Processing of Double-Strand Breaks Is Involved in the Precise Excision of Paramecium Internal Eliminated Sequences

ABSTRACT In ciliates, the development of the somatic macronucleus involves the programmed excision of thousands of internal eliminated sequences (IES) scattered throughout the germ line genome. Previous work with Tetrahymena thermophila has suggested that excision is initiated by a staggered double-strand break (DSB) at one IES end. Nucleophilic attack of the other end by the 3′OH group carried by the firstly broken chromosome end leads to macronuclear junction closure. In this study, we mapped the 3′OH and 5′PO4 groups that are developmentally released at Paramecium IES boundaries, which are marked by two conserved TA dinucleotides, one of which remains in the macronuclear genome after excision. We show that initiating DSBs at both ends generate 4-base 5′ overhangs centered on the TA. Based on the observed processing of the 5′-terminal residue of each overhang, we present a new model for the precise closure of macronuclear chromosomes in Paramecium tetraurelia, different from that previously proposed for Tetrahymena. In our model, macronucleus-destined broken ends are aligned through the partial pairing of their 5′-nTAn-3′ extensions and joined after trimming of the 5′ flaps.

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The Homologous Chromosome Is an Effective Template for the Repair of Mitotic DNA Double-Strand Breaks in Drosophila

Genetics ◽

10.1093/genetics/165.4.1831 ◽

2003 ◽

Vol 165 (4) ◽

pp. 1831-1842 ◽

Cited By ~ 12

Author(s):

Yikang S Rong ◽

Kent G Golic

Keyword(s):

Gene Conversion ◽

Mammalian Cells ◽

Homologous Chromosome ◽

Germ Line ◽

Strand Break ◽

Double Strand Breaks ◽

Dna Double Strand Breaks ◽

Yeast Saccharomyces Cerevisiae ◽

Strand Breaks ◽

Mitotic Cells

AbstractIn recombinational DNA double-strand break repair a homologous template for gene conversion may be located at several different genomic positions: on the homologous chromosome in diploid organisms, on the sister chromatid after DNA replication, or at an ectopic position. The use of the homologous chromosome in mitotic gene conversion is thought to be limited in the yeast Saccharomyces cerevisiae and mammalian cells. In contrast, by studying the repair of double-strand breaks generated by the I-SceI rare-cutting endonuclease, we find that the homologous chromosome is frequently used in Drosophila melanogaster, which we suggest is attributable to somatic pairing of homologous chromosomes in mitotic cells of Drosophila. We also find that Drosophila mitotic cells of the germ line, like yeast, employ the homologous recombinational repair pathway more often than imperfect nonhomologous end joining.

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I-SceI Endonuclease, a New Tool for Studying DNA Double-Strand Break Repair Mechanisms in Drosophila

Genetics ◽

10.1093/genetics/152.3.1037 ◽

1999 ◽

Vol 152 (3) ◽

pp. 1037-1044 ◽

Cited By ~ 1

Author(s):

Yohanns Bellaiche ◽

Vladic Mogila ◽

Norbert Perrimon

Keyword(s):

Germ Line ◽

Marker Gene ◽

Strand Break ◽

Double Strand Breaks ◽

Drosophila Genome ◽

Strand Breaks ◽

Recombination System ◽

Dna Double Strand Break ◽

Repair Mechanisms ◽

Specific Position

Abstract As a step toward the development of a homologous recombination system in Drosophila, we have developed a methodology to target double-strand breaks (DSBs) to a specific position in the Drosophila genome. This method uses the mitochondrial endonuclease I-SceI that recognizes and cuts an 18-bp restriction site. We find that >6% of the progeny derived from males that carry a marker gene bordered by two I-SceI sites and that express I-SceI in their germ line lose the marker gene. Southern blot analysis and sequencing of the regions surrounding the I-SceI sites revealed that in the majority of the cases, the introduction of DSBs at the I-SceI sites resulted in the complete deletion of the marker gene; the other events were associated with partial deletion of the marker gene. We discuss a number of applications for this novel technique, in particular its use to study DSB repair mechanisms.

