Populations of seven Ancistrus species were analyzed from streams and rivers of three hydrographic Brazilian basins. All populations showed different diploid numbers (2n), fundamental numbers (FNs), and karyotypes. Some representatives of Loricariidae have 2n = 54 chromosomes, which is very likely an ancestral cytotaxonomic characteristic, but many other representatives show extensive karyotype diversification. In the Ancistrus species studied, extensive karyotypic differentiation, which is generally associated with chromosome number reduction and rearrangement of the ribosomal RNA gene (rDNA) sites, was verified. Chromosomal locations of 18S and 5S rDNA were jointly detected using fluorescence in situ hybridization (FISH). In all the Ancistrus species analyzed, 18S rDNA sites were detected only on one chromosome pair, though this differed among species. 5S rDNA was located on 1–3 chromosome pairs either separately or in synteny with 18S rDNA in four of the seven species/populations. Hence the karyotype differentiation in Ancistrus species could be associated with a morphological speciation process, suggesting that chromosome fusions, inversions, deletions, duplications, and heterochromatination could contribute to the karyotype evolution of these neotropical armored catfishes.
Four populations of Ancistrus cf. dubius (Loricariidae, Ancistrinae) were analyzed cytogenetically. They were from different rivers and creeks of the Pantanal Basin, in the state of Mato Grosso, Brazil. The populations were from four distinct locations: population A (4F and 8M), Coxip6 river, in the county of Chapada dos Guimaraes; population B (4F and 11M), Pari Creek, in the county of Cuiabii; population C (18F and 24M), Flechas Creek, the county of Caceres and population D (15F and 7M), Fundo Creek, in the county of Pocone. The modal diploid number is 2n=42 chromosomes (24M, lOSM and 8ST) and FN=84. Band C shows a system of sexual chromosomes XX/XY in populations B, C and D. The Ag-RONs are simple, with markers on pair 16 of the specimens analyzed. Sexual chromosomes aren't rare in fishes butAncistrus shows the unique case of two systems of sexual chromosomes, ZZ/ZW and XX/XY, in the specie identified as Ancistrus cf. dubius, and specimens of population A has no differentiation of the macro and micro chromosomatic structure between males and females. This suggests an alopatric speciation event of Ancistrus cf. dubius and a complex of species thus contributing to the understanding of citotaxonomic-evolutive relations in the Ancistrinae.
Cytogenetic and FISH analyses were performed in 30 Ancistrus cuiabae specimens from a bay near the town of Poconé, in the Pantanal of Mato Grosso, Brazil. The observed diploid number was 2n = 34 chromosomes for both sexes and three distinct katyotypic formulae were found, namely cytotype A (20m, 8sm, 6st, Fundamental Number/FN = 68; 6 males and 11 females), cytotype B (19m, 8sm, 6st, 1a, FN = 67; 8 males and 4 females) and cytotype C (18m, 8sm, 6st, 2a, FN = 66; a single male). NORs's analyses showed that these regions were located in distinct sites on the NOR-bearing chromosome pair, according to cytotypes. Thus, in cytotype A, NORs were located in the terminal region of the short arm of the second metacentric chromosome pair; in cytotype B, they were detected in the short arm of the metacentric chromosome and interstitially on the acrocentric chromosome and, in cytotype C, NORs were observed in the interstitial region of the acrocentric chromosome pair. C-positive heterochromatic bands were adjacent to the rDNA sites in the corresponding chromosomes. Thus, the chromosomal polymorphism of A. cuiabae was probably originated through a pericentric inversion in chromosome pair nº 2 involving the NOR sites, which represents a novelty in the Ancistrini tribe. The results also broaden the knowledge of the chromosomal evolution in Ancistrus, the most derived genus of the Ancistrini tribe.Foram analisados, com técnicas convencionais de citogenética e FISH, 30 exemplares da espécie Ancistrus cuiabae da baía Arrombado, próximo a Poconé, Pantanal do Mato Grosso. Foram observadas metáfases com número diploide 2n = 34 cromossomos para ambos os sexos e três fórmulas cariotípicas distintas, aqui denominadas de citótipo A, verificado em 06 machos e 11 fêmeas (20m, 8sm, 6st, Número Fundamental, NF = 68); citótipo B, em 08 machos e 04 fêmeas (19m, 8sm, 6st, 1a, NF = 67) e citótipo C em apenas 01 macho (18m, 8sm, 6st, 2a, NF = 66). As NORs confirmaram os distintos citótipos verificados, além de evidenciar que os cromossomos portadores de rDNA são os que representam o polimorfismo na espécie Ancistrus cuiabae. No citótipo A, as NORs foram verificadas na região terminal do braço curto do segundo par de cromossomos metacêntricos; no citótipo B, foram evidenciadas no segundo par, heteromórfico, no braço curto do cromossomo metacêntrico e intersticial no seu homólogo acrocêntrico; no citótipo C as NORs foram observadas na região intersticial num par de cromossomos acrocêntricos. A análise da heterocromatina constitutiva evidenciou blocos discretos adjacentes ao rDNA no segundo par de cromossomos de ambos os citótipos. Uma provável inversão pericêntrica é a hipótese proposta para a origem deste polimorfismo na espécie Ancistrus cuiabae. Estes resultados ampliam o conhecimento sobre o gênero Ancistrus, o mais derivado da tribo, contribuem para o conhecimento sobre este grupo de peixes e para inferir sobre a evolução cromossômica dos Ancistrini.
