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1. Classification and molecular organization of satellites elucidated by phylogenetic network analysis – examples from Triturus salamanders and Palorus beetles

Author

Arntzen Jw

Subjects
Genetics, Genetic diversity, biology, Satellite DNA, Genetic Variation, Phylogenetic network, DNA, Satellite, biology.organism_classification, Triturus, DNA sequencing, Coleoptera, Tandem repeat, Phylogenetics, Genus, Animals, Phylogeny, Genetics (clinical)
Abstract

A phylogenetic network of 244 satellite DNA sequences across five species of aquatic salamanders (genus Triturus) revealed four types of satellite DNAs in a 'p'-shaped 1-2*-3-4-2* arrangement. Analysis of dimer and trimer DNA sequences revealed a prevalence of homosequential (e.g. 1-1, 2-2) and particular (1-4 and 2-3) heterosequential repeat motifs. Genetic diversity across types and species phylogeny indicated that type 1 and type 4 are derived from types 2 and 3. Support was also found for alternating motifs in Palorus flour beetle tandem repeats. The results were statistically significant, whether or not the underlying satellite DNA phylogenies were robust under bootstrap analysis.

Published
2002

2. Lampbrush chromosomes and chiasmata of sex-reversed crested newts

Author

B. M. N. Wallace, Gamal M. Badawy, and H. Wallace

Subjects
Male, Sex Characteristics, Somatic cell, Disorders of Sex Development, Chromosome Mapping, Anatomy, Breeding, Biology, Long arm, biology.organism_classification, Triturus, Chromosomes, Bivalent (genetics), Chiasma, Sexual dimorphism, Meiosis, Lampbrush chromosome, Genetics, Animals, Female, Genetics (clinical)
Abstract

Triturus cristatus carnifex provides a particularly clear example of sexual dimorphism for chiasma frequency and localisation. Oocytes from normal XX females routinely carry one proximal chiasma on each arm of their lampbrush bivalents. Spermatocytes from normal XY males have more numerous and relatively distal chiasmata. Lampbrush chromosomes from the oocytes of sex-reversed XY neofemales are found to resemble those from normal oocytes in having one proximal chiasma on each bivalent arm. A comparison of particular markers on the heteromorphic long arm of chromosome 1 provides evidence to equate the lampbrush 1A to somatic 1A, and confirms previous reports that lampbrush chromosome 1A is slightly longer than 1B. The XY sex bivalent of neofemales does not show any obvious heteromorphy of recognised marker loops.

Published
1998

3. Molecular structure of the rDNA intergenic spacer (IGS) in Triturus: implications for the hypervariability of rDNA loci

Author

F. Andronico, Irma Nardi, S. De Lucchini, DE LUCCHINI, Stefania, Andronico, F, and Nardi, I.

Subjects
Genetics, RIBOSOMAL-RNA GENES, VULGARIS-MERIDIONALIS AMPHIBIA, REPETITIVE DNA-SEQUENCE, FLANKING SEQUENCES, TRANSCRIPTION, NUCLEOLUS, URODELA, Base Sequence, Deoxyribonuclease BamHI, Recombination hotspot, Molecular Sequence Data, Nucleic acid sequence, Genetic Variation, Sequence alignment, Biology, Ribosomal RNA, DNA, Ribosomal, Triturus, Chromosomes, Sequence Homology, Nucleic Acid, 28S ribosomal RNA, Animals, Sequence motif, Sequence Alignment, Ribosomal DNA, Gene, Genetics (clinical), Repetitive Sequences, Nucleic Acid
Abstract

Ribosomal DNA (rDNA) variation in the species Triturus vulgaris meridionalis (Amphibia, Urodela) is remarkable because of unusually high intraspecific variability in the number and distribution of ribosomal loci in the karyotype; in addition, portions of the intergenic spacer (IGS) are clustered at chromosomal loci where they are not associated with ribosomal 18S and 28S RNA genes. These clusters are referred to as extraribosomal, and they appear to consist mostly of repetitive BamHI elements. In this paper, we report the complete nucleotide sequence of an IGS of T. v. meridionalis; this structural analysis is aimed to get insight into the molecular mechanism(s) of spreading of the ribosomal cistrons as well as its possible functional significance. We found that the IGS of T. vulgaris has a modular structure: modular repetitive elements contain sequences possibly related to the regulation of transcription of the ribosomal units. In particular, both ribosomal and extraribosomal IGS elements contain presumptive enhancers. Interestingly, the enhancer-containing region is mostly conserved between ribosomal and extraribosomal elements, while mutations accumulate in a region characterized by repetitions of a simple sequence motif, that we consider as a possible recombination hotspot. Our data suggest that extraribosomal elements most probably originated from ribosomal enhancer-containing elements able to move independently from the ribosomal unit at novel chromosomal positions, perhaps with the aid of the simple repetitive motif. We argue that a similar mechanism may lead to the spreading of complete repetition units as well, giving rise to multiple, and variable, ribosomal sites. We propose that hypervariability in the number and distribution of the rDNA loci, as seen in T. vulgaris, is a further mechanism to ensure redundancy, which seems to be an intrinsic property of rDNA biology, the occurrence of IGS elements independently clustered at separate chromosomal loci being a by-product of this mechanism.

Published
1997

4. Characterisation of a short, highly repeated and centromerically localised DNA sequence in crested and marbled newts of the genus Triturus

Author

Herbert C. Macgregor, Lesley Barnett, and Jennifer Varley

Subjects
Satellite DNA, Centromere, Molecular Sequence Data, Restriction Mapping, DNA, Satellite, DNA sequencing, HaeIII, Gene Frequency, Genetics, medicine, Consensus sequence, Animals, Cloning, Molecular, Repeated sequence, Genetics (clinical), Repetitive Sequences, Nucleic Acid, Genomic Library, biology, Base Sequence, Nucleic acid sequence, Genetic Variation, biology.organism_classification, Triturus, Restriction enzyme, medicine.drug
Abstract

A 32–33 bp highly repeated DNA sequence, TkS1, has been isolated from genomic DNA of the newt Triturus karelini digested with the restriction endonucleases HaeIII or AluI. TkS1 is known to be localised in the centromeric heterochromatin of all the chromosomes in T. karelini and the related species T. cristatus TkS1 has been shown to be present in varying amounts in the genomic DNA of a range of species of Triturus, including representatives of the two main subgenera Triturus and Palaeotriton. A programme of sequencing of monomers, dimers and trimers of TkS1 was carried out in order to determine the level of conservation of the sequence within and between species of Triturus. Altogether 204 monomer (32/33 bp) clones were made of TkS1 from three individuals of T. karelini, and one individual each of T. cristatus, T. carnifex, T. dobrogicus and T. marmoratus, all members of the subgenus Triturus and the cristatus species group. A number of dimer (64 bp) and trimer (96 bp) clones were also made from DNA of a single specimen of T. karelini digested with HaeIII or AluI. Three distinct types of TkS1 were identified in all species examined, except for T. marmoratus where only two of the types were found. The types were distinguished on the basis of certain recurring divergent patterns in monomers sequenced from T. karelini. Type 1 is mainly characterised by the presence of an AluI site at positions 24–27 and type 3 mainly by the presence of an additional base (C) at position 14. Type 2 normally lacks the AluI site and the C at position 14, as well as having a number of other distinguishing features. TkS1 and its three types have remained remarkably constant in sequence since before the divergence of T. marmoratus from other species in the cristatus species group, about 10 million years ago. Examination of all 204 monomer clones and comparison with consensus sequences for the three types shows less than 5% divergence at any one position in the sequence. There is good evidence from examination of dimer and trimer clones of TkS1 that the different types are intermingled with each other, and all three types are likely to be present on all chromosomes. Dimeric (64 bp) TkS1 clones constructed from AluI fragments of T. karelini DNA show evidence of a trimeric (96 bp) “supertype” with the pattern type 1-type 3-type 1 that is much more common than would be expected on a random basis. The properties of TkS1 are discussed in relation to models for the involvement of highly repeated satellite DNA in chromosomal growth and evolution.