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Transcription and Double-Strand Breaks Induce Similar Mitotic Recombination Events inSaccharomyces cerevisiae

Genetics ◽

10.1093/genetics/162.2.603 ◽

2002 ◽

Vol 162 (2) ◽

pp. 603-614 ◽

Cited By ~ 2

Author(s):

Sergio González-Barrera ◽

María García-Rubio ◽

Andrés Aguilera

Keyword(s):

Comparative Analysis ◽

Dna Sequence ◽

Recombination Event ◽

Strand Break ◽

Double Strand Breaks ◽

The Other ◽

Dna Breaks ◽

Strand Breaks ◽

Spontaneous Recombination ◽

Gene Conversions

AbstractWe have made a comparative analysis of double-strand-break (DSB)-induced recombination and spontaneous recombination under low- and high-transcription conditions in yeast. We constructed two different recombination substrates, one for the analysis of intermolecular gene conversions and the other for intramolecular gene conversions and inversions. Such substrates were based on the same leu2-HOr allele fused to the tet promoter and containing a 21-bp HO site. Gene conversions and inversions were differently affected by rad1, rad51, rad52, and rad59 single and double mutations, consistent with the actual view that such events occur by different recombination mechanisms. However, the effect of each mutation on each type of recombination event was the same, whether associated with transcription or induced by the HO-mediated DSB. Both the highly transcribed DNA and the HO-cut sequence acted as recipients of the gene conversion events. These results are consistent with the hypothesis that transcription promotes initiation of recombination along the DNA sequence being transcribed. The similarity between transcription-associated and DSB-induced recombination suggests that transcription promotes DNA breaks.

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Focused Genetic Recombination of Bacteriophage T4 Initiated by Double-Strand Breaks

Genetics ◽

10.1093/genetics/162.2.543 ◽

2002 ◽

Vol 162 (2) ◽

pp. 543-556

Author(s):

Victor Shcherbakov ◽

Igor Granovsky ◽

Lidiya Plugina ◽

Tamara Shcherbakova ◽

Svetlana Sizova ◽

...

Keyword(s):

Genetic Recombination ◽

Bacteriophage T4 ◽

Proximal Part ◽

Coupling Model ◽

Strand Break ◽

Double Strand Breaks ◽

Strand Breaks ◽

The Right ◽

Frequency Distance

Abstract A model system for studying double-strand-break (DSB)-induced genetic recombination in vivo based on the ets1 segCΔ strain of bacteriophage T4 was developed. The ets1, a 66-bp DNA fragment of phage T2L containing the cleavage site for the T4 SegC site-specific endonuclease, was inserted into the proximal part of the T4 rIIB gene. Under segC+ conditions, the ets1 behaves as a recombination hotspot. Crosses of the ets1 against rII markers located to the left and to the right of ets1 gave similar results, thus demonstrating the equal and symmetrical initiation of recombination by either part of the broken chromosome. Frequency/distance relationships were studied in a series of two- and three-factor crosses with other rIIB and rIIA mutants (all segC+) separated from ets1 by 12-2100 bp. The observed relationships were readily interpretable in terms of the modified splice/patch coupling model. The advantages of this localized or focused recombination over that distributed along the chromosome, as a model for studying the recombination-replication pathway in T4 in vivo, are discussed.

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End-resection at DNA double-strand breaks in the three domains of life

Biochemical Society Transactions ◽

10.1042/bst20120307 ◽

2013 ◽

Vol 41 (1) ◽

pp. 314-320 ◽

Cited By ~ 30

Author(s):

John K. Blackwood ◽

Neil J. Rzechorzek ◽

Sian M. Bray ◽

Joseph D. Maman ◽

Luca Pellegrini ◽

...

Keyword(s):

Dna Repair ◽

Homologous Recombination ◽

Strand Break ◽

Double Strand Breaks ◽

Dna Double Strand Breaks ◽

Strand Breaks ◽

Homologous Chromosomes ◽

Domains Of Life ◽

Strand Invasion ◽

End Resection

During DNA repair by HR (homologous recombination), the ends of a DNA DSB (double-strand break) must be resected to generate single-stranded tails, which are required for strand invasion and exchange with homologous chromosomes. This 5′–3′ end-resection of the DNA duplex is an essential process, conserved across all three domains of life: the bacteria, eukaryota and archaea. In the present review, we examine the numerous and redundant helicase and nuclease systems that function as the enzymatic analogues for this crucial process in the three major phylogenetic divisions.

