Your search keyword '"Replication Protein A metabolism"' showing total 845 results

1. Human hnRNPA1 reorganizes telomere-bound replication protein A.

Author

Granger SL, Sharma R, Kaushik V, Razzaghi M, Honda M, Gaur P, Bhat DS, Labenz SM, Heinen JE, Williams BA, Tabei SMA, Wlodarski MW, Antony E, and Spies M

Subjects

Humans, Single Molecule Imaging, G-Quadruplexes, Heterogeneous Nuclear Ribonucleoprotein A1 metabolism, Heterogeneous Nuclear Ribonucleoprotein A1 genetics, Heterogeneous Nuclear Ribonucleoprotein A1 chemistry, Replication Protein A metabolism, Replication Protein A chemistry, Replication Protein A genetics, Telomere metabolism, Telomere chemistry, DNA, Single-Stranded metabolism, DNA, Single-Stranded chemistry, DNA, Single-Stranded genetics, Protein Binding

Abstract

Human replication protein A (RPA) is a heterotrimeric ssDNA binding protein responsible for many aspects of cellular DNA metabolism. Dynamic interactions of the four RPA DNA binding domains (DBDs) with DNA control replacement of RPA by downstream proteins in various cellular metabolic pathways. RPA plays several important functions at telomeres where it binds to and melts telomeric G-quadruplexes, non-canonical DNA structures formed at the G-rich telomeric ssDNA overhangs. Here, we combine single-molecule total internal reflection fluorescence microscopy (smTIRFM) and mass photometry (MP) with biophysical and biochemical analyses to demonstrate that heterogeneous nuclear ribonucleoprotein A1 (hnRNPA1) specifically remodels RPA bound to telomeric ssDNA by dampening the RPA configurational dynamics and forming a ternary complex. Uniquely, among hnRNPA1 target RNAs, telomeric repeat-containing RNA (TERRA) is selectively capable of releasing hnRNPA1 from the RPA-telomeric DNA complex. We speculate that this telomere specific RPA-DNA-hnRNPA1 complex is an important structure in telomere protection., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

2. Molecular mechanism of parental H3/H4 recycling at a replication fork.

Author

Nagae F, Murayama Y, and Terakawa T

Subjects

Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, DNA Polymerase II metabolism, DNA Polymerase II genetics, Replication Protein A metabolism, DNA, Fungal metabolism, DNA, Fungal genetics, Protein Binding, Chromatin metabolism, Chromatin genetics, Histones metabolism, Histones genetics, DNA Replication, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae genetics, Molecular Dynamics Simulation

Abstract

In chromatin replication, faithful recycling of histones from parental DNA to replicated strands is essential for maintaining epigenetic information across generations. A previous experiment has revealed that disrupting interactions between the N-terminal tail of Mcm2, a subunit in DNA replication machinery, and a histone H3/H4 tetramer perturb the recycling. However, the molecular pathways and the factors that regulate the ratio recycled to each strand and the destination location are yet to be revealed. Here, we performed molecular dynamics simulations of yeast DNA replication machinery, an H3/H4 tetramer, and replicated DNA strands. The simulations demonstrated that histones are recycled via Cdc45-mediated and unmediated pathways without histone chaperones, as our in vitro biochemical assays supported. Also, RPA binding regulated the ratio recycled to each strand, whereas DNA bending by Pol ε modulated the destination location. Together, the simulations provided testable hypotheses, which are vital for elucidating the molecular mechanisms of histone recycling., (© 2024. The Author(s).)

Published

2024

3. Enhancing transcription-replication conflict targets ecDNA-positive cancers.

Author

Tang J, Weiser NE, Wang G, Chowdhry S, Curtis EJ, Zhao Y, Wong IT, Marinov GK, Li R, Hanoian P, Tse E, Mojica SG, Hansen R, Plum J, Steffy A, Milutinovic S, Meyer ST, Luebeck J, Wang Y, Zhang S, Altemose N, Curtis C, Greenleaf WJ, Bafna V, Benkovic SJ, Pinkerton AB, Kasibhatla S, Hassig CA, Mischel PS, and Chang HY

Subjects

Animals, Female, Humans, Male, Mice, Cell Death drug effects, Cell Line, Tumor, Checkpoint Kinase 1 metabolism, Checkpoint Kinase 1 genetics, Checkpoint Kinase 1 antagonists & inhibitors, DNA Breaks, Double-Stranded drug effects, DNA Repair drug effects, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, Protein Kinase Inhibitors pharmacology, Protein Kinase Inhibitors therapeutic use, Synthetic Lethal Mutations drug effects, Replication Protein A chemistry, Replication Protein A metabolism, Antineoplastic Agents pharmacology, Antineoplastic Agents therapeutic use, DNA Replication drug effects, Stomach Neoplasms drug therapy, Stomach Neoplasms genetics, Stomach Neoplasms pathology, Transcription, Genetic drug effects

Abstract

Extrachromosomal DNA (ecDNA) presents a major challenge for cancer patients. ecDNA renders tumours treatment resistant by facilitating massive oncogene transcription and rapid genome evolution, contributing to poor patient survival 1-7 . At present, there are no ecDNA-specific treatments. Here we show that enhancing transcription-replication conflict enables targeted elimination of ecDNA-containing cancers. Stepwise analyses of ecDNA transcription reveal pervasive RNA transcription and associated single-stranded DNA, leading to excessive transcription-replication conflicts and replication stress compared with chromosomal loci. Nucleotide incorporation on ecDNA is markedly slower, and replication stress is significantly higher in ecDNA-containing tumours regardless of cancer type or oncogene cargo. pRPA2-S33, a mediator of DNA damage repair that binds single-stranded DNA, shows elevated localization on ecDNA in a transcription-dependent manner, along with increased DNA double strand breaks, and activation of the S-phase checkpoint kinase, CHK1. Genetic or pharmacological CHK1 inhibition causes extensive and preferential tumour cell death in ecDNA-containing tumours. We advance a highly selective, potent and bioavailable oral CHK1 inhibitor, BBI-2779, that preferentially kills ecDNA-containing tumour cells. In a gastric cancer model containing FGFR2 amplified on ecDNA, BBI-2779 suppresses tumour growth and prevents ecDNA-mediated acquired resistance to the pan-FGFR inhibitor infigratinib, resulting in potent and sustained tumour regression in mice. Transcription-replication conflict emerges as a target for ecDNA-directed therapy, exploiting a synthetic lethality of excess to treat cancer., (© 2024. The Author(s).)

Published

2024

4. PRL1 interacts with and stabilizes RPA2A to regulate carbon deprivation-induced senescence in Arabidopsis.

Author

Meng J, Zhou W, Mao X, Lei P, An X, Xue H, Qi Y, Yu F, and Liu X

Subjects

Mutation genetics, Plant Leaves metabolism, Protein Stability, Seedlings genetics, Seedlings metabolism, Seedlings growth & development, Arabidopsis genetics, Arabidopsis metabolism, Arabidopsis physiology, Arabidopsis Proteins metabolism, Arabidopsis Proteins genetics, Carbon metabolism, Gene Expression Regulation, Plant, Plant Senescence, Protein Binding, Replication Protein A metabolism

Abstract

Leaf senescence is a developmental program regulated by both endogenous and environmental cues. Abiotic stresses such as nutrient deprivation can induce premature leaf senescence, which profoundly impacts plant growth and crop yield. However, the molecular mechanisms underlying stress-induced senescence are not fully understood. In this work, employing a carbon deprivation (C-deprivation)-induced senescence assay in Arabidopsis seedlings, we identified PLEIOTROPIC REGULATORY LOCUS 1 (PRL1), a component of the NineTeen Complex, as a negative regulator of C-deprivation-induced senescence. Furthermore, we demonstrated that PRL1 directly interacts with the RPA2A subunit of the single-stranded DNA-binding Replication Protein A (RPA) complex. Consistently, the loss of RPA2A leads to premature senescence, while increased expression of RPA2A inhibits senescence. Moreover, overexpression of RPA2A reverses the accelerated senescence in prl1 mutants, and the interaction with PRL1 stabilizes RPA2A under C-deprivation. In summary, our findings reveal the involvement of the PRL1-RPA2A functional module in C-deprivation-induced plant senescence., (© 2024 The Author(s). New Phytologist © 2024 New Phytologist Foundation.)

Published

2024

5. Mei5-Sae3 stabilizes Dmc1 nucleating clusters for efficient Dmc1 assembly on RPA-coated single-stranded DNA.

Author

Wei CD, Chang HY, Lu CH, Chang CC, Furukohri A, Mwaniki S, Shinohara A, Chi P, and Li HW

Subjects

Fluorescence Resonance Energy Transfer, Meiosis genetics, Protein Binding, Recombinases metabolism, Recombinases genetics, Single Molecule Imaging, Single-Strand Specific DNA and RNA Endonucleases metabolism, Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, Replication Protein A metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics

Abstract

Interhomolog recombination in meiosis requires a meiosis-specific recombinase, Dmc1. In Saccharomyces cerevisiae, the Mei5-Sae3 complex facilitates the loading of Dmc1 onto the replication protein A (RPA)-coated single-stranded DNA (ssDNA) to form nucleoprotein filaments. In vivo, Dmc1 and Mei5-Sae3 are interdependent in their colocalization on the chromosomes. However, the mechanistic role of Mei5-Sae3 in mediating Dmc1 activity remains unclear. We used single-molecule fluorescence resonance energy transfer and colocalization single-molecule spectroscopy experiments to elucidate how Mei5-Sae3 stimulates Dmc1 assembly on ssDNA and RPA-coated ssDNA. We showed that Mei5-Sae3 stabilized Dmc1 nucleating clusters with two to three molecules on naked DNA by preferentially reducing Dmc1 dissociation rates. Mei5-Sae3 also stimulated Dmc1 assembly on RPA-coated DNA. Using green fluorescent protein-labeled RPA, we showed the coexistence of an intermediate with Dmc1 and RPA on ssDNA before RPA dissociation. Moreover, the displacement efficiency of RPA depended on Dmc1 concentration, and its dependence was positively correlated with the stability of Dmc1 clusters on short ssDNA. These findings suggest a molecular model that Mei5-Sae3 mediates Dmc1 binding on RPA-coated ssDNA by stabilizing Dmc1 nucleating clusters, thus altering RPA dynamics on DNA to promote RPA dissociation., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

6. Partial wrapping of single-stranded DNA by replication protein A and modulation through phosphorylation.

Author

Chadda R, Kaushik V, Ahmad IM, Deveryshetty J, Holehouse AS, Sigurdsson ST, Biswas G, Levy Y, Bothner B, Cooley RB, Mehl RA, Dastvan R, Origanti S, and Antony E

Subjects

Phosphorylation, Models, Molecular, Fluorescence Resonance Energy Transfer, Humans, Replication Protein A metabolism, Replication Protein A chemistry, DNA, Single-Stranded metabolism, DNA, Single-Stranded chemistry, Protein Binding

Abstract

Single-stranded DNA (ssDNA) intermediates which emerge during DNA metabolic processes are shielded by replication protein A (RPA). RPA binds to ssDNA and acts as a gatekeeper to direct the ssDNA towards downstream DNA metabolic pathways with exceptional specificity. Understanding the mechanistic basis for such RPA-dependent functional specificity requires knowledge of the structural conformation of ssDNA when RPA-bound. Previous studies suggested a stretching of ssDNA by RPA. However, structural investigations uncovered a partial wrapping of ssDNA around RPA. Therefore, to reconcile the models, in this study, we measured the end-to-end distances of free ssDNA and RPA-ssDNA complexes using single-molecule FRET and double electron-electron resonance (DEER) spectroscopy and found only a small systematic increase in the end-to-end distance of ssDNA upon RPA binding. This change does not align with a linear stretching model but rather supports partial wrapping of ssDNA around the contour of DNA binding domains of RPA. Furthermore, we reveal how phosphorylation at the key Ser-384 site in the RPA70 subunit provides access to the wrapped ssDNA by remodeling the DNA-binding domains. These findings establish a precise structural model for RPA-bound ssDNA, providing valuable insights into how RPA facilitates the remodeling of ssDNA for subsequent downstream processes., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

7. Hypomorphic mutation in the large subunit of replication protein A affects mutagenesis by human APOBEC cytidine deaminases in yeast.

