Your search keyword '"Keeney, Scott"' showing total 41 results

1. Cryo-EM structures of the Spo11 core complex bound to DNA

Author

Yu, You, Wang, Juncheng, Liu, Kaixian, Zheng, Zhi, Arter, Meret, Claeys Bouuaert, Corentin, Pu, Stephen, Patel, Dinshaw J., and Keeney, Scott

Abstract

DNA double-strand breaks that initiate meiotic recombination are formed by the topoisomerase-relative enzyme Spo11, supported by conserved auxiliary factors. Because high-resolution structural data have not been available, many questions remain about the architecture of Spo11 and its partners and how they engage with DNA. We report cryo-electron microscopy structures at up to 3.3-Å resolution of DNA-bound core complexes of Saccharomyces cerevisiaeSpo11 with Rec102, Rec104 and Ski8. In these structures, monomeric core complexes make extensive contacts with the DNA backbone and with the recessed 3′-OH and first 5′ overhanging nucleotide, establishing the molecular determinants of DNA end-binding specificity and providing insight into DNA cleavage preferences in vivo. The structures of individual subunits and their interfaces, supported by functional data in yeast, provide insight into the role of metal ions in DNA binding and uncover unexpected structural variation in homologs of the Top6BL component of the core complex.

Published

2024

2. Divergence and conservation of the meiotic recombination machinery

Author

Arter, Meret and Keeney, Scott

Abstract

Sexually reproducing eukaryotes use recombination between homologous chromosomes to promote chromosome segregation during meiosis. Meiotic recombination is almost universally conserved in its broad strokes, but specific molecular details often differ considerably between taxa, and the proteins that constitute the recombination machinery show substantial sequence variability. The extent of this variation is becoming increasingly clear because of recent increases in genomic resources and advances in protein structure prediction. We discuss the tension between functional conservation and rapid evolutionary change with a focus on the proteins that are required for the formation and repair of meiotic DNA double-strand breaks. We highlight phylogenetic relationships on different time scales and propose that this remarkable evolutionary plasticity is a fundamental property of meiotic recombination that shapes our understanding of molecular mechanisms in reproductive biology.

Published

2024

3. Structure and DNA-bridging activity of the essential Rec114–Mei4 trimer interface

Author

Liu, Kaixian, Grasso, Emily M., Pu, Stephen, Zou, Mengyang, Liu, Shixin, Eliezer, David, and Keeney, Scott

Abstract

In this study, Liu et al. describe the structural interactions between the C terminus of Rec114 and N terminus of Mei4 within the evolutionarily conserved, heterotrimeric DNA double-strand break complex during meiotic recombination. They further show that the minimal Rec114–Mei4 complex can bind coaligned duplex DNA to facilitate nucleoprotein nucleation and condensate formation.

Published

2023

4. YTHDC2 control of gametogenesis requires helicase activity but not m6A binding

Author

Saito, Yuhki, Hawley, Ben R., Puno, M. Rhyan, Sarathy, Shreya N., Lima, Christopher D., Jaffrey, Samie R., Darnell, Robert B., Keeney, Scott, and Jain, Devanshi

Abstract

In this study, Saito et al. sought to understand how the N6-methyladenosine (m6A) reader and RNA helicase YTHDC2 switches cells from mitotic to meiotic gene expression programs. Their findings provide insight into YTHDC2's mechanism, and they propose a model in which YTHDC2 binds transcripts independent of m6A status and regulates gene expression during multiple stages of meiosis by distinct mechanisms.

Published

2022

5. Concerted cutting by Spo11 illuminates meiotic DNA break mechanics

Author

Johnson, Dominic, Crawford, Margaret, Cooper, Tim, Claeys Bouuaert, Corentin, Keeney, Scott, Llorente, Bertrand, Garcia, Valerie, and Neale, Matthew J.

Abstract

Genetic recombination arises during meiosis through the repair of DNA double-strand breaks (DSBs) that are created by Spo11, a topoisomerase-like protein1,2. Spo11 DSBs form preferentially in nucleosome-depleted regions termed hotspots3,4, yet how Spo11 engages with its DNA substrate to catalyse DNA cleavage is poorly understood. Although most recombination events are initiated by a single Spo11 cut, here we show in Saccharomyces cerevisiaethat hyperlocalized, concerted Spo11 DSBs separated by 33 to more than 100 base pairs also form, which we term ‘double cuts’. Notably, the lengths of double cuts vary with a periodicity of 10.5 base pairs, which is conserved in yeast and mice. This finding suggests a model in which the orientation of adjacent Spo11 molecules is fixed relative to the DNA helix—a proposal supported by the in vitro DNA-binding properties of the Spo11 core complex. Deep sequencing of meiotic progeny identifies recombination scars that are consistent with repair initiated from gaps generated by adjacent Spo11 DSBs. Collectively, these results revise our present understanding of the mechanics of Spo11-DSB formation and expand on the original concepts of gap repair during meiosis to include DNA gaps that are generated by Spo11 itself.