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Homologous recombination and the repair of double-strand breaks during cotransformation of Dictyostelium discoideum

Molecular and Cellular Biology ◽

10.1128/mcb.8.7.2779-2786.1988 ◽

1988 ◽

Vol 8 (7) ◽

pp. 2779-2786

Author(s):

K S Katz ◽

D I Ratner

Keyword(s):

Homologous Recombination ◽

Dictyostelium Discoideum ◽

Strand Break ◽

Double Strand Breaks ◽

Restriction Endonucleases ◽

Linear Molecule ◽

Strand Breaks ◽

Transformation Vector ◽

Closed Circle ◽

Primary Vector

We examined the ability of unlinked nonreplicating plasmid molecules to undergo homologous recombination during cotransformation of Dictyostelium amoebae. The transformation vector B10S confers resistance to the antibiotic G418 and was always presented to amoebae as a closed circle. Cotransforming DNA, containing a slime mold cDNA and sequences homologous to the primary vector, was presented either as a closed circle or as a linear molecule after digestion with restriction endonucleases which cut within one of three distinct regions of the plasmid. Remarkably, homologous recombination occurred in every clone examined. Moreover, the products of recombination were identical in all instances, irrespective of the presence or position of linearized ends. The ends of the linear templates were not recombinogenic. Repair of the introduced double-strand break occurred frequently during recombination. The repair could occur intermolecularly or, more likely, intramolecularly, i.e., by recircularization. Many of the recombination events were of a nonreciprocal nature. Despite the startlingly frequent level of homologous recombination, the use of cotransforming DNA which contains no homology to the selected vector established that such recombination was not required for cotransformation.

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i-BLESS is an ultra-sensitive method for detection of DNA double-strand breaks

Communications Biology ◽

10.1038/s42003-018-0165-9 ◽

2018 ◽

Vol 1 (1) ◽

Cited By ~ 22

Author(s):

Anna Biernacka ◽

Yingjie Zhu ◽

Magdalena Skrzypczak ◽

Romain Forey ◽

Benjamin Pardo ◽

...

Keyword(s):

Cell Fate ◽

Genome Stability ◽

Strand Break ◽

Double Strand Breaks ◽

Universal Method ◽

Dna Double Strand Breaks ◽

Strand Breaks ◽

Agarose Beads ◽

Genome Wide ◽

Dna Double Strand Break

AbstractMaintenance of genome stability is a key issue for cell fate that could be compromised by chromosome deletions and translocations caused by DNA double-strand breaks (DSBs). Thus development of precise and sensitive tools for DSBs labeling is of great importance for understanding mechanisms of DSB formation, their sensing and repair. Until now there has been no high resolution and specific DSB detection technique that would be applicable to any cells regardless of their size. Here, we present i-BLESS, a universal method for direct genome-wide DNA double-strand break labeling in cells immobilized in agarose beads. i-BLESS has three key advantages: it is the only unbiased method applicable to yeast, achieves a sensitivity of one break at a given position in 100,000 cells, and eliminates background noise while still allowing for fixation of samples. The method allows detection of ultra-rare breaks such as those forming spontaneously at G-quadruplexes.