Author

Dennen MS, Kockler ZW, Roberts SA, Burkholder AB, Klimczak LJ, and Gordenin DA

Subjects

Humans, APOBEC Deaminases metabolism, APOBEC Deaminases genetics, Cytidine Deaminase metabolism, Cytidine Deaminase genetics, DNA, Single-Stranded metabolism, APOBEC-1 Deaminase genetics, APOBEC-1 Deaminase metabolism, Protein Subunits metabolism, Protein Subunits genetics, Replication Protein A metabolism, Replication Protein A genetics, Mutagenesis, Mutation, Saccharomyces cerevisiae genetics

Abstract

Human APOBEC single-strand (ss) specific DNA and RNA cytidine deaminases change cytosines to uracils (U's) and function in antiviral innate immunity and RNA editing and can cause hypermutation in chromosomes. The resulting U's can be directly replicated, resulting in C to T mutations, or U-DNA glycosylase can convert the U's to abasic (AP) sites which are then fixed as C to T or C to G mutations by translesion DNA polymerases. We noticed that in yeast and in human cancers, contributions of C to T and C to G mutations depend on the origin of ssDNA mutagenized by APOBECs. Since ssDNA in eukaryotic genomes readily binds to replication protein A (RPA) we asked if RPA could affect APOBEC-induced mutation spectrum in yeast. For that purpose, we expressed human APOBECs in the wild-type (WT) yeast and in strains carrying a hypomorph mutation rfa1-t33 in the large RPA subunit. We confirmed that the rfa1-t33 allele can facilitate mutagenesis by APOBECs. We also found that the rfa1-t33 mutation changed the ratio of APOBEC3A-induced T to C and T to G mutations in replicating yeast to resemble a ratio observed in long persistent ssDNA in yeast and in cancers. We present the data suggesting that RPA may shield APOBEC formed U's in ssDNA from Ung1, thereby facilitating C to T mutagenesis through the accurate copying of U's by replicative DNA polymerases. Unexpectedly, we also found that for U's shielded from Ung1 by WT RPA, the mutagenic outcome is reduced in the presence of translesion DNA polymerase zeta., (Published by Oxford University Press on behalf of The Genetics Society of America 2024.)

Published

2024

8. Molecular architecture and functional dynamics of the pre-incision complex in nucleotide excision repair.

Author

Yu J, Yan C, Paul T, Brewer L, Tsutakawa SE, Tsai CL, Hamdan SM, Tainer JA, and Ivanov I

Subjects

Humans, Transcription Factor TFIIH metabolism, Transcription Factor TFIIH chemistry, Transcription Factor TFIIH genetics, Xeroderma Pigmentosum Group D Protein metabolism, Xeroderma Pigmentosum Group D Protein genetics, Xeroderma Pigmentosum Group D Protein chemistry, Cryoelectron Microscopy, Xeroderma Pigmentosum Group A Protein metabolism, Xeroderma Pigmentosum Group A Protein genetics, Transcription Factors metabolism, Transcription Factors genetics, Protein Binding, DNA metabolism, DNA chemistry, DNA genetics, Replication Protein A metabolism, Replication Protein A genetics, Models, Molecular, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, Excision Repair, Nuclear Proteins, DNA Repair, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins chemistry, Endonucleases metabolism, Endonucleases genetics

Abstract

Nucleotide excision repair (NER) is vital for genome integrity. Yet, our understanding of the complex NER protein machinery remains incomplete. Combining cryo-EM and XL-MS data with AlphaFold2 predictions, we build an integrative model of the NER pre-incision complex(PInC). Here TFIIH serves as a molecular ruler, defining the DNA bubble size and precisely positioning the XPG and XPF nucleases for incision. Using simulations and graph theoretical analyses, we unveil PInC's assembly, global motions, and partitioning into dynamic communities. Remarkably, XPG caps XPD's DNA-binding groove and bridges both junctions of the DNA bubble, suggesting a novel coordination mechanism of PInC's dual incision. XPA rigging interlaces XPF/ERCC1 with RPA, XPD, XPB, and 5' ssDNA, exposing XPA's crucial role in licensing the XPF/ERCC1 incision. Mapping disease mutations onto our models reveals clustering into distinct mechanistic classes, elucidating xeroderma pigmentosum and Cockayne syndrome disease etiology., (© 2024. The Author(s).)

Published

2024

9. DNA synthesis across DNA hairpins by human PrimPol.

Author

Boldinova EO, Baranovskiy AG, Esyunina D, Tahirov TH, and Makarova AV

Subjects

Humans, Multifunctional Enzymes metabolism, Multifunctional Enzymes genetics, Multifunctional Enzymes chemistry, Replication Protein A metabolism, Nucleic Acid Conformation, DNA-Directed DNA Polymerase metabolism, Inverted Repeat Sequences, Protein Binding, DNA Primase metabolism, DNA Primase chemistry, DNA Primase genetics, DNA metabolism, DNA Replication

Abstract

PrimPol is a human DNA primase involved in DNA damage tolerance pathways by restarting DNA replication downstream of DNA lesions and non-canonical DNA structures. Activity and affinity to DNA relays on the interaction of PrimPol with replication protein A (RPA). In this work, we report that PrimPol has an intrinsic ability to copy DNA hairpins with a stem length of 5-9 base pairs (bp) but shows pronounced pausing of DNA synthesis. RPA greatly stimulates DNA synthesis across inverted DNA repeats by PrimPol. Moreover, deletion of the C-terminal RPA binding motif (RBM) facilitates DNA hairpin bypass and makes it independent of RPA. This work supports the idea that RBM is a negative regulator of PrimPol and its interaction with RPA is required to achieve the fully active state., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

10. Heterozygous RPA2 variant as a novel genetic cause of telomere biology disorders.

Author

Kochman R, Ba I, Yates M, Pirabakaran V, Gourmelon F, Churikov D, Laffaille M, Kermasson L, Hamelin C, Marois I, Jourquin F, Braud L, Bechara M, Lainey E, Nunes H, Breton P, Penhouet M, David P, Géli V, Lachaud C, Maréchal A, Revy P, Kannengiesser C, Saintomé C, and Coulon S

Subjects

Humans, Heterozygote, Male, Female, Shelterin Complex, Telomere Shortening genetics, Mutation, Telomerase genetics, Telomerase metabolism, Ubiquitination genetics, Ubiquitin-Protein Ligases genetics, Replication Protein A genetics, Replication Protein A metabolism, Telomere genetics, Telomere-Binding Proteins genetics, Telomere-Binding Proteins metabolism

Abstract

Premature telomere shortening or telomere instability is associated with a group of rare and heterogeneous diseases collectively known as telomere biology disorders (TBDs). Here we identified two unrelated individuals with clinical manifestations of TBDs and short telomeres associated with the identical monoallelic variant c.767A>G; Y256C in RPA2 Although the replication protein A2 (RPA2) mutant did not affect ssDNA binding and G-quadruplex-unfolding properties of RPA, the mutation reduced the affinity of RPA2 with the ubiquitin ligase RFWD3 and reduced RPA ubiquitination. Using engineered knock-in cell lines, we found an accumulation of RPA at telomeres that did not trigger ATR activation but caused short and dysfunctional telomeres. Finally, both patients acquired, in a subset of blood cells, somatic genetic rescue events in either POT1 genes or TERT promoters known to counteract the accelerated telomere shortening. Collectively, our study indicates that variants in RPA2 represent a novel genetic cause of TBDs. Our results further support the fundamental role of the RPA complex in regulating telomere length and stability in humans., (© 2024 Kochman et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2024

11. Hyper-recombination in ribosomal DNA is driven by long-range resection-independent RAD51 accumulation.

Author

Gál Z, Boukoura S, Oxe KC, Badawi S, Nieto B, Korsholm LM, Geisler SB, Dulina E, Rasmussen AV, Dahl C, Lv W, Xu H, Pan X, Arampatzis S, Stratou DE, Galanos P, Lin L, Guldberg P, Bartek J, Luo Y, and Larsen DH

Subjects

Humans, Replication Protein A metabolism, Replication Protein A genetics, Homologous Recombination, Bloom Syndrome genetics, Bloom Syndrome metabolism, BRCA2 Protein metabolism, BRCA2 Protein genetics, BRCA1 Protein metabolism, BRCA1 Protein genetics, DNA Repair, Rad51 Recombinase metabolism, Rad51 Recombinase genetics, DNA, Ribosomal genetics, DNA, Ribosomal metabolism, RecQ Helicases metabolism, RecQ Helicases genetics, Genomic Instability

Abstract

Ribosomal DNA (rDNA) encodes the ribosomal RNA genes and represents an intrinsically unstable genomic region. However, the underlying mechanisms and implications for genome integrity remain elusive. Here, we use Bloom syndrome (BS), a rare genetic disease characterized by DNA repair defects and hyper-unstable rDNA, as a model to investigate the mechanisms leading to rDNA instability. We find that in Bloom helicase (BLM) proficient cells, the homologous recombination (HR) pathway in rDNA resembles that in nuclear chromatin; it is initiated by resection, replication protein A (RPA) loading and BRCA2-dependent RAD51 filament formation. However, BLM deficiency compromises RPA-loading and BRCA1/2 recruitment to rDNA, but not RAD51 accumulation. RAD51 accumulates at rDNA despite depletion of long-range resection nucleases and rDNA damage results in micronuclei when BLM is absent. In summary, our findings indicate that rDNA is permissive to RAD51 accumulation in the absence of BLM, leading to micronucleation and potentially global genomic instability., (© 2024. The Author(s).)

Published

2024

12. A glimpse into the hidden world of the flexible C-terminal protein binding domains of human RAD52.

Author

Struble LR, Lovelace JJ, and Borgstahl GEO

Subjects

Humans, Rad51 Recombinase metabolism, Rad51 Recombinase chemistry, Rad51 Recombinase genetics, X-Ray Diffraction methods, DNA Repair, Models, Molecular, Protein Domains, Rad52 DNA Repair and Recombination Protein metabolism, Rad52 DNA Repair and Recombination Protein genetics, Rad52 DNA Repair and Recombination Protein chemistry, Protein Binding, Scattering, Small Angle, Replication Protein A metabolism, Replication Protein A chemistry, Replication Protein A genetics

Abstract

Human RAD52 protein binds DNA and is involved in genomic stability maintenance and several forms of DNA repair, including homologous recombination and single-strand annealing. Despite its importance, there are very few structural details about the variability of the RAD52 ring size and the RAD52 C-terminal protein-protein interaction domains. Even recent attempts to employ cryogenic electron microscopy (cryoEM) methods on full-length yeast and human RAD52 do not reveal interpretable structures for the C-terminal half that contains the replication protein A (RPA) and RAD51 binding domains. In this study, we employed the monodisperse purification of two RAD52 deletion constructs and small angle X-ray scattering (SAXS) to construct a structural model that includes RAD52's RPA binding domain. This model is of interest to DNA repair specialists as well as for drug development against HR-deficient cancers., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

13. Molecular basis and functional consequences of the interaction between the base excision repair DNA glycosylase NEIL1 and RPA.

Author

Le Meur RA, Pecen TJ, Le Meur KV, Nagel ZD, and Chazin WJ

Subjects

Humans, Models, Molecular, Protein Domains, Excision Repair, Replication Protein A metabolism, Replication Protein A genetics, Replication Protein A chemistry, DNA Glycosylases metabolism, DNA Glycosylases chemistry, DNA Glycosylases genetics, DNA Repair, Protein Binding

Abstract

NEIL1 is a DNA glycosylase that recognizes and initiates base excision repair of oxidized bases. The ubiquitous ssDNA binding scaffolding protein, replication protein A (RPA), modulates NEIL1 activity in a manner that depends on DNA structure. Interaction between NEIL1 and RPA has been reported, but the molecular basis of this interaction has yet to be investigated. Using a combination of NMR spectroscopy and isothermal titration calorimetry (ITC), we show that NEIL1 interacts with RPA through two contact points. An interaction with the RPA32C protein recruitment domain was mapped to a motif in the common interaction domain (CID) of NEIL1 and a dissociation constant (Kd) of 200 nM was measured. A substantially weaker secondary interaction with the tandem RPA70AB ssDNA binding domains was also mapped to the CID. Together these two contact points reveal NEIL1 has a high overall affinity (Kd ∼ 20 nM) for RPA. A homology model of the complex of RPA32C with the NEIL1 RPA binding motif in the CID was generated and used to design a set of mutations in NEIL1 to disrupt the interaction, which was confirmed by ITC. The mutant NEIL1 remains catalytically active against a thymine glycol lesion in duplex DNA in vitro. Testing the functional effect of disrupting the NEIL1-RPA interaction in vivo using a Fluorescence Multiplex-Host Cell Reactivation (FM-HCR) reporter assay revealed an unexpected role for NEIL1 in nucleotide excision repair. These findings are discussed in the context of the role of NEIL1 in replication-associated repair., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

14. The DNA double-strand break repair proteins γH2AX, RAD51, BRCA1, RPA70, KU80, and XRCC4 exhibit follicle-specific expression differences in the postnatal mouse ovaries from early to older ages.

