The Pso4 mRNA Splicing and DNA Repair Complex Interacts with WRN for Processing of DNA Interstrand Cross-links

Zhang, Nianxiang; Kaur, Ramandeep; Lu, Xiaoyan; Shen, Xi; Li, Lei; Legerski, Randy J.

doi:10.1074/jbc.m508453200

Cited by 108 publications

(122 citation statements)

References 76 publications

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“…Our findings, reported here demonstrate that the mismatch repair factor MSH2 acts, presumably in concert with ERCC1-XPF, to uncouple the ICL [21]. Our previous findings have also implicated RPA, WRN, and a complex composed of PRP19, CDC5L, PLRG1, and SPF27 in the uncoupling process [34,37]. Subsequent to the uncoupling of the ICL, REV3 would act to bypass the remaining monoadduct.…”

Section: Discussionsupporting

confidence: 64%

“…In addition, MSH2 and ERCC1-XPF have been shown to interact by co-IP experiments [26]. We have also shown an involvement of RPA, WRN, and a four protein complex composed of PRP19/PSO4, CDC5L, SPF27, and PLRG1 in ICL repair processing using the CRS assay mentioned above [34]. The CRS assay measures the initial recognition and processing of the ICL, and thus the factors required for this assay are involved in the uncoupling stage of repair.…”

Section: Discussionmentioning

confidence: 57%

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Double-strand breaks induce homologous recombinational repair of interstrand cross-links via cooperation of MSH2, ERCC1-XPF, REV3, and the Fanconi anemia pathway

Zhang

Liu

et al. 2007

DNA Repair

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DNA interstrand cross-linking agents have been widely used in chemotherapeutic treatment of cancer. The majority of interstrand cross-links (ICLs) in mammalian cells are removed via a complex process that involves the formation of double strand breaks at replication forks, incision of the ICL, and subsequent error-free repair by homologous recombination. How double strand breaks effect the removal of ICLs and the downstream homologous recombination process is not clear. Here, we describe a plasmid-based recombination assay in which one copy of the CFP gene is inactivated by a site-specific psoralen ICL and can be repaired by gene conversion with a mutated homologous donor sequence. We found that the homology dependent recombination (HDR) is inhibited by the ICL. However, when we introduced a double strand break adjacent to the site of the ICL, the removal of the ICL was enhanced and the substrate was funneled into a HDR repair pathway. This process was not dependent on the nucleotide excision repair pathway, but did require the ERCC1-XPF endonuclease and REV3. In addition, both the Fanconi anemia pathway and the mismatch repair protein MSH2 were required for the recombinational repair processing of the ICL. These results suggest that the juxtaposition of an ICL and a DSB stimulates repair of ICLs through a process requiring components of mismatch repair, ERCC1-XPF, REV3, Fanconi anemia proteins, and homologous recombination repair factors.

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Section: Discussionsupporting

confidence: 64%

Section: Discussionmentioning

confidence: 57%

Double-strand breaks induce homologous recombinational repair of interstrand cross-links via cooperation of MSH2, ERCC1-XPF, REV3, and the Fanconi anemia pathway

Zhang

Liu

et al. 2007

DNA Repair

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“…siRNAs were purchased from Dharmacon. The sequence of the hPrp19 siRNA was previously described [21]. For treatment with DNA damaging agents, methyl-methane sulfonate (MMS) or mitomycin C (MMC) was added to the medium 24 hours after transfection.…”

Section: Cell Culture and Nucleic Acid Transfectionsmentioning

confidence: 99%

“…HeLa whole cell extracts were prepared and fractionated as described [21,22]. For responses to DNA damage, HeLa cells were transfected with the indicated plasmid, and MMS was added to the medium 24 hours later.…”

Section: Phosphocellulose Column Fractionation and Chromatin Isolationmentioning

confidence: 99%

“…Furthermore, the human protein has also been shown to interact with terminal deoxynucleotidyl transferase, and to be involved in mediating cell survival after DNA damage [20]. In addition, we have recently demonstrated a biochemical role for the core complex in processing of ICLs in vitro, and showed a direct physical interaction between Cdc5L and WRN [21]. These findings indicate that the Prp19/Pso4 core complex has a direct role in mediating the cellular response to DNA damage in addition to its demonstrated role in pre-mRNA splicing.…”

mentioning

confidence: 95%

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The Prp19/Pso4 core complex undergoes ubiquitylation and structural alterations in response to DNA damage

