4.3 Article

Fluorescent fusions of the N protein of phage Mu label DNA damage in living cells

Journal

DNA REPAIR
Volume 72, Issue -, Pages 86-92

Publisher

ELSEVIER SCIENCE BV
DOI: 10.1016/j.dnarep.2018.09.005

Keywords

DNA damage; Double-strand breaks; Escherichia coli; Phage Mu N protein; Phleomycin; RecBCD; Single-cell analysis

Funding

  1. National Institutes of Health [R35-GM122598, R01-CA190635, R01-GM088653, R01-GM106373]
  2. Baylor College of Medicine
  3. NIH [HD007495, DK56338, CA125123]
  4. Robert and Janice McNair Foundation/McNair Medical Institute M.D./Ph.D. Scholars program
  5. W.M. Keck Foundation

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The N protein of phage Mu was indicated from studies in Escherichia coil to hold linear Mu chromosomes in a circular conformation by non-covalent association, and thus suggested potentially to bind DNA double-stranded ends. Because of its role in association with linear Mu DNA, we tested whether fluorescent-protein fusions to N might provide a useful tool for labeling DNA damage including double-strand break (DSB) ends in single cells. We compared N-GFP with a biochemically well documented DSB-end binding protein, the Gam protein of phage Mu, also fused to GFP. We find that N-GFP produced in live E. coif forms foci in response to DNA damage induced by radiomimetic drug phleomycin, indicating that it labels damaged DNA. N-GFP also labels specific DSBs created enzymatically by I-Scel double-strand endonuclease, and by X-rays, with the numbers of foci corresponding with the numbers of DSBs generated, indicating DSB labeling. However, whereas N-GFP forms about half as many foci as GamGFP with phleomycin, its labeling of I-SceI-and X-ray-induced DSBs is far less efficient than that of GamGFP. The data imply that N-GFP binds and labels DNA damage including DSBs, but may additionally label phleomycin-induced non-DSB damage, with which DSB-specific GamGFP does not interact. The data indicate that N-GFP labels DNA damage, and may be useful for general, not DSB-specific, DNA-damage detection.

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