Published

2021

6. DNA-driven condensation assembles the meiotic DNA break machinery

Author

Claeys Bouuaert, Corentin, Pu, Stephen, Wang, Juncheng, Oger, Cédric, Daccache, Dima, Xie, Wei, Patel, Dinshaw J., and Keeney, Scott

Abstract

The accurate segregation of chromosomes during meiosis—which is critical for genome stability across sexual cycles—relies on homologous recombination initiated by DNA double-strand breaks (DSBs) made by the Spo11 protein1,2. The formation of DSBs is regulated and tied to the elaboration of large-scale chromosome structures3–5, but the protein assemblies that execute and control DNA breakage are poorly understood. Here we address this through the molecular characterization of Saccharomyces cerevisiaeRMM (Rec114, Mei4 and Mer2) proteins—essential, conserved components of the DSB machinery2. Each subcomplex of Rec114–Mei4 (a 2:1 heterotrimer) or Mer2 (a coiled-coil-containing homotetramer) is monodispersed in solution, but they independently condense with DNA into reversible nucleoprotein clusters that share properties with phase-separated systems. Multivalent interactions drive this condensation. Mutations that weaken protein–DNA interactions strongly disrupt both condensate formation and DSBs in vivo, and thus these processes are highly correlated. In vitro, condensates fuse into mixed RMM clusters that further recruit Spo11 complexes. Our data show how the DSB machinery self-assembles on chromosome axes to create centres of DSB activity. We propose that multilayered control of Spo11 arises from the recruitment of regulatory components and modulation of the biophysical properties of the condensates.

Published

2021

7. Structural and functional characterization of the Spo11 core complex

Author

Claeys Bouuaert, Corentin, Tischfield, Sam E., Pu, Stephen, Mimitou, Eleni P., Arias-Palomo, Ernesto, Berger, James M., and Keeney, Scott

Abstract

Spo11, which makes DNA double-strand breaks (DSBs) that are essential for meiotic recombination, has long been recalcitrant to biochemical study. We provide molecular analysis of SaccharomycescerevisiaeSpo11 purified with partners Rec102, Rec104 and Ski8. Rec102 and Rec104 jointly resemble the B subunit of archaeal topoisomerase VI, with Rec104 occupying a position similar to the Top6B GHKL-type ATPase domain. Unexpectedly, the Spo11 complex is monomeric (1:1:1:1 stoichiometry), consistent with dimerization controlling DSB formation. Reconstitution of DNA binding reveals topoisomerase-like preferences for duplex–duplex junctions and bent DNA. Spo11 also binds noncovalently but with high affinity to DNA ends mimicking cleavage products, suggesting a mechanism to cap DSB ends. Mutations that reduce DNA binding in vitro attenuate DSB formation, alter DSB processing and reshape the DSB landscape in vivo. Our data reveal structural and functional similarities between the Spo11 core complex and Topo VI, but also highlight differences reflecting their distinct biological roles.

Published

2021

8. Ensuring meiotic DNA break formation in the mouse pseudoautosomal region

Author

Acquaviva, Laurent, Boekhout, Michiel, Karasu, Mehmet E., Brick, Kevin, Pratto, Florencia, Li, Tao, van Overbeek, Megan, Kauppi, Liisa, Camerini-Otero, R. Daniel, Jasin, Maria, and Keeney, Scott

Abstract

Sex chromosomes in males of most eutherian mammals share only a small homologous segment, the pseudoautosomal region (PAR), in which the formation of double-strand breaks (DSBs), pairing and crossing over must occur for correct meiotic segregation1,2. How cells ensure that recombination occurs in the PAR is unknown. Here we present a dynamic ultrastructure of the PAR and identify controlling cis- and trans-acting factors that make the PAR the hottest segment for DSB formation in the male mouse genome. Before break formation, multiple DSB-promoting factors hyperaccumulate in the PAR, its chromosome axes elongate and the sister chromatids separate. These processes are linked to heterochromatic mo-2 minisatellite arrays, and require MEI4 and ANKRD31 proteins but not the axis components REC8 or HORMAD1. We propose that the repetitive DNA sequence of the PAR confers unique chromatin and higher-order structures that are crucial for recombination. Chromosome synapsis triggers collapse of the elongated PAR structure and, notably, oocytes can be reprogrammed to exhibit spermatocyte-like levels of DSBs in the PAR simply by delaying or preventing synapsis. Thus, the sexually dimorphic behaviour of the PAR is in part a result of kinetic differences between the sexes in a race between the maturation of the PAR structure, formation of DSBs and completion of pairing and synapsis. Our findings establish a mechanistic paradigm for the recombination of sex chromosomes during meiosis.

Published

2020

9. Multilayered mechanisms ensure that short chromosomes recombine in meiosis

Author

Murakami, Hajime, Lam, Isabel, Huang, Pei-Ching, Song, Jacquelyn, van Overbeek, Megan, and Keeney, Scott

