Your search keyword '"Julio S. Rufas"' showing total 72 results

1. Sex differences in the meiotic behavior of an XX sex chromosome pair in males and females of the mole vole Ellobius tancrei: turning an X into a Y chromosome?

Author

Julio S. Rufas, María Teresa Parra, Ana Gil-Fernández, Oxana Kolomiets, Jesús Page, Sergey Matveevsky, Irina Bakloushinskaya, Marta Martín-Ruiz, Marta Ribagorda, and Alberto Viera

Subjects

Male, X Chromosome, Heterochromatin, Y chromosome, 03 medical and health sciences, 0302 clinical medicine, Meiosis, Y Chromosome, Genetics, Animals, Genetics (clinical), X chromosome, 030304 developmental biology, 0303 health sciences, Sex Characteristics, Sex Chromosomes, biology, Arvicolinae, Synapsis, Chromosome, biology.organism_classification, Ellobius, Ellobius tancrei, Female, 030217 neurology & neurosurgery

Abstract

Sex determination in mammals is usually provided by a pair of chromosomes, XX in females and XY in males. Mole voles of the genus Ellobius are exceptions to this rule. In Ellobius tancrei, both males and females have a pair of XX chromosomes that are indistinguishable from each other in somatic cells. Nevertheless, several studies on Ellobius have reported that the two X chromosomes may have a differential organization and behavior during male meiosis. It has not yet been demonstrated if these differences also appear in female meiosis. To test this hypothesis, we have performed a comparative study of chromosome synapsis, recombination, and histone modifications during male and female meiosis in E. tancrei. We observed that synapsis between the two X chromosomes is limited to the short distal (telomeric) regions of the chromosomes in males, leaving the central region completely unsynapsed. This uneven behavior of sex chromosomes during male meiosis is accompanied by structural modifications of one of the X chromosomes, whose axial element tends to appear fragmented, accumulates the heterochromatin mark H3K9me3, and is associated with a specific nuclear body that accumulates epigenetic marks and proteins such as SUMO-1 and centromeric proteins but excludes others such as H3K4me, ubiH2A, and γH2AX. Unexpectedly, sex chromosome synapsis is delayed in female meiosis, leaving the central region unsynapsed during early pachytene. This region accumulates γH2AX up to the stage in which synapsis is completed. However, there are no structural or epigenetic differences similar to those found in males in either of the two X chromosomes. Finally, we observed that recombination in the sex chromosomes is restricted in both sexes. In males, crossover-associated MLH1 foci are located exclusively in the distal regions, indicating incipient differentiation of one of the sex chromosomes into a neo-Y. Notably, in female meiosis, the central region of the X chromosome is also devoid of MLH1 foci, revealing a lack of recombination, possibly due to insufficient homology. Overall, these results reveal new clues about the origin and evolution of sex chromosomes.

Published

2020

2. Meiosis reveals the early steps in the evolution of a neo-XY sex chromosome pair in the African pygmy mouse Mus minutoides

Author

Alberto Viera, María Teresa Parra, Nicolas Perrin, Jesús Page, Ana Gil-Fernández, Paul A. Saunders, Pablo López-Jiménez, Julio S. Rufas, Daniel L. Jeffries, Marta Martín-Ruiz, Marta Ribagorda, Frédéric Veyrunes, Institut des Sciences de l'Evolution de Montpellier (UMR ISEM), Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-École pratique des hautes études (EPHE), Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Université de Montpellier (UM)-Institut de recherche pour le développement [IRD] : UR226-Centre National de la Recherche Scientifique (CNRS), Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-École Pratique des Hautes Études (EPHE), and ANR-18-CE02-0018,SEXREV,Ménage à trois: un troisième chromosome sexuel féminisant. Conséquences évolutives et implications pour la génétique du déterminisme du sexe chez les mammifères(2018)

Subjects

0106 biological sciences, Male, Cancer Research, Sex Differentiation, [SDV]Life Sciences [q-bio], Pseudoautosomal region, Chromosomal translocation, QH426-470, 01 natural sciences, Biochemistry, Translocation, Genetic, Mice, Y Chromosome, Morphogenesis, sex chromosomes, meiosis, evolution, Cell Cycle and Cell Division, Genetics (clinical), Mammals, Pseudoautosomal Regions, 0303 health sciences, Sex Chromosomes, Sexual Differentiation, Eutheria, Chromosome Biology, Synapsis, Chromosome Mapping, Y Chromosomes, Chiasma, Chromosomal Aberrations, Nucleic acids, Meiosis, Cell Processes, Female, Research Article, X Chromosome, DNA recombination, DNA repair, Biology, Research and Analysis Methods, 010603 evolutionary biology, Chromosomes, 03 medical and health sciences, Genetics, Animals, Molecular Biology Techniques, Molecular Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Sexual differentiation, Autosome, Gene Mapping, Chromosome, Biology and Life Sciences, Cell Biology, DNA, Evolutionary biology, Chromosomal Translocations, Developmental Biology

Abstract

Sex chromosomes of eutherian mammals are highly different in size and gene content, and share only a small region of homology (pseudoautosomal region, PAR). They are thought to have evolved through an addition-attrition cycle involving the addition of autosomal segments to sex chromosomes and their subsequent differentiation. The events that drive this process are difficult to investigate because sex chromosomes in almost all mammals are at a very advanced stage of differentiation. Here, we have taken advantage of a recent translocation of an autosome to both sex chromosomes in the African pygmy mouse Mus minutoides, which has restored a large segment of homology (neo-PAR). By studying meiotic sex chromosome behavior and identifying fully sex-linked genetic markers in the neo-PAR, we demonstrate that this region shows unequivocal signs of early sex-differentiation. First, synapsis and resolution of DNA damage intermediates are delayed in the neo-PAR during meiosis. Second, recombination is suppressed or largely reduced in a large portion of the neo-PAR. However, the inactivation process that characterizes sex chromosomes during meiosis does not extend to this region. Finally, the sex chromosomes show a dual mechanism of association at metaphase-I that involves the formation of a chiasma in the neo-PAR and the preservation of an ancestral achiasmate mode of association in the non-homologous segments. We show that the study of meiosis is crucial to apprehend the onset of sex chromosome differentiation, as it introduces structural and functional constrains to sex chromosome evolution. Synapsis and DNA repair dynamics are the first processes affected in the incipient differentiation of X and Y chromosomes, and they may be involved in accelerating their evolution. This provides one of the very first reports of early steps in neo-sex chromosome differentiation in mammals, and for the first time a cellular framework for the addition-attrition model of sex chromosome evolution., Author summary Sex chromosomes seem to evolve and differentiate at different rates in different taxa. The reasons for this variability are still debated. It is well established that recombination suppression around the sex-determining region triggers differentiation, and several studies have investigated this process from a genetic point of view. However, the cellular context in which recombination arrest occurs has received little attention so far. In this report, we show that meiosis, the cellular division in which pairing and recombination between chromosomes takes place, can affect the incipient differentiation of X and Y chromosomes. Combining cytogenetic and genomic approaches, we found that in the African pygmy mouse Mus minutoides, which has recently undergone sex chromosome-autosome fusions, synapsis and DNA repair dynamics are disturbed along the newly added region of the sex chromosomes. We argue that these alterations are a by-product of the fusion itself, and cause recombination suppression across a large region of the neo-sex chromosome pair. Therefore, we propose that the meiotic context in which sex or neo-sex chromosomes arise is crucial to understand the very early stages of their differentiation, as it could promote or hinder recombination suppression, and therefore impact the rate at which these chromosomes differentiate.

Published

2020

3. Meiosis reveals the early steps in the evolution of a neo-XY sex chromosome pair in the African pygmy mouse Mus minutoides

Author

Ana Gil-Fernández, Julio S. Rufas, Marta Martín-Ruiz, Alberto Viera, Daniel L. Jeffries, Pablo López-Jiménez, María Teresa Parra, Nicolas Perrin, Frédéric Veyrunes, Marta Ribagorda, Jesús Page, and Paul A. Saunders

Subjects

0106 biological sciences, 0303 health sciences, Autosome, Pseudoautosomal region, Synapsis, Chromosome, Chromosomal translocation, Biology, Y chromosome, 010603 evolutionary biology, 01 natural sciences, Chiasma, 03 medical and health sciences, Meiosis, Evolutionary biology, 030304 developmental biology

Abstract

Sex chromosomes of eutherian mammals are highly different in size and gene content, and share only a small region of homology (pseudoautosomal region, PAR). They are thought to have evolved through an addition-attrition cycle involving the addition of autosomal segments to sex chromosomes and their subsequent differentiation. The events that drive this process are difficult to investigate because sex chromosomes in most mammals are at a very advanced stage of differentiation. Here, we have taken advantage of a recent translocation of an autosome to both sex chromosomes in the African pygmy mouse Mus minutoides, which has restored a large segment of homology (neo-PAR). By studying meiotic sex chromosome behavior and identifying fully sex-linked genetic markers in the neo-PAR, we demonstrate that this region shows unequivocal signs of early sex-differentiation. First, synapsis and resolution of DNA damage intermediates are delayed in the neo-PAR during meiosis. Second, recombination is suppressed in a large portion of the neo-PAR. However, the inactivation process that characterizes sex chromosomes during meiosis does not extend to this region. Finally, the sex chromosomes show a dual mechanism of association at metaphase-I that involves the formation of a chiasma in the neo-PAR and the preservation of an ancestral achiasmate mode of association in the non-homologous segments. We show that the study of meiosis is crucial to apprehend the onset of sex chromosome differentiation, as it introduces structural and functional constrains to sex chromosome evolution. Synapsis and DNA repair dynamics are the first processes affected in the incipient differentiation of X and Y chromosomes, and they may be involved in accelerating their evolution. This provides one of the very first reports of early steps in neo-sex chromosome differentiation in mammals, and for the first time a cellular framework for the addition-attrition model of sex chromosome evolution.AUTHOR SUMMARYThe early steps in the evolution of sex chromosomes are particularly difficult to study. Cessation of recombination around the sex-determining locus is thought to initiate the differentiation of sex chromosomes. Several studies have investigated this process from a genetic point of view. However, the cellular context in which recombination arrest occurs has not been considered as an important factor. In this report, we show that meiosis, the cellular division in which pairing and recombination between chromosomes takes place, can affect the incipient differentiation of X and Y chromosomes. Combining cytogenetic and genomic approaches, we found that in the African pygmy mouse Mus minutoides, which has recently undergone a sex chromosome-autosome fusion, synapsis and DNA repair dynamics are altered along the newly added region of the sex chromosomes, likely interfering with recombination and thus contributing to the genetic isolation of a large segment of the Y chromosome. Therefore, the cellular events that occur during meiosis are crucial to understand the very early stages of sex chromosome differentiation. This can help to explain why sex chromosomes evolve very fast in some organisms while in others they have barely changed for million years.

Published

2020

4. γ-H2AX is present at mouse meiotic kinetochores

Author

Andrea Guajardo, Alberto Viera, Julio S. Rufas, José A. Suja, Manuel M. Valdivia, and María Teresa Parra

Subjects

biology, urogenital system, Kinetochore, Chemistry, fungi, environment and public health, Chromatin, Cell biology, Serine, enzymes and coenzymes (carbohydrates), chemistry.chemical_compound, Meiotic Prophase I, Histone, Meiosis, biology.protein, biological phenomena, cell phenomena, and immunity, Homologous recombination, DNA

Abstract

The histone variant H2AX phosphorylated on serine 139, named γ-H2AX, is a canonical DNA double-strand breaks marker. During mammalian meiotic prophase I, γ-H2AX participates in meiotic recombination, meiotic sex chromosome inactivation and meiotic silencing of unsynapsed chromatin. In this study, we have analyzed the distribution of γ-H2AX during male mouse meiosis by immunofluorescence on spread and squashed spermatocytes. We have found that γ-H2AX locates at the inner kinetochore plate of meiotic kinetochores in both meiotic divisions. Therefore our results, for the first time, uncover a novel role for γ-H2AX at mammalian meiotic kinetochores.