Published
1990

5. Chromosome banding in amphibia

Author

M. Schmid, C. Klett, and J. Olert

Subjects
Genetics, biology, Karyotype, biology.organism_classification, Genetics (clinical), Triturus
Published
1979

6. Experimental hybridization within the genus Triturus (Urodela: Salamandridae)

Author

Matilde Ragghianti, Giorgio Mancino, and Stefania Bucci-Innocenti

Subjects
Male, Salamandridae, biology, Spermiogenesis, Chromosome, Zoology, biology.organism_classification, Triturus, Chromosomes, Chiasma, Chromosome Banding, Meiotic Prophase I, Genetics, Animals, Hybridization, Genetic, Female, Crossing Over, Genetic, Ploidy, Spermatogenesis, Genetics (clinical)
Abstract

The spermatogenesis of 9 F1 hybrids of Triturus cristatus carnifex female x T. vulgaris meridionalis male was studied in squash preparations of testicular fragments, treated by the C-staining method. The chromosome number of these hybrids was examined in spermatogonial metaphases and found to be diploid. The two parental sets were always recognized, which means that a regular, although heterospecific, amphimixis occurred (2n = nfemale + nmale). Meiotic prophase I is greatly altered owing to a failure of typical chromosome pairing and chiasma formation. At metaphase I and/or meta-anaphase I, the effects of the hybrid combination of the 2 specific parental sets are clearly visable. Most primary spermatocytes contain only univalents. A few show chromosome associations (bivalents, trivalents and, more rarely, quadrivalent chains) besides univalents. Such associations are of 2 types: (a) intragenomal associations = associations of 2 chromosomes by a terminal (a1) or subterminal chiasma (a2); (b) intergenomal associations = associations of 2 chromosomes by a terminal (b1) or subterminal chiasma (b2). Univalents segregate at random while the associations often lag on the equatorial plane or migrate entire to a spindle pole. Primary spermatocytes with chromosome multivalents can encounter greater difficulties in accomplishing the first cytokinesis. Secondary spermatocytes are numerically and qualitatively unbalanced; however, some of them undergo spermiogenesis and can give rise to a small number of sperms, generally abnormal and never united in bundles. --Problems related to the occurrence of "anomalous" chiasmata and of intra- and inter-genomal homologies are discussed.

Published
1978

7. Absence of chiasmata from the heteromorphic region of chromosome I during spermatogenesis in Triturus cristatus carnifex

Author

Garry T. Morgan

Subjects
Genetics, biology, biology.organism_classification, Oocyte, Triturus, Bivalent (genetics), Chiasma, medicine.anatomical_structure, Evolutionary biology, medicine, Feulgen stain, Developmental biology, Metaphase, Spermatogenesis, Genetics (clinical)
Abstract

Analysis of squash preparations of spermatocytes from crested newts, Triturus cristatus carnifex, has shown that in most cells at least one large bivalent regularly fails to form chiasmata in one arm-pair. Feulgen microphotometry of diplotene and metaphase bivalents has shown that it is the largest bivalent in each cell which shows chiasma failure in one arm-pair. A C-banding technique which identifies chromosome I by virtue of a long, darkly stained region in its long arm, was used to confirm the absence of chiasmata from one arm-pair of the longest bivalent, and specifically from the darkly stained region. The achiasmate region which chromosome I exhibits during spermatogenesis, corresponds to the “heteromorphic region” of oocyte lampbrush bivalent I in which chiasmata never form. A possible correlation between the complete absence of crossing-over from the heteromorphic region and unusual cytological and molecular features which it exhibits, are discussed.

Published
1978

8. Analysis of chromatin-associated fiber arrays

Author

Victoria E. Foe, Charles D. Laird, W. Yean Chooi, and L. E. Wilkinson

Subjects
Transcription, Genetic, Biology, Hemiptera, chemistry.chemical_compound, Transcription (biology), 28S ribosomal RNA, Genetics, Animals, Protein secondary structure, Genetics (clinical), Transcriptionally active chromatin, RNA, DNA, Ribosomal RNA, Triturus, Molecular biology, Chromatin, Microscopy, Electron, Drosophila melanogaster, Ribonucleoproteins, chemistry, RNA, Ribosomal, Biophysics
Abstract

Electron microscopic examination of chromatin from embryonic nuclei of Oncopeltus fasciatus and Drosophila melanogaster reveals arrays of chromatin associated fibers. The lengths and spacings of these fibers were analyzed to provide a basis for defining and interpreting regions of transcriptionally active chromatin. The results of the analysis are consistent with the interpretation of some fibers as nascent RNA with associated protein (RNP). The chromatin segments underlying these fiber arrays were classified as ribosomal or non-ribosomal transcription units according to definitions and criteria described by Foe et al. (1976). Nascent fibers on active ribosomal transcription units were analyzed and compared for Drosophila melanogaster, Triturus viridescens, and Oncopeltus fasciatus. A common feature of the fiber patterns on ribosomal TUs is that origin-distal fibers exhibit greater length variability and a lower slope relative to proximal fibers. The region of increased variability in fiber lengths is correlated with the expected location of 28S ribosomal RNA sequences in the distal half of each ribosomal transcription unit. Because 28S ribosomal RNA appears to contain more extensive regions of base sequence complementarity, we suggest that the length of ribosomal RNP fibers is influenced under our spreading conditions by the secondary structure of the nascent RNA. In order to calculate the RNA content of RNP fibers, chromatin morphology was used to estimate lengths of transcribed DNA. The packing ratio of DNA in chromatin, which we express as the length of B-structure DNA divided by length of chromatin, is 1.1-1.2 and 1.6 for the DNA in active ribosomal and non-ribosomal chromatins, respectively. These DNA packing ratios are used to determine the extent to which nascent RNP fibers are shorter than the transcribed DNA (expressed as DNA/RNP length ratio). For non-ribosomal transcription units and for proximal fibers of ribosomal transcription units. DNA/RNP length ratios are relatively constant within each array. However, considerable variability in this ratio (4-23) is observed for different arrays of fibers. Possible sources of this variability are considered by comparing ratios derived from the presumably identical ribosomal transcription units. Further analysis of the morphology of nascent fibers may elucidate the contributions of proteins and successive RNA sequences to RNP structure.

Published
1976

9. DNA reassociation kinetics in relation to genome size in four amphibian species

Author

Francesco Amaldi and Cosima T. Baldari

Subjects
Amphibian, Xenopus, Urodela, Bufo bufo, Amphibians, chemistry.chemical_compound, Cot analysis, Nucleic Acids, biology.animal, Genetics, Animals, Bufo, Genome size, Genetics (clinical), Base Sequence, biology, DNA, biology.organism_classification, Biological Evolution, Triturus, Nuclear DNA, Molecular Weight, Kinetics, Biochemistry, chemistry, Nucleic Acid Renaturation, Necturus maculosus
Abstract

DNA reassociation kinetics were studied, by means of the hydroxyapatite chromatography method, for four species of Amphibians with different nuclear DNA content: Xenopus laevis (3 pg DNA per haploid genome) and Bufo bufo (7 pg) of the Anura subclass and Triturus cristatus (23 pg) and Necturus maculosus (52 pg) of the Urodela subclass. Within each subclass the two species studied were found to have about the same absolute amount of unique DNA. The differences of total nuclear DNA can be accounted for by quantitative variations of the repetitive sequence classes, at least in part due to changes in the number of copies of the various sequences. On the contrary the great difference in nuclear DNA between the two subclasses, Anura and Urodela, involves all sequence classes in parallel; the slowly reassociating fraction appears to be unique in spite of a tenfold difference in absolute amount. The dependence of reassociation kinetics on DNA fragment length for the four species indicates for all of them an interspersed organization of the various sequence classes.

Published
1976

10. Chromosome and C-heterochromatin polymorphisms in the Italian newt, Triturus italicus

Author

Stefania Bucci-Innocenti, Giorgio Mancino, and Matilde Ragghianti

Subjects
Genetics, medicine.medical_specialty, Polymorphism, Genetic, Geography, Heterochromatin, Cytogenetics, Genetic Variation, Chromosome, Karyotype, Biology, Triturus, Chromosomes, Chromosome Banding, Italy, Larva, Centromere, medicine, Animals, Chromosomal polymorphism, Genetics (clinical), Chromosome 12, Chromosomal inversion
Abstract

A combined chromosome and C-heterochromatin polymorphism in pair 12 in the complement of the newt species, T. italicus is described. The C-heterochromatin polymorphism is presumably due to a loss in the proximal C-band, whereas the chromosomal polymorphism has its origin in two different independent pericentric inversions both including the centromere and the proximal C-band of chromosome 12. The double-inversion polymorphism has a wide distribution over the range and follows a clear bipolarity between a northern area where the karyotype is homomorphic for the standard type of pair 12 (ST/ST) and an opposite area where the ST type is completely replaced by variant M1 and M2 metacentric chromosomes 12. Various karyophylogenies are possible, but the simplest and the most probable presumes an ancestral karyotype of ST/ST and a mechanism of gradual replacement of the heterobrachial chromosome ST by two independent pericentric inversions. The present data are discussed in relation to existing theories on karyological evolution of Urodeles and the functional significance of telocentric chromosomes suggested by Sessions et al. (1982).

