4.1 Article

TREX2 exonuclease defective cells exhibit double-strand breaks and chromosomal fragments but not Robertsonian translocations

Publisher

ELSEVIER SCIENCE BV
DOI: 10.1016/j.mrfmmm.2008.11.012

Keywords

TREX2; Exonuclease; Double-strand breaks; Robertsonian translocations; Genomic stability

Funding

  1. [3P30CA054174-16S2]
  2. [UO1 ES11044]
  3. [1 RO1 CA123203-01A1]
  4. [T32 CA86800-03]

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TREX2 is a 3' -> 5' exonuclease that binds to DNA and removes 3' mismatched nucleotides. By an in vitro structure function analysis, we found a single amino acid change (H188A) completely ablates exonuclease activity and impairs DNA binding by about 60% while another change (R167A) impairs DNA binding by about 85% without impacting exonuclease activity. For a biological analysis, we generated trex2(null) cells by deleting the entire Trex2 coding sequences in mouse embryonic stem (ES) cells. We found Trex2 deletion caused high levels of Robertsonian translocations (RbTs) showing Trex2 is important for chromosomal maintenance. Here we evaluate the exonuclease and DNA binding domains by expressing in trex2(null) cells coding sequences for wild type human TREX2 (Trex2(hTX2)) or human TREX2 with the H188A change (Trex2(H188A)) or the R167A change (Trex2(R167A)). These cDNAs are positioned adjacent to the mouse Trex2 promoter by Cre-mediated knock-in. By observing metaphase spreads, we found Trex2(H188A) cells exhibited high levels of double-strand breaks (DSBs) and chromosomal fragments. Therefore. TREX2 may suppress spontaneous DSBs or exonuclease defective TREX2 may induce them in a dominate-negative manner. We also found Trex2(hTX2), hTrex2(H188A) and hTrex2(R167A) cells did not exhibit RbTs. Thus, neither the exonuclease nor DNA binding domains suppress RbTs suggesting TREX2 possesses additional biochemical activities. (C) 2008 Elsevier B.V. All rights reserved.

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