Legerski²

2007

Biochemical and Biophysical Research Communications

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Prp19/Pso4, a U-box containing E3 ligase, has a demonstrated role in pre-mRNA splicing, but has also been implicated in both yeast and mammalian cells as having a direct role in DNA damage processing. In this report we provide further evidence in support of this latter assertion. We show that hPrp19 forms an ubiquitylated oligomeric species that is resistant to disruption by SDS gel electrophoresis under nonreducing conditions suggesting that is mediated by a thiolester between ubiquitin and a cysteine residue in Prp19. The level of this species is significantly enhanced upon treatment of cells with DNA damaging agents, and its association with chromatin is increased. In addition, hPrp19 is known to form a stable core complex with Cdc5L, Plrg1, and Spf27; however, ubiquitylated hPrp19 fails to interact with either Cdc5L or Plrg1 indicating that DNA damage can induce profound alterations to the hPrp19 core complex. Finally, we show that overexpression of hPrp19 in human cells provides a pro-survival affect in that it reduces the levels of apoptosis observed after exposure of cells to DNA damage.The pso4-1 mutant of S. cerevisiae was isolated in a genetic screen for strains sensitive to the cross-linking agent psoralen plus UVA (PUVA) [1,2]. Characterization of this mutant indicated that it was particularly sensitive to bifunctional alkylating agents, but was also sensitive to a broad range of DNA damaging agents including IR, UV, and monofuntional alkylating compounds. Induced mutagenesis and induced and spontaneous mitotic recombination were all greatly reduced in this mutant suggesting that Pso4 is involved in a recombinational pathway of error-prone repair. Based on epistasis analysis PSO4 was assigned to both the yeast RAD6 and RAD52 groups indicating the pleiotropic nature of this mutation [3,4]. Interestingly, cloning of PSO4 showed that it was allelic to PRP19 a previously characterized component of the pre-mRNA splicing complex in both yeast and human cells [5][6][7][8][9][10].The complete function of Prp19 in mRNA splicing is not known, however, it has been shown that the Prp19p-associated complex is required for activation of the pre-mRNA splicesome and for the stable association of the small nuclear RNAs U5 and U6 with the spliceosome after U4 is dissociated [11,12]. These findings suggest a possible structural role for the Prp19-associated complex in pre-mRNA splicing. Mammalian Prp19 associates with a large number of splicing factors, although, it appears to form a core complex with three other proteins including Cdc5L, Plrg1, and Spf27 [9]. The structure of the Prp19 core complex is not completely resolved, however, it has been shown that yeast Prp19 forms a tetramer via its coiled coil domains, and that the tetramer interacts with one copy of Cdc5L through the associated coiled coil domains *Corresponding author. Fax. 713-792-1474; E-Mail: rlegersk@mdanderson.org. Publisher's Disclaimer: This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to ou...

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DNAInterstrand Crosslink Repair

Siede¹

2009

Encyclopedia of Life Sciences

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Crosslinking agents such as psoralens, nitrogen mustards or cisplatin are bifunctionally acting chemicals that generate a fraction of their adducts as covalent linkages between complementary deoxyribonucleic acid strands. Since many of these agents are of importance in genetic toxicology and cancer therapy, repair of interstrand crosslinks (ICL) has been studied extensively in prokaryotes and in lower and higher eukaryotes. The main repair pathway in E. coli involves the sequential action of nucleotide excision repair and recombinational repair. In eukaryotes, several repair pathways play important roles not only in repair including nucleotide excision repair, translesion synthesis, recombination, but also mismatch repair. Relative contributions of the various pathways depend on cell cycle position and agent used. Eukaryotic proteins that specifically enhance resistance to crosslinking agents have been identified ( SNM1 , FANC family of proteins). Key concepts: Chemicals with two or more correctly spaced reactive groups can covalently link opposing DNA strands. Several repair or tolerance pathways such as nucleotide excision repair, recombination and translesion synthesis can work together to overcome such complex damage. Cell cycle stage may determine the choice of repair pathway combinations. A seemingly deleterious consequence of complex DNA damage (replication fork collapse at a crosslinked site) can be an important integrated part of damage tolerance and repair. A heritable human syndrome with multiple diverse phenotypes (Fanconi anaemia) can be associated with a specific DNA repair deficiency (crosslink repair).

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The Pso4 mRNA Splicing and DNA Repair Complex Interacts with WRN for Processing of DNA Interstrand Cross-links

Cited by 108 publications

References 76 publications

Double-strand breaks induce homologous recombinational repair of interstrand cross-links via cooperation of MSH2, ERCC1-XPF, REV3, and the Fanconi anemia pathway

Double-strand breaks induce homologous recombinational repair of interstrand cross-links via cooperation of MSH2, ERCC1-XPF, REV3, and the Fanconi anemia pathway

The Prp19/Pso4 core complex undergoes ubiquitylation and structural alterations in response to DNA damage

DNAInterstrand Crosslink Repair

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