin cancers. UV damaged DNA is usually repaired by nucleotide excision repair (NER) or base excision repair (BER). After UV exposure, cells activate p53 and stall the cell cycle for repair. If the damage is too severe, the cell will trigger apoptosis to get rid of DNA damaged, potentially mutant cells.
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