Abstract
Comet assays to quantify DNA damage and repair in vivo and in vitro in blood cells-responses will be reported as %tail intensity and %tail moment.
Purpose
Assessment of DNA damage in spleen, liver, and gonads.
Keywords
DNA damage, Spleen, Liver, Gonad, Health assessment, Red snapper, Golden tilefish, Grouper, King snake eel
UDI
R1.x135.121:0005
Date
May 2016
Point of Contact
Name
Dana Wetzel
Organization
Mote Marine Laboratory / Environmental Laboratory of Forensics Program
Funding Source
RFP-1
DOI
10.7266/N7HT2MB1
Rights Information
This work is licensed under a
Creative Commons Public Domain Dedication 1.0 License.
Scholar Commons Citation
Wetzel, Dana. 2016. Fish Comet Assays, DeSoto Canyon, August 15-29, 2012. Distributed by: Gulf of Mexico Research Initiative Information and Data Cooperative (GRIIDC), Harte Research Institute, Texas A&M University–Corpus Christi. doi:10.7266/N7HT2MB1
Comments
Supplemental Information
Head Length, Tail Length, Head Intensity (% DNA in comet head), Tail Intensity (% DNA in comet tail), Tail Moment, Total Area, Mean Grey Level, Total Intensity, Width, Year, Month, Day, Hour, Minute, Second, Comment. Species [Gulf Hake, King Snake Eel, Red Snapper, Red Grouper, Greater Amberjack, Golden Tilefish, Yellowedge Grouper, Snowy Grouper]. The title of each file in this dataset indicates the location where the sample was collected, the sample ID, the organ being analyzed for DNA damage, the species of the sample, and year the sample was caught. For example, the file titled "WB-12-100-1-GOD-Gulf-Hake-2012.xlsx" would indicate that the: -the sample was collected from station WB-12-100 (see bellow for a list of stations and their locations) -the sample ID is 1 (additional information about the each sample can be fould in CIMAGE dataset R1.x135.120:0002) -the analysis was performed to identify gonad damage in the DNA of the specimen (there are three options: GOD = gonads, LID = liver, SPD = spleen) -the species of the specimen analyzed is Gulf Hake -the year the specimen was collected was 2012 The following is a list of stations where samples in the dataset were collected from (Station ID, Westbound Extent, Northbound Extent, Southbound Extent, Eastbound Extent): WB-12-100, -89.32078, 28.34337, 28.31415, -89.32016; WB-16-150, -90.00237, 28.38246, 28.34908, -89.58652; WB-GP2, -89.06051, 28.4325, 28.40069, -89.04501; WB-GP3, -89.12635, 28.45474, 28.42285, -89.11489; WB-SL8-40, -87.16775, 29.5302, 29.51386, -87.13137; WB-SL8-100, -87.14303, 29.445, 29.41751, -87.12102; WB-SL9-80, -88.00592, 29.17805, 29.16829, -88.04336; WB-SL9-150, -88.00322, 29.14935, 29.1495, -87.5974; WB-SL10-40, -88.53312, 29.1116, 29.08347, -88.52524; WB-SL14-60, -87.26249, 29.30115, 29.27621, -87.24361; WB-SL14-100, -87.3263, 29.24353, 29.22158, -87.29868; |Sample Collection Methods: - Collect a quarter size portion of each tissue into a scintillation vial and store on ice. - Wash 3 times with approximately 2 mL L-15 media. Discard each wash. - Add 2 mL of 4C Tissue Preparation solution and mince tissue into 1 mm pieces - Incubate on ice for 5 minutes - Liver – after 5 minute incubation, pass sample through 40 micron filter, stacked atop a 50 mL conical vial. Scrape tissue until all supernatant runs through. Additional PBS can be used, if needed. - Collect supernatant into a yellow capped centrifuge tube and centrifuge at 1200 rpm for 10 minutes. - Aspirate and discard supernatant and resuspend cell pellet in 1 mL 4C PBS - Count cells and check viability using a 1:1 dilution of Trypan blue with 10 uL cell suspension. - Adjust volume of PBS to the suspension to yield 1x105 cells/mL - Centrifuge at 1200 rpm for 10 minutes, aspirate and discard supernatant, and