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1.
J Genet ; 2019 Nov; 98: 1-14
Article | IMSEAR | ID: sea-215407

ABSTRACT

A wide range of diploid number of chromosomes and the body size of Channa congeners are useful combination of characters for studying the factors controlling the body size. In this study, the karyological information was superimposed on the evolutionary tree generated by 16S rRNA mitochondrial gene sequences. Here, the metaphase chromosome complements stained with Giemsa, AgNO3 and CMA3 were prepared from six snakehead murrel fish species collected from northeast India. The diploid chromosome numbers and the fundamental arms of C. aurantimaculata (2n = 52, NF = 98), C. gachua (2n = 56, NF = 84), C. marulius (2n = 44, NF = 58), C. orientalis (2n = 52, NF = 74), C. punctata (2n = 32, NF = 60) and C. striata (2n = 40, NF = 48) were calculated by the analysis of metaphase chromosome complements. Both methods of nucleolar organizer region (NOR) localization, silver nitrate and chromomycin A3, revealed NOR pairs of 1, 2, 3, 1, 4 and 3 in C. aurantimaculata, C. gachua, C. marulius, C. orientalis, C. punctata and C. striata, respectively. The subject species showed primitive type of asymmetrical chromosomes, except the C. punctata. The variation in 2n for C. orientalis (2n = 52, 78) and C. gachua (2n = 52, 78, 104) of a complete haploid set indicates the possibility of either ploidy change in . orientalisC and C. gachua, if we consider 2n = 52 or the Robertsonian rearrangements in different populations of these two species. The chromosome evolution tree was constructed on 16S rRNA ML-phylogenetic tree using ChromEvol 1.3. The analysis of chromosome evolution explained the loss or gain of chromosome, duplications or semiduplications mechanism. For time scaling the chromosomeevolution, the node age of available 16S rRNA gene of Channa species were estimated, which was also used for estimating the time when chromosomal changes occurred in context of geological time-scale.

2.
Neotrop. ichthyol ; 8(3): 667-671, 2010. ilus
Article in English | LILACS | ID: lil-562951

ABSTRACT

Cytogenetic analyses were performed in Astyanax jacuhiensis from lago Guaíba, Brazil. The diploid number was 50, with a karyotype composed of 8m+30sm+4st+8a chromosomes, FN = 92. The AgNORs were observed in 2 to 5 chromosomes, with intra- and interindividual variation. The sm pair 8 observed always carried NORs on the short arms, presenting size heteromorphism between homologous. Fluorescence in situ hybridization (FISH) with an 18S rDNA probe only confirmed the location of ribosomal cistrons in the sm pair 8, and heteromorphism of these regions between the homologous chromosomes. C-banding revealed the occurrence of weak C-positive heterochromatin in the pericentromeric regions of several chromosomes, in addition to more evident bands interstitially located on some chromosome pairs and in the terminal region of the short arms in pair 8. C-banding plus CMA3 revealed light fluorescent signals in different chromosomes of the karyotype, with a strong terminal site in pair 8, indicating the occurrence of several GC-rich heterochromatic regions in this species. Our results provide the first description of the Astyanax jacuhiensis karyotype, showing karyotype similarities when compared to various populations of A. altiparanae and A. bimaculatus, indicating that chromosomal features are very similar for these three species.


Análises citogenéticas foram realizadas em Astyanax jacuhiensis do lago Guaíba, Brasil. O número diplóide foi 50, sendo o cariótipo composto por 8m+30sm+4st+8a cromossomos, NF = 92. As regiões organizadoras de nucléolos (AgNORs) foram observadas em 2 a 5 cromossomos, evidenciando uma variação intra e interindividual nesta espécie. O par sm 8 foi constantemente detectado com NORs nos braços curtos, mostrando um heteromorfismo de tamanho entre os homólogos. Entretanto, a hibridação in situ fluorescente (FISH) com sonda de DNAr 18S, localizou cístrons ribossômicos apenas no par 8, confirmando o heteromorfismo de tamanho entre os homólogos. O bandamento C revelou a presença de bandas discretas de heterocromatina na região pericentromérica da maioria dos cromossomos, além de algumas bandas mais evidentes intersticiais, bem como na região terminal dos braços curtos do par 8. A associação de BC+CMA3 evidenciou marcações fluorescentes mais discretas em diferentes cromossomos e uma forte marcação terminal no par 8, confirmando vários sítios de heterocromatina GC-rica nessa espécie. Nossos resultados fornecem a primeira descrição do cariótipo de Astyanax jacuhiensis, apresentando semelhanças em relação ao cariótipo de diferentes populações de A. altiparanae e A. bimaculatus, indicando que as características cromossômicas são muito semelhantes para estas três espécies.


Subject(s)
Animals , /analysis , Nucleolus Organizer Region/genetics , Genetic Variation/genetics , Cytogenetic Analysis/veterinary , In Situ Hybridization, Fluorescence/veterinary , Fishes/genetics
3.
Genet. mol. res. (Online) ; 6(2): 284-291, 2007. ilus
Article in English | LILACS | ID: lil-482042

ABSTRACT

The karyotypes of two species of catfish, Rita rita (Hamilton) (2n = 54; 14m + 34sm + 6st; NF = 102) and Mystus gulio (Hamilton) (2n = 58; 30m + 12sm + 2st + 14t, NF = 100) were studied through Giemsa-, silver- and chromomycin A(3)-staining techniques. The silver-stained karyotypes in both sexes of R. rita and M. gulio revealed that the nucleolus organizing regions were located terminally at the shorter arms (Tp) of one pair of submetacentric chromosomes, placed at positions Nos. 2 and 1, respectively, which was confirmed by scanning electron microscopy. Staining with a GC-specific fluorochrome, chromomycin A(3), produced bright fluorescence in the Ag-positive nucleolus organizer regions, suggesting thereby that nucleolus organizing regions actually included GC-rich sites of active r-RNA genes in metaphase chromosomes of these two bagrids. Further such studies are needed due to the extreme paucity of data on fish.


Subject(s)
Animals , Male , Female , Chromosomes/ultrastructure , Catfishes/genetics , Nucleolus Organizer Region/genetics , Karyotyping , Staining and Labeling/methods , Base Composition , Chromomycins , Silver Staining , Microscopy, Electron, Scanning
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