Published

2020

5. Meiotic behavior of a complex hexavalent in heterozygous mice for Robertsonian translocations: insights for synapsis dynamics

Author

Riccardo Castiglia, Soledad Berríos, Marta Martín-Ruiz, Julio S. Rufas, Jesús Page, Emanuela Solano, María Teresa Parra, Raúl Fernández-Donoso, Eliana Ayarza, Marta Ribagorda, Ernesto Capanna, Ana Gil-Fernández, and Alberto Viera

Subjects

Male, Heterozygote, chromosome synapsis, Karyotype, Robertsonian translocation, Chromosomal translocation, Biology, medicine.disease_cause, Translocation, Genetic, Mice, 03 medical and health sciences, 0302 clinical medicine, Prophase, Meiosis, Spermatocytes, Chromosome regions, Genetics, medicine, Animals, meiosis, Meiotic Prophase I, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Synapsis, Chiasma, chromosome synapsis, meiosis, Robertsonian translocation, Chromosome Pairing, Female, 030217 neurology & neurosurgery

Abstract

Natural populations of the house mouse Mus musculus domesticus show great diversity in chromosomal number due to the presence of chromosomal rearrangements, mainly Robertsonian translocations. Breeding between two populations with different chromosomal configurations generates subfertile or sterile hybrid individuals due to impaired meiotic development. In this study, we have analyzed prophase-I spermatocytes of hybrids formed by crossing mice from Vulcano and Lipari island populations. Both populations have a 2n = 26 karyotype but different combinations of Robertsonian translocations. We studied the progress of synapsis, recombination, and meiotic silencing of unsynapsed chromosomes during prophase-I through the immunolocalization of the proteins SYCP3, SYCP1, γH2AX, RAD51, and MLH1. In these hybrids, a hexavalent is formed that, depending on the degree of synapsis between chromosomes, can adopt an open chain, a ring, or a closed configuration. The frequency of these configurations varies throughout meiosis, with the maximum degree of synapsis occurring at mid pachytene. In addition, we observed the appearance of heterologous synapsis between telocentric and metacentric chromosomes; however, this synapsis seems to be transient and unstable and unsynapsed regions are frequently observed in mid-late pachytene. Interestingly, we found that chiasmata are frequently located at the boundaries of unsynapsed chromosomal regions in the hexavalent during late pachytene. These results provide new clues about synapsis dynamics during meiosis. We propose that mechanical forces generated along chromosomes may induce premature desynapsis, which, in turn, might be counteracted by the location of chiasmata. Despite these and additional meiotic features, such as the accumulation of γH2AX on unsynapsed chromosome regions, we observed a large number of cells that progressed to late stages of prophase-I, indicating that synapsis defects may not trigger a meiotic crisis in these hybrids.

Published

2019

6. B1 Was the Ancestor B Chromosome Variant in the Western Mediterranean Area in the Grasshopper Eyprepocnemis plorans

Author

María Dolores López-León, Juan Pedro M. Camacho, Josefa Cabrero, Julio S. Rufas, Bruno Massa, M Kamel Ben Halima, E Petitpierre, Ricardo Gómez, and Mercedes Ruiz-Estévez

Subjects

Genetics, Mediterranean climate, Balearic islands, B chromosome, Satellite DNA, government.political_district, Biology, biology.organism_classification, Phylogeography, Evolutionary biology, government, Grasshopper, Molecular Biology, Ribosomal DNA, Genetics (clinical), X chromosome

Abstract

We analyzed the distribution of 2 repetitive DNAs, i.e. ribosomal DNA (rDNA) and a satellite DNA (satDNA), on the B chromosomes found in 17 natural populations of the grasshopper Eyprepocnemis ploransplorans sampled around the western Mediterranean region, including the Iberian Peninsula, Balearic Islands, Sicily, and Tunisia. Based on the amount of these repetitive DNAs, 4 types of B variants were found: B1, showing an equal or higher amount of rDNA than satDNA, and 3 other variants, B2, B24 and B5, bearing a higher amount of satDNA than rDNA. The variants B1 and B2 varied in size among populations: B1 was about half the size of the X chromosome in Balearic Islands, but two-thirds of the X in Iberian populations at Alicante, Murcia and Albacete provinces. Likewise, B2 was about one-third the size of the X chromosome in populations from the Granada province but half the size of the X in the populations collected at Málaga province. The widespread geographical distribution of the B1 variant makes it the best candidate for being the ancestor B chromosome in the whole western Mediterranean region.

Published

2013

7. Do Exogenous DNA Double-Strand Breaks Change Incomplete Synapsis and Chiasma Localization in the Grasshopper Stethophyma grossum?

Author

Juan Luis Santos, Julio S. Rufas, and Adela Calvente

Subjects

Male, 0301 basic medicine, Chromosomal Proteins, Non-Histone, Gene Expression, lcsh:Medicine, Cell Cycle Proteins, Biochemistry, Prophase, Chromosomal crossover, Chromosome segregation, Homologous Chromosomes, Animal Cells, Spermatocytes, DNA Breaks, Double-Stranded, Cell Cycle and Cell Division, Crossing Over, Genetic, Homologous Recombination, lcsh:Science, Genetics, Multidisciplinary, Chromosome Biology, Synapsis, Chromatin, Chiasma, Cell biology, Nucleic acids, Meiosis, Synaptonemal complex, Cell Processes, Epigenetics, Cellular Types, Research Article, DNA recombination, Grasshoppers, Biology, Chromosomes, 03 medical and health sciences, Homologous chromosome, Animals, Metaphase, Chromosome Aberrations, lcsh:R, Biology and Life Sciences, Cell Biology, DNA, Sperm, Chromosome Pairing, Germ Cells, 030104 developmental biology, lcsh:Q

Abstract

Meiotic recombination occurs as a programmed event that initiates by the formation of DNA double-strand breaks (DSBs) that give rise to the formation of crossovers that are observed as chiasmata. Chiasmata are essential for the accurate chromosome segregation and the generation of new combinations of parental alleles. Some treatments that provoke exogenous DSBs also lead to alterations in the recombination pattern of some species in which full homologous synapsis is achieved at pachytene. We have carried out a similar approach in males of the grasshopper Stethophyma grossum, whose homologues show incomplete synapsis and proximal chiasma localization. After irradiating males with γ rays we have studied the distribution of both the histone variant γ-H2AX and the recombinase RAD51. These proteins are cytological markers of DSBs at early prophase I. We have inferred synaptonemal complex (SC) formation via identification of SMC3 and RAD 21 cohesin subunits. Whereas thick and thin SMC3 filaments would correspond to synapsed and unsynapsed regions, the presence of RAD21 is only restricted to synapsed regions. Results show that irradiated spermatocytes maintain restricted synapsis between homologues. However, the frequency and distribution of chiasmata in metaphase I bivalents is slightly changed and quadrivalents were also observed. These results could be related to the singular nuclear polarization displayed by the spermatocytes of this species.

Published

2016

8. Meiosis inStethophyma(Mecostethus)Grossum(Orthoptera: Acrididae): An Exciting History

Author

Mónica Pradillo, Adela Calvente, Alberto Viera, Julio S. Rufas, and Juan L. Santos

Subjects

Genetics, B chromosome, Cohesin, Meiosis, Insect Science, Synapsis, Biology, X chromosome, Bivalent (genetics), Chiasma, Chromosomal crossover

Abstract

The present study is a sincere tribute from some of the cytogenetic laboratories of Madrid involved in the study of grasshopper meiosis, for the inestimable contribution of Professor Michael J.D. White to orthopteran cytogenetics, on the 100th anniversary of his birth. Here we review the knowledge accumulated over almost 90 y on the meiosis of the grasshopper Stethophyma grossum, especially on the male side, because of the very unusual meiotic characteristics shown by the spermatocytes, namely: whereas the three shortest bivalents achieve full synapsis and do not show chiasma localization and the single X chromosome remains asynapsed, the remaining eight bivalents show restricted synapsis and proximal chiasma localization. In addition, supernumerary segments and accessory chromosomes are present in some natural populations. Special attention is paid to the relationships among cohesin axis morphogenesis, initiation of recombination events and synapsis achievement.

Published

2010

9. Incomplete Synapsis and Chiasma Localization: The Chicken or the Egg?

Author

Adela Calvente, Alberto Viera, Rocío Gómez, José A. Suja, María Teresa Parra, C.G. de la Vega, Julio S. Rufas, Juan L. Santos, Jesús Page, and R. de la Fuente

Subjects

Male, Recombination, Genetic, Genetics, medicine.medical_specialty, Cohesin, Synapsis, Cytogenetics, Morphogenesis, Grasshoppers, Biology, Chromosomes, Chiasma, Chromosome Pairing, Meiosis, medicine, Animals, Crossing Over, Genetic, Homologous recombination, Molecular Biology, Genetics (clinical), Recombination

Abstract

In the present study, and as a sincere tribute from the Cytogenetics teams from Madrid to Professor Máximo Drets on his 80th birthday, we have analyzed and compared 3 different grasshopper species with different synaptic patterns, a standard pattern, a second pattern with synapsis restricted to the proximal regions, and a third pattern with synapsis restricted to the distal regions. In the 3 species we have thoroughly analyzed the relationships among cohesin axis morphogenesis, formation of double strand breaks (DSBs) and recombination initiation. Our results demonstrate that in every case recombination initiation precedes synapsis, and that there is a direct relationship between the absence of meiotic recombination and the existence of particular unsynapsed chromosomal regions during prophase I. Based on our results we propose and discuss the mechanisms underlying the existence of incomplete synapsis and the localization of chiasma in wild species.

Published

2010

10. Transcription reactivation during the first meiotic prophase in bugs is not dependent on synapsis

Author

Jesús Page, María Teresa Parra, Alberto Viera, Julio S. Rufas, and UAM. Departamento de Biología

Subjects

0301 basic medicine, Male, Transcriptional Activation, RNA polymerase II, Biology, MSUC, Bivalent (genetics), Chromosomal crossover, Heteroptera, 03 medical and health sciences, Meiotic Prophase I, Prophase, Meiosis, Spermatocytes, Genetics, Animals, Genetics (clinical), Recombination, Genetic, 030102 biochemistry & molecular biology, MSCI, Synapsis, Chromosome, Biología y Biomedicina / Biología, Chromosome Pairing, 030104 developmental biology, biology.protein, Transcription

Abstract

This is a post-peer-review, pre-copyedit version of an article published in Chromosoma. The final authenticated version is available online at: http://dx.doi.org/10.1007/s00412-016-0577-6, During meiosis, transcription is precisely regulated in relation to the process of chromosome synapsis. In mammals, transcription is very low until the completion of synapsis in early pachytene, and then reactivates during mid pachytene, up to the end of diplotene. Moreover, chromosomes or chromosomal regions that do not achieve synapsis undergo a specific process of inactivation called meiotic silencing of unpaired chromatin (MSUC). Sex chromosomes, which are mostly unsynapsed, present a special case of inactivation named meiotic sex chromosome inactivation (MSCI). Although processes that are similar to MSUC/MSCI have been described in other species like Sordaria and Caenorhabditis elegans, very few studies have been developed in insects. We present a study on the relationships between synapsis and transcription in two hemipteran species (Graphosoma italicum and Carpocoris fuscispinus) that possess holocentric chromosomes but develop different synaptic patterns. We have found that transcription, revealed by the presence of RNA polymerase II, is very low at the beginning of meiosis, but robustly increases during zygotene, long before the completion of synapsis, excepting in the sex chromosomes. In fact, we show that histone H3 methylation at lysine 9 (H3K9me3) may be present in the sex chromosomes at leptotene, thus acting as a likely epigenetic mark for this inactive state. Our results suggest that the meiotic transcription in these two species is differently regulated from that of mammals and, therefore, offer new opportunities to understand the relationship between synapsis and transcription and the mechanisms that govern MSUC/MSCI processes, This work was supported by grants BFU2009-10987 from Ministerio de Ciencia e Innovación and grants CGL2014-53106-P and BFU2014-53681-P from Ministerio de Economía y Competitividad (Spain)

Published

2015

11. The Program of Sex Chromosome Pairing in Meiosis Is Highly Conserved Across Marsupial Species

Author

Alberto Viera, Soledad Berríos, José A. Suja, María Teresa Parra, Jesús Page, Raúl Fernández-Donoso, Julio S. Rufas, José Luis Barbero, and Ignacio Prieto

Subjects

Genetics, Prophase, Meiosis, Evolution of sexual reproduction, Centromere, Homologous chromosome, Chromosome, Biology, Y chromosome, X chromosome

Abstract

Marsupials present a series of genetic and chromosomal features that are highly conserved in very distant species. One of these features is the absence of a homologous region between X and Y chromosomes. According to this genetic differentiation, sex chromosomes do not synapse during the first meiotic prophase in males, and a special structure, the dense plate, maintains sex chromosome association. In this report we present results on the process of meiotic sex chromosome pairing obtained from three different species, Thylamys elegans, Dromiciops gliroides, and Rhyncholestes raphanurus, representing the three orders of American marsupials. We have investigated the relationships between the axial structures organized along sex chromosomes and the formation of the dense plate. We found that in the three species the dense plate arises as a modification of sex chromosomal axial elements, but without the involvement of other meiotic axial structures, such as the cohesin axes. Considering the phylogenetic relationships among the marsupials studied here, our data reinforce the idea that the dense plate emerged early in marsupial evolution as an efficient mechanism to ensure the association of the nonhomologous sex chromosomes. This situation could have influenced the further evolution of sex chromosomes in marsupials.