Published
1983

11. The mitotic chromosomes of Notophthalmus (=Triturus) viridescens: Localization of C banding regions and DNA sequences complementary to 18S, 28S and 5S ribosomal RNA

Author

Mary Lou Pardue and N. Hutchison

Subjects
Male, Mitosis, In situ hybridization, Biology, Azure Stains, Chromosomes, chemistry.chemical_compound, 5S ribosomal RNA, Heterochromatin, 28S ribosomal RNA, Genetics, Animals, Genetics (clinical), Chromosome Mapping, Nucleic Acid Hybridization, Chromosome, RNA, Karyotype, DNA, Ribosomal RNA, Triturus, Molecular biology, Meiosis, Genes, chemistry, RNA, Ribosomal, Karyotyping
Abstract

The metaphase chromosomes of Notophthalmus (Triturus) viridescens have been studied by C-banding and in situ hybridization. The chromosomes show the pericentric C-banding seen in many organisms and in addition have interstitial C-bands located a short distance from the pericentric C-bands on each chromosome arm. A few C-bands are seen in telomeric regions. Regions which hybridize in situ with 18S and 28S ribosomal RNA were found on three chromosome pairs. The animals studied fell into three groups with respect to which of the six possible sites showed detectable hybridization with 18S and 28S RNA. Individual animals differed not only in the pattern of in situ hybridization of ribosomal RNA but also in the number of ribosomal RNA cistrons in the genome as measured by saturation hybridization on purified DNA. In situ hybridization showed five pairs of chromosomes which contained DNA complementary to 5S RNA. The four pairs of subtelocentric chromosomes in the N. viridescens karyotype all have 5S DNA in the pericentric regions. The fifth cluster of 5S DNA is in the middle of one arm of the chromosomes in one of the two smallest submetacentric pairs in the genome. The five sites of 5S DNA differ markedly in the level of in situ hybridization with 5S cRNA.

Published
1975

12. Experimental hybridization within the genus Triturus (Urodela: Salamandridae)

Author

Giorgio Mancino, Matilde Ragghianti, and Stefania Bucci-Innocenti

Subjects
Male, Salamandridae, biology, Chromosome, biology.organism_classification, Diploidy, Triturus, Chromosomes, Chiasma, Chromosomal crossover, Phenotype, Spermatocytes, Evolutionary biology, Genus, Karyotyping, Genetics, Animals, Hybridization, Genetic, Female, Chromatid, Crossing Over, Genetic, Spermatogenesis, Metaphase, Genetics (clinical)
Abstract

Spermatogenesis in the F1 hybrid (2n=24=12 female + 12 male) between the closely related newt species T. cristatus carnifex and T. marmoratus was apparently normal up to pachytene. Many unpaired chromosomes were present at diplotene and a typical diakinesis was lacking. Primary spermatocytes at meta- and meta-anaphase contained up to 12 regular intergenomal bivalents and a corresponding number of univalents when less then 12 II. Most chiasmata were terminal or subterminal, some intercalary. Chiasmata between corresponding heterospecific chromosomes can be reported as true: real crossing over has taken place, proving the presence of primary chromosomal homologies between the 2 sets of the parental species. Evidence for recombination is based on the segregation of particular markers (i.e., subterminal C-bands and NORs) observed in certain chromosomes at metaphase II. One chromatid of single chromosomes can show the T. cristatus "pheno-type" and the other the T. marmoratus phenotype". A few primary spermatocytes contain a certain number of irregular associations (intragenomal or intrahaploid bivalents, irregular intergenomal bivalents, chromosome multivalents) joined by chiasmata which can be defined as anomalous. Other abnormalities concern the occurrence of interlocked bivalents which occasionally show an anomalous exchange between heterologous chromatids. Cytogenetic criteria useful to evaluate the taxonomic relationships between different species have been discussed as well as some possible trends in chromosome evolution and speciation within the genus Triturus.

Published
1979

13. Length and interspersion of repetitive and non repetitive DNA sequences in four Amphibian species with different genome sizes

Author

Francesco Amaldi and Cosima T. Baldari

Subjects
Erythrocytes, Base pair, Xenopus, Urodela, Bufo bufo, chemistry.chemical_compound, Genetics, Animals, Bufo, Repeated sequence, Genome size, Genetics (clinical), Electrophoresis, Agar Gel, Base Sequence, biology, urogenital system, DNA, Interspersed Repetitive Sequences, biology.organism_classification, Triturus, Nuclear DNA, Microscopy, Electron, chemistry, Evolutionary biology, sense organs, Necturus maculosus
Abstract

The interspersion period of repetitive and unique sequences was analyzed by two different methods, electron microscopy and agarose gel electrophoresis, for four Amphibian species with different nuclear DNA content, namely the Anura Xenopus laevis (3 pg DNA per haploid genome) and Bufo bufo (7 pg) and the Urodela Triturus cristatus (23 pg) and Necturus maculosus (52 pg). Within each of the two subclasses it has been found that interspecific differences, in DNA content, due to variations in the amount of repetitive sequences, do not involve variations in length of the interspersed repetitive sequences. They remain about 380 base pairs. Furthermore, the unique sequences length has been found to be shorter in Bufo (760 base pairs) than in Xenopus (1600) and in Necturus (880) than in Triturus (1340). A study of the interspersion period has shown that the great difference in DNA content between Anura and Urodela, which had been previously shown not to have involved changes in the relative amounts of the various sequence classes, does not involve changes in the interspersion period.

Published
1977

14. Characterization of the lampbrush chromosomes of the marbled newt Triturus marmoratus (Latreille, 1800)

Author

Irma Nardi, Matilde Ragghianti, and Giorgio Mancino

Subjects
Heterozygote, Nucleolus, Mitosis, Urodela, Triturus marmoratus, Tritium, Ambystoma, Bivalent (genetics), Species Specificity, Genetics, Animals, Uridine, Genetics (clinical), Ovum, Sex Chromosomes, biology, Ovary, Chromosome Mapping, Rana esculenta, Anatomy, biology.organism_classification, Triturus, Lampbrush chromosome, Evolutionary biology, Autoradiography, RNA, Female, Developmental biology, Cell Nucleolus
Abstract

The maps of the lampbrush chromosomes of Triturus marmoratus oocytes were constructed on the basis of their lengths and major morphological characters such as giant fusing loops, dense matrix loops, lumpy objects, axial granules, lateral globules and reflected fusions; a nucleolus organizing region occurs subterminally on the right side of chromosome X. — Bivalent I appears morphologically asymmetrical, its two partners being of different lengths and bearing heteromorphic loops and other heterozygous structures: this heteromorphism may indicate that the two partners of bivalent I represent the ZW heterochromosomes of the species. Finally, an autoradiographic study has been performed in order to ascertain the pattern of 3H-uridine incorporation shown by the most typical landmarks and nucleoli.