resuspend in an equivalent amount of Cryopreservation media. - Place cryovials in cool cell overnight. In the morning, transfer to LN2. Sample Preparation in the laboratory: I. Solution Preparation A. Alkaline Electrophoresis Solution pH >13 (200 mM NaOH, 1mM EDTA) i. 8g Sodium Hydroxide (NaOH) ii. 2 mL 500 mM EDTA, pH 8 iii. Bring to 1000 mL with DI water (after NaOH is dissolved) iv. Chill at 4 ° C B. Lysis Solution i. Chill bottle at 4 ° C for at least 20 minutes C. Alkaline Solution i. 0.6g Sodium Hydroxide (NaOH) ii. 250 µl 200mM EDTA iii. 49.75 mL DI water iv. Allow to cool to room temperature II. Electrophoresis Unit Preparation A. Set up electrophoresis unit in the cold room, with alkaline electrophoresis solution i. 300 mA, constant amp, 21 V ii. Make sure unit is level iii. Clean jack ports with isopropyl alcohol III. LMAgarose Preparation A. Melt agarose by placing bottle in boiling water for 5 minutes. B. Aliquot enough agarose for Comet slides (500 µl per slide) into eppendorf tubes and float in 37°C water bath for a minimum of 20 minutes to cool. IV. Comet Slide Preparation A. Place appropriate number of comet slides in 37°C oven. V. Protocol 3. Thaw cell suspensions quickly to room temperature by submerging in 37°C water bath then placing on ice. 4. Centrifuge cells at 150 x g for 5 minutes and gently remove the supernatant. 5. Resuspend in ice cold PBS using the same volume the cells were preserved in. 6. Add 50 µl of 1 x 105 cells/mL cell suspension to 500ul 37°C LMAgarose 7. Gently mix by pipetting up and down. 8. Transfer 50µl to sample area on comet slide. Use pipette tip to spread mixture over entire sample area. 9. Repeat steps 2-4 for each sample. 10. Lay slides flat in a container with a small amount of desiccant and place at 4°C for 30 minutes. 11. Immerse slides in prechilled lysis solution and leave at 4°C for 30 minutes. 12. Drain excess lysis solution from slides and place slides in room temperature alkaline solution 13. Let stand in the dark for 20 minutes 14. Add 950 mL Alkaline Electrophoresis Solution to electrophoresis chamber 15. Place slides in electrophoresis unit slide tray a. Slide label on the side of the black cathode, samples towards the red anode b. 2 slides per slot 16. Cover slides with slide tray overlay 17. Place lid on electrophoresis unit ensuring proper connection of wires 18. Set power supply to constant amp, 300 mA, 21 volts; 30 minutes 19. Drain excess liquid form slides, immerse in DI water, incubate for 10 minutes 20. Repeat step 19 one time 21. Drain excess liquid form slides and immerse in 70% Ethanol 22. Incubate for 5 minutes 23. Dry samples for 10-15 at room temperature Samples may be stored at room temp with desiccant before scoring at this stage 24. Dilute SYBR green II (stable once prepared for several weeks when stored at 4°C in the dark) a. 1µl SYBR green b. 10mL TE buffer, pH 7.5 25. Place 100ul of diluted SYBR green onto each sample area and incubate at 4°C for 5 minutes 26. Gently tap slide to remove excess liquid 27. Dry at room temperature in the dark 28. View and score slides by epifluorescence microscopy Cellular DNA is identified using fluorescent markers and the migration of fragments from the cell nucleus through an agarose gel, under the influence of an electric field, results in a characteristic comet-like shape. Lower molecular weight DNA fragments migrate farther from the cell nucleus and form the 'comet tail'. The cell nucleus is commonly referred to as the 'comet head'. Trevigen human control cells are run once every month to confirm proper function of the electrophoresis unit.|Comet slide electrophoresis unit. Flourescent microscope. Comet scoring software (Comet Assay IV).|| |