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PhiC31 integrase induces a DNA damage response and chromosomal rearrangements in human adult fibroblasts

  • Jian Liu
  • , Tina Skjorringe
  • , Torben Gjetting
  • , Thomas G. Jensen
  • Kennedy Center
  • Rigshospitalet

Research output: Contribution to journalJournal articleResearchpeer-review

Abstract

Background: PhiC31 integrase facilitates efficient integration of transgenes into human and mouse genomes and is considered for clinical gene therapy. However recent studies have shown that the enzyme can induce various chromosomal abnormalities in primary human embryonic cells and mammalian cell lines. The mechanisms involved are unknown, but it has been proposed that PhiC31 attachment sites in the host genome recombine leading to chromosomal translocations. Results: We have studied possible effects of the PhiC31 integrase expression in human adult fibroblasts by karyotyping. All control cells were cytogenetically normal, whereas cells expressing PhiC31 integrase show chromosomal abnormalities confirming our previous results using primary embryonic fibroblasts. In order to study the early mechanisms involved we measured H2AX phosphorylation-a primary event in the response to DNA double-strand-breaks. Transient transfection with PhiC31 integrase encoding plasmids lead to an elevated number of cells positive for H2AX phosphorylation detected by immunofluorescence. Western blot analysis confirmed the upregulated H2AX phosphorylation, whereas markers for apoptosis as well as p53 and p21 were not induced. Cells transfected with plasmids encoding the Sleeping Beauty transposase remained cytogenetically normal, and in these cells less upregulation of H2AX phosphorylation could be detected. Conclusion: In primary human fibroblasts expression of PhiC31 integrase leads to a DNA damage response and chromosomal aberrations.
Keyword: GENOMIC INTEGRATION,IN-VIVO EVALUATION,HISTONE H2AX,GENE-THERAPY,MICE,TERM TRANSGENE EXPRESSION,BREAKS,SOMATIC INTEGRATION,PHI-C31 INTEGRASE,MAMMALIAN-CELLS
Original languageEnglish
JournalB M C Biotechnology
Volume9
Issue number31
ISSN1472-6750
DOIs
Publication statusPublished - 2009
Externally publishedYes

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