Abstract

In most species, homologous chromosomes must recombine in order to segregate accurately during meiosis1. Because small chromosomes would be at risk of missegregation if recombination were randomly distributed, the double-strand breaks (DSBs) that initiate recombination are not located arbitrarily2. How the nonrandomness of DSB distributions is controlled is not understood, although several pathways are known to regulate the timing, location and number of DSBs. Meiotic DSBs are generated by Spo11 and accessory DSB proteins, including Rec114 and Mer2, which assemble on chromosomes3–7and are nearly universal in eukaryotes8–11. Here we demonstrate how Saccharomyces cerevisiaeintegrates multiple temporally distinct pathways to regulate the binding of Rec114 and Mer2 to chromosomes, thereby controlling the duration of a DSB-competent state. The engagement of homologous chromosomes with each other regulates the dissociation of Rec114 and Mer2 later in prophase I, whereas the timing of replication and the proximity to centromeres or telomeres influence the accumulation of Rec114 and Mer2 early in prophase I. Another early mechanism enhances the binding of Rec114 and Mer2 specifically on the shortest chromosomes, and is subject to selection pressure to maintain the hyperrecombinogenic properties of these chromosomes. Thus, the karyotype of an organism and its risk of meiotic missegregation influence the shape and evolution of its recombination landscape. Our results provide a cohesive view of a multifaceted and evolutionarily constrained system that allocates DSBs to all pairs of homologous chromosomes.

Published

2020

10. Chromosome-autonomous feedback down-regulates meiotic DNA break competence upon synaptonemal complex formation

Author

Mu, Xiaojing, Murakami, Hajime, Mohibullah, Neeman, and Keeney, Scott

Abstract

In this study, Mu et al. set out to elucidate the mechanism underlying double-strand break (DSB) feedback control that arises due to a failure of homolog engagement. Using a novel approach to studying DSB control by using karyotypically abnormal yeast strains where homologous pairing and recombination defects are restricted to a small region of the genome, the authors show that DSB number is regulated in a chromosome-autonomous fashion and provide insight into how homeostatic DSB controls respond to aneuploidy during meiosis.

Published

2020

11. Molecular structures and mechanisms of DNA break processing in mouse meiosis

Author

Yamada, Shintaro, Hinch, Anjali Gupta, Kamido, Hisashi, Zhang, Yongwei, Edelmann, Winfried, and Keeney, Scott

Abstract

In this study, Yamada et al. set out to define structures of resected double-strand breaks (DSBs) in mouse spermatocytes genome-wide. Using S1-seq, a novel method that maps meiotic DSB resection endpoints genome-wide at single-nucleotide resolution, the authors report previously undocumented characteristics of resection, including global patterns, locus-to-locus variation, and the genetic pathways that control resection. The authors also report novel structures that appear to be intermolecular recombination intermediates and unexpected properties of these intermediates in mice shed light on the mechanism of meiotic recombination and the structure of chromatin at sites undergoing recombination.

Published

2020

12. Structure and DNA bridging activity of the essential Rec114-Mei4 trimer interface

Author

Liu, Kaixian, Grasso, Emily M., Pu, Stephen, Zou, Mengyang, Liu, Shixin, Eliezer, David, and Keeney, Scott

Published

2024

13. Pelvic fracture pattern predicts the need for hemorrhage control intervention-Results of an AAST multi-institutional study.

Author

Costantini, Todd W., Coimbra, Raul, Holcomb, John B., Podbielski, Jeanette M., Catalano, Richard D., Blackburn, Allie, Scalea, Thomas M., Stein, Deborah M., Williams, Lashonda, Conflitti, Joseph, Keeney, Scott, Hoey, Christy, Tianhua Zhou, Sperry, Jason, Skiada, Dimitra, Inaba, Kenji, Williams, Brian H., Minei, Joseph P., Privette, Alicia, and Mackersie, Robert C.

Published

2017

14. Control of meiotic double-strand-break formation by ATM: local and global views

Author

Lukaszewicz, Agnieszka, Lange, Julian, Keeney, Scott, and Jasin, Maria

Abstract

ABSTRACTDNA double-strand breaks (DSBs) generated by the SPO11 protein initiate meiotic recombination, an essential process for successful chromosome segregation during gametogenesis. The activity of SPO11 is controlled by multiple factors and regulatory mechanisms, such that the number of DSBs is limited and DSBs form at distinct positions in the genome and at the right time. Loss of this control can affect genome integrity or cause meiotic arrest by mechanisms that are not fully understood. Here we focus on the DSB-responsive kinase ATM and its functions in regulating meiotic DSB numbers and distribution. We review the recently discovered roles of ATM in this context, discuss their evolutionary conservation, and examine future research perspectives.

Published

2018

15. Current management of hemorrhage from severe pelvic fractures: Results of an American Association for the Surgery of Trauma multi-institutional trial.

Author

Costantini, Todd W., Coimbra, Raul, Holcomb, John B., Podbielski, Jeanette M., Catalano, Richard, Blackburn, Allie, Scalea, Thomas M., Stein, Deborah M., Williams, Lashonda, Conflitti, Joseph, Keeney, Scott, Suleiman, Ghada, Zhou, Tianhua, Sperry, Jason, Skiada, Dimitra, Inaba, Kenji, Williams, Brian H., Minei, Joseph P., Privette, Alicia, and Mackersie, Robert C.