Published
1972

15. The relationship of a specific chromosomal region to the development of the acrosome

Author

W. Krone and M. Schmid

Subjects
Male, Euchromatin, Spermiogenesis, Heterochromatin, Urodela, Biology, Ambystoma, Chromosomes, Genetics, medicine, Constitutive heterochromatin, Animals, Salamandra, Acrosome, Spermatogenesis, Genetics (clinical), Spermatid, Spermatozoon, Anatomy, Salamandridae, Spermatids, Spermatozoa, Triturus, medicine.anatomical_structure, Karyotyping, Chromosomal region
Abstract

In early spermatids of Urodeles the chromosome segments bearing constitutive heterochromatin are localized in one half of the round nucleus; this region becomes the basal part of the long nucleus of the spermatozoon. The euchromatic chromosome segments extend toward the anterior nuclear pole in a bouquet configuration (Macgregor and Walker, 1973). In the course of spermiohistogenesis, one of the heterochromatic regions (the acrosomal chromocenter) migrates from the basal part to the anterior half of the spermatid nucleus. This heterochromatic block is identical with a species-specific, definite C-band in the karyotype. This relationship between the acrosomal chromocenter and a specific chromosomal C-band was established in Triturus cristatus, T. marmoratus, T. alpestris and Cynops pyrrhogaster. In closely related species this particular C-band lies on similar chromosomes. — While the spermatid nucleus still retains its round shape the acrosomal chromocenter despiralizes into a long heterochromatic thread (acrosomal thread). Precisely at the position of this thread the nucleus evaginates and acquires a pear-like shape. During the elongation of the nuclear protrusion the acrosomal thread remains associated with the anterior end. At termination of spermiogenesis it lies closely below the acrosome in the tip of the spermatozoon. Spontaneous aberrations which affect the acrosomal chromocenter or the thread lead to the development of spermatozoa with defective tips. — Several euchromatic segments, interspersed between the heterochromatic segments, can be recognized in the completely despiralized acrosomal thread. Genes responsible for the morphogenetic activities of both, the acrosomal chromocenter and the acrosomal thread, in the development of the spermtip, might be localized in these interspersed euchromatic segments. The existence in higher vertebrates of an acrosomal chromocenter or an equivalent chromosomal region is discussed.

Published
1976

16. Chromosome location of the ribosomal RNA genes in Triturus vulgaris meridionalis (Amphibia, Urodela). II. Intraspecific variability in number and position of the chromosome loci for 18S + 28S ribosomal RNA

Author

Renata Batistoni, Irma Nardi, G. Barsacchi-Pilone, and F. Andronico

Subjects
Genetics, Male, Nucleolus, Chromosome, Mitosis, Biology, Ribosomal RNA, biology.organism_classification, Molecular biology, Triturus, Chromosomes, Meiosis, Lampbrush chromosome, Triturus vulgaris, Genes, RNA, Ribosomal, 28S ribosomal RNA, Karyotyping, Animals, Female, Nucleolus organizer region, Ribosomal DNA, Genetics (clinical)
Abstract

Ribosomal genes have been localized on mitotic and lampbrush chromosomes of 20 specimens of Triturus vulgaris meridionalis by in situ hybridization with 3H 18S + 28S rRNA. The results may be summarized as follows: 1) each individual shows positive in situ hybridization at the nucleolus organizing region (NOR) on chromosome XI; 2) in addition, many specimens exhibit a positive reaction in chromosomal sites other than the NOR (additional ribosomal sites); 3) the chromosomal distribution of the additional sites appears to be identical in different tissues from the same specimen and to follow a specific individual pattern; 4) the additional ribosomal sites are preferentially found at the telomeric, centromeric or C-band regions of the chromosomes involved.

Published
1977

17. Centromeric satellite DNA in the newt Triturus cristatus karelinii and related species: its distribution and transcription on lampbrush chromosomes

Author

Lise Baldwin and Herbert C. Macgregor

Subjects
Transcription, Genetic, Heterochromatin, Base pair, Satellite DNA, Biology, DNA, Satellite, Chromosomes, chemistry.chemical_compound, Species Specificity, Centromere, Genetics, Animals, Genetics (clinical), Base Sequence, Chromosome, Nucleic Acid Hybridization, DNA, DNA Restriction Enzymes, biology.organism_classification, Triturus, Chromosome Banding, Lampbrush chromosome, chemistry, Karyotyping, Plasmids
Abstract

Two abundant satellite DNA sequences have been identified in and cloned from the DNA of Triturus cristatus karelinii. The smaller of these with a repeat unit of 33 base pairs (bp) is designated TkS1, the larger with 68 bp is designated TkS2. These satellites are also present in DNA from T.c. cristatus, T.c. carnifex and T. marmoratus but in substantially lower copy number. In situ hybridisations to lampbrush chromosomes of T.c. karelinii and T.c. cristatus have shown that the satellites are concentrated in the heterochromatic centromere bars of T.c. karelinii and in a region around the centromere granule in T.c. cristatus. The satellites also bind specifically to the centromere regions of mitotic metaphase chromosomes. They do not bind to the heteromorphic arms of chromosome 1, which have previously been shown to be rich in highly repeated DNA. DNA/RNA-transcript in situ hybrids to lampbrush chromosomes with TkS1 suggest that this sequence is occasionally transcribed on lampbrush loops near the centromeres.

Published
1985

18. Chromosome location of the ribosomal genes in Triturus vulgaris meridionalis (Amphibia Urodela). III. Inheritance of the chromosomal sites for 18S + 28S ribosomal RNA

Author

Renata Batistoni, Irma Nardi, F. Andronico, and G. Barsacchi-Pilone

Subjects
Genetics, Male, Nucleolus, Chromosome, Chromosome Mapping, Nucleic Acid Hybridization, Ribosomal RNA, Biology, biology.organism_classification, Genome, Triturus, symbols.namesake, Triturus vulgaris, RNA, Ribosomal, 28S ribosomal RNA, Mendelian inheritance, symbols, Animals, Female, Gene, Genetics (clinical), Cell Nucleolus
Abstract

In Triturus vulgaris meridionalis, the 18S + 28S rDNA sequences have been shown to be located in a number of additional chromosomal sites besides the nucleolus organizing region. The additional ribosomal sites have been found to vary as to their number and chromosomal location in different individuals of the species.--The data presented in this study concern the chromosomal distribution of the ribosomal sequences as analyzed by in situ hybridization technique in two individuals as well as in their offspring. The evidence obtained by this analysis indicates quite clearly that all 18S + 28S rRNA sites present in each individual genome are inherited according to simple mendelian principles.

Published
1978

19. Heterochromatic DNA in Triturus (Amphibia, Urodela). I. A satellite DNA component of the pericentric C-bands

Author

F. Andronico, Renata Batistoni, Irma Nardi, Luigi Vitelli, and G. Barsacchi-Pilone

Subjects
Satellite DNA, Heterochromatin, Xenopus, Biology, DNA, Satellite, Haploidy, Genome, Ambystoma, Triturus vulgaris, Species Specificity, Genetics, Animals, Genetics (clinical), Pericentric heterochromatin, Genomic organization, Repetitive Sequences, Nucleic Acid, Necturus, Chromosome, Nucleic Acid Hybridization, DNA Restriction Enzymes, biology.organism_classification, Triturus, Lampbrush chromosome, Karyotyping, Oocytes, Female, Plasmids
Abstract

We have studied the structure, genome organization, chromosomal location, conservation across species and transcription on lampbrush chromosomes, of an AT-rich satellite DNA component of the newt, Triturus vulgaris meridionalis. The satellite (Sat G), originally isolated by gradient centrifugation, represents about 2% of the vulgaris genome and comprises a highly repetitive sequence family (HindIII family), whose monomers have been cloned. The repeat units are about 330 bp long, as measured on gels, and a cloned unit (pTvm1) is 310 bp long, as shown by sequencing. Abundant clusters of the HindIII family sequences are located within the pericentric heterochromatin (i.e. the C-bands placed at both sides of, and at a certain distance from, the centromeres) in most chromosomes. Both the sequence family and its overall pattern of chromosomal distribution are conserved within the genus Triturus, despite a few species-specific differences. The great majority of the HindIII family sequences are unexpressed on lampbrush chromosomes; they reside within pericentric, condensed segments of the chromosome axis ("loopless bars"). Only a few sequences are transcribed on some loops, suggesting that transcription promotion does not depend on the satellite sequences themselves.