Published

2005

12. DNA double‐strand breaks, recombination and synapsis: the timing of meiosis differs in grasshoppers and flies

Author

Alberto Viera, José A. Suja, Renee Lira, M. Teresa Parra, Rocío Gómez, Juan Luis Santos, Adela Calvente, Jesús Page, Julio S. Rufas, and Marta Cifuentes

Subjects

Male, cells, Scientific Report, Immunoblotting, RAD51, Fluorescent Antibody Technique, Grasshoppers, environment and public health, Biochemistry, Histones, Meiosis, Spermatocytes, Genetics, Recombinase, Animals, Molecular Biology, Recombination, Genetic, biology, Cohesin, Diptera, fungi, Synapsis, DNA-Binding Proteins, Chromosome Pairing, enzymes and coenzymes (carbohydrates), Synaptonemal complex, Histone, biology.protein, Rad51 Recombinase, biological phenomena, cell phenomena, and immunity, Homologous recombination

Abstract

The temporal and functional relationships between DNA events of meiotic recombination and synaptonemal complex formation are a matter of discussion within the meiotic field. To analyse this subject in grasshoppers, organisms that have been considered as models for meiotic studies for many years, we have studied the localization of phosphorylated histone H2AX (gamma-H2AX), which marks the sites of double-strand breaks (DSBs), in combination with localization of cohesin SMC3 and recombinase Rad51. We show that the loss of gamma-H2AX staining is spatially and temporally linked to synapsis, and that in grasshoppers the initiation of recombination, produced as a consequence of DSB formation, precedes synapsis. This result supports the idea that grasshoppers display a pairing pathway that is not present in other insects such as Drosophila melanogaster, but is similar to those reported in yeast, mouse and Arabidopsis. In addition, we have observed the presence of gamma-H2AX in the X chromosome from zygotene to late pachytene, indicating that the function of H2AX phosphorylation during grasshopper spermatogenesis is not restricted to the formation of gamma-H2AX foci at DNA DSBs.

Published

2004

13. Involvement of the cohesin Rad21 and SCP3 in monopolar attachment of sister kinetochores during mouse meiosis I

Author

María Teresa Parra, Alberto Viera, José A. Suja, Juan Luis Santos, Jesús Page, Rocío Gómez, Julio S. Rufas, and Ricardo Benavente

Subjects

Male, Centromere, Cell Cycle Proteins, Chromatids, Biology, Mice, Spermatocytes, Homologous chromosome, Animals, Acetyl-CoA C-Acetyltransferase, Telophase, Kinetochores, Genetics, Cohesin, Kinetochore, Meiosis II, Nuclear Proteins, Cell Biology, Phosphoproteins, Cell biology, DNA-Binding Proteins, Mice, Inbred C57BL, Establishment of sister chromatid cohesion, Meiosis, Microscopy, Electron, Synaptonemal complex, Microscopy, Fluorescence, Carrier Proteins

Abstract

SCP3 is a meiosis-specific structural protein appearing at axial elements and lateral elements of the synaptonemal complex. We have analysed the behaviour of SCP3 and the cohesin subunit Rad21 in mouse spermatocytes by means of a squashing technique. Our results demonstrate that both proteins colocalize and are partially released from chromosome arms during late prophase I stages, although they persist at the interchromatid domain of metaphase I bivalents. Thus, Rad21 cannot be considered a `mitotic'-specific variant, but coexists with Rec8. During late prophase I SCP3 and Rad21 accumulate at centromeres, and together with the chromosomal passenger proteins INCENP and aurora-B kinase, show a complex `double cornet'-like distribution at the inner domain of metaphase I centromeres beneath the associated sister kinetochores. We have observed that Rad21 and SCP3 are displaced from centromeres during telophase I when sister kinetochores separate, and are not present at metaphase II centromeres. Thus, we hypothesise that Rad21, and the superimposed SCP3 and SCP2, are involved in the monopolar attachment of sister kinetochores during meiosis I, and are not responsible for the maintenance of sister-chromatid centromere cohesion during meiosis II as previously suggested.

Published

2004

14. X and B chromosomes display similar meiotic characteristics in male grasshoppers

Author

Adela Calvente, Rocío Gómez, Juan Luis Santos, Alberto Viera, María Teresa Parra, Julio S. Rufas, José A. Suja, and Jesús Page

Subjects

Male, X Chromosome, Grasshoppers, Biology, Chromosomes, Histones, Meiosis, Chromosome regions, Genetics, Animals, Phosphorylation, Grasshopper, Molecular Biology, Metaphase, Genetics (clinical), X chromosome, B chromosome, Chromosome organisation, biology.organism_classification, DNA-Binding Proteins, Rad51 Recombinase, Chromosome 21, Antibodies, Phospho-Specific, Chromosome 22

Abstract

We have analysed the chromosome organisation and the location and temporal appearance of different proteins in X and B chromosomes in the grasshopper Eyprepocnemis plorans throughout the first meiotic prophase. We have used adult males that carry a B chromosome collected in natural Spanish populations. The scaffold organisation has been analysed by means of silver stained chromatid cores. In addition, we have detected by immunolabelling the presence of phosphoepitopes, the ensemble of cohesin axes, the location of histone γ-H2AX, and recombinase Rad51. Our observations demonstrate that X and B chromosomes share similarities in chromatin organisation and in the expression of the tested proteins, which strongly differ from those of the autosomes. These results could be interpreted either as a support to the hypothesis that the Bs analysed here originated from the X chromosome, and/or that their chromatin composition and precocious condensation could determine their meiotic behaviour.

Published

2004

15. Dynamic relocalization of the chromosomal passenger complex proteins inner centromere protein (INCENP) and aurora-B kinase during male mouse meiosis

Author

Alberto Viera, José A. Suja, Jesús Page, Rocío Gómez, William C. Earnshaw, María Teresa Parra, Mar Carmena, and Julio S. Rufas

Subjects

Male, Chromosomal Proteins, Non-Histone, Centromere, Immunoblotting, Aurora B kinase, Protein Serine-Threonine Kinases, Biology, Prophase, Histones, Chromosome segregation, Mice, Aurora Kinases, Spermatocytes, Heterochromatin, Animals, Aurora Kinase B, Humans, Phosphorylation, Kinetochores, Metaphase, Anaphase, Synaptonemal Complex, Kinetochore, INCENP, Spindle midzone, 3T3 Cells, Cell Biology, Cell biology, Meiosis, Sister Chromatid Exchange, HeLa Cells

Abstract

INCENP and aurora-B kinase are two chromosomal passenger proteins that are thought to play key roles in coordinating chromosome segregation with cytokinesis in somatic cells. Here we have analyzed their subcellular distribution, and that of phosphorylated histone H3, and the timing of their relative appearance in mouse spermatocytes during both meiotic divisions. Our results show that in mitotic spermatogonial cells, INCENP and aurora-B show the same pattern of distribution as they do in cultured somatic cells. INCENP labels the synaptonemal complex central element from zygotene up to late pachytene when it begins to relocalize to heterochromatic chromocentres. Aurora-B first appears at chromocentres in late diplotene before the initial phosphorylation of histone H3. INCENP and aurora-B concentrate at centromeres during diakinesis and appear during metaphase I as T-shaped signals at their inner domains, just below associated sister kinetochores. During late anaphase I both proteins relocalize to the spindle midzone. Both proteins colocalize at a connecting strand traversing the centromere region and joining sister kinetochores, in metaphase II centromeres. This strand disappears at the metaphase II/anaphase II transition and relocalizes to the spindle midzone. We discuss the complex dynamic relocalization of the chromosomal passenger complex during prophase I. Additionally, we suggest that this complex may regulate sister-chromatid centromere cohesion during both meiotic divisions.

Published

2003

16. Dynamic relocation of telomere complexes in mouse meiotic chromosomes

Author

Alberto Viera, José A. Suja, Juan Luis Santos, María Teresa Parra, Julio S. Rufas, and Jesús Page

Subjects

Male, Genetics, Synaptonemal Complex, Chromosome, Q-FISH, Telomere, Biology, Chromosomes, Mammalian, Mice, Inbred C57BL, Meiosis, Mice, Synaptonemal complex, Prophase, Spermatocytes, Centromere, Animals, Colchicine, Kinetochores, Anaphase

Abstract

Telomeric DNA repeats as well as different specific proteins such as TRF1 and Rap1 associate in functional telomere complexes found at chromosome ends. Using spreading techniques, the presence of TRF1 and Rap1 has been reported at mammalian meiotic telomeres during prophase I. In the present study, we have analysed, by fluorescence in-situ hybridization and immunofluorescence, the appearance and location of telomere complexes during both male mouse meiotic divisions. Additionally, we have studied their relationship with different centromere/kinetochore proteins and the synaptonemal complex protein SCP3. Our results show that telomere complexes are not located at condensed meiotic chromosome tips. Therefore, a change in chromosome structure may occur from pachytene up to metaphase I involving the dynamic relocation of telomere complexes in condensed chromosomes. Moreover, we have found that proximal telomere complexes are relocated internally to kinetochores from metaphase I up to anaphase II. We discuss the functional significance of the location of telomere complexes into internal domains of condensed meiotic chromosomes.

Published

2003

17. Chromatin Organization and Remodeling of Interstitial Telomeric Sites During Meiosis in the Mongolian Gerbil (Meriones unguiculatus)

Author

Manfred Alsheimer, Alberto Viera, Marcia Manterola, María Teresa Parra, Roberto de la Fuente, Jesús Page, and Julio S. Rufas

Subjects

Cell division, DNA Repair, DNA repair, Heterochromatin, Nuclear Envelope, Centromere, Biology, Investigations, Histones, Meiosis, Genetics, Animals, Recombination, Genetic, Cell Cycle, Telomere, Chromatin Assembly and Disassembly, Chromatin, Histone, biology.protein, Gerbillinae, Cell Division

Abstract

Telomeric DNA repeats are key features of chromosomes that allow the maintenance of integrity and stability in the telomeres. However, interstitial telomere sites (ITSs) can also be found along the chromosomes, especially near the centromere, where they may appear following chromosomal rearrangements like Robertsonian translocations. There is no defined role for ITSs, but they are linked to DNA damage-prone sites. We were interested in studying the structural organization of ITSs during meiosis, a kind of cell division in which programmed DNA damage events and noticeable chromatin reorganizations occur. Here we describe the presence of highly amplified ITSs in the pericentromeric region of Mongolian gerbil (Meriones unguiculatus) chromosomes. During meiosis, ITSs show a different chromatin conformation than DNA repeats at telomeres, appearing more extended and accumulating heterochromatin markers. Interestingly, ITSs also recruit the telomeric proteins RAP1 and TRF1, but in a stage-dependent manner, appearing mainly at late prophase I stages. We did not find a specific accumulation of DNA repair factors to the ITSs, such as γH2AX or RAD51 at these stages, but we could detect the presence of MLH1, a marker for reciprocal recombination. However, contrary to previous reports, we did not find a specific accumulation of crossovers at ITSs. Intriguingly, some centromeric regions of metacentric chromosomes may bind the nuclear envelope through the association to SUN1 protein, a feature usually performed by telomeres. Therefore, ITSs present a particular and dynamic chromatin configuration in meiosis, which could be involved in maintaining their genetic stability, but they additionally retain some features of distal telomeres, provided by their capability to associate to telomere-binding proteins.

Published

2014

18. Colchicine promotes a change in chromosome structure without loss of sister chromatid cohesion in prometaphase I-arrested bivalents

Author

Julio S. Rufas, María Teresa Parra, José A. Suja, and Eva M. Rodríguez

Subjects

Male, X Chromosome, Kinetochore, Grasshoppers, Chromatids, Biology, Spermatozoa, Chromosomes, Cell biology, Establishment of sister chromatid cohesion, Meiosis, Microscopy, Fluorescence, Centromere, Genetics, Animals, Sister chromatids, Chromatid, Prometaphase, Colchicine, Kinetochores, Sister Chromatid Exchange, Metaphase, Mitosis, Genetics (clinical)

Abstract

In somatic cells colchicine promotes the arrest of cell division at prometaphase, and chromosomes show a sequential loss of sister chromatid arm and centromere cohesion. In this study we used colchicine to analyse possible changes in chromosome structure and sister chromatid cohesion in prometaphase I-arrested bivalents of the katydid Pycnogaster cucullata. After silver staining we observed that in colchicine-arrested prometaphase I bivalents, and in contrast to what was found in control bivalents, sister kinetochores appeared individualised and sister chromatid axes were completely separated all along their length. However, this change in chromosome structure occurred without loss of sister chromatid arm cohesion. We also employed the MPM-2 monoclonal antibody against mitotic phosphoproteins on control and colchicine-treated spermatocytes. In control metaphase I bivalents this antibody labelled the tightly associated sister kinetochores and the interchromatid domain. By contrast, in colchicine-treated prometaphase I bivalents individualised sister kinetochores appeared labelled, but the interchromatid domain did not show labelling. These results support the notion that MPM-2 phosphoproteins, probably DNA topoisomerase IIalpha, located in the interchromatid domain act as "chromosomal staples" associating sister chromatid axes in metaphase I bivalents. The disappearance of these chromosomal staples would induce a change in chromosome structure, as reflected by the separation of sister kinetochores and sister axes, but without a concomitant loss of sister chromatid cohesion.

