S. M. M. K. Martins
University of São Paulo
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Featured researches published by S. M. M. K. Martins.
Reproduction in Domestic Animals | 2011
Afc De Andrade; Fabiane Gilli Zaffalon; E. C. C. Celeghini; Juliana Nascimento; Ofb Tarragó; S. M. M. K. Martins; Maria Augusta Alonso; Rubens Paes de Arruda
Effect of seminal plasma addition after thawing on viability or cryocapacitation is not definitively established. This experiment was performed to verify the effect of adding seminal plasma, autologous or homologous (from an animal with good semen freezability). Five ejaculates from each of four stallions with proven fertility were collected and cryopreserved. The semen was subsequently thawed and divided into the following three treatment groups: no seminal plasma addition after semen thawing (NOSP); the addition of homologous seminal plasma after semen thawing (HSP) and the addition of autologous seminal plasma after semen thawing (ASP). The addition of 20% of seminal plasma led to an increase in the cell population that simultaneously show plasma and acrosomal membrane integrity (p < 0.05). The addition of seminal plasma did not alter the total motility, the amount of cells with mitochondrial membrane potential or the sperm velocities (average path velocity, straight-line velocity and curvilinear velocity). However, the beat/cross-frequency, straightness and linearity were reduced in ASP and HSP groups (p < 0.05). Unexpectedly, the addition of homologous seminal plasma reduced the proportion of cells with progressive motility (p < 0.05) and the addition of autologous seminal plasma reduced the amplitude of the lateral head displacement (p < 0.05). Based on the increase in the cell populations that had the plasma and acrosomal membrane integrity simultaneously identified in this study, we proposed that the addition of seminal plasma (autologous or homologous) into post-thawed semen before insemination could increase semen fertility.
Andrologia | 2015
S. M. M. K. Martins; A. F. C. de Andrade; Fabiane Gilli Zaffalon; F. F. Bressan; S.M.P. Pugine; M.P. Melo; Marcos R. Chiaratti; Ct Marino; A. S. Moretti; Rubens Paes de Arruda
This study evaluated the effects of dietary organic selenium (Se) on viability of chilled boar semen. Twelve boars were divided into three groups: control (CON), 0.3 mg kg−1 sodium selenite; inorganic (INO), 0.5 mg kg−1 sodium selenite and organic (ORG), 0.5 mg kg−1 Se yeast. The experiment was conducted within 10 weeks, and analysis was performed fortnightly, in storage semen by 72 h. No effect was observed on motility; however, straightness and linearity percentages were higher (P < 0.05) in the animals receiving CON diet compared with INO group. Percentages of cells with both plasma and acrosomal intact membranes, lipidic membrane peroxidation and mitochondrial membrane potential were similar on all treatments. Animals receiving CON diet presented higher (P < 0.05) values of ATP when compared with INO group. The PHGPx was higher (P < 0.05) in animals that received ORG in comparison with INO group. In conclusion, organic selenium supplementation increases PHGPx but does not improve chilled semen viability in 72 h.
Journal of Animal Science | 2016
M. A. Torres; G. M. Ravagnani; D. F. Leal; S. M. M. K. Martins; B. B. D. Muro; F. V. Meirelles; F.O. Papa; J.A. Dell’Aqua; Marco Antonio Alvarenga; A. S. Moretti; A. F. C. de Andrade
Boar spermatozoa arising from the sperm-rich ejaculate fraction are reported to have a more stable plasma membrane and are more resistant to cold shock and premature acrosome reaction than spermatozoa from the whole ejaculate. Furthermore, seminal plasma (SP) can increase the cryotolerance of boar spermatozoa, and in other domestic species, it has the ability to reverse cryopreservation damage. This study aimed to evaluate the effects of boar SP arising from the whole sperm-rich ejaculate fraction (SP-SRF) on the integrity, stability, and peroxidation of sperm membranes after thawing. Each ejaculate ( = 24) was divided among 4 treatments: control (CT), centrifuged and suspended in autologous SP-SRF (CS), centrifuged with withdrawn SP-SRF (CW), and post-thawed SP arising from the whole sperm-rich fraction addition to CW (CWSP). After thawing, all treatments were incubated for 5, 60, and 120 min and were analyzed for membrane integrity, fluidity, and peroxidation by flow cytometer. The absence of SP-SRF increased the lipid disorder ( < 0.05) but had no effect on lipid peroxidation ( > 0.05) or membrane integrity ( > 0.05). However, the increase in lipid disorder by withdrawal of SP-SRF was reversed by SP-SRF addition ( < 0.05) to the post-thawing medium, whereas plasma and acrosomal membrane integrity ( > 0.05) and lipid peroxidation ( > 0.05) were unchanged. In conclusion, despite the centrifugation effects, the addition of SP arising from the whole sperm-rich fraction to post-thawed boar semen decreased sperm lipid disorder without an influence of the sperm membrane integrity and peroxidation.
