Your search keyword '"Felicia Scheffel"' showing total 3 results

1. SV40 T antigen helicase domain regions responsible for oligomerisation regulate Okazaki fragment synthesis initiation

Author

Nichodemus O. Onwubiko, Felicia Scheffel, Ingrid Tessmer, and Heinz Peter Nasheuer

Subjects

DNA polymerase α‐primase (Pol α), eukaryotic DNA replication, initiation reaction, Okazaki fragment synthesis, replication protein A (RPA), SV40 large T antigen, Biology (General), QH301-705.5

Abstract

The initiation of Okazaki fragment synthesis during cellular DNA replication is a crucial step for lagging strand synthesis, which is carried out by the primase function of DNA polymerase α‐primase (Pol‐prim). Since cellular replication protein A (RPA) prevents primase from starting RNA synthesis on single‐stranded DNA (ssDNA), primase requires auxiliary factors, such as the simian virus 40 (SV40) T antigen (Tag), for the initiation reaction on RPA‐bound ssDNA. Here, we investigated the ability of Tag variants and Tag protein complexes to bind to ssDNA and their resulting effects on the stimulation of Pol‐prim on free and RPA‐bound ssDNA. Atomic force microscopy imaging showed that while Tag131‐627(V350E/P417D) and Tag131‐627(L286D/R567E) (abbreviated as M1 and M2, respectively) could bind to ssDNA as monomers, these monomeric Tags could come together and bind to ssDNA as dimers as well. In a model assay for the initiation of Okazaki fragment synthesis, full‐length Tag SV40 Tag1‐708 and monomeric M2 stimulated DNA synthesis of Pol‐prim on ssDNA and on RPA‐bound ssDNA. In contrast, neither monomeric M1 nor M1‐M2 dimers could stimulate Pol‐prim, on ssDNA or on RPA‐bound ssDNA. Overall, we show that a lack of stimulatory activity of monomeric M1 and M1‐M2 dimers suggests that residues V350 and P417 are not only important for interactions between Tag molecules but also for protein–protein interactions within Okazaki fragment initiation complexes. Thus, we highlight that mutations in M1 are dominant negative with regard to Okazaki fragment initiation.

Published

2022

2. SV40 T antigen interactions with ssDNA and replication protein A: a regulatory role of T antigen monomers in lagging strand DNA replication

Author

Angela Borst, Felicia Scheffel, Nichodemus O. Onwubiko, Suraya A. Diaz, Heinz-Peter Nasheuer, Katharina Passkowski, and Ingrid Tessmer

Subjects

POLYMERASE ALPHA-PRIMASE, DNA Replication, DNA replication initiation, AcademicSubjects/SCI00010, Antigens, Polyomavirus Transforming, PRIMER SYNTHESIS, DNA, Single-Stranded, Eukaryotic DNA replication, DNA Primase, Simian virus 40, Genome Integrity, Repair and Replication, 03 medical and health sciences, chemistry.chemical_compound, Adenosine Triphosphate, Replication Protein A, SIMIAN-VIRUS-40 SPECIFIC PROTEINS, VIRAL ORIGIN, Genetics, LARGE TUMOR-ANTIGEN, ORIGIN-BINDING DOMAIN, HELICASE, Replication protein A, 030304 developmental biology, DIFFERENTIAL SCANNING FLUOROMETRY, 0303 health sciences, biology, Okazaki fragments, 030302 biochemistry & molecular biology, DNA replication, Helicase, DNA, DNA Polymerase I, chemistry, biology.protein, Biophysics, SPECIES-SPECIFIC REPLICATION, Primase, HUMAN RPA, Protein Binding

Abstract

DNA replication is a central process in all living organisms. Polyomavirus DNA replication serves as a model system for eukaryotic DNA replication and has considerably contributed to our understanding of basic replication mechanisms. However, the details of the involved processes are still unclear, in particular regarding lagging strand synthesis. To delineate the complex mechanism of coordination of various cellular proteins binding simultaneously or consecutively to DNA to initiate replication, we investigated single-stranded DNA (ssDNA) interactions by the SV40 large T antigen (Tag). Using single molecule imaging by atomic force microscopy (AFM) combined with biochemical and spectroscopic analyses we reveal independent activity of monomeric and oligomeric Tag in high affinity binding to ssDNA. Depending on ssDNA length, we obtain dissociation constants for Tag-ssDNA interactions (K-D values of 10-30 nM) that are in the same order of magnitude as ssDNA binding by human replication protein A (RPA). Furthermore, we observe the formation of RPA-Tag-ssDNA complexes containing hexameric as well as monomeric Tag forms. Importantly, our data clearly show stimulation of primase function in lagging strand Okazaki fragment synthesis by monomeric Tag whereas hexameric Tag inhibits the reaction, redefining DNA replication initiation on the lagging strand. Else Kröner-Fresenius-Stiftung (EKFS) [2013_A215]; PML Consortium (Washington, USA) [RIB1099] to H.P.N. Funding for open access charge: Funding by NUI Galway and University of Würzburg. peer-reviewed