Author

Talibova G, Bilmez Y, Tire B, and Ozturk S

Subjects

Animals, Female, Mice, Oocytes metabolism, Oocytes growth & development, Aging genetics, Aging metabolism, Replication Protein A metabolism, Replication Protein A genetics, Mice, Inbred BALB C, Rad51 Recombinase genetics, Rad51 Recombinase metabolism, DNA Breaks, Double-Stranded, Ku Autoantigen metabolism, Ku Autoantigen genetics, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, BRCA1 Protein genetics, BRCA1 Protein metabolism, DNA Repair genetics, Ovarian Follicle metabolism, Ovarian Follicle growth & development, Histones genetics, Histones metabolism, Ovary metabolism, Ovary growth & development

Abstract

Purpose: Ovarian aging is closely related to a decrease in follicular reserve and oocyte quality. The precise molecular mechanisms underlying these reductions have yet to be fully elucidated. Herein, we examine spatiotemporal distribution of key proteins responsible for DNA double-strand break (DSB) repair in ovaries from early to older ages. Functional studies have shown that the γH2AX, RAD51, BRCA1, and RPA70 proteins play indispensable roles in HR-based repair pathway, while the KU80 and XRCC4 proteins are essential for successfully operating cNHEJ pathway., Methods: Female Balb/C mice were divided into five groups as follows: Prepuberty (3 weeks old; n = 6), puberty (7 weeks old; n = 7), postpuberty (18 weeks old; n = 7), early aged (52 weeks old; n = 7), and late aged (60 weeks old; n = 7). The expression of DSB repair proteins, cellular senescence (β-GAL) and apoptosis (cCASP3) markers was evaluated in the ovaries using immunohistochemistry., Result: β-GAL and cCASP3 levels progressively increased from prepuberty to aged groups (P < 0.05). Notably, γH2AX levels varied in preantral and antral follicles among the groups (P < 0.05). In aged groups, RAD51, BRCA1, KU80, and XRCC4 levels increased (P < 0.05), while RPA70 levels decreased (P < 0.05) compared to the other groups., Conclusions: The observed alterations were primarily attributed to altered expression in oocytes and granulosa cells of the follicles and other ovarian cells. As a result, the findings indicate that these DSB repair proteins may play a role in the repair processes and even other related cellular events in ovarian cells from early to older ages., (© 2024. The Author(s).)

Published

2024

15. RPA transforms RNase H1 to a bidirectional exoribonuclease for processive RNA-DNA hybrid cleavage.

Author

Li Y, Liu C, Jia X, Bi L, Ren Z, Zhao Y, Zhang X, Guo L, Bao Y, Liu C, Li W, and Sun B

Subjects

DNA metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, RNA Stability, Nucleic Acid Hybridization, Ribonuclease H metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Exoribonucleases metabolism, Exoribonucleases genetics, RNA metabolism, RNA genetics, Replication Protein A metabolism

Abstract

RNase H1 has been acknowledged as an endoribonuclease specializing in the internal degradation of the RNA moiety within RNA-DNA hybrids, and its ribonuclease activity is indispensable in multifaceted aspects of nucleic acid metabolism. However, the molecular mechanism underlying RNase H1-mediated hybrid cleavage remains inadequately elucidated. Herein, using single-molecule approaches, we probe the dynamics of the hybrid cleavage by Saccharomyces cerevisiae RNase H1. Remarkably, a single RNase H1 enzyme displays 3'-to-5' exoribonuclease activity. The directional RNA degradation proceeds processively and yet discretely, wherein unwinding approximately 6-bp hybrids as a prerequisite for two consecutive 3-nt RNA excisions limits the overall rate within each catalytic cycle. Moreover, Replication Protein A (RPA) reinforces RNase H1's 3'-to-5' nucleolytic rate and processivity and stimulates its 5'-to-3' exoribonuclease activity. This stimulation is primarily realized through the pre-separation of the hybrids and consequently transfers RNase H1 to a bidirectional exoribonuclease, further potentiating its cleavage efficiency. These findings unveil unprecedented characteristics of an RNase and provide a dynamic view of RPA-enhanced processive hybrid cleavage by RNase H1., (© 2024. The Author(s).)

Published

2024

16. Single-molecule characterization of SV40 replisome and novel factors: human FPC and Mcm10.

Author

Ouyang Y, Al-Amodi A, Tehseen M, Alhudhali L, Shirbini A, Takahashi M, Raducanu VS, Yi G, Danazumi AU, De Biasio A, and Hamdan SM

Subjects

Humans, DNA Polymerase III metabolism, DNA Polymerase III genetics, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, DNA Helicases metabolism, DNA Helicases genetics, DNA, Viral metabolism, DNA, Viral genetics, Virus Replication, Single Molecule Imaging, Antigens, Polyomavirus Transforming metabolism, Antigens, Polyomavirus Transforming genetics, DNA, Single-Stranded metabolism, DNA-Directed DNA Polymerase, Multienzyme Complexes, Simian virus 40 metabolism, Simian virus 40 genetics, DNA Replication, Minichromosome Maintenance Proteins metabolism, Minichromosome Maintenance Proteins genetics, Replication Protein A metabolism

Abstract

The simian virus 40 (SV40) replisome only encodes for its helicase; large T-antigen (L-Tag), while relying on the host for the remaining proteins, making it an intriguing model system. Despite being one of the earliest reconstituted eukaryotic systems, the interactions coordinating its activities and the identification of new factors remain largely unexplored. Herein, we in vitro reconstituted the SV40 replisome activities at the single-molecule level, including DNA unwinding by L-Tag and the single-stranded DNA-binding protein Replication Protein A (RPA), primer extension by DNA polymerase δ, and their concerted leading-strand synthesis. We show that RPA stimulates the processivity of L-Tag without altering its rate and that DNA polymerase δ forms a stable complex with L-Tag during leading-strand synthesis. Furthermore, similar to human and budding yeast Cdc45-MCM-GINS helicase, L-Tag uses the fork protection complex (FPC) and the mini-chromosome maintenance protein 10 (Mcm10) during synthesis. Hereby, we demonstrate that FPC increases this rate, and both FPC and Mcm10 increase the processivity by stabilizing stalled replisomes and increasing their chances of restarting synthesis. The detailed kinetics and novel factors of the SV40 replisome establish it as a closer mimic of the host replisome and expand its application as a model replication system., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

17. The effect of replication protein A inhibition and post-translational modification on ATR kinase signaling.

Author

Jordan MR, Oakley GG, Mayo LD, Balakrishnan L, and Turchi JJ

Subjects

Humans, Phosphorylation, DNA-Binding Proteins metabolism, Protein Binding, Carrier Proteins, Nuclear Proteins, Replication Protein A metabolism, Ataxia Telangiectasia Mutated Proteins metabolism, Signal Transduction, Protein Processing, Post-Translational, DNA, Single-Stranded metabolism

Abstract

The ATR kinase responds to elevated levels of single-stranded DNA (ssDNA) to activate the G2/M checkpoint, regulate origin utilization, preserve fork stability, and allow DNA repair to ensure genome integrity. The intrinsic replication stress in cancer cells makes this pathway an attractive therapeutic target. The ssDNA that drives ATR signaling is sensed by the ssDNA-binding protein replication protein A (RPA), which acts as a platform for ATRIP recruitment and subsequent ATR activation by TopBP1. We have developed chemical RPA inhibitors (RPAi) that block RPA-ssDNA interactions (RPA-DBi) and RPA protein-protein interactions (RPA-PPIi); both activities are required for ATR activation. Here, we biochemically reconstitute the ATR kinase signaling pathway and demonstrate that RPA-DBi and RPA-PPIi abrogate ATR-dependent phosphorylation of target proteins with selectivity advantages over active site ATR inhibitors. We demonstrate that RPA post-translational modifications (PTMs) impact ATR kinase activation but do not alter sensitivity to RPAi. Specifically, phosphorylation of RPA32 and TopBP1 stimulate, while RPA70 acetylation does not affect ATR phosphorylation of target proteins. Collectively, this work reveals the RPAi mechanism of action to inhibit ATR signaling that can be regulated by RPA PTMs and offers insight into the anti-cancer activity of ATR pathway-targeted cancer therapeutics., (© 2024. The Author(s).)

Published

2024

18. The human Shu complex promotes RAD51 activity by modulating RPA dynamics on ssDNA.

Author

Hengel SR, Oppenheimer KG, Smith CM, Schaich MA, Rein HL, Martino J, Darrah KE, Witham M, Ezekwenna OC, Burton KR, Van Houten B, Spies M, and Bernstein KA

Subjects

Humans, DNA Repair, DNA-(Apurinic or Apyrimidinic Site) Lyase metabolism, DNA-(Apurinic or Apyrimidinic Site) Lyase genetics, Homologous Recombination, Poly(ADP-ribose) Polymerase Inhibitors pharmacology, Protein Binding, Single Molecule Imaging, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, Rad51 Recombinase metabolism, Rad51 Recombinase genetics, Replication Protein A metabolism, Replication Protein A genetics

Abstract

Templated DNA repair that occurs during homologous recombination and replication stress relies on RAD51. RAD51 activity is positively regulated by BRCA2 and the RAD51 paralogs. The Shu complex is a RAD51 paralog-containing complex consisting of SWSAP1, SWS1, and SPIDR. We demonstrate that SWSAP1-SWS1 binds RAD51, maintains RAD51 filament stability, and enables strand exchange. Using single-molecule confocal fluorescence microscopy combined with optical tweezers, we show that SWSAP1-SWS1 decorates RAD51 filaments proficient for homologous recombination. We also find SWSAP1-SWS1 enhances RPA diffusion on ssDNA. Importantly, we show human sgSWSAP1 and sgSWS1 knockout cells are sensitive to pharmacological inhibition of PARP and APE1. Lastly, we identify cancer variants in SWSAP1 that alter Shu complex formation. Together, we show that SWSAP1-SWS1 stimulates RAD51-dependent high-fidelity repair and may be an important new cancer therapeutic target., (© 2024. The Author(s).)

Published

2024

19. Rtt105 stimulates Rad51-ssDNA assembly and orchestrates Rad51 and RPA actions to promote homologous recombination repair.

Author

Wang X, Zhao X, Yu Z, Fan T, Guo Y, Liang J, Wang Y, Zhan J, Chen G, Zhou C, Zhang X, Li X, and Chen X

Subjects

Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae genetics, Protein Binding, Rad51 Recombinase metabolism, Replication Protein A metabolism, Replication Protein A genetics, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, Recombinational DNA Repair, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics

Abstract

Homologous recombination (HR) is essential for the maintenance of genome stability. During HR, Replication Protein A (RPA) rapidly coats the 3'-tailed single-strand DNA (ssDNA) generated by end resection. Then, the ssDNA-bound RPA must be timely replaced by Rad51 recombinase to form Rad51 nucleoprotein filaments that drive homology search and HR repair. How cells regulate Rad51 assembly dynamics and coordinate RPA and Rad51 actions to ensure proper HR remains poorly understood. Here, we identified that Rtt105, a Ty1 transposon regulator, acts to stimulate Rad51 assembly and orchestrate RPA and Rad51 actions during HR. We found that Rtt105 interacts with Rad51 in vitro and in vivo and restrains the adenosine 5' triphosphate (ATP) hydrolysis activity of Rad51. We showed that Rtt105 directly stimulates dynamic Rad51-ssDNA assembly, strand exchange, and D-loop formation in vitro. Notably, we found that Rtt105 physically regulates the binding of Rad51 and RPA to ssDNA via different motifs and that both regulations are necessary and epistatic in promoting Rad51 nucleation, strand exchange, and HR repair. Consequently, disrupting either of the interactions impaired HR and conferred DNA damage sensitivity, underscoring the importance of Rtt105 in orchestrating the actions of Rad51 and RPA. Our work reveals additional layers of mechanisms regulating Rad51 filament dynamics and the coordination of HR., Competing Interests: Competing interests statement:The authors declare no competing interest.