Published

2016

16. Histone H3 Threonine 11 Phosphorylation Is Catalyzed Directly by the Meiosis-Specific Kinase Mek1 and Provides a Molecular Readout of Mek1 Activity in Vivo

Author

Kniewel, Ryan, Murakami, Hajime, Liu, Yan, Ito, Masaru, Ohta, Kunihiro, Hollingsworth, Nancy M, and Keeney, Scott

Abstract

Saccharomyces cerevisiaeMek1 is a CHK2/Rad53-family kinase that regulates meiotic recombination and progression upon its activation in response to DNA double-strand breaks (DSBs). The full catalog of direct Mek1 phosphorylation targets remains unknown. Here, we show that phosphorylation of histone H3 on threonine 11 (H3 T11ph) is induced by meiotic DSBs in S. cerevisiaeand Schizosaccharomyces pombe. Molecular genetic experiments in S. cerevisiaeconfirmed that Mek1 is required for H3 T11ph and revealed that phosphorylation is rapidly reversed when Mek1 kinase is no longer active. Reconstituting histone phosphorylation in vitrowith recombinant proteins demonstrated that Mek1 directly catalyzes H3 T11 phosphorylation. Mutating H3 T11 to nonphosphorylatable residues conferred no detectable defects in otherwise unperturbed meiosis, although the mutations modestly reduced spore viability in certain strains where Rad51 is used for strand exchange in place of Dmc1. H3 T11ph is therefore mostly dispensable for Mek1 function. However, H3 T11ph provides an excellent marker of ongoing Mek1 kinase activity in vivo. Anti-H3 T11ph chromatin immunoprecipitation followed by deep sequencing demonstrated that H3 T11ph was highly enriched at presumed sites of attachment of chromatin to chromosome axes, gave a more modest signal along chromatin loops, and was present at still lower levels immediately adjacent to DSB hotspots. These localization patterns closely tracked the distribution of Red1 and Hop1, axis proteins required for Mek1 activation. These findings provide insight into the spatial disposition of Mek1 kinase activity and the higher order organization of recombining meiotic chromosomes.

Published

2017

17. Genomic and chromatin features shaping meiotic double-strand break formation and repair in mice

Author

Yamada, Shintaro, Kim, Seoyoung, Tischfield, Sam E., Jasin, Maria, Lange, Julian, and Keeney, Scott

Abstract

ABSTRACTThe SPO11-generated DNA double-strand breaks (DSBs) that initiate meiotic recombination occur non-randomly across genomes, but mechanisms shaping their distribution and repair remain incompletely understood. Here, we expand on recent studies of nucleotide-resolution DSB maps in mouse spermatocytes. We find that trimethylation of histone H3 lysine 36 around DSB hotspots is highly correlated, both spatially and quantitatively, with trimethylation of H3 lysine 4, consistent with coordinated formation and action of both PRDM9-dependent histone modifications. In contrast, the DSB-responsive kinase ATM contributes independently of PRDM9 to controlling hotspot activity, and combined action of ATM and PRDM9 can explain nearly two-thirds of the variation in DSB frequency between hotspots. DSBs were modestly underrepresented in most repetitive sequences such as segmental duplications and transposons. Nonetheless, numerous DSBs form within repetitive sequences in each meiosis and some classes of repeats are preferentially targeted. Implications of these findings are discussed for evolution of PRDM9 and its role in hybrid strain sterility in mice. Finally, we document the relationship between mouse strain-specific DNA sequence variants within PRDM9 recognition motifs and attendant differences in recombination outcomes. Our results provide further insights into the complex web of factors that influence meiotic recombination patterns.

Published

2017

18. Pelvic fracture pattern predicts the need for hemorrhage control intervention—Results of an AAST multi-institutional study

Author

Costantini, Todd W., Coimbra, Raul, Holcomb, John B., Podbielski, Jeanette M., Catalano, Richard D., Blackburn, Allie, Scalea, Thomas M., Stein, Deborah M., Williams, Lashonda, Conflitti, Joseph, Keeney, Scott, Hoey, Christy, Zhou, Tianhua, Sperry, Jason, Skiada, Dimitra, Inaba, Kenji, Williams, Brian H., Minei, Joseph P., Privette, Alicia, Mackersie, Robert C., Robinson, Brenton R., and Moore, Forrest O.

Abstract

Supplemental digital content is available in the text.

Published

2017

19. Numerical and spatial patterning of yeast meiotic DNA breaks by Tel1

Author

Mohibullah, Neeman and Keeney, Scott

Abstract

The Spo11-generated double-strand breaks (DSBs) that initiate meiotic recombination are dangerous lesions that can disrupt genome integrity, so meiotic cells regulate their number, timing, and distribution. Mechanisms of this regulation remain poorly understood. Here, we use Spo11-oligonucleotide complexes, a byproduct of DSB formation, to reveal aspects of the contribution of the Saccharomyces cerevisiaeDNA damage-responsive kinase Tel1 (ortholog of mammalian ATM). A tel1Δ mutant has globally increased amounts of Spo11-oligonucleotide complexes and altered Spo11-oligonucleotide lengths, consistent with conserved roles for Tel1 in control of DSB number and processing. A kinase-dead tel1mutation similarly increases Spo11-oligonucleotide levels but mutating known Tel1 phosphotargets on Hop1 and Rec114 does not, implicating Tel1 kinase activity and clarifying roles of Tel1 phosphorylation substrates. Deep sequencing of Spo11 oligonucleotides demonstrates that Tel1 shapes the genome-wide DSB landscape in unexpected ways. Early in meiosis, Tel1 absence causes widespread changes in DSB distributions across large chromosomal domains. Many of these changes are erased as meiosis proceeds, however, illustrating homeostatic behavior of DSB regulatory systems. We further find that effects of Tel1 are distinct but partially overlapping with previously described contributions of the recombination regulator Cst9 (also known as Zip3). Finally, we provide evidence indicating that Tel1-dependent DSB interference influences the population-average DSB landscape but also demonstrate that locally inhibitory effects of an artificial hotspot insertion can be both Tel1-independent and chromosomal context-dependent. Our findings delineate Tel1 roles in regulating number and location of DSBs and illuminate the complex interplay between Tel1 and other pathways for DSB control.

