Daniela dos Santos Brum
Universidade Federal de Santa Maria
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Featured researches published by Daniela dos Santos Brum.
Brazilian Journal of Veterinary Research and Animal Science | 2002
Daniela dos Santos Brum; Fábio Gallas Leivas; Mari Lourdes Bernardi; Lucio Pereira Rauber; Alceu Mezzalira; Karin Erica Brass; Carlos Antonio Mondino Silva; Mara Iolanda Batistella Rubin
In vitro produced bovine embryos were individually cultured from D7 to D9 to observe their development. Forty-nine blastocysts (early blastocyst, blastocyst and expanded blastocyst) were individually cultured, from D7 to D9 (D0= fertilization), in 50ml SOF medium plus 5% OCS. Between D7 and D8, blastocysts were cultured in straws (SC) or in plates (PC) and from D8 up to D9, they were cultured on plates. The ratio of early blastocyst, blastocyst, and expanded blastocyst advancing at least one stage of development were, respectively, 71%, 37%, 44% in PC and 100%, 66%, 36% in SC (P>;0.05). Overall development rates on D8 were not significantly different (P>;0.05) for PC (50%) and SC (60%). At D9, both culture systems produced similar (P>;0.05) hatching rates (29% and 24% for PC and SC, respectively). After fluorescent nuclei staining, the average number of cells counted in the hatched (182.7 vs. 202.8) and expanding (94.5 vs. 88.0) blastocysts were similar (P>;0.05) for PC and SC, respectively. In vitro produced bovine blastocysts can be individually cultured from D7 to D9, and the culture system employed (dishes or straws) has no effect on hatching rates and cell number of developed blastocysts.
Ciencia Rural | 2004
Fábio Gallas Leivas; Daniela dos Santos Brum; Alceu Mezzalira; Luis Fernando Cáceres Pilla; Mari Lourdes Bernardi; Mara Iolanda Batistella Rubin; Carlos Antonio Mondino Silva
Oocytes (n=1177) aspirated from 2 to 8mm follicles obtained from bovine slaughterhouse ovaries (11 replications) were randomly distributed in four treatments. Oocytes were matured for 24h with modified TCM-199 Earle salts, plus 25mM bicarbonate, 25 mM HEPES, rFSH-h, Estrus Cow Serum (ECS), and piruvate at 39oC, in incubator with 5% CO2 and saturated humidity (Control Group, n=296) or exposed to a simulated transport for 6 (T6, n=286), 12 (T12, n=294) or 18h (T18, n=301) in maturation medium containing TCM + HEPES, in a 39oC water bath, with the same components used in the Control Group, but with 1mM bicarbonate. At the conclusion of each transport period, oocytes were transferred to dishes with maturation medium to reach 24h in incubator, under the same conditions described for the Control group. Fertilization was accomplished during 18h, with the same temperature and gaseous atmosphere, in FERT-TALP plus heparin. The insemination dose was 1x106 spermatozoa/mL, sorted by swim-up. Presumptive zygotes were cultured in SOF medium + 5% ECS for 8 days, in incubator at 39oC using gasified bags with 5% CO2, 5% O2 and 90% N2. Cleavage rates did not differ between treatments. Embryonic development rates at D7 were similar for Control (20.9%), T6 (19.2%) and T12 (21.4%) groups, with a reduction (P 0.05) in hatched blastocyst rate. The average number of cells of hatched blastocysts was similar (P>0.05) in Control (136), T6 (125.5) and T12 (126.8) groups. These results indicate the possibility of transporting bovine oocytes in maturation medium containing TCM + HEPES, without controlled gaseous atmosphere environment, at 39oC, for up to 12 hours. This technique offers a practical and efficient alternative for the transport of bovine oocytes for in vitro production of bovine embryos (IVP).