Published

2001

19. Meiotic sister chromatid cohesion in holocentric sex chromosomes of three heteropteran species is maintained in absence of axial elements

Author

José A. Suja, Julio S. Rufas, Jesús Page, A. L. del Cerro, and Juan Luis Santos

Subjects

Cell Nucleus, Male, Genetics, Sex Chromosomes, Karyotype, Chromatids, Biology, Heteroptera, Establishment of sister chromatid cohesion, Meiosis, Synaptonemal complex, Meiotic sister chromatid cohesion, Chromosome Segregation, Karyotyping, Animals, Sister chromatids, Sister Chromatid Exchange, Metaphase, Cell Division, Genetics (clinical), Anaphase

Abstract

It has been suggested that in species with monocentric chromosomes axial element (AE) components may be responsible for sister chromatid cohesion during meiosis. To test this hypothesis in species with holocentric chromosomes we selected three heteropteran species with different sex-determining mechanisms. We observed in surface-spreads and sections using transmission electron microscopy that the univalent sex chromosomes form neither AEs nor synaptonemal complexes (SCs) during pachytene. We also found that a polyclonal antibody recognizing SCP3/Cor1, a protein present at AEs and SC lateral elements of rodents, labels the autosomal SCs but not AEs or SC stretches corresponding to the sex chromosomes. Cytological analysis of the segregational behaviour of the sex univalents demonstrates that although these chromosomes segregate equationally during anaphase I they never show precocious separation of sister chromatids during late prophase I or metaphase I. These results suggest that AEs are not responsible for sister cohesion in sex chromosomes. The segregational behaviour of these chromosomes during both meiotic divisions also indicates that different achiasmate modes of chromosome association exist in heteropteran species.

Published

2000

20. [Untitled]

Author

José A. Suja, Jesús Page, Francisco Panzera, Rubén Pérez, and Julio S. Rufas

Subjects

Chromosome segregation, Genetics, Meiosis, Holocentric, Sister chromatids, Karyotype, Chromatid, Biology, Metaphase, Bivalent (genetics)

Abstract

The meiotic behaviour of the X chromosome and one autosomal pair of the heteropteran Triatoma infestans was analysed by means of C-banding plus DAPI staining. At first metaphase, the X univalent is oriented with its long axis parallel to the equatorial plate, which suggests a holocentric interaction with the spindle fibres. After this initial orientation, kinetic activity is restricted to one of both chromatid ends. The election of the active chromatid end is random and it is independent of the end selected in the sister chromatid. At second metaphase, the X and Y chromatids associate side by side forming a pseudobivalent. After that, the kinetic activity is again restricted to either of both chromosomal ends in a random fashion. At first metaphase, the fourth autosomal bivalent shows two alternative random orientations depending on the chromosome end showing kinetic activity (DAPI positive or opposite). At second metaphase, half bivalents are oriented with their long axis parallel to the equatorial plate. Three different segregation patterns are observed. The kinetic activity can be localised: (i) in the end with the DAPI signal (46.9%), (ii) in the opposite end (44.6%) or (iii) in one DAPI-positive end in one chromatid and in the opposite end in the other one (8.5%). The existence of the last pattern indicates that the same end can show kinetic activity during both meiotic divisions. Our results provide new information on the comparative meiotic behaviour of autosomes and sex chromosomes in holocentric systems.

Published

2000

21. Effects of supernumerary heterochromatin on chiasma formation and chromosome segregation in Dociostaurus genei (Orthoptera)

Author

E Rodríguez Iñigo, P L Mason, Julio S. Rufas, and C. García de la Vega

Subjects

Genetics, Chromosome segregation, Autosome, Meiosis, Heterochromatin, Chromosome, Supernumerary, Biology, Chiasma, Genetics (clinical), Anaphase

Abstract

Dociostaurus genei is a grasshopper in which most of the autosomes present polymorphisms for distal heterochromatic supernumerary segments. C-banding, DAPI banding and fluorescence in situ hybridization (FISH) of a probe, which is representative of the highly repetitive DNA sequences comprising the segments, have been used to analyse the effects of the segments on chiasma formation. Results show that the supernumerary segments are associated with two major effects. First, a higher content of supernumerary heterochromatin is correlated with the formation of a lower number of chiasmata within a given chromosome complement. Secondly, because the methods used strongly suggest that the distal segments are truly terminal, they could be considered to be involved in the maintenance of achiasmate associations that persist up to the first anaphase migration. These terminal associations occurred in about 50 per cent of homozygous and heterozygous bivalents and did not impair the correct segregation of homologues at anaphase I.

Published

1998

22. [Untitled]

Author

Juan Luis Santos, José A. Suja, Jesús Page, and Julio S. Rufas

Subjects

Synaptonemal complex, Prophase, Meiosis, Polyclonal antibodies, Genetics, biology.protein, Chromosome, Nuclear protein, Biology, Cell Cycle Protein, Molecular biology, Mitosis, Cell biology

Abstract

Several techniques have been developed for protein immunolocalization in meiotic cells. However, most of them include treatments that lead to cell disruption and are only suitable for prophase-I cells. We describe a novel squash procedure of cell preparation for protein immunolabelling of different meiotic stages. This procedure is an alternative to both cryosectioning and whole spreading procedures. We present results obtained in mouse spermatocytes with three different antibodies: the MPM-2 mAb against mitotic phosphoepitopes, an anticentromere serum and a polyclonal serum against the SCP3 protein of the axial elements and lateral elements of the synaptonemal complex. The procedure was tested for single and double immunolabelling. With this technique a large number of cells at different meiotic stages can be analysed. Cell stages are easily identified and cell and chromosome structures are preserved. Thus, it allows the study of chromosome behaviour and the relationships between the different structural elements of the cell throughout meiotic divisions. Our procedure is also suitable for three-dimensional (3D) analyses and proved to be reliable in a wide range of systems including insects and mammals. In addition, the procedure may be interesting to obtain a rapid immunological diagnosis.

Published

1998

23. [Untitled]

Author

Francisco Panzera, Jesús Page, Rubén Pérez, Julio S. Rufas, and José A. Suja

Subjects

Chromosome segregation, Genetics, Prophase, Meiosis, Holocentric, Biology, Y chromosome, Metaphase, Chiasma, Anaphase

Abstract

The meiotic behaviour of the holocentric chromosomes of the heteropteran species Triatoma infestans has been analysed by means of orcein staining and C-banding on squashed spermatocytes. We have focused our analysis on chromosome 3, which shows a large distal heterochromatic band at one of the ends of both homologues. At metaphase I, and independently of the chiasma position, two alternative orientations have been observed: either the heterochromatic or the euchromatic ends of both homologues are directed to opposite poles. At anaphase I, the kinetic activity is restricted to the same chromosome end (euchromatic or heterochromatic) of each homologue. The frequencies of these two alternatives are not random and differ significantly among the five individuals analysed. However, the euchromatic ends present kinetic activity at a higher frequency than the heterochromatic ends. At metaphase II, half-bivalents also show the kinetic activity restricted to either of the chromosome ends (euchromatic or heterochromatic). The frequencies of each alternative are inverted in anaphase II compared with those scored in anaphase I. Accordingly, those ends that present kinetic activity at anaphase I segregate reductionally during the first meiotic division and equationally during the second meiotic division. These results provide sound evidence on the meiotic behaviour of holocentric chromosomes, as regards the absence of chiasma terminalization and the modes of orientation and segregation.

Published

1997

24. The osmium tetroxide-p-phenylenediamine procedure reveals the chromatid cores and kinetochores of meiotic chromosomes by light and electron microscopy

Author

José M. González-García, Carmen Antonio, J C Stockert, José A. Suja, Julio S. Rufas, and Jesús Page

Subjects

Male, Histology, Osmium Tetroxide, Scanning electron microscope, Analytical chemistry, chemistry.chemical_element, Grasshoppers, Chromatids, Phenylenediamines, Biology, Microanalysis, Chromosomes, law.invention, chemistry.chemical_compound, law, Microscopy, Animals, Osmium, Kinetochores, Staining and Labeling, Histocytochemistry, Molecular biology, Meiosis, Microscopy, Electron, Osmium tetroxide, chemistry, Transmission electron microscopy, Chromatid, Anatomy, Electron microscope

Abstract

We analyzed first-metaphase meiotic chromosomes of the grasshopper Chorthippus jucundus by two different methods, i.e., a silver impregnation technique and the osmium tetroxide-p-phenylenediamine (Os-PPD) procedure. The former was applied on squashed testes previously fixed in ethanol-acetic acid, whereas for Os-PPD the material was not subjected to any previous extraction treatment but was fixed in OsO4, treated with PPD, and embedded in Epon 812. Both techniques revealed chromatid cores and kinetochores regardless of the processing of the material (squashed or sectioned). Unstained Os-PPD sections were analyzed by light microscopy and transmission electron microscopy (TEM). The Os-PPD technique provided a high contrast of chromatid cores and kinetochores in relation to the chromatin, which revealed a low electron density. To determine the Os-PPD reaction mechanism, the PAS procedure, as well as scanning electron microscopy (SEM) backscattering and SEM X-ray microanalysis, was performed on sections. By use of the Os-PPD-PAS procedure, glycol groups formed by oxidation of osmium bound to aromatic substrates were detected in chromatid cores and kinetochores by brightfield and fluorescence microscopy. A high Z contrast was detected in these structures by backscattered electron imaging. SEM X-ray microanalysis showed osmium and phosphorus to be the main elements present on the chromatid cores. Taking into account the known reactivity of OsO4 and the present results, the possible participation of nucleic acids as well as proteins in the Os-PPD reaction mechanism and in the composition of chromatid cores and kinetochores is discussed.

Published

1996

25. Nucleolar cycle and localization of NORs in early embryos of Parascaris univalens

Author

José A. Suja, Carmen Antonio, José M. González-García, and Julio S. Rufas

Subjects

Nucleologenesis, Fibrillarin, Blastomeres, Staining and Labeling, Chromosomal Proteins, Non-Histone, Somatic cell, Nucleolus, Cell Cycle, Autoimmunity, Biology, Molecular biology, Chromatin, Prophase, Nucleolus Organizer Region, Genetics, Animals, Female, Horses, Ascaridida, Metaphase, Cell Nucleolus, In Situ Hybridization, Fluorescence, Genetics (clinical), Anaphase

Abstract

During early embryogenesis of the nematode Parascaris univalens (2n=2) the processes of chromatin diminution and segregation of the germ and somatic cell lineages take place simultaneously. In this study we analyzed the nucleolar cycle in early embryos, both in germinal and somatic blastomeres, by means of silver staining and antibodies against the nucleolar protein fibrillarin. We observed an identical nucleolar cycle in both types of blastomeres, hence, the chromatin diminution process has no effect on the nucleolar cycle of somatic blastomeres. We report the existence of outstanding differences between this cycle and those previously reported during early embryogenesis of other species. There is a true nucleolar cycle in early embryos that shows a peculiar nucleolar disorganization at prophase, and a preferential localization of prenucleolar bodies only on the euchromatic regions during nucleologenesis. Moreover, fibrillarin does not form a perichromosomal sheath in metaphase or anaphase holocentric chromosomes, probably owing to their special centromeric organization. The number and location of nucleolus organizer regions (NORs) in the chromosomal complement have been determined using silver impregnation, chromomycin A3/ distamycin A staining, and fluorescent in situ hybridization using an rDNA probe. There are only two NORs, one per chromosome, and these are located in the middle of the euchromatic central regions. This location implies that no rDNA sequences are lost in blastomeres after chromatin diminution. Moreover, the constant presence of two nucleoli in somatic blastomeres suggests that NORs are not affected during the fragmentation of euchromatic regions when this process occurs.

Published

1995

26. Dynamics of cohesin subunits in grasshopper meiotic divisions

Author

Alberto Viera, José A. Suja, Julio S. Rufas, María Teresa Parra, Adela Calvente, Jesús Page, Juan Luis Santos, José Luis Barbero, C. García de la Vega, and R. de la Fuente

Subjects

Genetics, Cohesin, Cohesin complex, Chromosomal Proteins, Non-Histone, Centromere, Mitosis, Cell Cycle Proteins, Grasshoppers, Biology, Chromosomes, Cell biology, Chromosome segregation, Establishment of sister chromatid cohesion, Meiotic Prophase I, Meiosis, Chromosome Segregation, Animals, biological phenomena, cell phenomena, and immunity, Separase, Anaphase, Genetics (clinical)

Abstract

The cohesin complex plays a key role for the maintenance of sister chromatid cohesion and faithful chromosome segregation in both mitosis and meiosis. This complex is formed by two structural maintenance of chromosomes protein family (SMC) subunits and two non-SMC subunits: an α-kleisin subunit SCC1/RAD21/REC8 and an SCC3-like protein. Several studies carried out in different species have revealed that the distribution of the cohesin subunits along the chromosomes during meiotic prophase I is not regular and that some subunits are distinctly incorporated at different cell stages. However, the accurate distribution of the different cohesin subunits in condensed meiotic chromosomes is still controversial. Here, we describe the dynamics of the cohesin subunits SMC1α, SMC3, RAD21 and SA1 during both meiotic divisions in grasshoppers. Although these subunits show a similar patched labelling at the interchromatid domain of metaphase I bivalents, SMCs and non-SMCs subunits do not always colocalise. Indeed, SA1 is the only cohesin subunit accumulated at the centromeric region of all metaphase I chromosomes. Additionally, non-SMC subunits do not appear at the interchromatid domain in either single X or B chromosomes. These data suggest the existence of several cohesin complexes during metaphase I. The cohesin subunits analysed are released from chromosomes at the beginning of anaphase I, with the exception of SA1 which can be detected at the centromeres until telophase II. These observations indicate that the cohesin components may be differentially loaded and released from meiotic chromosomes during the first and second meiotic divisions. The roles of these cohesin complexes for the maintenance of chromosome structure and their involvement in homologous segregation at first meiotic division are proposed and discussed.