Published

2024

20. CDC20 Holds Novel Regulation Mechanism in RPA1 during Different Stages of DNA Damage to Induce Radio-Chemoresistance.

Author

Gao Y, Wen P, Shao C, Ye C, Chen Y, You J, and Su Z

Subjects

Humans, Animals, Mice, Cell Line, Tumor, Mice, Inbred BALB C, Mice, Nude, DNA Repair drug effects, Xenograft Model Antitumor Assays, Cell Proliferation drug effects, Cisplatin pharmacology, HCT116 Cells, Gene Expression Regulation, Neoplastic drug effects, DNA Damage, Replication Protein A metabolism, Replication Protein A genetics, Radiation Tolerance drug effects, Radiation Tolerance genetics, Drug Resistance, Neoplasm genetics, Cdc20 Proteins metabolism, Cdc20 Proteins genetics

Abstract

Targeting CDC20 can enhance the radiosensitivity of tumor cells, but the function and mechanism of CDC20 on DNA damage repair response remains vague. To examine that issue, tumor cell lines, including KYSE200, KYSE450, and HCT116, were utilized to detect the expression, function, and underlying mechanism of CDC20 in radio-chemoresistance. Western blot and immunofluorescence staining were employed to confirm CDC20 expression and location, and radiation could upregulate the expression of CDC20 in the cell nucleus. The homologous recombination (HR) and non-homologous end joining (NHEJ) reporter gene systems were utilized to explore the impact of CDC20 on DNA damage repair, indicating that CDC20 could promote HR repair and radio/chemo-resistance. In the early stages of DNA damage, CDC20 stabilizes the RPA1 protein through protein-protein interactions, activating the ATR-mediated signaling cascade, thereby aiding in genomic repair. In the later stages, CDC20 assists in the subsequent steps of damage repair by the ubiquitin-mediated degradation of RPA1. CCK-8 and colony formation assay were used to detect the function of CDC20 in cell vitality and proliferation, and targeting CDC20 can exacerbate the increase in DNA damage levels caused by cisplatin or etoposide. A tumor xenograft model was conducted in BALB/c-nu/nu mice to confirm the function of CDC20 in vivo, confirming the in vitro results. In conclusion, this study provides further validation of the potential clinical significance of CDC20 as a strategy to overcome radio-chemoresistance via uncovering a novel role of CDC20 in regulating RPA1 during DNA damage repair.

Published

2024

21. Schlafen 11 further sensitizes BRCA-deficient cells to PARP inhibitors through single-strand DNA gap accumulation behind replication forks.

Author

Onji H, Tate S, Sakaue T, Fujiwara K, Nakano S, Kawaida M, Onishi N, Matsumoto T, Yamagami W, Sugiyama T, Higashiyama S, Pommier Y, Kobayashi Y, and Murai J

Subjects

Humans, Female, Cell Line, Tumor, Nuclear Proteins metabolism, Nuclear Proteins genetics, Replication Protein A metabolism, Replication Protein A genetics, Chromatin metabolism, Phthalazines pharmacology, Poly(ADP-ribose) Polymerase Inhibitors pharmacology, DNA Replication drug effects, DNA, Single-Stranded genetics, DNA, Single-Stranded metabolism, Ovarian Neoplasms drug therapy, Ovarian Neoplasms genetics, Ovarian Neoplasms pathology, Ovarian Neoplasms metabolism, BRCA2 Protein genetics, BRCA2 Protein metabolism, MRE11 Homologue Protein metabolism, MRE11 Homologue Protein genetics, BRCA1 Protein genetics, BRCA1 Protein metabolism

Abstract

The preferential response to PARP inhibitors (PARPis) in BRCA-deficient and Schlafen 11 (SLFN11)-expressing ovarian cancers has been documented, yet the underlying molecular mechanisms remain unclear. As the accumulation of single-strand DNA (ssDNA) gaps behind replication forks is key for the lethality effect of PARPis, we investigated the combined effects of SLFN11 expression and BRCA deficiency on PARPi sensitivity and ssDNA gap formation in human cancer cells. PARPis increased chromatin-bound RPA2 and ssDNA gaps in SLFN11-expressing cells and even more in cells with BRCA1 or BRCA2 deficiency. SLFN11 was co-localized with chromatin-bound RPA2 under PARPis treatment, with enhanced recruitment in BRCA2-deficient cells. Notably, the chromatin-bound SLFN11 under PARPis did not block replication, contrary to its function under replication stress. SLFN11 recruitment was attenuated by the inactivation of MRE11. Hence, under PARPi treatment, MRE11 expression and BRCA deficiency lead to ssDNA gaps behind replication forks, where SLFN11 binds and increases their accumulation. As ovarian cancer patients who responded (progression-free survival >2 years) to olaparib maintenance therapy had a significantly higher SLFN11-positivity than short-responders (<6 months), our findings provide a mechanistic understanding of the favorable responses to PARPis in SLFN11-expressing and BRCA-deficient tumors. It highlight the clinical implications of SLFN11., (© 2024. The Author(s).)

Published

2024

22. Replication protein A dynamically re-organizes on primer/template junctions to permit DNA polymerase δ holoenzyme assembly and initiation of DNA synthesis.

Author

Norris JL, Rogers LO, Pytko KG, Dannenberg RL, Perreault S, Kaushik V, Kuppa S, Antony E, and Hedglin M

Subjects

Holoenzymes metabolism, DNA Primers genetics, Fluorescence Resonance Energy Transfer, Humans, Replication Protein A metabolism, DNA Polymerase III metabolism, DNA Polymerase III genetics, Proliferating Cell Nuclear Antigen metabolism, Proliferating Cell Nuclear Antigen genetics, DNA metabolism, DNA biosynthesis, Replication Protein C metabolism, Replication Protein C genetics, DNA Replication, Templates, Genetic

Abstract

DNA polymerase δ (pol δ) holoenzymes, comprised of pol δ and the processivity sliding clamp, PCNA, carry out DNA synthesis during lagging strand replication, initiation of leading strand replication, and the major DNA damage repair and tolerance pathways. Pol δ holoenzymes are assembled at primer/template (P/T) junctions and initiate DNA synthesis in a stepwise process involving the major single strand DNA (ssDNA)-binding protein complex, RPA, the processivity sliding clamp loader, RFC, PCNA and pol δ. During this process, the interactions of RPA, RFC and pol δ with a P/T junction all significantly overlap. A burning issue that has yet to be resolved is how these overlapping interactions are accommodated during this process. To address this, we design and utilize novel, ensemble FRET assays that continuously monitor the interactions of RPA, RFC, PCNA and pol δ with DNA as pol δ holoenzymes are assembled and initiate DNA synthesis. Results from the present study reveal that RPA remains engaged with P/T junctions throughout this process and the RPA•DNA complexes dynamically re-organize to allow successive binding of RFC and pol δ. These results have broad implications as they highlight and distinguish the functional consequences of dynamic RPA•DNA interactions in RPA-dependent DNA metabolic processes., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

23. Dynamic stem-loop extension by Pol θ and templated insertion during DNA repair.

Author

Carvajal-Maldonado D, Li Y, Returan M, Averill AM, Doublié S, and Wood RD

Subjects

Humans, DNA End-Joining Repair, DNA Polymerase beta metabolism, DNA Polymerase beta genetics, DNA Polymerase beta chemistry, DNA Repair, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, DNA, Single-Stranded chemistry, Replication Protein A metabolism, Replication Protein A genetics, DNA Polymerase theta, DNA-Directed DNA Polymerase metabolism, DNA-Directed DNA Polymerase genetics

Abstract

Theta-mediated end joining (TMEJ) is critical for survival of cancer cells when other DNA double-stranded break repair pathways are impaired. Human DNA polymerase theta (Pol θ) can extend ssDNA oligonucleotides, but little is known about preferred substrates and mechanism. We show that Pol θ can extend both ssDNA and RNA substrates by unimolecular stem-loop synthesis initiated by only two 3' terminal base pairs. Given sufficient time, Pol θ uses alternative pairing configurations that greatly expand the repertoire of sequence outcomes. Further primer-template adjustments yield low-fidelity outcomes when the nucleotide pool is imbalanced. Unimolecular stem-loop synthesis competes with bimolecular end joining, even when a longer terminal microhomology for end joining is available. Both reactions are partially suppressed by the ssDNA-binding protein replication protein A. Protein-primer grasp residues that are specific to Pol θ are needed for rapid stem-loop synthesis. The ability to perform stem-loop synthesis from a minimally paired primer is rare among human DNA polymerases, but we show that human DNA polymerases Pol η and Pol λ can catalyze related reactions. Using purified human Pol θ, we reconstituted in vitro TMEJ incorporating an insertion arising from a stem-loop extension. These activities may help explain TMEJ repair events that include inverted repeat sequences., Competing Interests: Conflict of interest R. D. W. owns stock in Repare Therapeutics Inc. The other authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

24. In Situ Complexation of sgRNA and Cas12a Improves the Performance of a One-Pot RPA-CRISPR-Cas12 Assay.

Author

Lesinski JM, Moragues T, Mathur P, Shen Y, Paganini C, Bezinge L, Verberckmoes B, Van Eenooghe B, Stavrakis S, deMello AJ, and Richards DA

Subjects

Humans, Endodeoxyribonucleases metabolism, Endodeoxyribonucleases chemistry, Bacterial Proteins metabolism, Bacterial Proteins genetics, Bacterial Proteins chemistry, Nucleic Acid Amplification Techniques, Replication Protein A metabolism, Biosensing Techniques methods, CRISPR-Cas Systems genetics, CRISPR-Associated Proteins metabolism, RNA, Guide, CRISPR-Cas Systems metabolism

Abstract

Due to their ability to selectively target pathogen-specific nucleic acids, CRISPR-Cas systems are increasingly being employed as diagnostic tools. "One-pot" assays that combine nucleic acid amplification and CRISPR-Cas systems (NAAT-CRISPR-Cas) in a single step have emerged as one of the most popular CRISPR-Cas biosensing formats. However, operational simplicity comes at a cost, with one-pot assays typically being less sensitive than corresponding two-step NAAT-CRISPR-Cas assays and often failing to detect targets at low concentrations. It is thought that these performance reductions result from the competition between the two enzymatic processes driving the assay, namely, Cas-mediated cis -cleavage and polymerase-mediated amplification of the target DNA. Herein, we describe a novel one-pot RPA-Cas12a assay that circumvents this issue by leveraging in situ complexation of the target-specific sgRNA and Cas12a to purposefully limit the concentration of active Cas12a during the early stages of the assay. Using a clinically relevant assay against a DNA target for HPV-16, we show how this in situ format reduces competition between target cleavage and amplification and engenders significant improvements in detection limit when compared to the traditional one-pot assay format, even in patient-derived samples. Finally, to gain further insight into the assay, we use experimental data to formulate a mechanistic model describing the competition between the Cas enzyme and nucleic acid amplification. These findings suggest that purposefully limiting cis -cleavage rates of Cas proteins is a viable strategy for improving the performance of one-pot NAAT-CRISPR-Cas assays.

