Analysis of the Oxidative Damage Repair GenesNUDT1,OGG1, andMUTYHin Patients from Mismatch Repair Proficient HNPCC Families (MSS-HNPCC)

Garré, Pilar; Briceño, Verõnica F.; Xicola, Rosa M.; Doyle, Brian J.; Hoya, Miguel de la; Sanz, Julián; Llovet, Patricia; Pescador, Paula; Puente, Javier; Dı́az-Rubio, Eduardo; Llor, Xavier; Caldés, Trinidad

doi:10.1158/1078-0432.ccr-10-2491

Cited by 34 publications

(37 citation statements)

References 49 publications

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“…All variants are named according to the Human Genome Variation Society (HGVS) and to the reference transcript NM_000059 3. Variants were classified according to their pathogenicity risk.…”

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confidence: 99%

BRCA2 gene: a candidate for clinical testing in familial colorectal cancer type X

et al. 2014

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Familial colorectal cancer type X (FCCX) encompasses a group of families with dominant inheritance pattern of colorectal cancer (CRC) but no alteration in any known CRC susceptibility gene. Therefore, the explanation of their susceptibility is a priority to offer an accurate genetic counseling. We screened the 27 coding exons and exon-intron boundaries of BRCA2 in 48 FCCX probands. We identified 29 variants including a frameshift mutation. Deleterious variant c.3847_3848delGT p.(Val1283Lysfs*2) showed cosegregation with disease as well as loss of heterozygosity (LOH) in CRC tumor DNA. This is the first evidence of germline BRCA2 pathogenic mutation associated with CRC risk. Furthermore, missense variants c.502C>A p.(Pro168Thr), c.5744C>T p.(Thr1915Met) and c.7759C>T p.(Leu2587Phe) were proposed as candidate risk alleles based on cosegregation, LOH tumor analysis and in silico testing.

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“…All variants are named according to the Human Genome Variation Society (HGVS) and to the reference transcript NM_000059 3. Variants were classified according to their pathogenicity risk.…”

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confidence: 99%

BRCA2 gene: a candidate for clinical testing in familial colorectal cancer type X

et al. 2014

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“…The only variant identified in the OGG1 gene (NM_016821.2) with a population MAF < 1% was c.137G>A (p.R46Q) (rs104893751; MAF GnomAD = 0.22% (600/275,590)). It had been previously shown that this variant might affect splicing causing the insertion of intron 1 (Garre et al., ; Kohno et al., ), having been associated with CRC predisposition when occurring in the germline (Garre et al., ).…”

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confidence: 99%

Germline variation in the oxidative DNA repair genesNUDT1andOGG1is not associated with hereditary colorectal cancer or polyposis

et al. 2018

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The causal association of NUDT1 (=MTH1) and OGG1 with hereditary colorectal cancer (CRC) remains unclear. Here, we sought to provide additional evidence for or against the causal contribution of NUDT1 and OGG1 mutations to hereditary CRC and/or polyposis. Mutational screening was performed using pooled DNA amplification and targeted next-generation sequencing in 529 families (441 uncharacterized MMR-proficient familial nonpolyposis CRC and 88 polyposis cases). Cosegregation, in silico analyses, in vitro functional assays, and case-control associations were carried out to characterize the identified variants. Five heterozygous carriers of novel (n = 1) or rare (n = 4) NUDT1 variants were identified. In vitro deleterious effects were demonstrated for c.143G>A p.G48E (catalytic activity and protein stability) and c.403G>T p.G135W (protein stability), although cosegregation data in the carrier families were inconclusive or nonsupportive. The frequency of missense, loss-of-function, and splice-site NUDT1 variants in our familial CRC cohort was similar to the one observed in cancer-free individuals, suggesting lack of association with CRC predisposition. No OGG1 pathogenic mutations were identified. Our results suggest that the contribution of NUDT1 and OGG1 germline mutations to hereditary CRC and to polyposis is inexistent or, at most, negligible. The inclusion of these genes in routine genetic testing is not recommended.

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“…Next, we sought to determine changes in stress response proteins in β2-M knockdown prostate cancer cells. Using C4-2B control and β2-M knockdown prostate cancer cells (KD β2-M ) we tested the levels of stress response proteins such as heat shock protein 27 (HSP27) 17 and heat shock protein 70 (HSP70) 18 and DNA repair enzymes such as N-methylpurine-DNA glycosylase (MPG) 19 and nudix (nucleoside diphosphate linked moiety X)-type motif 1 (NUDT1) 20. Interestingly, the stress response and heat shock proteins were downregulated in β2-M knockdown clones KD β2-M (Figure 2D).…”

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confidence: 99%

Inhibition of β2-Microglobulin/Hemochromatosis Enhances Radiation Sensitivity by Induction of Iron Overload in Prostate Cancer Cells

et al. 2013

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BackgroundBone metastasis is the most lethal form of several cancers. The β2-microglobulin (β2-M)/hemochromatosis (HFE) complex plays an important role in cancer development and bone metastasis. We demonstrated previously that overexpression of β2-M in prostate, breast, lung and renal cancer leads to increased bone metastasis in mouse models. Therefore, we hypothesized that β2-M is a rational target to treat prostate cancer bone metastasis.ResultsIn this study, we demonstrate the role of β2-M and its binding partner, HFE, in modulating radiation sensitivity and chemo-sensitivity of prostate cancer. By genetic deletion of β2-M or HFE or using an anti-β2-M antibody (Ab), we demonstrate that prostate cancer cells are sensitive to radiation in vitro and in vivo. Inhibition of β2-M or HFE sensitized prostate cancer cells to radiation by increasing iron and reactive oxygen species and decreasing DNA repair and stress response proteins. Using xenograft mouse model, we demonstrate that anti-β2-M Ab sensitizes prostate cancer cells to radiation treatment. Additionally, anti-β2-M Ab was able to prevent tumor growth in an immunocompetent spontaneous prostate cancer mouse model. Since bone metastasis is lethal, we used a bone xenograft model to test the ability of anti-β2-M Ab and radiation to block tumor growth in the bone. Combination treatment significantly prevented tumor growth in the bone xenograft model by inhibiting β2-M and inducing iron overload. In addition to radiation sensitive effects, inhibition of β2-M sensitized prostate cancer cells to chemotherapeutic agents.ConclusionSince prostate cancer bone metastatic patients have high β2-M in the tumor tissue and in the secreted form, targeting β2-M with anti-β2-M Ab is a promising therapeutic agent. Additionally, inhibition of β2-M sensitizes cancer cells to clinically used therapies such as radiation by inducing iron overload and decreasing DNA repair enzymes.

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Analysis of the Oxidative Damage Repair GenesNUDT1,OGG1, andMUTYHin Patients from Mismatch Repair Proficient HNPCC Families (MSS-HNPCC)

Cited by 34 publications

References 49 publications

BRCA2 gene: a candidate for clinical testing in familial colorectal cancer type X

BRCA2 gene: a candidate for clinical testing in familial colorectal cancer type X

Germline variation in the oxidative DNA repair genesNUDT1andOGG1is not associated with hereditary colorectal cancer or polyposis

Inhibition of β2-Microglobulin/Hemochromatosis Enhances Radiation Sensitivity by Induction of Iron Overload in Prostate Cancer Cells

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