Published

2012

27. Supernumerary chromosome segments and intrabivalent chiasma redistribution in Pyrgomorpha conica (Orthoptera)

Author

José A. Suja, Carmen Antonio, Carlos Vega, and Julio S. Rufas

Subjects

Genetics, medicine.medical_specialty, Heterochromatin, Cytogenetics, Chromosome, Aneuploidy, Biology, medicine.disease, Chiasma, Loss of heterozygosity, Meiosis, medicine, Supernumerary, Genetics (clinical)

Abstract

Two kinds of supernumerary chromosome segments have been found on the megameric chromosome of the grasshopper Pyrgomorpha conica. One of them is euchromatic and distally located while the other one is heterochromatic and proximally located. Their effects on chiasma distribution in heterozygous, homozygous and doubly heterozygous bivalents for these segments have been analyzed. Both segments distort chiasma distribution so that the single chiasma is preferentially formed far from the location of each supernumerary segment. This effect is more pronounced in bivalents that are homozygous for the presence of the proximal heterochromatic segment. In doubly heterozygous bivalents that possess both segments on the same chromosome the chiasma distribution is significantly different from that observed in heterozygous bivalents for each segment and a significant frequency of univalents was scored.

Published

1994

28. Inactivation or non-reactivation: what accounts better for the silence of sex chromosomes during mammalian male meiosis?

Author

Jesús Page, Alberto Viera, María Teresa Parra, Marcia Manterola, Soledad Berríos, Raúl Fernández-Donoso, Roberto de la Fuente, and Julio S. Rufas

Subjects

Male, X Chromosome, DNA Repair, Transcription, Genetic, SUMO-1 Protein, Cell Cycle Proteins, Y chromosome, Histones, Meiotic Prophase I, Histone H3, Mice, Prophase, Meiosis, Y Chromosome, Genetics, Animals, DNA Breaks, Double-Stranded, Gene Silencing, Genetics (clinical), biology, Synapsis, Nuclear Proteins, RNA-Binding Proteins, Chromatin, DNA-Binding Proteins, Chromosome Pairing, Histone, biology.protein, Pachytene Stage, RNA Polymerase II, Carrier Proteins

Abstract

During the first meiotic prophase in male mammals, sex chromosomes undergo a program of transcriptional silencing called meiotic sex chromosome inactivation (MSCI). MSCI is triggered by accumulation of proteins like BRCA1, ATR, and γH2AX on unsynapsed chromosomes, followed by local changes on the sex chromatin, including histone modifications, incorporation of specific histone variants, non-histone proteins, and RNAs. It is generally thought that MSCI represents the transition of unsynapsed chromatin from a transcriptionally active state to a repressed state. However, transcription is generally low in the whole nucleus during the early stages of the first meiotic prophase, when markers of MSCI first appear, and is then reactivated globally during pachytene. Thus, an alternative possibility is that MSCI represents the targeted maintenance and/or reinforcement of a prior repressed state, i.e., a failure to reactivate. Here, we present an analysis of the temporal and spatial appearance of transcriptional and MSCI markers, as well as chromatin modifications related to transcriptional regulation. We show that levels of RNA pol II and histone H3 acetylated at lysine 9 (H3K9ac) are low during leptotene, zygotene, and early pachytene, but increase strongly in mid-pachytene, indicating that reactivation occurs with some delay after synapsis. However, while transcription markers appear abundantly on the autosomes at mid-pachytene, they are not directed to the sex chromosomes. Interestingly, we found that chromatin modifications related to transcriptional silencing and/or MSCI, namely, histone H3 trimethylated at lysine 9 (H3K9me3), histone H3 monomethylated at lysine 4 (H3K4me1), γH2AX, SUMO1, and XMR, appear on the sex chromosomes before autosomes become reactivated. These results suggest that the onset of MSCI during late zygotene and early pachytene may prevent sex chromosome reactivation during mid-pachytene instead of promoting inactivation de novo. Additionally, we found temporal differences between the X and Y chromosomes in the recruitment of DNA repair and MSCI markers, indicating a differential regulation of these processes. We propose that many of the meiotic defects attributed to failure to silence sex chromosomes could be interpreted as a more general process of transcriptional misregulation that occurs under certain pathological circumstances in zygotene and early pachytene.

Published

2011

29. Marsupial Sex Chromosome Behaviour During Male Meiosis

Author

Jesús Page, Julio S. Rufas, Raúl Fernández-Donoso, and Soledad Berríos

Subjects

Chromosome segregation, Autosome, Meiosis, biology, Evolution of sexual reproduction, Evolutionary biology, Synapsis, Chromosome, biology.organism_classification, Chiasma, Marsupial

Abstract

The absence of homology between sex chromosomes in marsupials strongly influences their behaviour during male meiosis. The highly differentiated X and Y chromosomes perform a precise and specific meiotic program that includes pairing and segregation, but lacks the usual mechanisms of synapsis, recombination and chiasma formation that occur in the autosomes and also in the sex chromosomes of eutherian mammals. The most relevant feature of marsupial male meiosis is the development of a synaptonemal complex-derived structure called the dense plate (DP). This structure maintains the association between the asynaptic and achiasmatic sex chromosomes during the first meiotic division, contributing to the proper segregation of sex chromosomes into daughter cells. Comparison of the meiotic mechanism present in marsupials with those present in some eutherian mammals opens new perspectives concerning the origin of sex chromosomes and sex chromosome segregation in the ancestor of marsupials and placental mammals. Similarly, recent characterisation of the mechanisms involved in the inactivation of sex chromosomes during marsupial meiosis has led to the idea that somatic inactivation of sex chromosomes in mammals may have originated from the more ancient and conserved mechanism of meiotic sex chromosome inactivation. This clearly places marsupial meiosis at the heart of the discussion concerning sex chromosome evolution and the origin of gene dosage compensation in mammals.

Published

2010

30. Meiotic chromosome structure: relationship between the synaptonemal complex and the chromatid cores

Author

Julio S. Rufas, José A. Suja, Juan Luis Santos, and M. Diez

Subjects

Genetics, Spermatid, Chromosome, General Medicine, Biology, law.invention, Cell biology, Synaptonemal complex, medicine.anatomical_structure, Meiosis, law, Transmission electron microscopy, Microscopy, medicine, Chromatid, Electron microscope, Molecular Biology, Biotechnology

Abstract

The development of silver-stained synaptonemal complexes (SCs) and of chromatid cores was analyzed in squashed and surface-spread grasshopper spermatocytes using light and electron microscopy, respectively. This study was conducted to determine the relationship of the two chromosome structures and then obtain more insight into the meiotic chromosome structure. Pachytene cells observed by light microscopy showed thin silver-stained threads, representing SCs, along the centre of the bivalents. However, fully formed SCs, and an axial element corresponding to the univalent sex chromosome, appeared when these cells were observed by electron microscopy. During early diplotene no silver-stained threads were observed by light microscopy. However, fragmentation of the SCs was apparent in cells at the same stage when observed by electron microscopy. Both light and electron microscopy showed that chromosome cores were first detected in homologues of late diplotene – early diakinesis cells. During diakinesis the cores were not continuous but were interrupted where interstitial chiasmata occur. In prometaphase I – metaphase I cells these cores appeared continuous and double, i.e., each chromatid clearly showed its own core. We propose a model whereby the associated cores of sister chromatids act as frameworks for the formation of the SC lateral elements.Key words: meiosis, chromosome structure, synaptonemal complex, chromatid core.

Published

1992

31. Involvement of chromatid cohesiveness at the centromere and chromosome arms in meiotic chromosome segregation: A cytological approach

Author

José A. Suja, Carmen Antonio, and Julio S. Rufas

Subjects

Male, Genetics, Sex Chromosomes, Cohesin, Centromere, Grasshoppers, Meiotic chromosome segregation, Chromatids, Biology, Spindle apparatus, Establishment of sister chromatid cohesion, Meiosis, Animals, Sister chromatids, Chromatid, Genetics (clinical), Anaphase

Abstract

Kinetochores and chromatid cores of meiotic chromosomes of the grasshopper species Arcyptera fusca and Eyprepocnemis plorans were differentially silver stained to analyse the possible involvement of both structures in chromatid cohesiveness and meiotic chromosome segregation. Special attention was paid to the behaviour of these structures in the univalent sex chromosome, and in B univalents with different orientations during the first meiotic division. It was observed that while sister chromatid of univalents are associated at metaphase I, chromatid cores are individualised independently of their orientation. We think that cohesive proteins on the inner surface of sister chromatids, and not the chromatid cores, are involved in the chromatid cohesiveness that maintains associated sister chromatids of bivalents and univalents until anaphase I. At anaphase I sister chromatids of amphitelically oriented B univalents or spontaneous autosomal univalents separate but do not reach the poles because they remain connected at the centromere by a long strand which can be visualized by silver staining, that joins stretched sister kinetochores. This strand is normally observed between sister kinetochores of half-bivalents at metaphase II and early anaphase II. We suggest that certain centromere proteins that form the silver-stainable strand assure chromosome integrity until metaphase II. These cohesive centromere proteins would be released or modified during anaphase II to allow normal chromatid segregation. Failure of this process during the first meiotic division could lead to the lagging of amphitelically oriented univalents. Based on our results we propose a model of meiotic chromosome segregation. During mitosis the cohesive proteins located at the centromere and chromosome arms are released during the same cellular division. During meiosis those proteins must be sequentially inactivated, i.e. those situated on the inner surface of the chromatids must be eliminated during the first meiotic division while those located at the centromere must be released during the second meiotic division.

Published

1992

32. A high incidence of meiotic silencing of unsynapsed chromatin is not associated with substantial pachytene loss in heterozygous male mice carrying multiple simple robertsonian translocations

Author

Alberto Viera, María Teresa Parra, Jesús Page, Julio S. Rufas, Chiara Vasco, Maurizio Zuccotti, Soledad Berríos, Raúl Fernández-Donoso, Marcia Manterola, Silvia Garagna, and UAM. Departamento de Biología

Subjects

Male, Heterozygote, Cancer Research, Developmental Biology/Germ Cells, lcsh:QH426-470, Biología, Cell Biology/Cell Growth and Division, Chromosomal translocation, Meiocyte, Biology, Translocation, Genetic, Mice, Meiosis, Spermatocytes, Genetics, Homologous chromosome, Animals, Gene Silencing, Molecular Biology, Metaphase, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Sex Chromosomes, Autosome, Synapsis, Chromosome, Chromatin, Genetics and Genomics/Chromosome Biology, Chromosome Pairing, lcsh:Genetics, Evolutionary Biology/Nuclear Structure and Function, Female, Pachytene Stage, Research Article

Abstract

Meiosis is a complex type of cell division that involves homologous chromosome pairing, synapsis, recombination, and segregation. When any of these processes is altered, cellular checkpoints arrest meiosis progression and induce cell elimination. Meiotic impairment is particularly frequent in organisms bearing chromosomal translocations. When chromosomal translocations appear in heterozygosis, the chromosomes involved may not correctly complete synapsis, recombination, and/or segregation, thus promoting the activation of checkpoints that lead to the death of the meiocytes. In mammals and other organisms, the unsynapsed chromosomal regions are subject to a process called meiotic silencing of unsynapsed chromatin (MSUC). Different degrees of asynapsis could contribute to disturb the normal loading of MSUC proteins, interfering with autosome and sex chromosome gene expression and triggering a massive pachytene cell death. We report that in mice that are heterozygous for eight multiple simple Robertsonian translocations, most pachytene spermatocytes bear trivalents with unsynapsed regions that incorporate, in a stage-dependent manner, proteins involved in MSUC (e.g., γH2AX, ATR, ubiquitinated-H2A, SUMO-1, and XMR). These spermatocytes have a correct MSUC response and are not eliminated during pachytene and most of them proceed into diplotene. However, we found a high incidence of apoptotic spermatocytes at the metaphase stage. These results suggest that in Robertsonian heterozygous mice synapsis defects on most pachytene cells do not trigger a prophase-I checkpoint. Instead, meiotic impairment seems to mainly rely on the action of a checkpoint acting at the metaphase stage. We propose that a low stringency of the pachytene checkpoint could help to increase the chances that spermatocytes with synaptic defects will complete meiotic divisions and differentiate into viable gametes. This scenario, despite a reduction of fertility, allows the spreading of Robertsonian translocations, explaining the multitude of natural Robertsonian populations described in the mouse., Author Summary Cells have different mechanisms to assess the proper occurrence of cellular events. These mechanisms are called checkpoints and are involved in the surveillance of processes such as DNA replication and cell division. A checkpoint at the pachytene stage arrests meiosis when defects in the process of homologous chromosome synapsis and recombination are detected. In mammals, both transcriptional inactivation of chromosomal regions that are not correctly synapsed at pachytene and activation of sex chromosome genes that are normally silent during this stage could contribute to meiotic arrest. We found that when Robertsonian translocations appear in heterozygosis, many synapsis defects occur, and mechanisms that trigger transcriptional silencing of the unsynapsed chromatin are activated. However, meiotic prophase-I progression is not greatly compromised. This questions the ability of the meiotic checkpoints to halt meiosis progression when synapsis is not completed, allowing cells with synapsis defects to reach the first meiotic division. The fertility reduction of Robertsonian heterozygous mice seems to be mainly caused by errors detected by the metaphase-I checkpoint, when most of the spermatocytes die, rather than by synapsis defects. In an evolutionary context, a permissive pachytene checkpoint could contribute to increasing the chances of Robertsonian translocations to spread into natural populations.