Published

2024

25. Cdc13 exhibits dynamic DNA strand exchange in the presence of telomeric DNA.

Author

Nickens DG, Feng Z, Shen J, Gray SJ, Simmons RH 3rd, Niu H, and Bochman ML

Subjects

Binding Sites, DNA, Fungal metabolism, DNA, Fungal genetics, DNA-Binding Proteins metabolism, Protein Binding, RecQ Helicases, Replication Protein A metabolism, Telomerase metabolism, DNA Helicases metabolism, DNA, Single-Stranded metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Telomere metabolism, Telomere-Binding Proteins metabolism

Abstract

Telomerase is the enzyme that lengthens telomeres and is tightly regulated by a variety of means to maintain genome integrity. Several DNA helicases function at telomeres, and we previously found that the Saccharomyces cerevisiae helicases Hrq1 and Pif1 directly regulate telomerase. To extend these findings, we are investigating the interplay between helicases, single-stranded DNA (ssDNA) binding proteins (ssBPs), and telomerase. The yeast ssBPs Cdc13 and RPA differentially affect Hrq1 and Pif1 helicase activity, and experiments to measure helicase disruption of Cdc13/ssDNA complexes instead revealed that Cdc13 can exchange between substrates. Although other ssBPs display dynamic binding, this was unexpected with Cdc13 due to the reported in vitro stability of the Cdc13/telomeric ssDNA complex. We found that the DNA exchange by Cdc13 occurs rapidly at physiological temperatures, requires telomeric repeat sequence DNA, and is affected by ssDNA length. Cdc13 truncations revealed that the low-affinity binding site (OB1), which is distal from the high-affinity binding site (OB3), is required for this intermolecular dynamic DNA exchange (DDE). We hypothesize that DDE by Cdc13 is the basis for how Cdc13 'moves' at telomeres to alternate between modes where it regulates telomerase activity and assists in telomere replication., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

26. Di- and tri-methylation of histone H3K36 play distinct roles in DNA double-strand break repair.

Author

Chen R, Zhao MJ, Li YM, Liu AH, Wang RX, Mei YC, Chen X, and Du HN

Subjects

Humans, Methylation, Ku Autoantigen metabolism, Ku Autoantigen genetics, Replication Protein A metabolism, Replication Protein A genetics, Homologous Recombination, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, DNA Repair, Chromatin metabolism, Chromatin genetics, DNA Breaks, Double-Stranded, Histones metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, DNA End-Joining Repair, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism

Abstract

Histone H3 Lys36 (H3K36) methylation and its associated modifiers are crucial for DNA double-strand break (DSB) repair, but the mechanism governing whether and how different H3K36 methylation forms impact repair pathways is unclear. Here, we unveil the distinct roles of H3K36 dimethylation (H3K36me2) and H3K36 trimethylation (H3K36me3) in DSB repair via non-homologous end joining (NHEJ) or homologous recombination (HR). Yeast cells lacking H3K36me2 or H3K36me3 exhibit reduced NHEJ or HR efficiency. yKu70 and Rfa1 bind H3K36me2- or H3K36me3-modified peptides and chromatin, respectively. Disrupting these interactions impairs yKu70 and Rfa1 recruitment to damaged H3K36me2- or H3K36me3-rich loci, increasing DNA damage sensitivity and decreasing repair efficiency. Conversely, H3K36me2-enriched intergenic regions and H3K36me3-enriched gene bodies independently recruit yKu70 or Rfa1 under DSB stress. Importantly, human KU70 and RPA1, the homologs of yKu70 and Rfa1, exclusively associate with H3K36me2 and H3K36me3 in a conserved manner. These findings provide valuable insights into how H3K36me2 and H3K36me3 regulate distinct DSB repair pathways, highlighting H3K36 methylation as a critical element in the choice of DSB repair pathway., (© 2024. Science China Press.)

Published

2024

27. CK2-dependent degradation of CBX3 dictates replication fork stalling and PARP inhibitor sensitivity.

Author

Ma J, Ren D, Wang Z, Li W, Li L, Liu T, Ye Q, Lei Y, Jian Y, Ma B, Fan Y, Liu J, Gao Y, Jin X, Huang H, and Li L

Subjects

Humans, Cell Line, Tumor, Proteolysis, DNA Damage, Phosphorylation, Chromosomal Proteins, Non-Histone, Casein Kinase II metabolism, Casein Kinase II genetics, Poly(ADP-ribose) Polymerase Inhibitors pharmacology, DNA Replication, Replication Protein A metabolism, Replication Protein A genetics

Abstract

DNA replication is a vulnerable cellular process, and its deregulation leads to genomic instability. Here, we demonstrate that chromobox protein homolog 3 (CBX3) binds replication protein A 32-kDa subunit (RPA2) and regulates RPA2 retention at stalled replication forks. CBX3 is recruited to stalled replication forks by RPA2 and inhibits ring finger and WD repeat domain 3 (RFWD3)-facilitated replication restart. Phosphorylation of CBX3 at serine-95 by casein kinase 2 (CK2) kinase augments cadherin 1 (CDH1)-mediated CBX3 degradation and RPA2 dynamics at stalled replication forks, which permits replication fork restart. Increased expression of CBX3 due to gene amplification or CK2 inhibitor treatment sensitizes prostate cancer cells to poly(ADP-ribose) polymerase (PARP) inhibitors while inducing replication stress and DNA damage. Our work reveals CBX3 as a key regulator of RPA2 function and DNA replication, suggesting that CBX3 could serve as an indicator for targeted therapy of cancer using PARP inhibitors.

Published

2024

28. Inhibition of intracellular ATP synthesis impairs the recruitment of homologous recombination factors after ionizing radiation.

Author

Hayashi R, Okumura H, Isono M, Yamauchi M, Unami D, Lusi RT, Yamamoto M, Kato Y, Uchihara Y, and Shibata A

Subjects

Humans, DNA Breaks, Double-Stranded radiation effects, Replication Protein A metabolism, Cell Line, Tumor, Intracellular Space metabolism, Intracellular Space radiation effects, DNA Repair, Histones metabolism, Adenosine Triphosphate metabolism, Adenosine Triphosphate biosynthesis, Homologous Recombination radiation effects, Radiation, Ionizing, Rad51 Recombinase metabolism, BRCA1 Protein metabolism

Abstract

Ionizing radiation (IR)-induced double-strand breaks (DSBs) are primarily repaired by non-homologous end joining or homologous recombination (HR) in human cells. DSB repair requires adenosine-5'-triphosphate (ATP) for protein kinase activities in the multiple steps of DSB repair, such as DNA ligation, chromatin remodeling, and DNA damage signaling via protein kinase and ATPase activities. To investigate whether low ATP culture conditions affect the recruitment of repair proteins at DSB sites, IR-induced foci were examined in the presence of ATP synthesis inhibitors. We found that p53 binding protein 1 foci formation was modestly reduced under low ATP conditions after IR, although phosphorylated histone H2AX and mediator of DNA damage checkpoint 1 foci formation were not impaired. Next, we examined the foci formation of breast cancer susceptibility gene I (BRCA1), replication protein A (RPA) and radiation 51 (RAD51), which are HR factors, in G2 phase cells following IR. Interestingly, BRCA1 and RPA foci in the G2 phase were significantly reduced under low ATP conditions compared to that under normal culture conditions. Notably, RAD51 foci were drastically impaired under low ATP conditions. These results suggest that HR does not effectively progress under low ATP conditions; in particular, ATP shortages impair downstream steps in HR, such as RAD51 loading. Taken together, these results suggest that the maintenance of cellular ATP levels is critical for DNA damage response and HR progression after IR., (© The Author(s) 2024. Published by Oxford University Press on behalf of The Japanese Radiation Research Society and Japanese Society for Radiation Oncology.)

Published

2024

29. CSB and SMARCAL1 compete for RPA32 at stalled forks and differentially control the fate of stalled forks in BRCA2-deficient cells.

Author

Batenburg NL, Sowa DJ, Walker JR, Andres SN, and Zhu XD

Subjects

Humans, Protein Binding, Cell Line, Tumor, DNA Repair, DNA Helicases metabolism, DNA Helicases genetics, Poly-ADP-Ribose Binding Proteins metabolism, Poly-ADP-Ribose Binding Proteins genetics, BRCA2 Protein metabolism, BRCA2 Protein genetics, DNA Replication, DNA Repair Enzymes metabolism, DNA Repair Enzymes genetics, Replication Protein A metabolism, Replication Protein A genetics

Abstract

CSB (Cockayne syndrome group B) and SMARCAL1 (SWI/SNF-related, matrix-associated, actin-dependent, regulator of chromatin, subfamily A-like 1) are DNA translocases that belong to the SNF2 helicase family. They both are enriched at stalled replication forks. While SMARCAL1 is recruited by RPA32 to stalled forks, little is known about whether RPA32 also regulates CSB's association with stalled forks. Here, we report that CSB directly interacts with RPA, at least in part via a RPA32C-interacting motif within the N-terminal region of CSB. Modeling of the CSB-RPA32C interaction suggests that CSB binds the RPA32C surface previously shown to be important for binding of UNG2 and SMARCAL1. We show that this interaction is necessary for promoting fork slowing and fork degradation in BRCA2-deficient cells but dispensable for mediating restart of stalled forks. CSB competes with SMARCAL1 for RPA32 at stalled forks and acts non-redundantly with SMARCAL1 to restrain fork progression in response to mild replication stress. In contrast to CSB stimulated restart of stalled forks, SMARCAL1 inhibits restart of stalled forks in BRCA2-deficient cells, likely by suppressing BIR-mediated repair of collapsed forks. Loss of CSB leads to re-sensitization of SMARCAL1-depleted BRCA2-deficient cells to chemodrugs, underscoring a role of CSB in targeted cancer therapy., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

30. Physical interactions between specifically regulated subpopulations of the MCM and RNR complexes prevent genetic instability.

Author

Yáñez-Vilches A, Romero AM, Barrientos-Moreno M, Cruz E, González-Prieto R, Sharma S, Vertegaal ACO, and Prado F

Subjects

Protein Serine-Threonine Kinases genetics, Protein Serine-Threonine Kinases metabolism, DNA Helicases genetics, DNA Helicases metabolism, Minichromosome Maintenance Proteins metabolism, Minichromosome Maintenance Proteins genetics, Replication Protein A metabolism, Replication Protein A genetics, Ribonucleoside Diphosphate Reductase genetics, Ribonucleoside Diphosphate Reductase metabolism, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism, DNA Replication genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, DNA Damage genetics, Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, Rad52 DNA Repair and Recombination Protein metabolism, Rad52 DNA Repair and Recombination Protein genetics, Genomic Instability, Ribonucleotide Reductases genetics, Ribonucleotide Reductases metabolism, DNA Repair genetics

Abstract

The helicase MCM and the ribonucleotide reductase RNR are the complexes that provide the substrates (ssDNA templates and dNTPs, respectively) for DNA replication. Here, we demonstrate that MCM interacts physically with RNR and some of its regulators, including the kinase Dun1. These physical interactions encompass small subpopulations of MCM and RNR, are independent of the major subcellular locations of these two complexes, augment in response to DNA damage and, in the case of the Rnr2 and Rnr4 subunits of RNR, depend on Dun1. Partial disruption of the MCM/RNR interactions impairs the release of Rad52 -but not RPA-from the DNA repair centers despite the lesions are repaired, a phenotype that is associated with hypermutagenesis but not with alterations in the levels of dNTPs. These results suggest that a specifically regulated pool of MCM and RNR complexes plays non-canonical roles in genetic stability preventing persistent Rad52 centers and hypermutagenesis., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Yáñez-Vilches et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

31. Mechanism of single-stranded DNA annealing by RAD52-RPA complex.

Author

Liang CC, Greenhough LA, Masino L, Maslen S, Bajrami I, Tuppi M, Skehel M, Taylor IA, and West SC

Subjects

Humans, Models, Molecular, Protein Binding, Protein Domains, Binding Sites, Cryoelectron Microscopy, DNA, Single-Stranded chemistry, DNA, Single-Stranded metabolism, DNA, Single-Stranded ultrastructure, Rad52 DNA Repair and Recombination Protein chemistry, Rad52 DNA Repair and Recombination Protein metabolism, Rad52 DNA Repair and Recombination Protein ultrastructure, Replication Protein A chemistry, Replication Protein A metabolism, Replication Protein A ultrastructure, Multiprotein Complexes chemistry, Multiprotein Complexes metabolism, Multiprotein Complexes ultrastructure

Abstract

RAD52 is important for the repair of DNA double-stranded breaks 1,2 , mitotic DNA synthesis 3-5 and alternative telomere length maintenance 6,7 . Central to these functions, RAD52 promotes the annealing of complementary single-stranded DNA (ssDNA) 8,9 and provides an alternative to BRCA2/RAD51-dependent homologous recombination repair 10 . Inactivation of RAD52 in homologous-recombination-deficient BRCA1- or BRCA2-defective cells is synthetically lethal 11,12 , and aberrant expression of RAD52 is associated with poor cancer prognosis 13,14 . As a consequence, RAD52 is an attractive therapeutic target against homologous-recombination-deficient breast, ovarian and prostate cancers 15-17 . Here we describe the structure of RAD52 and define the mechanism of annealing. As reported previously 18-20 , RAD52 forms undecameric (11-subunit) ring structures, but these rings do not represent the active form of the enzyme. Instead, cryo-electron microscopy and biochemical analyses revealed that ssDNA annealing is driven by RAD52 open rings in association with replication protein-A (RPA). Atomic models of the RAD52-ssDNA complex show that ssDNA sits in a positively charged channel around the ring. Annealing is driven by the RAD52 N-terminal domains, whereas the C-terminal regions modulate the open-ring conformation and RPA interaction. RPA associates with RAD52 at the site of ring opening with critical interactions occurring between the RPA-interacting domain of RAD52 and the winged helix domain of RPA2. Our studies provide structural snapshots throughout the annealing process and define the molecular mechanism of ssDNA annealing by the RAD52-RPA complex., (© 2024. The Author(s).)