Published

2017

20. ATM suppresses c-Myc overexpression in the mammary epithelium in response to estrogen

Author

Najnin, Rifat Ara, Al Mahmud, Md Rasel, Rahman, Md Maminur, Takeda, Shunichi, Sasanuma, Hiroyuki, Tanaka, Hisashi, Murakawa, Yasuhiro, Shimizu, Naoto, Akter, Salma, Takagi, Masatoshi, Sunada, Takuro, Akamatsu, Shusuke, He, Gang, Itou, Junji, Toi, Masakazu, Miyaji, Mary, Tsutsui, Kimiko M., Keeney, Scott, and Yamada, Shintaro

Abstract

ATM gene mutation carriers are predisposed to estrogen-receptor-positive breast cancer (BC). ATM prevents BC oncogenesis by activating p53 in every cell; however, much remains unknown about tissue-specific oncogenesis after ATM loss. Here, we report that ATM controls the early transcriptional response to estrogens. This response depends on topoisomerase II (TOP2), which generates TOP2-DNA double-strand break (DSB) complexes and rejoins the breaks. When TOP2-mediated ligation fails, ATM facilitates DSB repair. After estrogen exposure, TOP2-dependent DSBs arise at the c-MYCenhancer in human BC cells, and their defective repair changes the activation profile of enhancers and induces the overexpression of many genes, including the c-MYConcogene. CRISPR/Cas9 cleavage at the enhancer also causes c-MYCoverexpression, indicating that this DSB causes c-MYCoverexpression. Estrogen treatment induced c-Myc protein overexpression in mammary epithelial cells of ATM-deficient mice. In conclusion, ATM suppresses the c-Myc-driven proliferative effects of estrogens, possibly explaining such tissue-specific oncogenesis.

Published

2023

21. Meiotic DNA break formation requires the unsynapsed chromosome axis-binding protein IHO1 (CCDC36) in mice

Author

Stanzione, Marcello, Baumann, Marek, Papanikos, Frantzeskos, Dereli, Ihsan, Lange, Julian, Ramlal, Angelique, Tränkner, Daniel, Shibuya, Hiroki, de Massy, Bernard, Watanabe, Yoshinori, Jasin, Maria, Keeney, Scott, and Tóth, Attila

Abstract

DNA double-strand breaks (DSBs) are induced by SPO11 during meiosis to initiate recombination-mediated pairing and synapsis of homologous chromosomes. Germline genome integrity requires spatiotemporal control of DSB formation, which involves the proteinaceous chromosome axis along the core of each meiotic chromosome. In particular, a component of unsynapsed axes, HORMAD1, promotes DSB formation in unsynapsed regions where DSB formation must occur to ensure completion of synapsis. Despite its importance, the underlying mechanism has remained elusive. We identify CCDC36 as a direct interactor of HORMAD1 (IHO1) that is essential for DSB formation. Underpinning this function, IHO1 and conserved SPO11-auxiliary proteins MEI4 and REC114 assemble chromatin-bound recombinosomes that are predicted activators of DSB formation. HORMAD1 is needed for robust recruitment of IHO1 to unsynapsed axes and efficient formation and/or stabilization of these recombinosomes. Thus, we propose that HORMAD1–IHO1 interaction provides a mechanism for the selective promotion of DSB formation along unsynapsed chromosome axes.

Published

2016

22. Current management of hemorrhage from severe pelvic fractures: Results of an American Association for the Surgery of Trauma multi-institutional trial

Author

Costantini, Todd W., Coimbra, Raul, Holcomb, John B., Podbielski, Jeanette M., Catalano, Richard, Blackburn, Allie, Scalea, Thomas M., Stein, Deborah M., Williams, Lashonda, Conflitti, Joseph, Keeney, Scott, Suleiman, Ghada, Zhou, Tianhua, Sperry, Jason, Skiada, Dimitra, Inaba, Kenji, Williams, Brian H., Minei, Joseph P., Privette, Alicia, Mackersie, Robert C., Robinson, Brenton R., and Moore, Forrest O.