Published

2009

33. Sequential Assembly of Centromeric Proteins in Male Mouse Meiosis

Author

Alberto Viera, José A. Suja, Rocío Gómez, María Teresa Parra, Alberto M. Pendás, Elena Llano, Julio S. Rufas, and UAM. Departamento de Biología

Subjects

Male, Cancer Research, lcsh:QH426-470, Chromosomal Proteins, Non-Histone, Biología, Centromere, Genetics and Genomics/Nuclear Structure and Function, Kinesins, Cell Cycle Proteins, Protein Serine-Threonine Kinases, Biology, Mice, Meiotic Prophase I, Prophase, Meiosis, Spermatocytes, Genetics, Animals, Interkinesis, Kinetochores, Molecular Biology, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Metaphase, Anaphase, Centromeres, INCENP, Kinetochore, Cell Biology, Cell biology, Genetics and Genomics/Chromosome Biology, lcsh:Genetics, Research Article

Abstract

10 páginas, 6 figuras.-- et al., The assembly of the mitotic centromere has been extensively studied in recent years, revealing the sequence and regulation of protein loading to this chromosome domain. However, few studies have analyzed centromere assembly during mammalian meiosis. This study specifically targets this approach on mouse spermatocytes. We have found that during prophase I, the proteins of the chromosomal passenger complex Borealin, INCENP, and Aurora-B load sequentially to the inner centromere before Shugoshin 2 and MCAK. The last proteins to be assembled are the outer kinetochore proteins BubR1 and CENP-E. All these proteins are not detected at the centromere during anaphase/telophase I and are then reloaded during interkinesis. The loading sequence of the analyzed proteins is similar during prophase I and interkinesis. These findings demonstrate that the interkinesis stage, regularly overlooked, is essential for centromere and kinetochore maturation and reorganization previous to the second meiotic division. We also demonstrate that Shugoshin 2 is necessary for the loading of MCAK at the inner centromere, but is dispensable for the loading of the outer kinetochore proteins BubR1 and CENP-E., This work was supported by grants BFU2008-00300, BFU2006-06655 and SAF-2008-03172 from Ministerio de Ciencia e Innovacion. RG has been supported by a Fundación Francisco Cobos and Ministerio de Ciencia e Innovación predoctoral fellowships.

Published

2009

34. Relationship between incomplete synapsis and chiasma localization

Author

Alberto Viera, Juan L. Santos, and Julio S. Rufas

Subjects

Genetics, Cohesin loading, Male, Cohesin, Chromosomal Proteins, Non-Histone, Synaptonemal Complex, Synapsis, Cell Cycle Proteins, Biology, Chiasma, Cell biology, Synaptonemal complex, Chromosome Pairing, Meiosis, Spermatocytes, Recombinase, Animals, Insect Proteins, Orthoptera, Homologous recombination, Genetics (clinical)

Abstract

One of the subjects within the meiotic field that has been actively investigated in the recent years is the temporal and functional relationships between meiotic recombination, cohesin loading and synaptonemal complex (SC) assembly. Although the study of meiotic mutants has shed some light, many questions remain to be answered. Here, we have studied this topic in the orthopteran Paratettix meridionalis, a species with telocentric chromosomes, which shows two unusual cytological features: pairing and synapsis of homologues during prophase I are restricted to the non-centromeric distal regions and extremely distal chiasma localization in metaphase I bivalents. In order to determine whether there is a relationship between both phenomena, we have used: (1) a spreading technique for following the ultrastructure of SC assembly and (2) immunofluorescence for SMC3 and SMC1alpha cohesin subunits, which mark the development of the axial element (a SC component); the histone gamma-H2AX, which mostly labels the sites of double-strand breaks; and the recombinase RAD51. Spermatocytes showed conspicuous polarization of both the maturation of cohesin axes and the initiation of meiotic recombination events. Consequently, it is proposed that maturation of cohesin axes, which begins in very distal regions, could drive the latter loading of recombinases to such regions. This restricted distribution of recombination events along homologues would finally be responsible for the incomplete pairing and synapsis observed in all autosomes of the complement and hence for chiasma localization.

Published

2008

35. Inverted Meiosis: The True Bugs as a Model to Study

Author

Julio S. Rufas, Jesús Page, and Alberto Viera

Subjects

Genetics, Meiosis, Haploidisation, fungi, Holocentric, Synapsis, Homologous chromosome, Interkinesis, Biology, Genetic recombination, Chromosomal crossover

Abstract

Most of the meiotic literature is based on species with monocentric chromosomes, however meiosis in protoctist, plant and animal species with holocentric chromosomes is less characterized. In some ca

Published

2008

36. A Screen for Retrotransposed Imprinted Genes Reveals an Association between X Chromosome Homology and Maternal Germ-Line Methylation

Author

María Teresa Parra, Ignacio Prieto, Margarete M. S. Heck, Ana Valdeolmillos, Julio S. Rufas, Jesús Page, Carlos Martínez-A, Juan L. Santos, Alberto Viera, José A. Suja, José Luis Barbero, and UAM. Departamento de Biología

Subjects

Male, Cancer Research, Amino Acid Transport System A, Chromosomal Proteins, Non-Histone, Biología, Cell Cycle Proteins, Chromosome segregation, 0302 clinical medicine, Spermatocytes, Testis, Tissue Distribution, Meiotic Prophase I, Genetics (clinical), Cells, Cultured, Genetics, 0303 health sciences, Nuclear Proteins, Chromatin, Cell biology, 3. Good health, Establishment of sister chromatid cohesion, Insects, Chromatid, Drosophila, Separase, biological phenomena, cell phenomena, and immunity, Research Article, Cohesin complex, lcsh:QH426-470, Grasshoppers, Biology, Chromatids, Models, Biological, Chromosomes, 03 medical and health sciences, Sister chromatids, Animals, Molecular Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Cohesin, Genetics and Genomics, Cell Biology, Spermatogonia, Chromosome Pairing, Protein Subunits, lcsh:Genetics, 030217 neurology & neurosurgery

Abstract

A previous version of this article appeared as an Early Online Release on January 2, 2007 (doi:10.1371/journal.pgen.0030028.eor)., The cohesin complexes play a key role in chromosome segregation during both mitosis and meiosis. They establish sister chromatid cohesion between duplicating DNA molecules during S-phase, but they also have an important role during postreplicative double-strand break repair in mitosis, as well as during recombination between homologous chromosomes in meiosis. An additional function in meiosis is related to the sister kinetochore cohesion, so they can be pulled by microtubules to the same pole at anaphase I. Data about the dynamics of cohesin subunits during meiosis are scarce; therefore, it is of great interest to characterize how the formation of the cohesin complexes is achieved in order to understand the roles of the different subunits within them. We have investigated the spatio-temporal distribution of three different cohesin subunits in prophase I grasshopper spermatocytes. We found that structural maintenance of chromosome protein 3 (SMC3) appears as early as preleptotene, and its localization resembles the location of the unsynapsed axial elements, whereas radiation-sensitive mutant 21 (RAD21) (sister chromatid cohesion protein 1, SCC1) and stromal antigen protein 1 (SA1) (sister chromatid cohesion protein 3, SCC3) are not visualized until zygotene, since they are located in the synapsed regions of the bivalents. During pachytene, the distribution of the three cohesin subunits is very similar and all appear along the trajectories of the lateral elements of the autosomal synaptonemal complexes. However, whereas SMC3 also appears over the single and unsynapsed X chromosome, RAD21 and SA1 do not. We conclude that the loading of SMC3 and the non-SMC subunits, RAD21 and SA1, occurs in different steps throughout prophase I grasshopper meiosis. These results strongly suggest the participation of SMC3 in the initial cohesin axis formation as early as preleptotene, thus contributing to sister chromatid cohesion, with a later association of both RAD21 and SA1 subunits at zygotene to reinforce and stabilize the bivalent structure. Therefore, we speculate that more than one cohesin complex participates in the sister chromatid cohesion at prophase I., This work was supported by grants BFU2005–05668-C03–01, BFU2006–06655, BFU2005–01266, BFU2005–02431, and BFU2006–04406 from Ministerio de Educación y Ciencia, España, and grants 1001160016 and 11/BCB/013 from Universidad Autónoma de Madrid and Comunidad de Madrid. The Department of Immunology and Oncology was founded and is supported by the Spanish Council for Scientific Research (CSIC).

Published

2007

37. Chromatid Cores in Meiotic Chromosome Structure and Segregation

Author

Julio S. Rufas and José A. Suja

Subjects

Synaptonemal complex, Cohesin, biology, Meiosis, Condensin, Prophase I, Meiotic chromosome, biology.protein, Chromatid, biological phenomena, cell phenomena, and immunity, Mitosis, Cell biology

Abstract

There is an extensive literature concerning the structure of mitotic chromosomes and the participation of proteinaceous axial structures, the chromatid cores, in their organization. However, the involvement of the chromatid cores in the structure and segregation of meiotic chromosomes is less known. This chapter reviews the occurrence and behaviour of the chromatid cores in condensed meiotic chromosomes, particularly in grasshopper species. We present current models that relate chromatid cores with the lateral elements of the synaptonemal complex, a tripartite structure present along synapsed homologues during the pachytene stage of prophase I. Additionally, we summarize recent data about the relationship between the chromatid cores, DNA topoisomerase IIα, condensin and cohesin complexes.

Published

2007

38. Condensin I reveals new insights on mouse meiotic chromosome structure and dynamics

Author

Alberto Viera, José A. Suja, Julio S. Rufas, María Teresa Parra, Kyoko Yokomori, John A. Schmiesing, Rocío Gómez, and UAM. Departamento de Biología

Subjects

Male, Condensin, Biología, Mitosis, lcsh:Medicine, macromolecular substances, Chromatids, Mice, Prophase, Spermatocytes, Centromere, Medicine and Health Sciences, Animals, Humans, Prometaphase, lcsh:Science, Metaphase, Genetics, Adenosine Triphosphatases, Multidisciplinary, Cohesin, biology, lcsh:R, Cell Biology, Telomere, Chromosomes, Mammalian, Spermatogonia, Cell biology, DNA-Binding Proteins, Mice, Inbred C57BL, Meiosis, Protein Subunits, Telomeres, Chromosome Structures, Multiprotein Complexes, biology.protein, Chromatid, lcsh:Q, Research Article

Abstract

Chromosome shaping and individualization are necessary requisites to warrant the correct segregation of genomes in either mitotic or meiotic cell divisions. These processes are mainly prompted in vertebrates by three multiprotein complexes termed cohesin and condensin I and II. In the present study we have analyzed by immunostaining the appearance and subcellular distribution of condensin I in mouse mitotic and meiotic chromosomes. Our results demonstrate that in either mitotically or meiotically dividing cells, condensin I is loaded onto chromosomes by prometaphase. Condensin I is detectable as a fuzzy axial structure running inside chromatids of condensed chromosomes. The distribution of condensin I along the chromosome length is not uniform, since it preferentially accumulates close to the chromosome ends. Interestingly, these round accumulations found at the condensin I axes termini colocalized with telomere complexes. Additionally, we present the relative distribution of the condensin I and cohesin complexes in metaphase I bivalents. All these new data have allowed us to propose a comprehensive model for meiotic chromosome structure.