Published

2024

32. Modulation of the microhomology-mediated end joining pathway suppresses large deletions and enhances homology-directed repair following CRISPR-Cas9-induced DNA breaks.

Author

Yuan B, Bi C, Tian Y, Wang J, Jin Y, Alsayegh K, Tehseen M, Yi G, Zhou X, Shao Y, Romero FV, Fischle W, Izpisua Belmonte JC, Hamdan S, Huang Y, and Li M

Subjects

Humans, DNA Breaks, Recombinational DNA Repair, Sequence Deletion, DNA Polymerase theta, Replication Protein A metabolism, Replication Protein A genetics, CRISPR-Cas Systems, DNA End-Joining Repair, Gene Editing methods

Abstract

Background: CRISPR-Cas9 genome editing often induces unintended, large genomic rearrangements, posing potential safety risks. However, there are no methods for mitigating these risks., Results: Using long-read individual-molecule sequencing (IDMseq), we found the microhomology-mediated end joining (MMEJ) DNA repair pathway plays a predominant role in Cas9-induced large deletions (LDs). We targeted MMEJ-associated genes genetically and/or pharmacologically and analyzed Cas9-induced LDs at multiple gene loci using flow cytometry and long-read sequencing. Reducing POLQ levels or activity significantly decreases LDs, while depleting or overexpressing RPA increases or reduces LD frequency, respectively. Interestingly, small-molecule inhibition of POLQ and delivery of recombinant RPA proteins also dramatically promote homology-directed repair (HDR) at multiple disease-relevant gene loci in human pluripotent stem cells and hematopoietic progenitor cells., Conclusions: Our findings reveal the contrasting roles of RPA and POLQ in Cas9-induced LD and HDR, suggesting new strategies for safer and more precise genome editing., (© 2024. The Author(s).)

Published

2024

33. Replication protein-A, RPA, plays a pivotal role in the maintenance of recombination checkpoint in yeast meiosis.

Author

Sampathkumar A, Zhong C, Tang Y, Fujita Y, Ito M, and Shinohara A

Subjects

Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, Recombination, Genetic, Homologous Recombination, MAP Kinase Kinase 1 metabolism, MAP Kinase Kinase 1 genetics, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, Nuclear Proteins metabolism, Nuclear Proteins genetics, Replication Protein A metabolism, Replication Protein A genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Meiosis, DNA Breaks, Double-Stranded, Transcription Factors

Abstract

DNA double-strand breaks (DSBs) activate DNA damage responses (DDRs) in both mitotic and meiotic cells. A single-stranded DNA (ssDNA) binding protein, Replication protein-A (RPA) binds to the ssDNA formed at DSBs to activate ATR/Mec1 kinase for the response. Meiotic DSBs induce homologous recombination monitored by a meiotic DDR called the recombination checkpoint that blocks the pachytene exit in meiotic prophase I. In this study, we further characterized the essential role of RPA in the maintenance of the recombination checkpoint during Saccharomyces cerevisiae meiosis. The depletion of an RPA subunit, Rfa1, in a recombination-defective dmc1 mutant, fully alleviates the pachytene arrest with the persistent unrepaired DSBs. RPA depletion decreases the activity of a meiosis-specific CHK2 homolog, Mek1 kinase, which in turn activates the Ndt80 transcriptional regulator for pachytene exit. These support the idea that RPA is a sensor of ssDNAs for the activation of meiotic DDR. Rfa1 depletion also accelerates the prophase I delay in the zip1 mutant defective in both chromosome synapsis and the recombination, consistent with the notion that the accumulation of ssDNAs rather than defective synapsis triggers prophase I delay in the zip1 mutant., (© 2024. The Author(s).)

Published

2024

34. RPA interacts with Rad52 to promote meiotic crossover and noncrossover recombination.

Author

Joo JH, Hong S, Higashide MT, Choi EH, Yoon S, Lee MS, Kang HA, Shinohara A, Kleckner N, and Kim KP

Subjects

Recombination, Genetic, DNA, Single-Stranded metabolism, DNA, Single-Stranded genetics, Homologous Recombination genetics, Rad52 DNA Repair and Recombination Protein metabolism, Rad52 DNA Repair and Recombination Protein genetics, Replication Protein A metabolism, Replication Protein A genetics, Meiosis genetics, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Crossing Over, Genetic, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, DNA Breaks, Double-Stranded

Abstract

Meiotic recombination is initiated by programmed double-strand breaks (DSBs). Studies in Saccharomyces cerevisiae have shown that, following rapid resection to generate 3' single-stranded DNA (ssDNA) tails, one DSB end engages a homolog partner chromatid and is extended by DNA synthesis, whereas the other end remains associated with its sister. Then, after regulated differentiation into crossover- and noncrossover-fated types, the second DSB end participates in the reaction by strand annealing with the extended first end, along both pathways. This second-end capture is dependent on Rad52, presumably via its known capacity to anneal two ssDNAs. Here, using physical analysis of DNA recombination, we demonstrate that this process is dependent on direct interaction of Rad52 with the ssDNA binding protein, replication protein A (RPA). Furthermore, the absence of this Rad52-RPA joint activity results in a cytologically-prominent RPA spike, which emerges from the homolog axes at sites of crossovers during the pachytene stage of the meiotic prophase. Our findings suggest that this spike represents the DSB end of a broken chromatid caused by either the displaced leading DSB end or the second DSB end, which has been unable to engage with the partner homolog-associated ssDNA. These and other results imply a close correspondence between Rad52-RPA roles in meiotic recombination and mitotic DSB repair., (© The Author(s) 2024. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

35. SMARCAL1 ubiquitylation controls its association with RPA-coated ssDNA and promotes replication fork stability.

Author

Yates M, Marois I, St-Hilaire E, Ronato DA, Djerir B, Brochu C, Morin T, Hammond-Martel I, Gezzar-Dandashi S, Casimir L, Drobetsky E, Cappadocia L, Masson JY, Wurtele H, and Maréchal A

Subjects

Humans, Replication Protein A genetics, Replication Protein A metabolism, Protein Binding, Ubiquitination, DNA Damage, Genomic Instability, DNA Helicases genetics, DNA Helicases metabolism, Ubiquitin-Protein Ligases genetics, Ubiquitin-Protein Ligases metabolism, DNA, Single-Stranded genetics, DNA Replication genetics

Abstract

Impediments in replication fork progression cause genomic instability, mutagenesis, and severe pathologies. At stalled forks, RPA-coated single-stranded DNA (ssDNA) activates the ATR kinase and directs fork remodeling, 2 key early events of the replication stress response. RFWD3, a recently described Fanconi anemia (FA) ubiquitin ligase, associates with RPA and promotes its ubiquitylation, facilitating late steps of homologous recombination (HR). Intriguingly, RFWD3 also regulates fork progression, restart and stability via poorly understood mechanisms. Here, we used proteomics to identify putative RFWD3 substrates during replication stress in human cells. We show that RFWD3 interacts with and ubiquitylates the SMARCAL1 DNA translocase directly in vitro and following DNA damage in vivo. SMARCAL1 ubiquitylation does not trigger its subsequent proteasomal degradation but instead disengages it from RPA thereby regulating its function at replication forks. Proper regulation of SMARCAL1 by RFWD3 at stalled forks protects them from excessive MUS81-mediated cleavage in response to UV irradiation, thereby limiting DNA replication stress. Collectively, our results identify RFWD3-mediated SMARCAL1 ubiquitylation as a novel mechanism that modulates fork remodeling to avoid genome instability triggered by aberrant fork processing., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Yates et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

36. Rapid Long-distance Migration of RPA on Single Stranded DNA Occurs Through Intersegmental Transfer Utilizing Multivalent Interactions.

Author

Pangeni S, Biswas G, Kaushik V, Kuppa S, Yang O, Lin CT, Mishra G, Levy Y, Antony E, and Ha T

Subjects

DNA Replication, Protein Binding genetics, DNA, Single-Stranded chemistry, DNA, Single-Stranded metabolism, Replication Protein A chemistry, Replication Protein A genetics, Replication Protein A metabolism

Abstract

Replication Protein A (RPA) is asingle strandedDNA(ssDNA)binding protein that coordinates diverse DNA metabolic processes including DNA replication, repair, and recombination. RPA is a heterotrimeric protein with six functional oligosaccharide/oligonucleotide (OB) domains and flexible linkers. Flexibility enables RPA to adopt multiple configurations andis thought to modulate its function. Here, usingsingle moleculeconfocal fluorescencemicroscopy combinedwith optical tweezers and coarse-grained molecular dynamics simulations, we investigated the diffusional migration of single RPA molecules on ssDNA undertension.The diffusioncoefficientDis the highest (20,000nucleotides 2 /s) at 3pNtension and in 100 mMKCl and markedly decreases whentensionor salt concentrationincreases. We attribute the tension effect to intersegmental transfer which is hindered by DNA stretching and the salt effect to an increase in binding site size and interaction energy of RPA-ssDNA. Our integrative study allowed us to estimate the size and frequency of intersegmental transfer events that occur through transient bridging of distant sites on DNA by multiple binding sites on RPA. Interestingly, deletion of RPA trimeric core still allowed significant ssDNA binding although the reduced contact area made RPA 15-fold more mobile. Finally, we characterized the effect of RPA crowding on RPA migration. These findings reveal how the high affinity RPA-ssDNA interactions are remodeled to yield access, a key step in several DNA metabolic processes., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Chang-Ting Lin was previously employed by LUMICKS B.V and Olivia Yang is currently employed by LUMICS B.V. Y. L. holds The Morton and Gladys Pickman professional chair in Structural Biology., (Copyright © 2024 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2024

37. ZNF827 is a single-stranded DNA binding protein that regulates the ATR-CHK1 DNA damage response pathway.

Author

Yang SF, Nelson CB, Wells JK, Fernando M, Lu R, Allen JAM, Malloy L, Lamm N, Murphy VJ, Mackay JP, Deans AJ, Cesare AJ, Sobinoff AP, and Pickett HA

Subjects

Phosphorylation, Replication Protein A metabolism, Ataxia Telangiectasia Mutated Proteins metabolism, DNA-Binding Proteins metabolism, DNA Replication, DNA Damage, DNA, Single-Stranded, DNA Repair, Protein Kinases metabolism, Signal Transduction

Abstract

The ATR-CHK1 DNA damage response pathway becomes activated by the exposure of RPA-coated single-stranded DNA (ssDNA) that forms as an intermediate during DNA damage and repair, and as a part of the replication stress response. Here, we identify ZNF827 as a component of the ATR-CHK1 kinase pathway. We demonstrate that ZNF827 is a ssDNA binding protein that associates with RPA through concurrent binding to ssDNA intermediates. These interactions are dependent on two clusters of C2H2 zinc finger motifs within ZNF827. We find that ZNF827 accumulates at stalled forks and DNA damage sites, where it activates ATR and promotes the engagement of homologous recombination-mediated DNA repair. Additionally, we demonstrate that ZNF827 depletion inhibits replication initiation and sensitizes cancer cells to the topoisomerase inhibitor topotecan, revealing ZNF827 as a therapeutic target within the DNA damage response pathway., (© 2024. The Author(s).)