Published

2016

23. Scale matters

Author

Tischfield, Sam E. and Keeney, Scott

Abstract

During meiosis in many organisms, homologous chromosomes engage in numerous recombination events initiated by DNA double-strand breaks (DSBs) formed by the Spo11 protein. DSBs are distributed nonrandomly, which governs how recombination influences inheritance and genome evolution. The chromosomal features that shape DSB distribution are not well understood. In the budding yeast Saccharomyces cerevisiae, trimethylation of lysine 4 of histone H3 (H3K4me3) has been suggested to play a causal role in targeting Spo11 activity to small regions of preferred DSB formation called hotspots. The link between H3K4me3 and DSBs is supported in part by a genome-wide spatial correlation between the two. However, this correlation has only been evaluated using relatively low-resolution maps of DSBs, H3K4me3 or both. These maps illuminate chromosomal features that influence DSB distributions on a large scale (several kb and greater) but do not adequately resolve features, such as chromatin structure, that act on finer scales (kb and shorter). Using recent nucleotide-resolution maps of DSBs and meiotic chromatin structure, we find that the previously described spatial correlation between H3K4me3 and DSB hotspots is principally attributable to coincident localization of both to gene promoters. Once proximity to the nucleosome-depleted regions in promoters is accounted for, H3K4me3 status has only modest predictive power for determining DSB frequency or location. This analysis provides a cautionary tale about the importance of scale in genome-wide analyses of DSB and recombination patterns.

Published

2012

24. H2B (Ser10) Phosphorylation is Induced during Apoptosis and Meiosis in S. cerevisiae

Author

Ahn, Sung-Hee, Henderson, Kiersten A., Keeney, Scott, and Allis, C. David

Abstract

The nucleosome, composed of an octamer of highly conserved histone proteins and associated DNA, is the fundamental unit of eukaryotic chromatin. How arrays of nucleosomes are folded into higher-order structures, and how the dynamics of such compaction are regulated, are questions that remain largely unanswered. Our recent studies demonstrated that phosphorylation of histone H2B is necessary to induce cell death that exhibits phenotypic hallmarks of apoptosis including DNA fragmentation and chromatin condensation in yeast (serine 10)1 and in mammalian cells (serine 14).2 In this article, we extend these findings by uncovering a role for H2B phosphorylation at serine 10 (Ser10) in another biological event that is associated with dramatic alterations in higher-order chromatin structure, meiosis. Our data show strong staining, indicative of H2B (Ser10) phosphorylation, during the pachytene stage of yeast meiotic prophase. These data broaden the use of this phosphorylation mark in chromatin remodeling that closely correlates with chromatin compaction. How phosphorylation marks are translated into meaningful downstream events during processes as diverse as apoptosis and meiosis remains a challenge for future studies.

Published

2005

25. Identification of Residues in Yeast Spo11p Critical for Meiotic DNA Double-Strand Break Formation

Author

Diaz, Robert L., Alcid, Alston D., Berger, James M., and Keeney, Scott

Abstract

ABSTRACTSaccharomyces cerevisiaeSpo11 protein (Spo11p) is thought to generate the DNA double-strand breaks (DSBs) that initiate homologous recombination during meiosis. Spo11p is related to a subunit of archaebacterial topoisomerase VI and appears to cleave DNA through a topoisomerase-like transesterase mechanism. In this work, we used the crystal structure of a fragment of topoisomerase VI to model the Spo11p structure and to identify amino acid residues in yeast Spo11p potentially involved in DSB catalysis and/or DNA binding. These residues were mutated to determine which are critical for Spo11p function in vivo. Mutation of Glu-233 or Asp-288, which lie in a conserved structural motif called the Toprim domain, abolished meiotic recombination. These Toprim domain residues have been implicated in binding a metal ion cofactor in topoisomerases and bacterial primases, supporting the idea that DNA cleavage by Spo11p is Mg2+dependent. Mutations at an invariant arginine (Arg-131) within a second conserved structural motif known as the 5Y-CAP domain, as well as three other mutations (E235A, F260R, and D290A), caused marked changes in the DSB pattern at a recombination hotspot, suggesting that Spo11p contributes directly to the choice of DNA cleavage site. Finally, certain DSB-defective mutant alleles generated in this study conferred a semidominant negative phenotype but only when Spo11p activity was partially compromised by the presence of an epitope tag. These results are consistent with a multimeric structure for Spo11p in vivo but may also indicate that the amount of Spo11 protein is not a limiting factor for DSB formation in normal cells.

Published

2002

26. Identification of Residues in Yeast Spo11p Critical for Meiotic DNA Double-Strand Break Formation

Author

Diaz, Robert L., Alcid, Alston D., Berger, James M., and Keeney, Scott

Abstract

Saccharomyces cerevisiaeSpo11 protein (Spo11p) is thought to generate the DNA double-strand breaks (DSBs) that initiate homologous recombination during meiosis. Spo11p is related to a subunit of archaebacterial topoisomerase VI and appears to cleave DNA through a topoisomerase-like transesterase mechanism. In this work, we used the crystal structure of a fragment of topoisomerase VI to model the Spo11p structure and to identify amino acid residues in yeast Spo11p potentially involved in DSB catalysis and/or DNA binding. These residues were mutated to determine which are critical for Spo11p function in vivo. Mutation of Glu-233 or Asp-288, which lie in a conserved structural motif called the Toprim domain, abolished meiotic recombination. These Toprim domain residues have been implicated in binding a metal ion cofactor in topoisomerases and bacterial primases, supporting the idea that DNA cleavage by Spo11p is Mg2+dependent. Mutations at an invariant arginine (Arg-131) within a second conserved structural motif known as the 5Y-CAP domain, as well as three other mutations (E235A, F260R, and D290A), caused marked changes in the DSB pattern at a recombination hotspot, suggesting that Spo11p contributes directly to the choice of DNA cleavage site. Finally, certain DSB-defective mutant alleles generated in this study conferred a semidominant negative phenotype but only when Spo11p activity was partially compromised by the presence of an epitope tag. These results are consistent with a multimeric structure for Spo11p in vivo but may also indicate that the amount of Spo11 protein is not a limiting factor for DSB formation in normal cells.

