Improve Research Reproducibility A Bio-protocol resource
- Home
- Protocols
-
Preprint
Quantification of cytosolic DNA
Last updated date: Oct 24, 2024 DOI: 10.21769/p2736 Views: 65 Forks: 0
Download PDF
Ask a
question
How to
cite
Favorite
1. Buffers and reagents preparation
- Permeabilization buffer (0.1%Tween 20, 0.01% Triton-X in Phosphate Buffer Saline): Mix 50mL of 1×Phosphate Buffer Saline (PBS) with 50μL of Tween 20 and 5μL of Triton-X.
- PBST: Mix 100mL PBS and 100μL Tween 20.
- 1% BSA-PBST: Dissolve 1g of bovine serum albumin (BSA) in 100mL of PBST.
- Blocking buffer (1% BSA, 0.1% Tween 20, 2.25% Glycine): Dissolve 1.126g of glycine in 50mL of 1% BSA-PBST.
2. Procedure
- Seed 50,000–100,000 cells/well in 1 mL of growth medium.
- Wash the cells with 1× PBS.
- Fix the cells with fresh 4% of para-formaldehyde (4% PFA; Santa Cruz Biotechnology #sc-281692) for 10min at room temperature.
- Discard the 4% PFA in an appropriate container.
- Wash the cells in 1× PBS.
- Incubate the cells with the permeabilization buffer for 7min at room temperature.
- After three additional washes with 1× PBS (for 5min at room temperature), block nonspecific binding sites by incubating the cells with the blocking buffer for 30min at room temperature.
- Remove the blocking buffer (Do not wash).
- Dilute anti-dsDNA antibody (sc-58749, Santa Cruz Biotechnology) at 1:100 in 1% BSA-PBST.
- Incubate your sample with the diluted anti-dsDNA antibody in humidified chamber overnight at 4°C.
- Wash 3 times by 1× PBS (for 5min at room temperature).
- Dilute the secondary antibody (goat anti-mouse IgG H&L Alexa Fluor® 488 preabsorbed, abcam, # ab150117) at 1:200 in 1% BSA-PBST.
- Wash 3 times by 1 × PBS (for 5 min at room temperature).
- Let it sit for 1–3h at room temperature (Note: protect from the light).
- Keep the slide overnight at 4°C in slide box (Note: upside, protect from the light).
- Observe and acquire pictures with a fluorescence microscope using the RFP/GFP and DAPI channels the next day to ensure that the mounting medium is completely dry.
- Slides can be stored at 4°C.
- Upon adherence (16–24 h after seeding, according to cell type), cells are treated if needed.
- Incubate samples with the diluted secondary antibody for 1 h at room temperature (Note: protect from the light).
- Drop mounting media containing DAPI (Vector laboratories, Vectashield® Hardset™ Anti-fade mounting medium with DAPI, #H-1500) on a slide, and put carefully the cover slip.−
- Let it sit for 1–3h at room temperature (Note: protect from the light).
- Keep the slide overnight at 4°C in slide box (Note: upside, protect from the light).
- Observe and acquire pictures with a fluorescence microscope using the RFP/GFP and DAPI channels the next day to ensure that the mounting medium is completely dry.
- Slides can be stored at 4°C.
Related files
Cytosolic DNA staning protocol.docx 
Copyright: © 2024 The Author(s); This is an open-access article under the CC BY license (https://creativecommons.org/licenses/by/4.0/).
How to cite:
Readers should cite both the Bio-protocol preprint and the original research article where this protocol was used:
- Wen, H, CHEN, J and Dong, H(2024). Quantification of cytosolic DNA. Bio-protocol Preprint. DOI: 10.21769/p2736.
- Chen, J., Zhao, B., Dong, H., Li, T., Cheng, X., Gong, W., Wang, J., Zhang, J., Xin, G., Yu, Y., Lei, Y. L., Black, J. D., Li, Z. and Wen, H.(2024). Inhibition of O-GlcNAc transferase activates type I interferon-dependent antitumor immunity by bridging cGAS-STING pathway. eLife. DOI: 10.7554/eLife.94849
Do you have any questions about this protocol?
Post your question to gather feedback from the community. We will also invite the authors of this article to respond.
0/150
Tips for asking effective questions
+ Description
Write a detailed description. Include all information that will help others answer your question including experimental processes, conditions, and relevant images.
Post a Question0 Q&A
This protocol preprint was submitted via the "Request
a Protocol" track.