Published

2024

38. Harmonin homology domain-mediated interaction of RTEL1 helicase with RPA and DNA provides insights into its recruitment to DNA repair sites.

Author

Kumar N, Taneja A, Ghosh M, Rothweiler U, Sundaresan NR, and Singh M

Subjects

DNA genetics, DNA Repair, DNA Replication, Humans, Replication Protein A metabolism, Telomere metabolism, DNA Helicases chemistry, DNA Helicases metabolism

Abstract

The regulator of telomere elongation helicase 1 (RTEL1) plays roles in telomere DNA maintenance, DNA repair, and genome stability by dismantling D-loops and unwinding G-quadruplex structures. RTEL1 comprises a helicase domain, two tandem harmonin homology domains 1&2 (HHD1 and HHD2), and a Zn2+-binding RING domain. In vitro D-loop disassembly by RTEL1 is enhanced in the presence of replication protein A (RPA). However, the mechanism of RTEL1 recruitment at non-telomeric D-loops remains unknown. In this study, we have unravelled a direct physical interaction between RTEL1 and RPA. Under DNA damage conditions, we showed that RTEL1 and RPA colocalise in the cell. Coimmunoprecipitation showed that RTEL1 and RPA interact, and the deletion of HHDs of RTEL1 significantly reduced this interaction. NMR chemical shift perturbations (CSPs) showed that RPA uses its 32C domain to interact with the HHD2 of RTEL1. Interestingly, HHD2 also interacted with DNA in the in vitro experiments. HHD2 structure was determined using X-ray crystallography, and NMR CSPs mapping revealed that both RPA 32C and DNA competitively bind to HHD2 on an overlapping surface. These results establish novel roles of accessory HHDs in RTEL1's functions and provide mechanistic insights into the RPA-mediated recruitment of RTEL1 to DNA repair sites., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

39. The chromatin-associated lncREST ensures effective replication stress response by promoting the assembly of fork signaling factors.

Author

Statello L, Fernandez-Justel JM, González J, Montes M, Ranieri A, Goñi E, Mas AM, and Huarte M

Subjects

DNA Replication genetics, Replication Protein A metabolism, S Phase genetics, DNA Damage, Chromatin genetics, RNA, Long Noncoding genetics

Abstract

Besides the well-characterized protein network involved in the replication stress response, several regulatory RNAs have been shown to play a role in this critical process. However, it has remained elusive whether they act locally at the stressed forks. Here, by investigating the RNAs localizing on chromatin upon replication stress induced by hydroxyurea, we identified a set of lncRNAs upregulated in S-phase and controlled by stress transcription factors. Among them, we demonstrate that the previously uncharacterized lncRNA lncREST (long non-coding RNA REplication STress) is transcriptionally controlled by p53 and localizes at stressed replication forks. LncREST-depleted cells experience sustained replication fork progression and accumulate un-signaled DNA damage. Under replication stress, lncREST interacts with the protein NCL and assists in engaging its interaction with RPA. The loss of lncREST is associated with a reduced NCL-RPA interaction and decreased RPA on chromatin, leading to defective replication stress signaling and accumulation of mitotic defects, resulting in apoptosis and a reduction in tumorigenic potential of cancer cells. These findings uncover the function of a lncRNA in favoring the recruitment of replication proteins to sites of DNA replication., (© 2024. The Author(s).)

Published

2024

40. The Intriguing Mystery of RPA Phosphorylation in DNA Double-Strand Break Repair.

Author

Fousek-Schuller VJ and Borgstahl GEO

Subjects

Humans, DNA, Single-Stranded, Phosphorylation, DNA metabolism, DNA Breaks, Double-Stranded, DNA Repair genetics, Replication Protein A metabolism

Abstract

Human Replication Protein A (RPA) was historically discovered as one of the six components needed to reconstitute simian virus 40 DNA replication from purified components. RPA is now known to be involved in all DNA metabolism pathways that involve single-stranded DNA (ssDNA). Heterotrimeric RPA comprises several domains connected by flexible linkers and is heavily regulated by post-translational modifications (PTMs). The structure of RPA has been challenging to obtain. Various structural methods have been applied, but a complete understanding of RPA's flexible structure, its function, and how it is regulated by PTMs has yet to be obtained. This review will summarize recent literature concerning how RPA is phosphorylated in the cell cycle, the structural analysis of RPA, DNA and protein interactions involving RPA, and how PTMs regulate RPA activity and complex formation in double-strand break repair. There are many holes in our understanding of this research area. We will conclude with perspectives for future research on how RPA PTMs control double-strand break repair in the cell cycle.

Published

2024

41. RPA guides UNG to uracil in ssDNA to facilitate antibody class switching and repair of mutagenic uracil at the replication fork.

Author

Hayran AB, Liabakk NB, Aas PA, Kusnierczyk A, Vågbø CB, Sarno A, Iveland TS, Chawla K, Zahn A, Di Noia JM, Slupphaug G, and Kavli B

Subjects

Cytidine Deaminase genetics, Cytidine Deaminase metabolism, DNA Repair genetics, DNA, Single-Stranded genetics, Immunoglobulin Class Switching genetics, Immunoglobulin Isotypes genetics, Immunoglobulins genetics, Mutagens, Uracil metabolism, Humans, Animals, Mice, Replication Protein A genetics, Replication Protein A metabolism, Uracil-DNA Glycosidase genetics, Uracil-DNA Glycosidase metabolism

Abstract

Activation-induced cytidine deaminase (AID) interacts with replication protein A (RPA), the major ssDNA-binding protein, to promote deamination of cytosine to uracil in transcribed immunoglobulin (Ig) genes. Uracil-DNA glycosylase (UNG) acts in concert with AID during Ig diversification. In addition, UNG preserves genome integrity by base-excision repair (BER) in the overall genome. How UNG is regulated to support both mutagenic processing and error-free repair remains unknown. UNG is expressed as two isoforms, UNG1 and UNG2, which both contain an RPA-binding helix that facilitates uracil excision from RPA-coated ssDNA. However, the impact of this interaction in antibody diversification and genome maintenance has not been investigated. Here, we generated B-cell clones with targeted mutations in the UNG RPA-binding motif, and analysed class switch recombination (CSR), mutation frequency (5' Ig Sμ), and genomic uracil in clones representing seven Ung genotypes. We show that the UNG:RPA interaction plays a crucial role in both CSR and repair of AID-induced uracil at the Ig loci. By contrast, the interaction had no significant impact on total genomic uracil levels. Thus, RPA coordinates UNG during CSR and pre-replicative repair of mutagenic uracil in ssDNA but is not essential in post-replicative and canonical BER of uracil in dsDNA., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2024

42. Direct, ensemble FRET approaches to monitor transient state kinetics of human DNA polymerase δ holoenzyme assembly and initiation of DNA synthesis.

Author

Norris JL and Hedglin M

Subjects

Humans, Kinetics, Holoenzymes metabolism, Holoenzymes chemistry, Replication Protein A metabolism, Replication Protein A chemistry, Replication Protein C metabolism, Replication Protein C genetics, Replication Protein C chemistry, Fluorescence Resonance Energy Transfer methods, DNA Polymerase III metabolism, DNA Polymerase III chemistry, Proliferating Cell Nuclear Antigen metabolism, Proliferating Cell Nuclear Antigen chemistry, Proliferating Cell Nuclear Antigen genetics, DNA Replication, DNA metabolism, DNA chemistry

Abstract

In humans, DNA polymerase δ (pol δ) holoenzymes, comprised of pol δ and the processivity sliding clamp, proliferating cell nuclear antigen (PCNA), carry out DNA synthesis during lagging strand replication, the initiation of leading strand DNA replication as well as most of the major DNA damage repair pathways. In each of these contexts, pol δ holoenzymes are assembled at primer/template (P/T) junctions and initiate DNA synthesis in a stepwise process that involves the PCNA clamp loader, replication factor C and, depending on the DNA synthesis pathway, the major single strand DNA-binding protein complex, replication protein A (RPA). In a recent report from our laboratory, we designed and utilized direct, ensemble Förster Resonance Energy Transfer approaches to monitor the transient state kinetics of pol δ holoenzyme assembly and initiation of DNA synthesis on P/T junctions engaged by RPA. In this chapter, we detail the original approaches and discuss adaptations that can be utilized to monitor fast kinetic reactions in the millisecond (ms) timescale. All approaches described in this chapter utilize a commercially-available fluorescence spectrophotometer, can be readily evolved for alternative DNA polymerases and P/T DNA substrates, and permit incorporation of protein posttranslational modifications, accessory factors, DNA covalent modifications, accessory factors, enzymes, etc. Hence, these approaches are widely accessible and broadly applicable for characterizing DNA polymerase holoenzyme assembly and initiation of DNA synthesis during any PCNA-dependent DNA synthesis pathway., (Copyright © 2024. Published by Elsevier Inc.)

Published

2024

43. Human RAD52 stimulates the RAD51-mediated homology search.

Author

Muhammad AA, Basto C, Peterlini T, Guirouilh-Barbat J, Thomas M, Veaute X, Busso D, Lopez B, Mazon G, Le Cam E, Masson JY, and Dupaigne P

Subjects

Humans, DNA, Single-Stranded genetics, DNA Repair genetics, Homologous Recombination genetics, Rad52 DNA Repair and Recombination Protein genetics, Rad52 DNA Repair and Recombination Protein metabolism, Replication Protein A genetics, Replication Protein A metabolism, Rad51 Recombinase genetics

Abstract

Homologous recombination (HR) is a DNA repair mechanism of double-strand breaks and blocked replication forks, involving a process of homology search leading to the formation of synaptic intermediates that are regulated to ensure genome integrity. RAD51 recombinase plays a central role in this mechanism, supported by its RAD52 and BRCA2 partners. If the mediator function of BRCA2 to load RAD51 on RPA-ssDNA is well established, the role of RAD52 in HR is still far from understood. We used transmission electron microscopy combined with biochemistry to characterize the sequential participation of RPA, RAD52, and BRCA2 in the assembly of the RAD51 filament and its activity. Although our results confirm that RAD52 lacks a mediator activity, RAD52 can tightly bind to RPA-coated ssDNA, inhibit the mediator activity of BRCA2, and form shorter RAD51-RAD52 mixed filaments that are more efficient in the formation of synaptic complexes and D-loops, resulting in more frequent multi-invasions as well. We confirm the in situ interaction between RAD51 and RAD52 after double-strand break induction in vivo. This study provides new molecular insights into the formation and regulation of presynaptic and synaptic intermediates by BRCA2 and RAD52 during human HR., (© 2023 Muhammad et al.)

Published

2023

44. Characterization of meiotic recombination intermediates through gene knockouts in founder hybrid mice.

Author

Davies B, Zhang G, Moralli D, Alghadban S, Biggs D, Preece C, Donnelly P, and Hinch AG

Subjects

Animals, Mice, DNA Breaks, Double-Stranded, Phosphate-Binding Proteins genetics, Phosphate-Binding Proteins metabolism, Replication Protein A metabolism, Replication Protein A genetics, Recombination, Genetic, Male, CRISPR-Cas Systems, Gene Knockout Techniques, Female, Homologous Recombination, Meiosis genetics, Rad51 Recombinase genetics, Rad51 Recombinase metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Cell Cycle Proteins genetics, Cell Cycle Proteins metabolism, Mice, Knockout

Abstract

Mammalian meiotic recombination proceeds via repair of hundreds of programmed DNA double-strand breaks, which requires choreographed binding of RPA, DMC1, and RAD51 to single-stranded DNA substrates. High-resolution in vivo binding maps of these proteins provide insights into the underlying molecular mechanisms. When assayed in F 1 -hybrid mice, these maps can distinguish the broken chromosome from the chromosome used as template for repair, revealing more mechanistic detail and enabling the structure of the recombination intermediates to be inferred. By applying CRISPR-Cas9 mutagenesis directly on F 1 -hybrid embryos, we have extended this approach to explore the molecular detail of recombination when a key component is knocked out. As a proof of concept, we have generated hybrid biallelic knockouts of Dmc1 and built maps of meiotic binding of RAD51 and RPA in them. DMC1 is essential for meiotic recombination, and comparison of these maps with those from wild-type mice is informative about the structure and timing of critical recombination intermediates. We observe redistribution of RAD51 binding and complete abrogation of D-loop recombination intermediates at a molecular level in Dmc1 mutants. These data provide insight on the configuration of RPA in D-loop intermediates and suggest that stable strand exchange proceeds via multiple rounds of strand invasion with template switching in mouse. Our methodology provides a high-throughput approach for characterization of gene function in meiotic recombination at low animal cost., (© 2023 Davies et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2023

45. Upregulated RPA2 in endometrial tissues of repeated implantation failure patients impairs the endometrial decidualization.