Published

2002

27. Chromosome Synapsis Defects and Sexually Dimorphic Meiotic Progression in Mice Lacking Spo11

Author

Baudat, Frédéric, Manova, Katia, Yuen, Julie Pui, Jasin, Maria, and Keeney, Scott

Abstract

Spo11, a protein first identified in yeast, is thought to generate the chromosome breaks that initiate meiotic recombination. We now report that disruption of mouse Spo11leads to severe gonadal abnormalities from defective meiosis. Spermatocytes suffer apoptotic death during early prophase; oocytes reach the diplotene/dictyate stage in nearly normal numbers, but most die soon after birth. Consistent with a conserved function in initiating meiotic recombination, Dmc1/Rad51 focus formation is abolished. Spo11−/−meiocytes also display homologous chromosome synapsis defects, similar to fungi but distinct from flies and nematodes. We propose that recombination initiation precedes and is required for normal synapsis in mammals. Our results also support the view that mammalian checkpoint responses to meiotic recombination and/or synapsis defects are sexually dimorphic.

Published

2000

28. YTHDC2 is essential for pachytene progression and prevents aberrant microtubule-driven telomere clustering in male meiosis

Author

Liu, Rong, Kasowitz, Seth D., Homolka, David, Leu, N. Adrian, Shaked, Jordan T., Ruthel, Gordon, Jain, Devanshi, Lin, Huijuan, Keeney, Scott, Luo, Mengcheng, Pillai, Ramesh S., and Wang, P. Jeremy

Abstract

Mechanisms driving the prolonged meiotic prophase I in mammals are poorly understood. RNA helicase YTHDC2 is critical for mitosis to meiosis transition. However, YTHDC2 is highly expressed in pachytene cells. Here we identify an essential role for YTHDC2 in meiotic progression. Specifically, YTHDC2 deficiency causes microtubule-dependent telomere clustering and apoptosis at the pachytene stage of prophase I. Depletion of YTHDC2 results in a massively dysregulated transcriptome in pachytene cells, with a tendency toward upregulation of genes normally expressed in mitotic germ cells and downregulation of meiotic transcripts. Dysregulation does not correlate with m6A status, and YTHDC2-bound mRNAs are enriched in genes upregulated in mutant germ cells, revealing that YTHDC2 primarily targets mRNAs for degradation. Furthermore, altered transcripts in mutant pachytene cells encode microtubule network proteins. Our results demonstrate that YTHDC2 regulates the pachytene stage by perpetuating a meiotic transcriptome and preventing microtubule network changes that could lead to telomere clustering.

Published

2021

29. A Mouse Homolog of the Saccharomyces cerevisiaeMeiotic Recombination DNA Transesterase Spo11p

Author

Keeney, Scott, Baudat, Frederic, Angeles, Michael, Zhou, Zhi-Hong, Copeland, Neal G., Jenkins, Nancy A., Manova, Katia, and Jasin, Maria

Abstract

The Saccharomyces cerevisiaeSpo11 protein is thought to catalyze formation of the DNA double-strand breaks that initiate meiotic recombination. We have cloned cDNA and genomic DNA for a mouse gene encoding a protein with significant sequence similarity to conserved domains found in proteins of the Spo11p family. This putative mouse Spo11gene maps to the distal region of chromosome 2 (homologous to human chromosome 20q13.2–q13.3) and comprises at least 12 exons, spanning approximately 15–18 kb. Strong expression of the Spo11message is seen in juvenile and adult testis by RNA in situhybridization, RT-PCR, and Northern blot, with much weaker expression in thymus and brain. In situhybridization detects expression in oocytes of embryonic ovary, but not of adult ovary. RT-PCR and in situhybridization analyses of a time course of juvenile testis development indicate that Spo11expression begins in early meiotic Prophase I, prior to the pachytene stage, with increasing accumulation of mRNA through the pachytene stage. Taken together, these results strongly suggest that this gene encodes the functional homolog of yeast Spo11p, which in turn suggests that the mechanism of meiotic recombination initiation is conserved between yeast and mammals.

Published

1999

30. Biochemical heterogeneity in xeroderma pigmentosum complementation group E

Author

Keeney, Scott, Wein, Harrison, and Linn, Stuart

Abstract

Cells from two patients with xeroderma pigmentosum complementation group E (XP-E) have been shown to lack an activity which binds specifically to UV-irradiated DNA (Chu and Chang, 1988). We investigated the occurrence of this binding activity in cell strains from nine additional, unrelated XP-E patients and found that all but one of these strains contained normal levels of the binding protein. Furthermore, the binding activity from these XP-E strains was indistinguishable from that of normal controls in thermal stability, behavior on ion-exchange chromatography, and electrophoretic mobility of protein-DNA complexes, indicating that there were no gross structural alterations in the protein. The association of XP-E with a deficiency in DNA-damage binding protein in cells from 3 of 12 XP-E patients (compared to 0 of 20 non-XP-E controls) is statistically significant (p< 0.05), but there is no obvious correlation between the biochemical defect and the clinical or cellular characteristics of individual patients. Implications of these findings for the role of the binding protein in XP-E are discussed.

