Literature DB >> 28645898

DNA-PK facilitates piggyBac transposition by promoting paired-end complex formation.

Yan Jin1, Yaohui Chen2, Shimin Zhao2, Kun-Liang Guan2,3, Yuan Zhuang1,4, Wenhao Zhou1, Xiaohui Wu5, Tian Xu5,6,7.   

Abstract

The involvement of host factors is critical to our understanding of underlying mechanisms of transposition and the applications of transposon-based technologies. Modified piggyBac (PB) is one of the most potent transposon systems in mammals. However, varying transposition efficiencies of PB among different cell lines have restricted its application. We discovered that the DNA-PK complex facilitates PB transposition by binding to PB transposase (PBase) and promoting paired-end complex formation. Mass spectrometry analysis and coimmunoprecipitation revealed physical interaction between PBase and the DNA-PK components Ku70, Ku80, and DNA-PKcs Overexpression or knockdown of DNA-PK components enhances or suppresses PB transposition in tissue culture cells, respectively. Furthermore, germ-line transposition efficiency of PB is significantly reduced in Ku80 heterozygous mutant mice, confirming the role of DNA-PK in facilitating PB transposition in vivo. Fused dimer PBase can efficiently promote transposition. FRET experiments with tagged dimer PBase molecules indicated that DNA-PK promotes the paired-end complex formation of the PB transposon. These data provide a mechanistic explanation for the role of DNA-PK in facilitating PB transposition and suggest a transposition-promoting manipulation by enhancing the interaction of the PB ends. Consistent with this, deletions shortening the distance between the two PB ends, such as PB vectors with closer ends (PB-CE vectors), have a profound effect on transposition efficiency. Taken together, our study indicates that in addition to regulating DNA repair fidelity during transposition, DNA-PK also affects transposition efficiency by promoting paired-end complex formation. The approach of CE vectors provides a simple practical solution for designing efficient transposon vectors.

Entities:  

Keywords:  CE transposon vectors; DNA–PK; paired-end complex formation; piggyBac; transposition efficiency

Mesh:

Substances:

Year:  2017        PMID: 28645898      PMCID: PMC5514698          DOI: 10.1073/pnas.1612980114

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  31 in total

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Authors:  Sareina Chiung-Yuan Wu; Yaa-Jyuhn James Meir; Craig J Coates; Alfred M Handler; Pawel Pelczar; Stefan Moisyadi; Joseph M Kaminski
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8.  Nonhomologous-end-joining factors regulate DNA repair fidelity during Sleeping Beauty element transposition in mammalian cells.

Authors:  Stephen R Yant; Mark A Kay
Journal:  Mol Cell Biol       Date:  2003-12       Impact factor: 4.272

9.  Molecular architecture of the Mos1 paired-end complex: the structural basis of DNA transposition in a eukaryote.

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5.  Six domesticated PiggyBac transposases together carry out programmed DNA elimination in Paramecium.

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