Published
1986

20. DNA replication in the amphibia

Author

Barbara G. Wilson

Subjects
DNA Replication, Ranidae, DNA replication, Bufo cognatus, Biology, Tritium, Virology, Molecular biology, Triturus, Scaphiopus couchi, Bufonidae, Nuclear DNA, Amphibians, Autoradiograph, Isotope Labeling, Replication (statistics), Genetics, Animals, Autoradiography, Anura, Floxuridine, Rana clamitans, Uridine, Genetics (clinical), Thymidine
Abstract

Autoradiographic techniques were used to measure rate of replication and length of the replication unit in cultured cells of Scaphiopus couchi, Bufo cognatus, Rana clamitans, and Triturus viridescens, having nuclear DNA amounts in the ratio 1:4:7:39 respectively. The autoradiographic experiments were designed to show whether the larger amounts of nuclear DNA are correlated with more rapid rates of synthesis and/or with longer replication units. -- The DNA replication rate was 2.5 mu/minute (corrected for two growing points) with 10 minutes 3H-thymidine label at 22 degrees C, but decreased with longer labelling durations. The length of the replication unit (estimated by the distance from the center of one autoradiograph to the center of the next in sequence) was most commonly in the 10-25 mu range with a 30 minute label, in all four species. The average center-to-center distance was 8 mu at 10 minutes and increased with label duration, to over 45 mu with 24 hours label. Replication was predominantly but not exclusively bidirectional. Neither rate of replication nor length of the replication unit was proportional to the amount of DNA in these species.

Published
1975

21. In situ hybridization of ribosomal DNA labelled with 125iodine to metaphase and lampbrush chromosomes from newts

Author

Sally Hennen, H. C. Macgregor, and S. Mizuno

Subjects
Male, Xenopus, Mitosis, In situ hybridization, Biology, Bivalent (genetics), Chromosomes, Iodine Radioisotopes, Genetics, Centrifugation, Density Gradient, Methods, Animals, Microscopy, Phase-Contrast, Metaphase, Ribosomal DNA, Genetics (clinical), Ovum, Ovary, Chromosome, Nucleic Acid Hybridization, Karyotype, DNA, Molecular biology, Triturus, Lampbrush chromosome, Karyotyping, Autoradiography, Female, Ribosomes
Abstract

Methods are described for in situ hybridization of ribosomal DNA from Xenopus laevis, labelled in vitro with 125iodine, to mitotic and lampbrush chromosomes from Triturus cristatus carnifex. The hybridization reaction was carried out in a mixture containing 50% formamide, 4 X SSC, 0.1 M KI, at 37 degrees C, or in 2 X SSC, 0.1 M KI at 65 degrees C. Autoradiographs of mitotic metaphases from 2 males showed labelling over the middle of the short arm of one chromosome IX in each metaphase. In some cases, a region near the end of a longer chromosome was also labelled. In a lampbrush preparations, labelling was confined to a region identified as about 53 units, near the middle of the short arm of both halves of bivalent IX. The usefulness of the technique and the significance of the labelling of only 1 of the 2 chromosomes IX in mitotic preparations are discussed.

Published
1975

22. Ultrastructure of segmentation mitoses in cleaving newt eggs after blocking of centrospheres by quinoline

Author

Paul Sentein and Yadigar Ates

Subjects
Centriole, Zygote, Mitosis, Urodela, Anatomy, Biology, Salamandridae, Triturus, Chromosomes, Cell biology, Spindle apparatus, Organoids, Prophase, Microtubule, Genetics, Ultrastructure, Quinolines, Animals, Female, Centriole replication, Metaphase, Genetics (clinical)
Abstract

In quinoline treated blastomeres of Triturus helveticus Raz. and Pleurodeles waltlii Michah., microtubules disappear and around the centrioles markedly enlarged dense bodies accompanied by striated bodies are accumulated, from prophase beyond metaphase. It is concluded that these bodies in untreated cells play a role in the formation of the spindle microtubules. — During metaphase the chromosome are smooth-surfaced and show a pronounced tendency to stickiness. During ana-telophase they become surrounded by nuclear membranes and form caryomeres. — Quinoline does not interfere with centriole replication, but prevents the separation if diplosomes that have been already formed, if it acts before that separation. — Some centrioles exhibit different degrees of ultrastructural disarrangement.

Published
1976

23. The structure of chromosome-derived ribonucleoprotein in oocytes of Triturus cristatus carnifex (Laurenti)

Author

John Sommerville and David B. Malcolm

Subjects
Transcription, Genetic, Detergents, Fibril, Chromosomes, Ribonucleases, Transcription (biology), Genetics, Animals, Ribonuclease, Genetics (clinical), Ovum, Ribonucleoprotein, Cell Nucleus, Deoxyribonucleases, biology, Ribonucleoprotein particle, RNA, Chromosome, Triturus, Molecular biology, Microscopy, Electron, Nucleoproteins, Models, Chemical, Oocytes, biology.protein, Biophysics, Female, High voltage electron microscopy, Peptide Hydrolases
Abstract

The morphology of the lateral loops of newt oocyte chromosomes results from the state of aggregation of the ribonucleoprotein which constitutes the loop matrix. This ribonucleoprotein consists of the RNA products of transcription in association with various non-basic proteins. During vitellogenesis there is marked variation in the size and appearance of the different loops of a chromosome complement. Variation in morphology is due largely to the extent to which fibrous arrays of particles, approximately 20 nm in diameter, interact to form larger particulate aggregates. Increased aggregation may accompany individual loop maturation. Ribonucleoprotein particles, which closely resemble the particulate material seen on the chromosomes (i.e. composites of fibrous aggregates of 20 nm subparticles), can be isolated from homogenates of oocytes. The structure of intact particles has been examined by high voltage electron microscopy. Disrupted particles have been prepared by droplet diffusion on to the surfaces of grids. The substructure of the particles is further revealed by treatment with various detergents and with ribonuclease and protease. The interpretation of the observations is that the RNA is transcribed from the loop axis as long continuous strands which interact with protein to form 20 nm subparticles along their length. These linear arrays of 20 nm subparticles are often loosely arranged, both on the chromosome and in nuclear ribonucleoprotein extracts, as highly hydrated irregular particles. Whether the 20 nm particles are preformed complexes of protein which attach to an RNA backbone or whether they are periodic condensates of RNP along the length of an RNP fibril is discussed.

Published
1974

24. In situ hybridization of highly repetitive DNA to chromosomes of Triturus cristatus

Author

Herbert C. Macgregor

Subjects
DNA Replication, Transcription, Genetic, G banding, Chromosome, Nucleic Acid Hybridization, DNA, Biology, Eukaryotic chromosome structure, Molecular biology, Triturus, Bivalent (genetics), Chromosomes, Chromosomal crossover, Lampbrush chromosome, Genetics, Animals, RNA, Nick translation, Mitosis, Genetics (clinical)
Abstract

Highly repetitive DNA of C0t 0--0.2 was purified from whole DNA of Triturus cristatus carnifex, labelled by nick translation, and in situ hybridized to RNA transcripts on the loops of lampbrush chromosomes and to the DNA of mitotic chromosomes from intestinal epithelium from the same species. The labelled DNA bound to 20--30 loops on the long arms of lampbrush bivalent 1, a pair of loops near the centromere on bivalent 10, and a number of other loops most of which were localized in pericentric regions. In mitotic preparations the same labelled DNA bound to the heteromorphic regions of the long arms of both chromosomes 1, and to the centromeric regions of all chromosomes. Centromeric labelling was light on chromosomes 4 and particularly clear on the 3 shortest chromosomes of the set. The heavy labelling of the heteromorphic arms of chromosome 1 is discussed in relation to several other peculiar properties of these arms, including their extraordinary lengths, their Giemsa banding patterns, and the absence of meiotic crossing over. It is suggested that insofar as the results with DNA/DNA hybridization and mitotic chromosomes match those obtained with the DNA/RNA-transcript hybridization and lampbrush chromosomes, confidence in the latter technique may be increased accordingly.

Published
1979

25. Chromosome location of the ribosomal RNA genes in Triturus vulgaris meridionalis (Amphibia, Urodela)

Author

I, Nardi, S, De Lucchini, G, Barsacchi-Pilone, and F, Andronico

Subjects
Male, Silver, Genes, Species Specificity, Staining and Labeling, RNA, Ribosomal, Animals, Chromosome Mapping, Nucleic Acid Hybridization, Triturus, Cell Nucleolus
Abstract

The mitotic chromosomes of six specimens from Triturus vulgaris meridionalis have been examined by both in situ hybridization with 3H 18S + 28S rRNA and AS-SAT staining method. The results of these two sets of experiments can be summarized as follows: 1) in each specimen the NORs and the additional ribosomal sites, which react positively to in situ hybridization with 3H 18S + 28S rRNA, are also stained by silver; 2) other chromosomal regions, which do not hybridize in situ with 3H 18S + 28S rRNA, are on the other hand stained by the AS-SAT method. These latter AG-positive sites show a species-specific pattern of chromosomal distribution.

