Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork

Double-strand break (DSB) repair is associated with a 1000-fold increase in mutations compared to normal replication of the same sequences. In budding yeast, repair of an HO endonuclease-induced DSB at the MATα locus can be repaired by using a homologous, heterochromatic HMR::Kl-URA3 donor harboring...

Descripción completa

Detalles Bibliográficos
Autores principales: Dalin, Simona, Webster, Sophie, Sugawara, Neal, Zhang, Shu, Wu, Qiuqin, Cui, Tracy, Liang, Victoria, Beroukhim, Rameen, Haber, James E.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Cold Spring Harbor Laboratory 2023
Materias:
Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10592705/
https://www.ncbi.nlm.nih.gov/pubmed/37873277
http://dx.doi.org/10.1101/2023.10.09.561461
_version_ 1785124331171348480
author Dalin, Simona
Webster, Sophie
Sugawara, Neal
Zhang, Shu
Wu, Qiuqin
Cui, Tracy
Liang, Victoria
Beroukhim, Rameen
Haber, James E.
author_facet Dalin, Simona
Webster, Sophie
Sugawara, Neal
Zhang, Shu
Wu, Qiuqin
Cui, Tracy
Liang, Victoria
Beroukhim, Rameen
Haber, James E.
author_sort Dalin, Simona
collection PubMed
description Double-strand break (DSB) repair is associated with a 1000-fold increase in mutations compared to normal replication of the same sequences. In budding yeast, repair of an HO endonuclease-induced DSB at the MATα locus can be repaired by using a homologous, heterochromatic HMR::Kl-URA3 donor harboring a transcriptionally silenced URA3 gene, resulting in a MAT::URA3 (Ura(+)) repair product where URA3 is expressed. Repair-associated ura3− mutations can be selected by resistance to 5-fluoroorotic acid (FOA). Using this system, we find that a major class of mutations are −1 deletions, almost always in homonucleotide runs, but there are few +1 insertions. In contrast, +1 and −1 insertions in homonucleotide runs are nearly equal among spontaneous mutations. Approximately 10% of repair-associated mutations are interchromosomal template switches (ICTS), even though the K. lactis URA3 sequence embedded in HMR is only 72% identical with S. cerevisiae ura3-52 sequences on a different chromosome. ICTS events begin and end in regions of short microhomology, averaging 7 bp. Long microhomologies are favored, but some ICTS junctions are as short as 2 bp. Both repair-associated intragenic deletions (IDs) and tandem duplications (TDs) are recovered, with junctions sharing short stretches of, on average, 6 bp of microhomology. Intragenic deletions are more than 5 times more frequent than TDs. IDs have a mean length of 60 bp, but, surprisingly there are almost no deletions shorter than 25 bp. In contrast, TDs average only 12 bp. The usage of microhomologies among intragenic deletions is not strongly influenced by the degree of adjacent homeology. Together, these data provide a picture of the structure of the repair replication fork. We suggest that IDs and TDs occur within the migrating D-loop in which DNA polymerase δ copies the template, where the 3’ end of a partly copied new DNA strand can dissociate and anneal with a single-stranded region of microhomology that lies either in front or behind the 3’ end, within the open structure of a migrating D-loop. Our data suggest that ~100 bp ahead of the polymerase is “open,” but that part of the repair replication apparatus remains bound in the 25 bp ahead of the newly copied DNA, preventing annealing. In contrast, the template region behind the polymerase appears to be rapidly reannealed, limiting template switching to a very short region.
format Online
Article
Text
id pubmed-10592705
institution National Center for Biotechnology Information
language English
publishDate 2023
publisher Cold Spring Harbor Laboratory
record_format MEDLINE/PubMed
spelling pubmed-105927052023-10-24 Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork Dalin, Simona Webster, Sophie Sugawara, Neal Zhang, Shu Wu, Qiuqin Cui, Tracy Liang, Victoria Beroukhim, Rameen Haber, James E. bioRxiv Article Double-strand break (DSB) repair is associated with a 1000-fold increase in mutations compared to normal replication of the same sequences. In budding yeast, repair of an HO endonuclease-induced DSB at the MATα locus can be repaired by using a homologous, heterochromatic HMR::Kl-URA3 donor harboring a transcriptionally silenced URA3 gene, resulting in a MAT::URA3 (Ura(+)) repair product where URA3 is expressed. Repair-associated ura3− mutations can be selected by resistance to 5-fluoroorotic acid (FOA). Using this system, we find that a major class of mutations are −1 deletions, almost always in homonucleotide runs, but there are few +1 insertions. In contrast, +1 and −1 insertions in homonucleotide runs are nearly equal among spontaneous mutations. Approximately 10% of repair-associated mutations are interchromosomal template switches (ICTS), even though the K. lactis URA3 sequence embedded in HMR is only 72% identical with S. cerevisiae ura3-52 sequences on a different chromosome. ICTS events begin and end in regions of short microhomology, averaging 7 bp. Long microhomologies are favored, but some ICTS junctions are as short as 2 bp. Both repair-associated intragenic deletions (IDs) and tandem duplications (TDs) are recovered, with junctions sharing short stretches of, on average, 6 bp of microhomology. Intragenic deletions are more than 5 times more frequent than TDs. IDs have a mean length of 60 bp, but, surprisingly there are almost no deletions shorter than 25 bp. In contrast, TDs average only 12 bp. The usage of microhomologies among intragenic deletions is not strongly influenced by the degree of adjacent homeology. Together, these data provide a picture of the structure of the repair replication fork. We suggest that IDs and TDs occur within the migrating D-loop in which DNA polymerase δ copies the template, where the 3’ end of a partly copied new DNA strand can dissociate and anneal with a single-stranded region of microhomology that lies either in front or behind the 3’ end, within the open structure of a migrating D-loop. Our data suggest that ~100 bp ahead of the polymerase is “open,” but that part of the repair replication apparatus remains bound in the 25 bp ahead of the newly copied DNA, preventing annealing. In contrast, the template region behind the polymerase appears to be rapidly reannealed, limiting template switching to a very short region. Cold Spring Harbor Laboratory 2023-10-13 /pmc/articles/PMC10592705/ /pubmed/37873277 http://dx.doi.org/10.1101/2023.10.09.561461 Text en https://creativecommons.org/licenses/by-nc-nd/4.0/This work is licensed under a Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License (https://creativecommons.org/licenses/by-nc-nd/4.0/) , which allows reusers to copy and distribute the material in any medium or format in unadapted form only, for noncommercial purposes only, and only so long as attribution is given to the creator.
spellingShingle Article
Dalin, Simona
Webster, Sophie
Sugawara, Neal
Zhang, Shu
Wu, Qiuqin
Cui, Tracy
Liang, Victoria
Beroukhim, Rameen
Haber, James E.
Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
title Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
title_full Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
title_fullStr Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
title_full_unstemmed Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
title_short Double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
title_sort double-strand break repair-associated intragenic deletions and tandem duplications suggest the architecture of the repair replication fork
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10592705/
https://www.ncbi.nlm.nih.gov/pubmed/37873277
http://dx.doi.org/10.1101/2023.10.09.561461
work_keys_str_mv AT dalinsimona doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT webstersophie doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT sugawaraneal doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT zhangshu doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT wuqiuqin doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT cuitracy doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT liangvictoria doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT beroukhimrameen doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork
AT haberjamese doublestrandbreakrepairassociatedintragenicdeletionsandtandemduplicationssuggestthearchitectureoftherepairreplicationfork

Ejemplares similares