Reproduction in Domestic Animals | 2014
Oho Eckhardt; S. M. M. K. Martins; Me Pinese; Fc Horta; Ac Rosseto; Ma Torres; Afc De Andrade; Bbd Muro; Ct Marino; Phm Rodrigues; Aníbal de Sant'Anna Moretti
The aim of this study was to evaluate the reproductive performance of three parities of gilts treated or not treated with gonadotropin to induce puberty. Sixty gilts received 600 IU of equine chorionic gonadotropin (eCG) followed by 2.5 mg of porcine luteinizing hormone (LH) 72 h later. Fifty-nine other gilts were exposed only to a mature boar for 15 min twice daily. Artificial insemination (AI) was performed at 0, 12 and 24 h after the detection of oestrus, and gestation was confirmed by ultrasound after 35 days. Sows were inseminated at the first post-weaning oestrus. The total numbers of piglets born, piglets born alive, stillborn, mummified foetuses, as well as pregnancy and farrowing rates were evaluated for each of the three parities. Culling rates, farrowing intervals and weaning-to-oestrous intervals (WEI) were also analysed. Mean age at puberty and oestrous manifestation were not significantly different between treatments (p = 0.0639; 179.20 ± 17.52 compared with 173.96 ± 16.94, 91.66% compared with 94.92%) across the experimental period. However, females that underwent puberty induction showed modest increases both in the number of total pigs born and in the number of piglets born alive. In conclusion, puberty induction through exogenous gonadotropin administration in field conditions did not induce a more concentrated first oestrous manifestation, but trended to a modest increase in the number of pigs born alive in the first parity and a reduced culling rate during the first gestation.
Animal Reproduction Science | 2018
D. F. Leal; M. A. Torres; G. M. Ravagnani; S. M. M. K. Martins; F. V. Meirelles; A. F. C. de Andrade
Seminal plasma (SP), the fluid that surrounds the sperm cells, is known to exert substantial influence on sperm physiology. The SP has a pivotal role in sperm function in vivo, and due to its components, it functions in an ambiguous manner in vitro, simultaneously possessing deleterious and beneficial effects. This experiment aimed to describe the differences between the presence or absence of SP from the sperm-rich fraction on some spermatozoa characteristics (kinetics, plasma and acrosome membrane integrity, lipid peroxidation and capacitation-like changes). Furthermore, this experiment focused on distinguishing the effects of SP on the variables evaluated from the effects of centrifugation during SP removal. Total and progressive sperm motility, as well as integrity of plasma and acrosome membranes, were less (P < 0.05) in the absence of SP. Membrane lipid peroxidation (P < 0.05) and sperm membrane stability (P < 0.05) did not differ among treatments. The SP from the sperm-rich fraction is important for the maintenance of adequate structural and functional characteristics of extended liquid boar semen and should be present in seminal doses throughout storage. Furthermore, the detrimental effect on the variables evaluated was caused solely by the absence of SP and not by the process of removal through centrifugation at 500 x g for 10 min.
Reproduction in Domestic Animals | 2007
Afc De Andrade; R. P. de Arruda; E. C. C. Celeghini; Juliana Nascimento; S. M. M. K. Martins; Cláudia Fernandes Raphael; Aníbal de Sant'Anna Moretti
Livestock Science | 2014
S. M. M. K. Martins; A. F. C. de Andrade; Fabiane Gilli Zaffalon; Larissa José Parazzi; F. F. Bressan; S.M.P. Pugine; M.P. Melo; Marcos R. Chiaratti; Ct Marino; Esther Ramalho Afonso; A. S. Moretti; Rubens Paes de Arruda
Animal Reproduction Science | 2008
Rubens Paes de Arruda; André Furugen Cesar de Andrade; Cláudia Fernandes Raphael; K.R. Peres; Juliana Nascimento; S. M. M. K. Martins; L.L. Bianconi
Animal reproduction | 2017
V. H. B. Rigo; M. A. Torres; D. F. Leal; B. B. D. Muro; S. M. M. K. Martins; M. S. Monteiro; G. M. Ravagnani; A. P. P. Pavaneli; M. S. Passarelli; A. F. C. de Andrade
Animal reproduction | 2017
V. H. B. Rigo; M. A. Torres; D. F. Leal; B. B. D. Muro; S. M. M. K. Martins; G. M. Ravagnani; A. P. P. Pavaneli; M. S. Monteiro; M. S. Passarelli; A. F. C. de Andrade