We investigated the chromosomal distribution of 18S ribosomal DNA (rDNA) in different populations of 11 species of Hypostomus collected in important Brazilian basins, namely South Atlantic, Upper Paraná, and Paraguay applying the fluorescence in situ hybridization (FISH). Hypostomus cochliodon, Hypostomus commersoni, Hypostomus hermanni, Hypostomus regani, Hypostomus albopunctatus, Hypostomus paulinus, Hypostomus aff. paulinus, Hypostomus iheringii, and Hypostomus mutucae presented multiple 18S rDNA sites while Hypostomus strigaticeps and Hypostomus nigromaculatus exhibited a single pair of chromosomes with 18S rDNA sites. The studied species presented variations in the number and position of these sites. The results accomplished were similar to those obtained by the analysis of AgNORs, revealing the same interspecific variability. Each species exhibited distinctive patterns of AgNOR and 18S rDNA distribution, which can be considered cytogenetic markers in each species of the genus and help improve the discussions on the phylogeny of the group.
Astyanax is one of the most abundant and diverse taxa of fishes in the Neotropical region. In order to increase the amount of cytogenetic information for Astyanax as well as to exhibit data to subsidize future taxonomic studies, this work analyzed three species of Astyanax: two species are cryptic, and are here reported to live in syntopy (A. abramis and A. lacustris); the first karyotype description for A. pirapuan is also presented. Cytogenetic analyzes reveal a diploid number of 2n=50 chromosomes for three species, yet with differences in their karyotype morphology. The physical mapping of 18S rDNA showed up to thirteen sites in A. pirapuan and two in A. abramis and A. lacustris. The physical mapping of 5S rDNA has proven to be an effective marker for the characterization of species of Astyanax studied in this work.
Cytogenetic analyses were carried out in 117 specimens of seven species of the genus Ancistrus from three hydrographic in Mato Grosso State: Paraguay, Araguaia-Tocantins and Amazon basins. Conventional cytogenetic techniques were used to obtain mitotic chromosomes. C-banding was performed to detect heterochromatic regions and silver nitrate staining was used to identify nucleolar organizer regions (Ag-NORs). The counted and paired chromosomes revealed diploid numbers ranging from 2n = 40 to 2n = 54 with karyotype formulae varying from FN = 80 to FN = 86. Single marks in distinct chromosomes identified the nucleolar organizer regions. The constitutive heterochromatin was scarce in the diploid number from 2n = 50 to 2n = 54 and conspicuous blocks were observed in a single species with 2n = 40 chromosomes. These data corroborate the hypotheses of reduction of diploid number in species with derived features such as presence of sex chromosomes and polymorphisms, besides allowing inferences about the evolutionary mechanisms and the ancestor karyotype that favored the diversification of this important genus in the tribe Ancistrini. Foram realizadas análises citogenéticas de 117 espécimes do gênero Ancistrus de três bacias hidrográficas do estado de MatoGrosso: Paraguai, Araguaia-Tocantins e Amazônica, utilizando as técnicas de citogenética convencional para obtenção de cromossomos mitóticos, visualização de regiões heterocromáticas e regiões organizadoras de nucléolos. Os cromossomos pareados revelaram uma variação no número diploide de 2n = 40 a 2n = 54 e número fundamental de NF = 80 a NF = 86. As regiões organizadoras de nucléolos foram evidenciadas em um único par de cromossomos para todas as espécies e a heterocromatina é escassa nas espécies com números diploides elevados (2n = 50 a 2n = 54). Os blocos heterocromáticos mais evidentes foram observados nos pares portadores das AgRONs e em cromossomos da espécie com 2n = 40. Estes dados contribuem para a hipótese de redução do número diploide nas espécies que apresentam polimorfismos cromossômicos e cromossomos sexuais, além de contribuir para inferências sobre os mecanismos de evolução cariotípica que favoreceu a diversificação do gênero Ancistrus, o mais representativo na tribo Ancistrini.
The present study was stimulated by the growing demand for healthy food and the technology available for the detection and identification of microbial organisms in fishery products. Molecular tools were used to identify the bacterial community and detect the presence of pathogenic species in samples of farmed and wild-caught fish. Samples of muscle tissue were obtained from the local market in Cuiabá, Mato Grosso, Brazil. The 16S rDNA gene was used to detect 11 bacterial genera: Enterobacter (29.29%), Aeromonas (24.24%), Pseudomonnas (17.17%), Enterococcus (10.10%), Acinetobacter (6.06%), Citrobacter (4.04%), Bacillus (3.03%), Klebsiella and Lactococcus (2.02%), and Clostridium and Lysinibacillus (1.01%). High percentages of deleterious bacteria were recorded. Species-specific primers were used to detect the presence of Escherichia coli (35.71%), Staphylococcus aureus (12.5%), and Salmonella (7.14%), although Shigella was absent. These concentrations exceeded the limits established by the currently public health legislation. The molecular techniques used in the present study provide an alternative approach for the reliable diagnosis of contamination, which can be used on a large scale.
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