Published

2020

3. SV40 T antigen helicase domain regions responsible for oligomerisation regulate Okazaki fragment synthesis initiation

Author

Nichodemus O. Onwubiko, Felicia Scheffel, Ingrid Tessmer, and Heinz Peter Nasheuer

Subjects

Okazaki fragment synthesis, SV40 large T antigen, Antigens, Viral, Tumor/genetics/metabolism, DNA, Simian virus 40, DNA/genetics, DNA polymerase ¿-primase (Pol ¿), General Biochemistry, Genetics and Molecular Biology, replication protein A (RPA), Replication Protein A/genetics/metabolism, Replication Protein A, Simian virus 40/genetics/metabolism, eukaryotic DNA replication, Antigens, Viral, Tumor, initiation reaction

Abstract

The initiation of Okazaki fragment synthesis during cellular DNA replication is a crucial step for lagging strand synthesis, which is carried out by the primase function of DNA polymerase ¿-primase (Pol-prim). Since cellular replication protein A (RPA) prevents primase from starting RNA synthesis on single-stranded DNA (ssDNA), primase requires auxiliary factors, such as the simian virus 40 (SV40) T antigen (Tag), for the initiation reaction on RPA-bound ssDNA. Here, we investigated the ability of Tag variants and Tag protein complexes to bind to ssDNA and their resulting effects on the stimulation of Pol-prim on free and RPA-bound ssDNA. Atomic force microscopy imaging showed that while Tag(131-627) (V350E/P417D) and Tag(131-627) (L286D/R567E) (abbreviated as M1 and M2, respectively) could bind to ssDNA as monomers, these monomeric Tags could come together and bind to ssDNA as dimers as well. In a model assay for the initiation of Okazaki fragment synthesis, full-length Tag SV40 Tag(1-708) and monomeric M2 stimulated DNA synthesis of Pol-prim on ssDNA and on RPA-bound ssDNA. In contrast, neither monomeric M1 nor M1-M2 dimers could stimulate Pol-prim, on ssDNA or on RPA-bound ssDNA. Overall, we show that a lack of stimulatory activity of monomeric M1 and M1-M2 dimers suggests that residues V350 and P417 are not only important for interactions between Tag molecules but also for protein-protein interactions within Okazaki fragment initiation complexes. Thus, we highlight that mutations in M1 are dominant negative with regard to Okazaki fragment initiation. This work was supported by funding from the Deutsche Forschungsgemeinschaft (DFG, grant TE-671/4-2 to IT) and from the Else Kröner-Fresenius-Stiftung (EKFS 2013_A215) and the PML Consortium (Washington, USA; RIB1099) to HPN. The authors thank Patricia Nyland for expert technical assistance and Dr Lars Schönemann (Recombinant Protein Expression Facility, University of Würzburg) for his expert purification of wild type and mutant Tag131-627. We acknowledge Angela Borst for her contributions to AFM data collection and analyses, and Maciej Doczyk (NUI Galway) for his graphical work. We would also like to acknowledge the FP7 WeNMR (project# 261572), H2020 West-Life (project# 675858), the EOSC-hub (project #777536) and the EGI-ACE (project# 101017567) European e-Infrastructure projects for the use of their web portals, which make use of the EGI infrastructure with the dedicated support of CESNET-MCC, INFN-PADOVA-STACK, INFN-LNL-2, NCG-INGRID-PT, TW-NCHC, CESGA, IFCA-LCG2, UA-BITP, SURFsara and NIKHEF, and the additional support of the national GRID Initiatives of Belgium, France, Italy, Germany, the Netherlands, Poland, Portugal, Spain, UK, Taiwan and the US Open Science Grid. peer-reviewed

Published

2021