Published

1992

31. Chromosomal Localization and cDNA Cloning of the Genes (DDB1 and DDB2) for the p127 and p48 Subunits of a Human Damage-Specific DNA Binding Protein

Author

Dualan, Rachel, Brody, Tom, Keeney, Scott, Nichols, Anne F., Admon, Arie, and Linn, Stuart

Abstract

DDB is a damage-specific DNA binding protein whose binding activity is absent from a minority of cell strains from individuals with xeroderma pigmentosum Group E, a human hereditary disease characterized by defective nucleotide excision DNA repair and an increased incidence of skin cancer. The binding activity from Hela cells is associated with polypeptides of M_r 124,000 and 41,000 as determined by SDS-polyacrylamide gels. This report describes the isolation of full-length human cDNAs encoding each polypeptide of DDB. The predicted peptide molecular masses based on open reading frames are 127,000 and 48,000. When expressed in an in vitro rabbit reticulocyte system, the p48 subunit migrates with an M_r of 41 kDa on SDS-polyacrylamide gels, similarly to the peptide purified from Hela cells. There is no significant homology between the derived p48 peptide sequence and any proteins in current databases, and the derived peptide sequence of pl27 has homology only with the monkey DDB p127 (98% nucleotide identity and only one conserved amino acid substitution. Using a fluorescence in situ hybridization technique, the DDB p127 locus (DDB1) was assigned to the chromosomal location 11q12-q13, and the DDB p48 locus (DDB2) to 11p11-p12. Copyright 1995, 1999 Academic Press

Published

1995

32. A critical review of permeabilized cell systems for studying mammalian DNA repair

Author

Keeney, Scott and Linn, Stuart

Abstract

Permeabilized cell systems have proven valuable for studies of the enzymology of mammalian DNA repair and this review will summarize and contrast the different systems used to this end. Results from permeable cell studies will be reviewed which pertain to 3 questions of DNA repair: the role(s) of ATP, DNA polymerase enzymology, and the isolation of repair factors by in vitro correction of repair-defective cells.

Published

1990

33. A Case of Gastric Metastatic Melanoma 15 Years after the Initial Diagnosis of Cutaneous Melanoma

Author

Farshad, Sohail, Keeney, Scott, Halalau, Alexandra, and Ghaith, Gehad

Abstract

Melanoma is the most common cancer to metastasize to the gastrointestinal tract; however, metastasis to the stomach is a rare occurrence. We present the case of a patient with a history of melanoma of the chest wall 15 years prior to presentation who initially presented to the hospital with sepsis but was later found to have metastatic melanoma in the gastric cardia. This case illustrates the rare occurrence of metastatic melanoma to the stomach which occurred 15 years after the initial skin diagnosis of melanoma was made, its endoscopic appearance, and how the nonspecific symptoms frequently lead to a delayed diagnosis or one that is not made at all until after autopsy. For these reasons, endoscopy should be promptly performed if there is a suspicion of gastrointestinal metastatic melanoma.

Published

2018

34. DDK links replication and recombination in meiosis

Author

Murakami, Hajime and Keeney, Scott

Published

2014

35. Zip it up to shut it down

Author

Zhu, Xuan and Keeney, Scott

Published

2014

36. How much is enough? Control of DNA double-strand break numbers in mouse meiosis

Author

Kauppi, Liisa, Jasin, Maria, and Keeney, Scott

Published

2013

37. It Is the Day (Poem).

Author

Keeney, Scott

Subjects

IT Is the Day (Poem), KEENEY, Scott

Abstract

Presents the poem "It Is the Day," by Scott Keeney.

Published

2004

38. POETA NASCITUR SED FIT.

Author

Keeney, Scott

Subjects

POETA Nascitur Sed Fit (Poem), KEENEY, Scott

Abstract

The poem "Poeta Nascitur Sed Fit," by Scott Keeney is presented. First Line: Stark-minded and spiritually naked, Allen Ginsberg; Last Line: Stark mad and raving naked, I thought I was a girl.

Published

2009

39. Subterranean Apartment Blue (Poem).

Author

Keeney, Scott

Subjects

SUBTERRANEAN Apartment Blue (Poem), KEENEY, Scott

Abstract

Presents the poem "Subterranean Apartment Blue," by Scott Keeney.

Published

2004

40. LITTLE GIRL LOST: SHE CLIMBS.

Author

Keeney, Scott

Subjects

LITTLE Girl Lost: She Climbs (Poem), KEENEY, Scott

Abstract

Presents the poem "Little Girl Lost: She Climbs," by Scott Keeney.

Published

2003

41. LETTERS.

Author

Perrell, Charles, Tipishe, Leo, Sweet, David Kevin, Grillos, John, Landry, Julie, Vyakarnam, Shailendra, Keeney, Scott, and Kapoor, Reena

Abstract

Presents letters to the editor referencing articles and topics discussed in previous issues. "Editor," which discussed the threats of terrorism in the U.S.; "Against the Grain," which expounded on the agbio industry; "Reload," which analyzed investors' perception; "Market Values," which explained the role of entrepreneurs and capitalists.

Published

2001