Crystal structure of a Fanconi anemia-associated nuclease homolog bound to 5′ flap DNA: basis of interstrand cross-link repair by FAN1

Gwon, G.H.; Kim, Youngran; Liu, Yaqi; Watson, Adam T.; Jo, Aera; Etheridge, Thomas J.; Yuan, Fenghua; Zhang, Yanbin; Kim, Young Chang; Carr, Antony; Cho, Yunje

doi:10.1101/gad.248492.114

Cited by 20 publications

(33 citation statements)

References 59 publications

(107 reference statements)

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“…Recent crystallographic data revealed that the SAP domain interacts extensively with the DNA (Gwon et al 2014;Wang et al 2014;Zhang and Walter 2014), suggesting that direct DNA binding to the ICL might be responsible for the recruitment of FAN1 to sites of DNA damage. To investigate the contribution of the UBZ and the SAP domains to the localization of FAN1 at ICLs, we studied the recruitment of human GFP-tagged FAN1 (GFP-hFAN1) to psoralen-induced ICLs in U2OS cells ( Fig.…”

Section: Fan1 Is Required For Resistance To Dna Icl-inducing Agents Imentioning

confidence: 99%

Fan1 deficiency results in DNA interstrand cross-link repair defects, enhanced tissue karyomegaly, and organ dysfunction

et al. 2016

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Deficiency of FANCD2/FANCI-associated nuclease 1 (FAN1) in humans leads to karyomegalic interstitial nephritis (KIN), a rare hereditary kidney disease characterized by chronic renal fibrosis, tubular degeneration, and characteristic polyploid nuclei in multiple tissues. The mechanism of how FAN1 protects cells is largely unknown but is thought to involve FAN1's function in DNA interstrand cross-link (ICL) repair. Here, we describe a Fan1-deficient mouse and show that FAN1 is required for cellular and organismal resistance to ICLs. We show that the ubiquitinbinding zinc finger (UBZ) domain of FAN1, which is needed for interaction with FANCD2, is not required for the initial rapid recruitment of FAN1 to ICLs or for its role in DNA ICL resistance. Epistasis analyses reveal that FAN1 has cross-link repair activities that are independent of the Fanconi anemia proteins and that this activity is redundant with the 5 ′ -3 ′ exonuclease SNM1A. Karyomegaly becomes prominent in kidneys and livers of Fan1-deficient mice with age, and mice develop liver dysfunction. Treatment of Fan1-deficient mice with ICL-inducing agents results in pronounced thymic and bone marrow hypocellularity and the disappearance of c-kit + cells. Our results provide insight into the mechanism of FAN1 in ICL repair and demonstrate that the Fan1 mouse model effectively recapitulates the pathological features of human FAN1 deficiency.

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Section: Fan1 Is Required For Resistance To Dna Icl-inducing Agents Imentioning

confidence: 99%

Fan1 deficiency results in DNA interstrand cross-link repair defects, enhanced tissue karyomegaly, and organ dysfunction

et al. 2016

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“…1A) with T4 polynucleotide kinase (New England Biolabs) and [␥- 32 P]ATP and annealing with oligonucleotide III as described above. The 3Ј-labeled cross-linked substrates (Figs.…”

Section: Methodsmentioning

confidence: 99%

FANCD2-associated Nuclease 1, but Not Exonuclease 1 or Flap Endonuclease 1, Is Able to Unhook DNA Interstrand Cross-links in Vitro

Pizzolato

Mukherjee

Schärer

et al. 2015

Journal of Biological Chemistry

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Background:We studied how the endo/exonucleases EXO1, FAN1, and FEN1 process substrates resembling replication forks blocked by interstrand cross-links (ICLs). Results: All three enzymes cleaved off the single-stranded 5Ј flap, but FAN1 was also able to incise the substrate behind the ICL. Conclusion: FAN1 can unhook ICLs. Significance: In vivo, FAN1 may not require a 3Ј flap nuclease to unhook ICLs.