Published
1978

26. Evolutionary conservation of a common pattern of activity of nucleolus organizers during spermatogenesis in vertebrates

Author

Wolfgang Engel, C. Löser, M. Schmid, and Jörg Schmidtke

Subjects
Male, Nucleolus, Biology, 03 medical and health sciences, Prophase, Meiosis, Species Specificity, Bone Marrow, Genetics, medicine, Animals, 14. Life underwater, Spermatogenesis, Ribosomal DNA, Gene, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Spermatid, 030302 biochemistry & molecular biology, Fishes, RNA, Snakes, Biological Evolution, Triturus, Bufonidae, Turtles, medicine.anatomical_structure, Organ Specificity, Karyotyping, Nucleolus organizer region, Colchicine, Chickens, Cell Nucleolus
Abstract

The patterns of activity of the nucleolus organizer regions (NORs) in the spermatogeneses of ten species of all non-mammalian classes of vertebrates and one species of the cephalochordates were investigated with the silver (Ag)-staining technique. The Ag-stainability of the NORs is a measure of the transcriptional activity of the ribosomal RNA genes. In all species, there is a very similar pattern of NOR-activity in the various stages of Spermatogenesis. The qualitative analysis of the Ag-stainability of the NORs was in very good agreement with the results obtained for mammals: Ag-stained NORs are detectable during the entire meiotic prophase up to the pachytene stage, completely absent in the meiotic metaphases I and II, and again demonstrable in early spermatid nuclei. The results confirm the occurrence of postmeiotic reactivation of the RNA genes. The preferential inhibition of rRNA synthesis by low doses of actinomycin D induced a rapid decline of the Ag-stainability of the postmeiotically reactivated NORs. The significance of the evolutionary conservation of the postmeiotic NOR-reactivation is discussed.

Published
1982

27. Multiple ribosomal gene sites revealed by in situ hybridization of Xenopus rDNA to Triturus lampbrush chromosomes

Author

Alan Colman, Garry T. Morgan, and Herbert C. Macgregor

Subjects
Ribosomal Proteins, Transcription, Genetic, Nucleolus, Xenopus, Nucleic Acid Hybridization, DNA, DNA-Directed RNA Polymerases, Biology, Ribosomal RNA, Molecular biology, Triturus, Lampbrush chromosome, Genes, Species Specificity, Extrachromosomal DNA, 28S ribosomal RNA, Genetics, RNA polymerase I, Nucleolus Organizer Region, Animals, Nucleolus organizer region, Ribosomal DNA, Genetics (clinical)
Abstract

A variety of 3H-labelled ribosomal gene probes were hybridized in situ to the nascent transcripts of lampbrush chromosomes from the crested newt, Triturus cristatus carnifex. The probes were from Xenopus laevis and included rDNA isolated by CsCl gradient centrifugation, recombinant plasmids and purified restriction fragments of rDNA. All the probes gave essentially the same result. About 10-15 loop pairs were distinctly labelled in each preparation, almost all of them located on the heteromorphic arms (HTAs) of chromosome 1. Ribosomal gene probes were also hybridized in situ to the DNA of denatured mitotic chromosomes from some of the individuals used to provide lampbrush preparations. Minor, scattered sites of hybridization were found in the HTAs, but the main clusters of ribosomal genes were found on chromosomes 6 and/or 9, in agreement with previous determinations of nucleolus organizer position in this species. However, the nucleolus organizers were not sites of labelled loops in lampbrush transcript hybridizations.--We have incubated isolated lampbrush-stage nuclei in media containing alpha-amanitin and labelled RNA precursors. Although extrachromosomal nucleolar genes incorporated label, supposedly due to transcription by RNA polymerase I, no lampbrush loops were labelled.--It appears that in T. c. carnifex there are ribosomal gene sequences at the main nucleolus organizers and at a number of sites scattered along the HTAs. The ribosomal genes at the nucleolus organizers are not extended in the form of actively transcribing loops unlike the ribosomal sequences on the HTAs, which are heavily labelled in transcript hybridization. The ribosomal sequences on the HTAs appear not to be transcribed by the same RNA polymerase that transcribes the ribosomal genes of extrachromosomal nucleoli.

Published
1980

28. Cytological evidence of transcription of highly repeated DNA sequences during the lampbrush stage in Triturus cristatus carnifex

Author

Christine Andrews, Irma Nardi, Jennifer Varley, Harry P. Erba, and Herbert C. Macgregor

Subjects
DNA Replication, Transcription, Genetic, Satellite DNA, Heterochromatin, Biology, DNA, Satellite, DNA sequencing, chemistry.chemical_compound, Oogenesis, Transcription (biology), Genetics, Animals, Genetics (clinical), Nucleic Acid Hybridization, DNA, DNA Restriction Enzymes, biology.organism_classification, Molecular biology, Triturus, Restriction enzyme, Lampbrush chromosome, chemistry, RNA, Female
Abstract

Highly repeated, or satellite, DNA fractions have been isolated from total Triturus cristatus carnifex DNA by renaturation kinetics, caesium salt centrifugation and restriction endonuclease digestion. We have shown by DNA/DNA in situ hybridisation and autoradiography that all of these probes bind to C-band positive regions on mitotic or lampbrush chromosomes of T.c. carnifex. Under conditions of DNA to RNA-transcript in situ hybridisation labelled satellite DNA binds to nascent RNA transcripts that are still associated with the DNA axes of many lampbrush loops. The majority of the loops that label heavily in these experiments are located on the long arms of chromosome I, a region previously shown to be rich in highly repeated DNA and to have many of the properties of heterochromatin. These satellite DNA probes also label many loops on a comparable chromosome region in T. marmoratus, a species closely related to T. cristatus. However, in DNA/RNA-transcript hybrids to other more distantly related species of Triturus, there are no chromosome regions that have the same concentration of labelled loop pairs as the long arms of T.c. carnifex and T. marmoratus, although some loop pairs do label. We have cloned two satellite sequences in pBR322, and have obtained the same results using these pure probes as we obtained using satellite probes isolated by other techniques. These results demonstrate unequivocally that satellite DNA is transcribed on lampbrush chromosomes during oogenesis in crested newts.

Published
1980

29. Heterochromatic DNA in Triturus (Amphibia, Urodela) II. A centromeric satellite DNA

Author

Renata Batistoni, Giuseppina Barsacchi, Federico Cremisi, and Robert Vignali

Subjects
Heterochromatin, Satellite DNA, Centromere, Immunoblotting, Molecular Sequence Data, Restriction Mapping, DNA, Satellite, Genome, Chromosomes, Conserved sequence, Triturus vulgaris, Genetics, Animals, Cloning, Molecular, Genetics (clinical), Genomic organization, Repetitive Sequences, Nucleic Acid, biology, Nucleic Acid Hybridization, biology.organism_classification, Triturus, Blotting, Southern, Karyotyping
Abstract

The MspI family of highly repeated sequences is a centromeric satellite DNA representing about 1% of the genome of the Italian smooth newt, Triturus vulgaris meridionalis. We have studied the structure, genomic organization, chromosomal localization and conservation across species of this family. MspI sequences are around 197 bp long, as shown by sequencing of three cloned units. The family is organized in large clusters of tandemly arrayed units, present at almost all the centromeres of T.v. meridionalis, and is well conserved in the T.v. vulgaris subspecies. Conserved MspI sequences are also present in the related species T. helveticus, where they appear to be clustered at the centromeres of only a few chromosomes. MspI sequences are not found in other Triturus species analysed. The correlation of these sequences with the overall distribution pattern of heterochromatin and the extent of their conservation within the genus Triturus, are discussed.