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ATM-dependent pathways of chromatin remodelling and oxidative DNA damage responses

Philosophical Transactions of the Royal Society B Biological Sciences ◽

10.1098/rstb.2016.0283 ◽

2017 ◽

Vol 372 (1731) ◽

pp. 20160283 ◽

Cited By ~ 25

Author(s):

N. Daniel Berger ◽

Fintan K. T. Stanley ◽

Shaun Moore ◽

Aaron A. Goodarzi

Keyword(s):

Dna Damage ◽

Oxidative Dna Damage ◽

Strand Break ◽

Chromatin Remodelling ◽

Double Strand Breaks ◽

Biochemical Network ◽

Regulatory Function ◽

Dna Double Strand Breaks ◽

Strand Breaks ◽

The Impact

Ataxia-telangiectasia mutated (ATM) is a serine/threonine protein kinase with a master regulatory function in the DNA damage response. In this role, ATM commands a complex biochemical network that signals the presence of oxidative DNA damage, including the dangerous DNA double-strand break, and facilitates subsequent repair. Here, we review the current state of knowledge regarding ATM-dependent chromatin remodelling and epigenomic alterations that are required to maintain genomic integrity in the presence of DNA double-strand breaks and/or oxidative stress. We will focus particularly on the roles of ATM in adjusting nucleosome spacing at sites of unresolved DNA double-strand breaks within complex chromatin environments, and the impact of ATM on preserving the health of cells within the mammalian central nervous system. This article is part of the themed issue ‘Chromatin modifiers and remodellers in DNA repair and signalling’.

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Double-strand DNA breaks recruit the centromeric histone CENP-A

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.0908233106 ◽

2009 ◽

Vol 106 (37) ◽

pp. 15762-15767 ◽

Cited By ~ 90

Author(s):

Samantha G. Zeitlin ◽

Norman M. Baker ◽

Brian R. Chapados ◽

Evi Soutoglou ◽

Jean Y. J. Wang ◽

...

Keyword(s):

Dna Cleavage ◽

Strand Break ◽

Double Strand Breaks ◽

Dna Breaks ◽

End Joining ◽

Strand Breaks ◽

Double Strand Dna Breaks ◽

Histone H3 Variant ◽

Radiation Induced ◽

Non Homologous End Joining

The histone H3 variant CENP-A is required for epigenetic specification of centromere identity through a loading mechanism independent of DNA sequence. Using multiphoton absorption and DNA cleavage at unique sites by I-SceI endonuclease, we demonstrate that CENP-A is rapidly recruited to double-strand breaks in DNA, along with three components (CENP-N, CENP-T, and CENP-U) associated with CENP-A at centromeres. The centromere-targeting domain of CENP-A is both necessary and sufficient for recruitment to double-strand breaks. CENP-A accumulation at DNA breaks is enhanced by active non-homologous end-joining but does not require DNA-PKcs or Ligase IV, and is independent of H2AX. Thus, induction of a double-strand break is sufficient to recruit CENP-A in human and mouse cells. Finally, since cell survival after radiation-induced DNA damage correlates with CENP-A expression level, we propose that CENP-A may have a function in DNA repair.

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RAP80 suppresses the vulnerability of R-loops during DNA double-strand break repair

10.1101/2021.04.23.440542 ◽

2021 ◽

Author(s):

Takaaki Yasuhara ◽

Reona Kato ◽

Motohiro Yamauchi ◽

Yuki Uchihara ◽

Lee Zou ◽

...

Keyword(s):

Active Regions ◽

Strand Break ◽

Double Strand Breaks ◽

Critical Component ◽

Dna Double Strand Breaks ◽

End Joining ◽

Dsb Repair ◽

Strand Breaks ◽

Chromosome Translocations ◽

Dna Double Strand Break

AbstractR-loops, consisting of ssDNA and DNA-RNA hybrids, are potentially vulnerable unless they are appropriately processed. Recent evidence suggests that R-loops can form in the proximity of DNA double-strand breaks (DSBs) within transcriptionally active regions. Yet, how the vulnerability of R-loops is overcome during DSB repair remains unclear. Here, we identify RAP80 as a factor suppressing the vulnerability of ssDNA in R-loops and chromosome translocations and deletions during DSB repair. Mechanistically, RAP80 prevents unscheduled nucleolytic processing of ssDNA in R-loops by CtIP. This mechanism promotes efficient DSB repair via transcription-associated end-joining dependent on BRCA1, Polθ, and LIG1/3. Thus, RAP80 suppresses the vulnerability of R-loops during DSB repair, thereby precluding genomic abnormalities in a critical component of the genome caused by deleterious R-loop processing.

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