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“…However, a number of studies suggested that the cross-link repair function of FAN1 is not within the FA pathway as: (i) homologs of FAN1 have been found in bacteria, archaea, and unicellular eukaryotes which lack FA proteins (19,(21)(22)(23), (ii) mutations in FAN1 do not cause FA, but instead a kidney disorder called karyomegalic interstitial nephritis (KIN) (24), (iii) N-terminal UBZ domain is dispensable for ICL repair, but is required for genomic maintenance, suggesting that the interaction of FAN1 with ID serves a function outside of ICL repair (25)(26)(27). Nevertheless, the sensitivity of FAN1-deficient cells to ICL-forming agents implicates FAN1 in ICL resolution independently of the FA pathway.…”

Section: Dna Synthesis (Tls) and The Second Strand Is Repaired By Hommentioning

confidence: 99%

“…FAN1 incises substrates 2-5 nucleotides into the duplex from the ss/ds junction of DNA with a 5' flap or a nick, followed by 5' to 3' exonucleolytic cleavage of the duplex even in presence of an ICL (17)(18)(19)(20)23,(32)(33)(34).…”

Section: Dna Synthesis (Tls) and The Second Strand Is Repaired By Hommentioning

confidence: 99%

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Structural mechanism of DNA interstrand cross-link unhooking by the bacterial FAN1 nuclease

Jin

Roy

Lee

et al. 2018

Journal of Biological Chemistry

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The mechanism of ICL unhooking by bacterial FAN1 4 a "head to tail" dimer in the presence of DNA (34).The authors suggest that FAN1 dimer scans, latches, and unwinds DNA to pull the single-stranded DNA to the active site of a FAN1. Mutations of the residues at the dimeric interface abolished the nuclease activity of the HsFAN1, raising the possibility that the dimerization is important for its activity.Bacterial FAN1 homologs share a high similarity with HsFAN1 (Fig. 1A, 23,35). Second, PaFAN1 does not have a specific basic pocket that is critical for the proposed "3-nt exonuclease" mechanism (Fig. 1B, C, 33). Third, PaFAN1 lacks the basic motif in the SAP domain required for dimerization in one of the structures of the human nuclease (Fig. 1A, 34). These features raise the question if PaFAN1 can unhook ICLs, and if so, by which mechanism.To address these issues, we examined the ICL Based on these findings, we provide insights into how FAN1 might have evolved to have two basic regions to guide its nuclease activity and maintain genomic stability. RESULTS Substrate specificity of PaFAN1In previous study, we have used a DNA substrate with a four nucleotide 5' flap (23). (Fig. S1E-F). PaFAN1 efficiently incises ICL lesionTo examine whether the bacterial FAN1homolog shares the ICL resolving activity of mammalian FAN1, we examined the in vitro ICL unhooking activity of PaFAN1 using various DNA ICL substrates (Fig. 1D). We first analyzed ifPaFAN1 can unhook the ICL near the ss/ds junction.We used DNA substrates containing a nitrogen-like ICL, which is free of duplex distortion (15,36,37), The mechanism of ICL unhooking by bacterial FAN1 7 how PaFAN1 can catalyze multiple cleavage events.

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Crystal structure of a Fanconi anemia-associated nuclease homolog bound to 5′ flap DNA: basis of interstrand cross-link repair by FAN1

Cited by 20 publications

References 59 publications

Fan1 deficiency results in DNA interstrand cross-link repair defects, enhanced tissue karyomegaly, and organ dysfunction

Fan1 deficiency results in DNA interstrand cross-link repair defects, enhanced tissue karyomegaly, and organ dysfunction

FANCD2-associated Nuclease 1, but Not Exonuclease 1 or Flap Endonuclease 1, Is Able to Unhook DNA Interstrand Cross-links in Vitro

Structural mechanism of DNA interstrand cross-link unhooking by the bacterial FAN1 nuclease

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