Published
1988

31. The maps of the lampbrush chromosomes of Triturus (Amphibia Urodela). IV. Triturus vulgaris meridionalis

Author

Giuseppina Barsacchi, Giorgio Mancino, and Luciana Bussotti

Subjects
Germinal vesicle, Morphology (linguistics), biology, Chromosome, Chromosome Mapping, Mitosis, Anatomy, biology.organism_classification, Triturus, Chiasma, Chromosomes, Amphibians, Cytogenetics, Lampbrush chromosome, Triturus vulgaris, Centromere, Genetics, Animals, Female, Genetics (clinical), Ovum
Abstract

The lampbrush chromosomes of Triturus vulgaris meridionalis were isolated from the germinal vesicle of medium and large-sized oocytes and studied with phase-contrast microscope. The maps were constructed on the basis of the lengths and major morphological features of the chromosomes. The length of each map is equal to the mean of the relative lengths of the corresponding chromosome from different oocytes (the relative length of each chromosome is represented by the ratio between its absolute length and that of chromosome XII from the same complement, conventionally considered as 100 units long). The maps arranged in decreasing length order, were oriented according to the most frequent position of chiasmata, as centromeres were not always evident. — Chromosomes VI and XI bear a sphere in subterminal position. Landmarks typical for T. vulgaris meridionalis are the loops inserted on chromosomes VIII (47 units), X (23 units), XI (34 units) and XII (34 units) frequently presenting themselves under the form of double loop bridges of considerable extension. On chromosomes I (4 units), VI (13 units), X (4 units) and XI (36 units) giant bodies were found that are sometimes comparable to dense-matrix loops. Chromosome XI includes a nucleolus-organizing region, sometimes identifiable by the presence of an inserted nucleolus. Normal and granular loops (much extended at times), axial granules, globules, and loopless bars supplement the morphology of the lampbrush chromosomes of this species.

Published
1970

32. Delayed termination of nuclear histone doubling after premeiotic DNA synthesis in Triturus vulgaris male meiosis

Author

Yu. F. Bogdanov and E. N. Antropova

Subjects
DNA Replication, Male, Insecta, Statistics as Topic, Mitosis, Meiocyte, Chromosomes, Histones, Photometry, chemistry.chemical_compound, Cytogenetics, Meiosis, Genetics, Homologous chromosome, Animals, Spermatogenesis, Genetics (clinical), Cell Nucleus, biology, DNA, Molecular biology, Spermatozoa, Triturus, Histone, chemistry, biology.protein, Interphase, Developmental biology
Abstract

It has been shown by means of double wavelength cytophotometry of DNA (Feulgen reaction) and histone (fast green, pH 8.2) inTriturus vulgaris spermatocytes that the doubling of DNA content in nuclei terminates at the end of preleptotene to beginning of leptotene whereas the doubling of histone content begun at premeiotic interphase is delayed and proceeds till the end of leptotene to beginning of zygotene. As a result preleptotene spermatocytes contain approximately 4C DNA and only 3C histone. Histone content in leptotene amounts to 93% of 4C, and in zygotene, pachytene and metaphase I both DNA and histone contents equal 4C. Thus, the temporal pattern of nucleo-histone doubling in meiotic chromosomes ofT. vulgaris differs from the synchronous DNA and histone doubling in mitotic chromosomes of all previously studied species. The delay of histone doubling inT. vulgaris meiocytes is less pronounced than in the previously studied insectsAcheta domestica andPyrrhocoris apterus where the histone content amounts to 3C in leptotene—zygotene and the equal histone/DNA ratio is restored only in pachytene.—Responsibilities for this phenomenon and its biolgoical sinnificance are discussed in connection with recent hypotheses concerning mechanisms of homologous chromosome pairing.

Published
1971

34. Ultrastructure of segmentation mitoses in cleaving newt eggs after blocking of centrospheres by quinoline.

Author

Sentein P and Ates Y

Subjects
Animals, Chromosomes ultrastructure, Female, Organoids ultrastructure, Triturus, Zygote ultrastructure, Mitosis drug effects, Quinolines pharmacology, Salamandridae, Urodela
Abstract

In quinoline treated blastomeres of Triturus helveticus Raz. and Pleurodeles waltlii Michah., microtubules disappear and around the centrioles markedly enlarged dense bodies accompanied by striated bodies are accumulated, from prophase beyond metaphase. It is concluded that these bodies in untreated cells play a role in the formation of the spindle microtubules. - During metaphase the chromosome are smooth-surfaced and show a pronounced tendency to stickiness. During ana-telophase they become surrounded by nuclear membranes and form caryomeres. - Qinoline does not interfere with centriole replication, but prevents the separation if diplosomes that have been already formed, if it acts before that separation. - Some centrioles exhibit different degrees of ultrastructural disarrangement.

Published
1976
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35. Analysis of chromatin-associated fiber arrays.

Author

Laird CD, Wilkinson LE, Foe VE, and Chooi WY

Subjects
Animals, Chromatin ultrastructure, DNA analysis, Drosophila melanogaster, Hemiptera, Microscopy, Electron, RNA biosynthesis, RNA, Ribosomal biosynthesis, Ribonucleoproteins analysis, Triturus, Chromatin analysis, Transcription, Genetic
Abstract

Electron microscopic examination of chromatin from embryonic nuclei of Oncopeltus fasciatus and Drosophila melanogaster reveals arrays of chromatin associated fibers. The lengths and spacings of these fibers were analyzed to provide a basis for defining and interpreting regions of transcriptionally active chromatin. The results of the analysis are consistent with the interpretation of some fibers as nascent RNA with associated protein (RNP). The chromatin segments underlying these fiber arrays were classified as ribosomal or non-ribosomal transcription units according to definitions and criteria described by Foe et al. (1976). Nascent fibers on active ribosomal transcription units were analyzed and compared for Drosophila melanogaster, Triturus viridescens, and Oncopeltus fasciatus. A common feature of the fiber patterns on ribosomal TUs is that origin-distal fibers exhibit greater length variability and a lower slope relative to proximal fibers. The region of increased variability in fiber lengths is correlated with the expected location of 28S ribosomal RNA sequences in the distal half of each ribosomal transcription unit. Because 28S ribosomal RNA appears to contain more extensive regions of base sequence complementarity, we suggest that the length of ribosomal RNP fibers is influenced under our spreading conditions by the secondary structure of the nascent RNA. In order to calculate the RNA content of RNP fibers, chromatin morphology was used to estimate lengths of transcribed DNA. The packing ratio of DNA in chromatin, which we express as the length of B-structure DNA divided by length of chromatin, is 1.1-1.2 and 1.6 for the DNA in active ribosomal and non-ribosomal chromatins, respectively. These DNA packing ratios are used to determine the extent to which nascent RNP fibers are shorter than the transcribed DNA (expressed as DNA/RNP length ratio). For non-ribosomal transcription units and for proximal fibers of ribosomal transcription units. DNA/RNP length ratios are relatively constant within each array. However, considerable variability in this ratio (4-23) is observed for different arrays of fibers. Possible sources of this variability are considered by comparing ratios derived from the presumably identical ribosomal transcription units. Further analysis of the morphology of nascent fibers may elucidate the contributions of proteins and successive RNA sequences to RNP structure.

Published
1976
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36. Evolutionary conservation of a common pattern of activity of nucleolus organizers during spermatogenesis in vertebrates.

Author

Schmid M, Löser C, Schmidtke J, and Engel W

Subjects
Animals, Bone Marrow physiology, Bufonidae, Chickens, Colchicine pharmacology, Fishes, Karyotyping, Male, Organ Specificity, Snakes, Species Specificity, Triturus, Turtles, Biological Evolution, Cell Nucleolus physiology, Spermatogenesis
Abstract

The patterns of activity of the nucleolus organizer regions (NORs) in the spermatogeneses of ten species of all non-mammalian classes of vertebrates and one species of the cephalochordates were investigated with the silver (Ag)-staining technique. The Ag-stainability of the NORs is a measure of the transcriptional activity of the ribosomal RNA genes. In all species, there is a very similar pattern of NOR-activity in the various stages of spermatogenesis. The qualitative analysis of the Ag-stainability of the NORs was in very good agreement with the results obtained for mammals: Ag-stained NORs are detectable during the entire meiotic prophase up to the pachytene stage, completely absent in the meiotic metaphases I and II, and again demonstrable in early spermatid nuclei. The results confirm the occurrence of postmeiotic reactivation of the RNA genes. The preferential inhibition of rRNA synthesis by low doses of actinomycin D induced a rapid decline of the Ag-stainability of the postmeiotically reactivated NORs. The significance of the evolutionary conservation of the postmeiotic NOR-reactivation is discussed.

Published
1982
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37. The structure of chromosome-derived ribonucleoprotein in oocytes of Triturus cristatus carnifex (Laurenti).