Author

Zhao H, Lv N, Cong J, Chen G, Bao H, and Liu X

Subjects

Humans, Female, Fertility, Biomarkers metabolism, Immunohistochemistry, Stromal Cells metabolism, Embryo Implantation genetics, Replication Protein A metabolism, Decidua metabolism, Endometrium metabolism

Abstract

Purpose: To investigate the expression and underlying mechanism of RPA2 in endometrium of patients with repeated implantation failure (RIF)., Methods: In this study, we retrieved the expression profiles from GEO databases and filtered the differentially expressed genes between RIF and the fertile control group. Ultimately, RPA2 was confirmed as a target gene. RPA2 expression in endometrial tissues of RIF patients, the control group, and different phases was detected by RT-qPCR, immunohistochemistry, and Western blotting. The role of RPA2 in endometrial decidualization was performed by in vitro decidualization inducing by 8-Br-cAMP and MPA. Furthermore, RT-qPCR was used to detect changes in the decidual biomarkers after transfection of RPA2 overexpression vector in human endometrium stromal cell (HESC)., Results: RPA2 was significantly upregulated in the mid-secretory endometrium of patients with RIF. As a proliferation-related gene, RPA2 was obviously higher expressed at proliferative phase during the normal menstrual cycles. Moreover, the downregulation of RPA2 was discovered during decidualization of HESC. Furthermore, RPA2 overexpression impaired decidualization by inhibiting the expression of prolactin (PRL) and insulin-like growth factor-binding protein 1 (IGFBP1)., Conclusions: Our finding indicated that aberrant upregulation of RPA2 attenuated decidualization of HESC in RIF women and provided new potential therapeutic targets., (© 2023. The Author(s), under exclusive licence to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

46. Distinct RPA functions promote eukaryotic DNA replication initiation and elongation.

Author

Pike AM, Friend CM, and Bell SP

Subjects

DNA, Single-Stranded genetics, DNA, Single-Stranded metabolism, Protein Binding, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Bacteriophage T4 metabolism, DNA Replication, DNA-Binding Proteins metabolism, Replication Protein A genetics, Replication Protein A metabolism

Abstract

Replication protein A (RPA) binds single-stranded DNA (ssDNA) and serves critical functions in eukaryotic DNA replication, the DNA damage response, and DNA repair. During DNA replication, RPA is required for extended origin DNA unwinding and DNA synthesis. To determine the requirements for RPA during these processes, we tested ssDNA-binding proteins (SSBs) from different domains of life in reconstituted Saccharomyces cerevisiae origin unwinding and DNA replication reactions. Interestingly, Escherichia coli SSB, but not T4 bacteriophage Gp32, fully substitutes for RPA in promoting origin DNA unwinding. Using RPA mutants, we demonstrated that specific ssDNA-binding properties of RPA are required for origin unwinding but that its protein-interaction domains are dispensable. In contrast, we found that each of these auxiliary RPA domains have distinct functions at the eukaryotic replication fork. The Rfa1 OB-F domain negatively regulates lagging-strand synthesis, while the Rfa2 winged-helix domain stimulates nascent strand initiation. Together, our findings reveal a requirement for specific modes of ssDNA binding in the transition to extensive origin DNA unwinding and identify RPA domains that differentially impact replication fork function., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023

47. Antagonistic roles of canonical and Alternative-RPA in disease-associated tandem CAG repeat instability.

Author

Gall-Duncan T, Luo J, Jurkovic CM, Fischer LA, Fujita K, Deshmukh AL, Harding RJ, Tran S, Mehkary M, Li V, Leib DE, Chen R, Tanaka H, Mason AG, Lévesque D, Khan M, Razzaghi M, Prasolava T, Lanni S, Sato N, Caron MC, Panigrahi GB, Wang P, Lau R, Castel AL, Masson JY, Tippett L, Turner C, Spies M, La Spada AR, Campos EI, Curtis MA, Boisvert FM, Faull RLM, Davidson BL, Nakamori M, Okazawa H, Wold MS, and Pearson CE

Subjects

Animals, Humans, Mice, DNA genetics, DNA Mismatch Repair, Huntington Disease genetics, Proteins genetics, Spinocerebellar Ataxias genetics, Trinucleotide Repeat Expansion, Replication Protein A metabolism

Abstract

Expansions of repeat DNA tracts cause >70 diseases, and ongoing expansions in brains exacerbate disease. During expansion mutations, single-stranded DNAs (ssDNAs) form slipped-DNAs. We find the ssDNA-binding complexes canonical replication protein A (RPA1, RPA2, and RPA3) and Alternative-RPA (RPA1, RPA3, and primate-specific RPA4) are upregulated in Huntington disease and spinocerebellar ataxia type 1 (SCA1) patient brains. Protein interactomes of RPA and Alt-RPA reveal unique and shared partners, including modifiers of CAG instability and disease presentation. RPA enhances in vitro melting, FAN1 excision, and repair of slipped-CAGs and protects against CAG expansions in human cells. RPA overexpression in SCA1 mouse brains ablates expansions, coincident with decreased ATXN1 aggregation, reduced brain DNA damage, improved neuron morphology, and rescued motor phenotypes. In contrast, Alt-RPA inhibits melting, FAN1 excision, and repair of slipped-CAGs and promotes CAG expansions. These findings suggest a functional interplay between the two RPAs where Alt-RPA may antagonistically offset RPA's suppression of disease-associated repeat expansions, which may extend to other DNA processes., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023

48. Chemical Inhibition of RPA by HAMNO Alters Cell Cycle Dynamics by Impeding DNA Replication and G2-to-M Transition but Has Little Effect on the Radiation-Induced DNA Damage Response.

Author

Dueva R, Krieger LM, Li F, Luo D, Xiao H, Stuschke M, Metzen E, and Iliakis G

Subjects

Humans, Cell Cycle genetics, DNA-Binding Proteins metabolism, DNA Replication, DNA Repair, DNA Damage, DNA, Mitosis, DNA, Single-Stranded, Replication Protein A metabolism, Neoplasms

Abstract

Replication protein A (RPA) is the major single-stranded DNA (ssDNA) binding protein that is essential for DNA replication and processing of DNA double-strand breaks (DSBs) by homology-directed repair pathways. Recently, small molecule inhibitors have been developed targeting the RPA70 subunit and preventing RPA interactions with ssDNA and various DNA repair proteins. The rationale of this development is the potential utility of such compounds as cancer therapeutics, owing to their ability to inhibit DNA replication that sustains tumor growth. Among these compounds, (1Z)-1-[(2-hydroxyanilino) methylidene] naphthalen-2-one (HAMNO) has been more extensively studied and its efficacy against tumor growth was shown to arise from the associated DNA replication stress. Here, we study the effects of HAMNO on cells exposed to ionizing radiation (IR), focusing on the effects on the DNA damage response and the processing of DSBs and explore its potential as a radiosensitizer. We show that HAMNO by itself slows down the progression of cells through the cell cycle by dramatically decreasing DNA synthesis. Notably, HAMNO also attenuates the progression of G2-phase cells into mitosis by a mechanism that remains to be elucidated. Furthermore, HAMNO increases the fraction of chromatin-bound RPA in S-phase but not in G2-phase cells and suppresses DSB repair by homologous recombination. Despite these marked effects on the cell cycle and the DNA damage response, radiosensitization could neither be detected in exponentially growing cultures, nor in cultures enriched in G2-phase cells. Our results complement existing data on RPA inhibitors, specifically HAMNO, and suggest that their antitumor activity by replication stress induction may not extend to radiosensitization. However, it may render cells more vulnerable to other forms of DNA damaging agents through synthetically lethal interactions, which requires further investigation.

Published

2023

49. Pot1b -/- tumors activate G-quadruplex-induced DNA damage to promote telomere hyper-elongation.

Author

Takasugi T, Gu P, Liang F, Staco I, and Chang S

Subjects

Mice, Humans, Animals, Telomere-Binding Proteins genetics, Telomere-Binding Proteins metabolism, Telomere genetics, Telomere metabolism, DNA Damage, Replication Protein A metabolism, DNA-Binding Proteins genetics, Shelterin Complex, Sarcoma

Abstract

Malignant cancers must activate telomere maintenance mechanisms to achieve replicative immortality. Mutations in the human Protection of Telomeres 1 (POT1) gene are frequently detected in cancers with abnormally long telomeres, suggesting that the loss of POT1 function disrupts the regulation of telomere length homeostasis to promote telomere elongation. However, our understanding of the mechanisms leading to elongated telomeres remains incomplete. The mouse genome encodes two POT1 proteins, POT1a and POT1b possessing separation of hPOT1 functions. We performed serial transplantation of Pot1b-/- sarcomas to better understand the role of POT1b in regulating telomere length maintenance. While early-generation Pot1b-/- sarcomas initially possessed shortened telomeres, late-generation Pot1b-/- cells display markedly hyper-elongated telomeres that were recognized as damaged DNA by the Replication Protein A (RPA) complex. The RPA-ATR-dependent DNA damage response at telomeres promotes telomerase recruitment to facilitate telomere hyper-elongation. POT1b, but not POT1a, was able to unfold G-quadruplex present in hyper-elongated telomeres to repress the DNA damage response. Our findings demonstrate that the repression of the RPA-ATR DDR is conserved between POT1b and human POT1, suggesting that similar mechanisms may underly the phenotypes observed in human cancers harboring human POT1 mutations., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023

50. Alteration of replication protein A binding mode on single-stranded DNA by NSMF potentiates RPA phosphorylation by ATR kinase.

Author

Kang Y, Han YG, Khim KW, Choi WG, Ju MK, Park K, Shin KJ, Chae YC, Choi JH, Kim H, and Lee JY

Subjects

Ataxia Telangiectasia Mutated Proteins metabolism, Checkpoint Kinase 1 metabolism, DNA Damage, DNA Replication, DNA, Single-Stranded, DNA-Binding Proteins genetics, Phosphorylation, Protein Binding, Protein Kinases genetics, Humans, Protein Serine-Threonine Kinases metabolism, Replication Protein A metabolism

Abstract

Replication protein A (RPA), a eukaryotic single-stranded DNA (ssDNA) binding protein, dynamically interacts with ssDNA in different binding modes and plays essential roles in DNA metabolism such as replication, repair, and recombination. RPA accumulation on ssDNA due to replication stress triggers the DNA damage response (DDR) by activating the ataxia telangiectasia and RAD3-related (ATR) kinase, which phosphorylates itself and downstream DDR factors, including RPA. We recently reported that the N-methyl-D-aspartate receptor synaptonuclear signaling and neuronal migration factor (NSMF), a neuronal protein associated with Kallmann syndrome, promotes RPA32 phosphorylation via ATR upon replication stress. However, how NSMF enhances ATR-mediated RPA32 phosphorylation remains elusive. Here, we demonstrate that NSMF colocalizes and physically interacts with RPA at DNA damage sites in vivo and in vitro. Using purified RPA and NSMF in biochemical and single-molecule assays, we find that NSMF selectively displaces RPA in the more weakly bound 8- and 20-nucleotide binding modes from ssDNA, allowing the retention of more stable RPA molecules in the 30-nt binding mode. The 30-nt binding mode of RPA enhances RPA32 phosphorylation by ATR, and phosphorylated RPA becomes stabilized on ssDNA. Our findings provide new mechanistic insight into how NSMF facilitates the role of RPA in the ATR pathway., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023