Published

2007

39. Meiotic pairing and segregation of achiasmate sex chromosomes in Eutherian mammals: The role of SYCP3 protein

Author

María Teresa Parra, Alberto Viera, Jesús Page, José A. Suja, Roberto de la Fuente, Rocío Gómez, Adela Calvente, Julio S. Rufas, and UAM. Departamento de Biología

Subjects

Male, Cancer Research, lcsh:QH426-470, Biología, Pseudoautosomal region, Centromere, Biology, Y chromosome, Eukaryotic chromosome structure, Chromosome segregation, Histones, Mongolian gerbil (Meriones unguiculatus), Spermatocytes, Chromosome Segregation, Genetics, Animals, Small supernumerary marker chromosome, Molecular Biology, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Recombination, Genetic, Recombinant proteins, B chromosome, Sex Chromosomes, Models, Genetic, Synaptonemal Complex, Synapsis, Nuclear Proteins, Cell Biology, Chromatin, Synaptonemal complex, lcsh:Genetics, Chromosome Pairing, Rad51 Recombinase, Gerbillinae, Research Article

Abstract

In most eutherian mammals, sex chromosomes synapse and recombine during male meiosis in a small region called pseudoautosomal region. However in some species sex chromosomes do not synapse, and how these chromosomes manage to ensure their proper segregation is under discussion. Here we present a study of the meiotic structure and behavior of sex chromosomes in one of these species, the Mongolian gerbil (Meriones unguiculatus). We have analyzed the location of synaptonemal complex (SC) proteins SYCP1 and SYCP3, as well as three proteins involved in the process of meiotic recombination (RAD51, MLH1, and γ-H2AX). Our results show that although X and Y chromosomes are associated at pachytene and form a sex body, their axial elements (AEs) do not contact, and they never assemble a SC central element. Furthermore, MLH1 is not detected on the AEs of the sex chromosomes, indicating the absence of reciprocal recombination. At diplotene the organization of sex chromosomes changes strikingly, their AEs associate end to end, and SYCP3 forms an intricate network that occupies the Y chromosome and the distal region of the X chromosome long arm. Both the association of sex chromosomes and the SYCP3 structure are maintained until metaphase I. In anaphase I sex chromosomes migrate to opposite poles, but SYCP3 filaments connecting both chromosomes are observed. Hence, one can assume that SYCP3 modifications detected from diplotene onwards are correlated with the maintenance of sex chromosome association. These results demonstrate that some components of the SC may participate in the segregation of achiasmate sex chromosomes in eutherian mammals., Author Summary Meiosis is a special kind of cell division that leads to the formation of gametes. During meiosis the number of chromosomes must be halved in the daughter cells, and to do this properly, most organisms use an amazing strategy: during the first of the two meiotic divisions, homologous chromosomes associate in pairs, undergo a reciprocal genetic interchange, and then each member of the pair segregates into a different daughter cell. Genetic exchange, called meiotic recombination, is a key process to ensure that homologous chromosomes remain tightly associated until they segregate. In general, sex chromosomes are subjected to the same processes as the rest of chromosomes. But, of course, exceptions exist. This is the case in the Mongolian gerbil, a mammal whose sex chromosomes pair and segregate during male meiosis without undergoing meiotic recombination. We have found that they are able to do this because some proteins of a meiosis-specific structure, the synaptonemal complex, are reorganized to maintain sex chromosomes associated until they segregate into daughter cells. This kind of behavior resembles the situation found in marsupials and some insect species, indicating a recurrent role of synaptonemal complex components in chromosome segregation when meiotic recombination is missing.

Published

2007

40. Involvement of synaptonemal complex proteins in sex chromosome segregation during marsupial male meiosis

Author

Ignacio Prieto, Jesús Page, Raúl Fernández-Donoso, José Luis Barbero, Soledad Berríos, María Teresa Parra, Julio S. Rufas, Roberto de la Fuente, Alberto Viera, José A. Suja, and UAM. Departamento de Biología

Subjects

Male, Cancer Research, lcsh:QH426-470, Biología, Biology, Lateral element, Marsupials, Chromosomal crossover, Chromosome segregation, Meiosis, Spermatocytes, Chromosome Segregation, Phosphoprotein Phosphatases, Genetics, Animals, Meiotic Prophase I, Central element, Molecular Biology, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Anaphase, Sex Chromosomes, Synaptonemal Complex, Synapsis, Nuclear Proteins, Cromosomas Sexuales, Cell Biology, Telomere, Genetics/Chromosome Biology, Chromosome Pairing, Synaptonemal complex, lcsh:Genetics, Marsupialia, Evolutionary biology, Research Article

Abstract

Marsupial sex chromosomes break the rule that recombination during first meiotic prophase is necessary to ensure reductional segregation during first meiotic division. It is widely accepted that in marsupials X and Y chromosomes do not share homologous regions, and during male first meiotic prophase the synaptonemal complex is absent between them. Although these sex chromosomes do not recombine, they segregate reductionally in anaphase I. We have investigated the nature of sex chromosome association in spermatocytes of the marsupial Thylamys elegans, in order to discern the mechanisms involved in ensuring their proper segregation. We focused on the localization of the axial/lateral element protein SCP3 and the cohesin subunit STAG3. Our results show that X and Y chromosomes never appear as univalents in metaphase I, but they remain associated until they orientate and segregate to opposite poles. However, they must not be tied by a chiasma since their separation precedes the release of the sister chromatid cohesion. Instead, we show they are associated by the dense plate, a SCP3-rich structure that is organized during the first meiotic prophase and that is still present at metaphase I. Surprisingly, the dense plate incorporates SCP1, the main protein of the central element of the synaptonemal complex, from diplotene until telophase I. Once sex chromosomes are under spindle tension, they move to opposite poles losing contact with the dense plate and undergoing early segregation. Thus, the segregation of the achiasmatic T. elegans sex chromosomes seems to be ensured by the presence in metaphase I of a synaptonemal complex-derived structure. This feature, unique among vertebrates, indicates that synaptonemal complex elements may play a role in chromosome segregation., Synopsis Meiosis is the fascinating kind of cell division that leads to the formation of gametes, and thus is essential for sexual reproduction. During meiosis, the part of our genome coming from our father and that coming from our mother play the last act of a love story initiated at the very moment of fertilization. This performance includes the search and close pairing of each chromosome with its homolog, the interchange of their genetic information, and their ultimate segregation into different cells. Everything occurs in an ordered and proper fashion because each chromosome is able to recognize its homolog and recombine with it. This ensures they are correctly transmitted to the next generation. But exceptions exist to this general rule. The authors show in this report that in the meiosis of the South American marsupial, Thylamys elegans, the sex chromosomes have the ability to segregate without undergoing meiotic recombination. The sex chromosomes take profit of the organization of a structure only present in marsupials, the dense plate, which serves the purpose of maintaining X and Y chromosomes associated until they segregate to different daughter cells. Surprisingly, this dense plate is composed of two proteins of the synaptonemal complex not meant to be at that place at that time. This finding teaches us that wildlife has plenty of way-out species, most of them unexplored, which challenge our accepted paradigms.

Published

2006

41. A Perikinetochoric Ring Defined by MCAK and Aurora-B as a Novel Centromere Domain

Author

Alberto Viera, José A. Suja, Julio S. Rufas, Adela Calvente, María Teresa Parra, Linda Wordeman, Rocío Gómez, Jesús Page, and UAM. Departamento de Biología

Subjects

Male, Cancer Research, lcsh:QH426-470, Biología, Centromere, Aurora B kinase, Mitosis, Kinesins, Cell Cycle Proteins, Spindle Apparatus, Biology, Protein Serine-Threonine Kinases, Models, Biological, Aurora-B, Chromosomes, Chromosome segregation, Mice, Aurora Kinases, Spermatocytes, Chromosome Segregation, Genetics, Animals, Aurora Kinase B, Tissue Distribution, Telophase, Prometaphase, Meiotic Prophase I, Kinetochores, Molecular Biology, Metaphase, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Anaphase, Kinetochore, Nuclear Proteins, Cell Biology, Genetics/Chromosome Biology, Cell biology, DNA-Binding Proteins, Mice, Inbred C57BL, lcsh:Genetics, Meiosis, Tension, Research Article, MCAK

Abstract

Mitotic Centromere-Associated Kinesin (MCAK) is a member of the kinesin-13 subfamily of kinesin-related proteins. In mitosis, this microtubule-depolymerising kinesin seems to be implicated in chromosome segregation and in the correction of improper kinetochore-microtubule interactions, and its activity is regulated by the Aurora-B kinase. However, there are no published data on its behaviour and function during mammalian meiosis. We have analysed by immunofluorescence in squashed mouse spermatocytes, the distribution and possible function of MCAK, together with Aurora-B, during both meiotic divisions. Our results demonstrate that MCAK and Aurora-B colocalise at the inner domain of metaphase I centromeres. Thus, MCAK shows a “cone”-like three-dimensional distribution beneath and surrounding the closely associated sister kinetochores. During the second meiotic division, MCAK and Aurora-B also colocalise at the inner centromere domain as a band that joins sister kinetochores, but only during prometaphase II in unattached chromosomes. During chromosome congression to the metaphase II plate, MCAK relocalises and appears as a ring below each sister kinetochore. Aurora-B also relocalises to appear as a ring surrounding and beneath kinetochores but during late metaphase II. Our results demonstrate that the redistribution of MCAK at prometaphase II/metaphase II centromeres depends on tension across the centromere and/or on the interaction of microtubules with kinetochores. We propose that the perikinetochoric rings of MCAK and Aurora-B define a novel transient centromere domain at least in mouse chromosomes during meiosis. We discuss the possible functions of MCAK at the inner centromere domain and at the perikinetochoric ring during both meiotic divisions., Synopsis The centromere is a chromosome domain essential for the correct partitioning of chromosomes during mitotic and meiotic cell divisions. MCAK is a centromeric protein that depolymerises microtubules, and seems to be implicated in chromosome segregation, and in the correction of improper microtubule interactions with the chromosome. However, there are no published data on its behaviour and function during meiotic divisions. Here, Parra et al. analyse the pattern of distribution of MCAK during male mouse meiosis in relation to Aurora-B, a kinase that regulates its activity. They show that MCAK and Aurora-B appear at the inner domain of metaphase I bivalents and unaligned metaphase II chromosomes. Most importantly, the authors discovered that these proteins relocalise to a novel perikinetochoric ring in aligned metaphase II chromosomes. The discovery of this novel structure adds a new dimension to the understanding of kinetochore structure and biology. The authors propose that, at least for mouse centromeres, the perikinetochoric ring represents a transient centromere domain whose appearance depends on tension across centromeres once microtubules interact with both sister kinetochores. This study shows that the analysis of the behaviour of different centromere proteins during meiosis can offer new insights concerning the centromere functionality.

Published

2006

42. Mammalian SGO2 appears at the inner centromere domain and redistributes depending on tension across centromeres during meiosis II and mitosis

Author

Rocío Gómez, José Luis Barbero, Fernando Roncal, María Teresa Parra, Candelas Carreiro, Ana Valdeolmillos, Alberto Viera, Julio S. Rufas, and José A. Suja

Subjects

Male, Condensin, Centromere, Scientific Report, Fluorescent Antibody Technique, Cell Cycle Proteins, Biology, Biochemistry, Mice, Spermatocytes, Genetics, Sister chromatids, Animals, Interkinesis, Telophase, Molecular Biology, Cohesin, Meiosis II, Synapsis, Nuclear Proteins, Phosphoproteins, Cell biology, Establishment of sister chromatid cohesion, DNA-Binding Proteins, Meiosis, biology.protein

Abstract

Shugoshin (SGO) is a family of proteins that protect centromeric cohesin complexes from release during mitotic prophase and from degradation during meiosis I. Two mammalian SGO paralogues - SGO1 and SGO2 - have been identified, but their distribution and function during mammalian meiosis have not been reported. Here, we analysed the expression of SGO2 during male mouse meiosis and mitosis. During meiosis I, SGO2 accumulates at centromeres during diplotene, and colocalizes differentially with the cohesin subunits RAD21 and REC8 at metaphase I centromeres. However, SGO2 and RAD21 change their relative distributions during telophase I when sister-kinetochore association is lost. During meiosis II, SGO2 shows a striking tension-dependent redistribution within centromeres throughout chromosome congression during prometaphase II, as it does during mitosis. We propose a model by which the redistribution of SGO2 would unmask cohesive centromere proteins, which would be then released or cleaved by separase, to trigger chromatid segregation to opposite poles.

Published

2006

43. Sex chromosomes, synapsis, and cohesins: a complex affair

Author

Alberto Viera, Adela Calvente, José A. Suja, Roberto de la Fuente, María Teresa Parra, Rocío Gómez, Soledad Berríos, Julio S. Rufas, Jesús Page, Raúl Fernández-Donoso, Juan L. Santos, and UAM. Departamento de Biología

Subjects

Bioquímica, Cohesin complex, GeneralLiterature_INTRODUCTORYANDSURVEY, Chromosomal Proteins, Non-Histone, Cell Cycle Proteins, Biology, Protein Serine-Threonine Kinases, Chromosomal crossover, Prophase, Meiosis, Genetics, Homologous chromosome, Animals, Humans, GeneralLiterature_REFERENCE(e.g.,dictionaries,encyclopedias,glossaries), Genetics (clinical), Sex Chromosomes, Cohesin, Biología celular, BRCA1 Protein, Microbiología Eucariota, Synapsis, Nuclear Proteins, Synaptonemal complex, Chromosome Pairing, ComputingMethodologies_DOCUMENTANDTEXTPROCESSING

Abstract

During first meiotic prophase, homologous chromosomes are held together by the synaptonemal complex, a tripartite proteinaceous structure that extends along the entire length of meiotic bivalents. While this feature is applicable for autosomes, sex chromosomes often escape from this rule. Many species present sex chromosomes that differ between them in their morphology, length, and gene content. Moreover, in some species, sex chromosomes appear in a single dose in one of the sexes. In all of these cases, the behavior of sex chromosomes during meiosis is conspicuously affected, and this includes the assembly and dynamics of the synaptonemal complex. We review in this study the structure of the synaptonemal complex in the sex chromosomes of three groups of organisms, namely: mammals, orthopterans, and hemipterans, which present different patterns of sex chromosome structure and behavior. Of special interest is the analysis of the organization of the axial/lateral elements of the synaptonemal complex in relation to other axial structures organized along meiotic chromosomes, mainly the cohesin axis. The differences found in the behavior of both axial structures reveal that while the organization of a cohesin axis along sex chromosomes is a conserved feature in most organisms and it shows very little morphological variations, the axial/lateral elements of the synaptonemal complex present a wide range of structural modifications on these chromosomes.