Author

Malcolm DB and Sommerville J

Subjects
Animals, Cell Nucleus ultrastructure, Chromosomes analysis, Deoxyribonucleases pharmacology, Detergents pharmacology, Female, Microscopy, Electron, Models, Chemical, Oocytes analysis, Peptide Hydrolases pharmacology, Ribonucleases pharmacology, Transcription, Genetic, Chromosomes ultrastructure, Nucleoproteins analysis, Oocytes ultrastructure, Ovum ultrastructure, RNA analysis, Triturus
Published
1974
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38. Expermental hybridization within the genus Triturus (Urodela: Salamandridae). III. Evidence for crossing-over, true chiasmata and chomosomal homologies in the spermatogenesis of F1 species hybrids, T. cristatus carnifex female X T. marmoratus male.

Author

Mancino G, Ragghianti M, and Bucci-Innocenti S

Subjects
Animals, Chromosomes analysis, Diploidy, Female, Karyotyping, Male, Phenotype, Spermatocytes analysis, Triturus, Crossing Over, Genetic, Hybridization, Genetic, Spermatogenesis
Abstract

Spermatogenesis in the F1 hybrid (2n=24=12 female + 12 male) between the closely related newt species T. cristatus carnifex and T. marmoratus was apparently normal up to pachytene. Many unpaired chromosomes were present at diplotene and a typical diakinesis was lacking. Primary spermatocytes at meta- and meta-anaphase contained up to 12 regular intergenomal bivalents and a corresponding number of univalents when less then 12 II. Most chiasmata were terminal or subterminal, some intercalary. Chiasmata between corresponding heterospecific chromosomes can be reported as true: real crossing over has taken place, proving the presence of primary chromosomal homologies between the 2 sets of the parental species. Evidence for recombination is based on the segregation of particular markers (i.e., subterminal C-bands and NORs) observed in certain chromosomes at metaphase II. One chromatid of single chromosomes can show the T. cristatus "pheno-type" and the other the T. marmoratus phenotype". A few primary spermatocytes contain a certain number of irregular associations (intragenomal or intrahaploid bivalents, irregular intergenomal bivalents, chromosome multivalents) joined by chiasmata which can be defined as anomalous. Other abnormalities concern the occurrence of interlocked bivalents which occasionally show an anomalous exchange between heterologous chromatids. Cytogenetic criteria useful to evaluate the taxonomic relationships between different species have been discussed as well as some possible trends in chromosome evolution and speciation within the genus Triturus.

Published
1979
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39. In situ hybridization of ribosomal DNA labelled with 125iodine to metaphase and lampbrush chromosomes from newts.

Author

Hennen S, Mizuno S, and Macgregor HC

Subjects
Animals, Autoradiography, Centrifugation, Density Gradient, Female, Iodine Radioisotopes, Karyotyping, Male, Methods, Microscopy, Phase-Contrast, Ovary, Ovum cytology, Ribosomes, Triturus, Xenopus, Chromosomes, DNA, Mitosis, Nucleic Acid Hybridization
Abstract

Methods are described for in situ hybridization of ribosomal DNA from Xenopus laevis, labelled in vitro with 125iodine, to mitotic and lampbrush chromosomes from Triturus cristatus carnifex. The hybridization reaction was carried out in a mixture containing 50% formamide, 4 X SSC, 0.1 M KI, at 37 degrees C, or in 2 X SSC, 0.1 M KI at 65 degrees C. Autoradiographs of mitotic metaphases from 2 males showed labelling over the middle of the short arm of one chromosome IX in each metaphase. In some cases, a region near the end of a longer chromosome was also labelled. In a lampbrush preparations, labelling was confined to a region identified as about 53 units, near the middle of the short arm of both halves of bivalent IX. The usefulness of the technique and the significance of the labelling of only 1 of the 2 chromosomes IX in mitotic preparations are discussed.

Published
1975
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40. Length and interspersion of repetitive and non repetitive DNA sequences in four amphibian species with different genome sizes.

Author

Baldari CT and Amaldi F

Subjects
Animals, Base Sequence, Electrophoresis, Agar Gel, Erythrocytes, Microscopy, Electron, Bufo bufo, DNA, Triturus, Urodela, Xenopus
Abstract

The interspersion period of repetitive and unique sequences was analyzed by two different methods, electron microscopy and agarose gel electrophoresis, for four Amphibian species with different nuclear DNA content, namely the Anura Xenopus laevis (3 pg DNA per haploid genome) and Bufo bufo (7 pg) and the Urodela Triturus cristatus (23 pg) and Necturus maculosus (52 pg). Within each of the two subclasses it has been found that interspecific differences, in DNA content, due to variations in the amount of repetitive sequences, do not involve variations in length of the interspersed repetitive sequences. They remain about 380 base pairs. Furthermore, the unique sequences length has been found to be shorter in Bufo (760 base pairs) than in Xenopus (1600) and in Necturus (880) than in Triturus (1340). A study of the interspersion period has shown that the great difference in DNA content between Anura and Urodela, which had been previously shown not to have involved changes in the relative amounts of the various sequence classes, does not involve changes in the interspersion period.

Published
1977
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41. The relationship of a specific chromosomal region to the development of the acrosome.

Author

Schmid M and Krone W

Subjects
Ambystoma, Animals, Heterochromatin, Karyotyping, Male, Salamandra, Salamandridae, Spermatids, Spermatogenesis, Triturus, Urodela, Acrosome, Chromosomes, Spermatozoa
Abstract

In early spermatids of Urodeles the chromosome segments bearing constitutive heterochromatin are localized in one half of the round nucleus; this region becomes the basal part of the long nucleus of the spermatozoon. The euchromatic chromosome segments extend toward the anterior nuclear pole in a bouquet configuration (Macgregor and Walker, 1973). In the course of spermiohistogenesis, one of the heterochromatic regions (the acrosomal chromocenter) migrates from the basal part to the anterior half of the spermatid nucleus. This heterochromatic block is identical with a species-specific, definite C-band in the karyotype. This relationship between the acrosomal chromocenter and a specific chromosomal C-band was established in Triturus cristatus, T. marmoratus, T. alpestric and Cynops pyrrhogaster. In closely related species this particular C-band lies on similar chromosomes. - While the spermatid nucleus still retains its round shape the acrosomal chromocenter despiralizes into a long heterochromatic thread (acrosomal thread). Precisely at the position of this thread the nucleus evaginates and acquires a pear-like shape. During the elongation of the nuclear protrusion the acrosomal thread remains associated with the anterior end. At termination of spermiogenesis it lies closely below the acrosome in the tip of the spermatozoon. Spontaneous aberrations which affect the acrosomal chromocenter or the thread lead to the development of spermatozoa with defective tips. - Several euchromatic segments, interspersed between the heterchromatic segments, can be recognized in the completely despiralized acrosomal thread. Genes responsible for the morphogenetic activities of both, the acrosomal chromocenter and the acrosomal thread, in the development of the spermtip, might be localized in these interspersed euchromatic segments. The existence in higher vertebrates of an acrosomal chromocenter or an equivalent chromosomal region is discussed.

Published
1976
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42. DNA replication in the amphibia.

Author

Wilson BG

Subjects
Animals, Anura, Autoradiography, Bufonidae, Floxuridine metabolism, Floxuridine pharmacology, Isotope Labeling methods, Ranidae, Thymidine metabolism, Tritium, Triturus, Uridine metabolism, Amphibians, DNA Replication drug effects
Abstract

Autoradiographic techniques were used to measure rate of replication and length of the replication unit in cultured cells of Scaphiopus couchi, Bufo cognatus, Rana clamitans, and Triturus viridescens, having nuclear DNA amounts in the ratio 1:4:7:39 respectively. The autoradiographic experiments were designed to show whether the larger amounts of nuclear DNA are correlated with more rapid rates of synthesis and/or with longer replication units. -- The DNA replication rate was 2.5 mu/minute (corrected for two growing points) with 10 minutes 3H-thymidine label at 22 degrees C, but decreased with longer labelling durations. The length of the replication unit (estimated by the distance from the center of one autoradiograph to the center of the next in sequence) was most commonly in the 10-25 mu range with a 30 minute label, in all four species. The average center-to-center distance was 8 mu at 10 minutes and increased with label duration, to over 45 mu with 24 hours label. Replication was predominantly but not exclusively bidirectional. Neither rate of replication nor length of the replication unit was proportional to the amount of DNA in these species.

Published
1975
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