Brazilian Journal of Veterinary Research and Animal Science | 2003
Lucio Pereira Rauber; Denis Faustino Alves; Giuliano Moraes Figueiró; Daniela dos Santos Brum; Tiago Fernando Hilgert; Mari Lourdes Bernardi; Carlos Antonio Mondino Silva; Mara Iolanda Batistella Rubin
Bovine oocytes have been maintained in the follicular fluid to be transported and to increase their competence, before maturation. Eight hundred eighty-one (881) oocytes, aspirated from bovine slaughterhouse ovaries, were used to evaluate the effect of holding bovine oocytes in follicular fluid (FF) of bovine follicles of different diameters on the rate of embryo development. The oocytes were randomly distributed in four treatments with seven replicates each: The control group (n=217) was constituted by oocytes matured for 24h in modified TCM-199 with Estrus Mare Serum (EMS), pyruvate and rFSH-h in incubator with 5,00% CO2, 39°C and saturated humidity. In the FFsmall group (3 to 5mm follicles; n=216), the oocytes were held for 6h in follicular fluid at 30°C and matured for 18h in the same conditions of the Control-group. The oocytes of the FFmedium group (5,1-8mm follicles; n=226) and of the FFlarge group (>8,1mm follicles; n=222) were held in follicular fluid and matured like FFsmall. Fertilization was accomplished during 18h and, after this, the zygotes were cultured for 8 days in SOFaaci medium + 5,00% EMS in incubator at 39°C using plastic bags gasified with 5,00%CO2, 5,00%O2 and 90,00%N2. FFsmall oocytes produced a lower (P 0,05) between the groups. Follicular fluid of medium and large follicles could be used to hold for 6h at 30°C bovine oocytes before their maturation for 18h.
Animal Reproduction Science | 2018
Daniele Missio; Natália Picolli Folchini; Fábio Gallas Leivas; Cecilia Urquiza Machado Pavin; Hirya Fernandes Pinto; Francielli Weber Santos Cibin; Daniela dos Santos Brum
The aim of the present study was to evaluate the effects of Percoll volume on recovery rate, sperm quality, and embryo development kinetics in in vitro production of cattle embryos. Straws of conventional and sex-sorted semen were allocated to three different volumes of Percoll: 300 μL of each Percoll gradient (90%, 60%, and 30%), Control; 100 μL of each Percoll gradient, P100; and 200 μL of each Percoll gradient, P200. Sperm quality, fertilization rate, and embryo morpho-kinetic development using time lapse cinematography up to 48 h post-insemination were evaluated. For conventionally processed semen, sperm motility, vigor, and recovery rate were greater in the P100 and P200 treatment groups compared to the Control (P < 0.05), whereas reactive oxygen species (ROS) concentrations, lipid peroxidation, and superoxide dismutase enzyme activity were not influenced by treatments. For sex-sorted semen, treatment with P100 increased sperm curvilinear velocity, average path velocity, and amplitude of lateral head displacement (P < 0.05). Recovery rate was greater in the P100 group than Control and P200 groups (P < 0.05), formation of ROS was less in the P100 than Control and P200 groups, and superoxide dismutase enzyme activity was less in the P100 than Control group. Fertilization and cleavage rates, time of first cleavage, and cell number were similar between the P100 and Control groups (P > 0.05). The inclusion of Percoll volumes of 100 μL resulted in an increased sperm recovery rate without damage to sperm quality or affecting early embryonic development.
Brazilian Journal of Veterinary Research and Animal Science | 2006
Daniela dos Santos Brum; Fábio Gallas Leivas; Mari Lourdes Bernardi; Fabrício Desconzi Mozzaquatro; Carlos Antonio Mondino Silva; Mara Iolanda Batistella Rubin
Archive | 2002
Giuliano Moraes Figueiró; Sergio da Silva Fialho; Daniela dos Santos Brum; Marta Pasin; Lucio Pereira Rauber; Mari Lourdes Bernardi; Alceu Mezzalira; Mara Iolanda Batistella Rubin; Carlos Antonio Mondino Silva
Anais do Salão Internacional de Ensino, Pesquisa e Extensão | 2017
Aryele Pinto Izaguirry; Francielli Weber Santos Cibin; Luana Roberta Michels; Daniela dos Santos Brum; Sandra Elisa Haas
Anais do Salão Internacional de Ensino, Pesquisa e Extensão | 2017
Tainara Bremm; Daniela dos Santos Brum; Karine de Mattos; Gabriela Ceratti Hoch
Anais do Salão Internacional de Ensino, Pesquisa e Extensão | 2017
Pauline Souza; Daniela dos Santos Brum; Tainara Bremm; Daniele Missio; Fábio Gallas Leivas
Anais do Salão Internacional de Ensino, Pesquisa e Extensão | 2017
Karine de Mattos; Daniela dos Santos Brum; Wilson Viotto; Marcelo Becker; Cassiane Aguiar