Published

2006

44. DNA double-strand breaks and homology search: inferences from a species with incomplete pairing and synapsis

Author

Rocío Gómez, M. Teresa Parra, Jesús Page, Adela Calvente, Alberto Viera, Julio S. Rufas, José A. Suja, and Juan L. Santos

Subjects

Male, X Chromosome, RAD51, Grasshoppers, Biology, Chromosomes, Chromosomal crossover, Histones, Meiosis, Spermatocytes, Homologous chromosome, Animals, Meiotic Prophase I, Genetics, Cell Nucleus, Chromosome Aberrations, Cohesin, Synaptonemal Complex, Synapsis, Cell Biology, DNA, Chiasma, Cell biology, Synaptonemal complex, Chromosome Pairing, biological phenomena, cell phenomena, and immunity, DNA Damage

Abstract

The relationship between meiotic recombination events and different patterns of pairing and synapsis has been analysed in prophase I spermatocytes of the grasshopper Stethophyma grossum, which exhibit very unusual meiotic characteristics, namely (1) the three shortest bivalents achieve full synapsis and do not show chiasma localisation; (2) the remaining eight bivalents show restricted synapsis and proximal chiasma localisation, and (3) the X chromosome remains unsynapsed. We have studied by means of immunofluorescence the localisation of the phosphorylated histone H2AX (γ-H2AX), which marks the sites of double-strand breaks; the SMC3 cohesin subunit, which is thought to have a close relationship to the development of the axial element (a synaptonemal complex component); and the recombinase RAD51. We observed a marked nuclear polarization of both the maturation of SMC3 cohesin axis and the ulterior appearance of γ-H2AX and RAD51 foci, these being exclusively restricted to those chromosomal regions that first form cohesin axis stretches. This polarised distribution of recombination events is maintained throughout prophase I over those autosomal regions that are undergoing, or about to undergo, synapsis. We propose that the restricted distribution of recombination events along the chromosomal axes in the spermatocytes is responsible for the incomplete presynaptic homologous alignment and, hence, for the partial synaptonemal complex formation displayed by most bivalents.

Published

2005

45. Size heterogeneity of telomeric DNA in mouse meiotic chromosomes

Author

Julio S. Rufas, Alberto Viera, María Teresa Parra, and José A. Suja

Subjects

Male, Biology, chemistry.chemical_compound, Mice, Meiosis, Genetics, medicine, Animals, Molecular Biology, Metaphase, Mitosis, Genetics (clinical), In Situ Hybridization, Fluorescence, Polymorphism, Genetic, medicine.diagnostic_test, Peptide nucleic acid, Chromosome, DNA, Telomere, Chromosomes, Mammalian, Chromatin, Mice, Inbred C57BL, chemistry, Fluorescence in situ hybridization

Abstract

Heterogeneity for the length of telomeric DNA sequences has been found among different mitotic chromosomes in several mammalian species. However, there are no studies reporting such heterogeneity in meiotic chromosomes. To analyse this heterogeneity we have performed fluorescence in situ hybridization with a telomeric (C3TA2)3 peptide nucleic acid (PNA) probe on spread metaphase chromosomes during both male mouse meiotic divisions. Our results show that independently of the meiotic division, telomeric DNA signals were always surrounded by DAPI-stained chromatin, even at centromeric regions. Moreover, we have found heterogeneity for the size of telomeric DNA signals among different chromosomes, between homologues, and even within a given chromosome. We discuss the functional significance of the location of telomeric DNA in condensed meiotic chromosomes, and then the possible origin for the different polymorphisms found.

Published

2002

46. Expression and behaviour of CENP-E at kinetochores during mouse spermatogenesis

Author

Ana Valdeolmillos, José A. Suja, María Teresa Parra, Julio S. Rufas, Tim J. Yen, Jesús Page, and Dacheng He

Subjects

Male, Chromosomal Proteins, Non-Histone, Macromolecular Substances, Immunoblotting, Fluorescent Antibody Technique, macromolecular substances, Centromere protein E, Biology, Mice, Centromere, Genetics, Homologous chromosome, Animals, Prometaphase, Kinetochores, Spermatogenesis, Genetics (clinical), Metaphase, Kinetochore, Meiosis II, Spindle apparatus, Cell biology, Mice, Inbred C57BL, Spindle checkpoint, Meiosis, Anaphase, Biomarkers

Abstract

Centromere protein E (CENP-E) is a microtubule motor protein localised in the outer kinetochore plate and in the fibrous corona that relocalises to the midzone in early anaphase. While its expression in somatic cells has been widely analysed, an accurate description of its behaviour during the two meiotic divisions has not yet been reported. We have carefully analysed by immunofluorescence the subcellular distribution of CENP-E during mouse spermatogenesis. CENP-E first appears during late diakinesis/early prometaphase I as very bright C-shaped or "crescent" signals at each homologous centromere. These crescent CENP-E signals are also observed in unaligned prometaphase I bivalents that are not attached to spindle microtubules, while in bioriented metaphase I bivalents two kinds of fainter signals are observed. Thus, some bivalents present a plate-like signal while others show a pair of spots representing sister kinetochores at each homologous centromere. Double labelling of CENP-E with CENP-G and an anti-centromere serum indicates that in meiosis CENP-E is also located at the outer kinetochore plate and the fibrous corona. During early anaphase I CENP-E relocalises from kinetochores to the midzone where it is detected as fibrous strands, although some residual labelling persists at kinetochores until telophase I. During this stage CENP-E is detected as two parallel plates at the intercellular bridge. The general pattern of labelling during meiosis II is similar to that found during meiosis I. Our results suggest that CENP-E is implicated in the spindle checkpoint, and in chromosome alignment, during the two meiotic divisions in vertebrate males. We also demonstrate that the centromere changes its structure once alignment of all bivalents at the metaphase I plate has been reached.

Published

2002

47. Mammalian STAG3 is a cohesin specific to sister chromatid arms in meiosis I

Author

Leonor Kremer, Ignacio Prieto, José A. Suja, Nieves Pezzi, Julio S. Rufas, Carlos Martínez-A, and José Luis Barbero

Subjects

Male, Cohesin complex, Chromosomal Proteins, Non-Histone, Centromere, Fluorescent Antibody Technique, Cell Cycle Proteins, Biology, Chromatids, Chromosome segregation, Fungal Proteins, Mice, Organ Culture Techniques, Spermatocytes, Chromosome Segregation, Testis, Sister chromatids, Animals, Genetics, Mammals, Cohesin, Synapsis, Nuclear Proteins, Cell Biology, Haplorhini, Cell biology, Establishment of sister chromatid cohesion, DNA-Binding Proteins, Meiosis, Chromatid, biological phenomena, cell phenomena, and immunity, Separase, Sister Chromatid Exchange

Abstract

Cohesins, which have been characterized in budding yeast1,2 and Xenopus3, are multisubunit protein complexes involved in sister chromatid cohesion. Regulation of the interactions among different cohesin subunits and the assembly/disassembly of the cohesin complex to chromatin are key steps in chromosome segregation. We previously characterized the mammalian STAG3 protein as a component of the synaptonemal complex that is specifically expressed in germinal cells4, although its function in meiosis remains unknown. Here we show that STAG3 has a role in sister chromatid arm cohesion during mammalian meiosis I. Immunofluorescence results in prophase I cells suggest that STAG3 is a component of the axial/lateral element of the synaptonemal complex. In metaphase I, STAG3 is located at the interchromatid domain and is absent from the chiasma region. In late anaphase I and the later stages of meiosis, STAG3 is not detected. STAG3 interacts with the structural maintenance chromosome proteins SMC1 and SMC3, which have been reported to be subunits of the mitotic cohesin complex2,3. We propose that STAG3 is a sister chromatid arm cohesin that is specific to mammalian meiosis I.

Published

2001

48. Phosphorylated proteins are involved in sister-chromatid arm cohesion during meiosis I

Author

Carmen Antonio, Julio S. Rufas, José A. Suja, and Alain Debec

Subjects

Male, Silver Staining, Grasshoppers, Biology, Chromatids, Protein Serine-Threonine Kinases, Meiosis, Spermatocytes, Sister chromatids, Animals, Phosphorylation, Kinetochores, Mitosis, Metaphase, Anaphase, Genetics, Chromosome, Cell Biology, Telomere, Phosphoproteins, Chiasma, Establishment of sister chromatid cohesion, Microscopy, Electron, Microscopy, Fluorescence, Insect Proteins, Chromatid, Protein Processing, Post-Translational, Sister Chromatid Exchange

Abstract

Sister-chromatid arm cohesion is lost during the metaphase I/anaphase I transition to allow homologue separation. To obtain needed information on this process we have analysed in grasshopper bivalents the sequential release of arm cohesion in relation to the behaviour of chromatid axes. Results show that sister axes are associated during early metaphase I but separate during late metaphase I leading to a concomitant change of chromosome structure that implies the loss of sister-kinetochore cohesion. Afterwards, homologues initiate their separation asynchronously depending on their size, and number and position of chiasmata. In all bivalents thin chromatin strands at the telomeres appeared as the last point of contact between sister chromatids. Additionally, we have analysed the participation of phosphoproteins recognised by the MPM-2 monoclonal antibody against mitotic phosphoproteins in arm cohesion in bivalents and two different kinds of univalents. Results show the absence of MPM-2 phosphoproteins at the interchromatid domain in mitotic chromosomes and meiotic univalents, but their presence in metaphase I bivalents. These phosphoproteins are lost at the onset of anaphase I. Taken together, these data have prompted us to propose a ‘working’ model for the release of arm cohesion during meiosis I. The model suggests that MPM-2 phosphoproteins may act as cohesive proteins associating sister axes. Their modification, once all bivalents are correctly aligned at the metaphase plate, would trigger a change of chromosome structure and the sequential release of sister-kinetochore, arm, and telomere cohesions.

Published

1999

49. Meiosis in holocentric chromosomes: kinetic activity is randomly restricted to the chromatid ends of sex univalents in Graphosoma italicum (Heteroptera)

Author

José M. González-García, José A. Suja, Carmen Antonio, and Julio S. Rufas

Subjects

Male, Silver Staining, Insecta, X Chromosome, Biology, Chromatids, Chromosome segregation, chemistry.chemical_compound, Meiosis, Spermatocytes, Genetics, Nucleolus Organizer Region, Sister chromatids, Animals, Metaphase, X chromosome, In Situ Hybridization, Fluorescence, Cell biology, chemistry, Sex Chromatin, Holocentric, Microscopy, Electron, Scanning, Chromatid, Chromomycin A3, Female, biological phenomena, cell phenomena, and immunity

Abstract

We have determined the number and location of the nucleolar organizing regions in spermatocytes of Graphosoma italicum (2n = 12A + XYmale/XXfemale) by means of silver impregnation, chromomycin A3/distamycin A staining and fluorescence in situ hybridization. The identification of only one nucleolar organizing region located at one of the X chromosome ends has provided a suitable cytological marker to analyse the segregation of this univalent and that of the XY pseudobivalent during the first and second meiotic divisions respectively. Our results clearly show that at first meiotic metaphase the chromatids of the X chromosome are orientated with their long axes perpendicular to the polar axis. Although the kinetic activity is restricted to only one end in both X chromatids during the first meiotic division, both ends of the same chromatid have the same probability of showing such kinetic activity. In this sense, we also report that the chromatid segregation may be initiated either at the same sister chromatid ends or at opposite ends in each chromatid. Thus, this indicates a sex chromatid independence as regards to the chromatid segregation during the first meiotic division. Throughout the second meiotic division both ends of the X chromatid are involved with the same probability in the end-to-end association to conform the XY pseudobivalent. This also implies a random localization of the kinetic activity at the ends opposite to those involved in the end-to-end association.

Published

1996

50. The telochore: a telomeric differentiation of the chromosome axis

Author

Julio S. Rufas and José A. Suja

Subjects

Genetics, Male, Silver Staining, Cohesin, Base Sequence, Molecular Sequence Data, Grasshoppers, Biology, Chromatids, Telomere, Chiasma, Meiosis, Nucleoproteins, Spermatocytes, Homologous chromosome, Sister chromatids, Animals, Chromatid, Metaphase, Satellite chromosome, Anaphase

Abstract

We have analysed by means of silver staining the structure of the chromosome axis at the telomeres of meiotic chromosomes in three different grasshopper species. At metaphase I the chromatid axes run the length of the chromatids although they do not reach the chromosome ends. The axes of sister chromatids are associated and show a round differentiation at their distal ends that we have named the 'telochore'. Telochores never contact the chromosome ends: there is always some chromatin beyond them. In late metaphase I bivalents with a distal chiasma, anaphase I and metaphase II half-bivalents and anaphase II chromatids, the axes clearly possess one telochore in each chromosome end. These results seem to indicate that telochores are differentiations of the distal ends of chromatids. We discuss the possible structural significance of telochores according to the current scaffold/radial loop model of chromatin organization of eukaryotic metaphase chromosomes. Additionally, we suggest the possible functional role of the telochore as a nucleoprotein domain forming a protective cap for telomeric DNA.

Published

1994