Skip NavigationSkip to Content
Return Return to Search Results

? Recombineering Used to Engineer the Genome of Phage T7

  1. Author:
    Jensen, Jordan D
    Parks, Adam R
    Adhya, Sankar
    Rattray,Alison
    Court,Don

  2. Author Address

    RNA Biology Laboratory, Center for Cancer Research, The National Cancer Institute at Frederick, Frederick, MD 21702, USA., Laboratory of Molecular Biology, Center for Cancer Research, The National Cancer Institute, Bethesda, MD 20814, USA.,
    1. Year: 2020
    2. Date: Nov 13
    3. Epub Date: 2020 11 13
  2. Journal: Antibiotics (Basel, Switzerland)
    1. 9
    2. 11
    3. Pages: pii: E805
  4. Type of Article: Article
  5. Article Number: 805
  1. Abstract:

    Bacteriophage T7 and T7-like bacteriophages are valuable genetic models for lytic phage biology that have heretofore been intractable with in vivo genetic engineering methods. This manuscript describes that the presence of ? Red recombination proteins makes in vivo recombineering of T7 possible, so that single base changes and whole gene replacements on the T7 genome can be made. Red recombination functions also increase the efficiency of T7 genome DNA transfection of cells by ~100-fold. Likewise, Red function enables two other T7-like bacteriophages that do not normally propagate in E. coli to be recovered following genome transfection. These results constitute major technical advances in the speed and efficiency of bacteriophage T7 engineering and will aid in the rapid development of new phage variants for a variety of applications.

    See More

  1. Keywords:

External Sources

  1. View Full Text
  2. DOI: 10.3390/antibiotics9110805
  3. PMID: 33202746
  4. View record in Web of ScienceĀ®
  5. WOS: 000593625600001
  6. PII : antibiotics9110805

Library Notes

  1. Fiscal Year: FY2020-2021
NCI at Frederick

You are leaving a government website.

This external link provides additional information that is consistent with the intended purpose of this site. The government cannot attest to the accuracy of a non-federal site.

Linking to a non-federal site does not constitute an endorsement by this institution or any of its employees of the sponsors or the information and products presented on the site. You will be subject to the destination site's privacy policy when you follow the link.

ContinueCancel