960 resultados para extended liquid boar semen
Resumo:
O plasma seminal é o constituintes não celular do sêmen suíno e contém uma série de componentes orgânicos e inorgânico que desempenham ações variadas tanto no trato reprodutivo masculino como no feminino. No entanto, este fluido de constituição complexa, exerce ações ambiguas sobre os espermatozoides suínos, pois pode atuar ao mesmo tempo de forma benéfica ou deletéria sobre a viabilidade destas células. Nesse sentido, alguns estudos sugerem que este não é o melhor meio para a conservação de espermatozoides. Desta forma o objetivo deste trabalho foi avaliar os efeitos do plasma seminal sobre a integridade das membranas plasmática e acrossomal e o potencial de membrana mitocondrial do espermatozoide suíno armazenado sob refrigeração a 17°C por 72 horas. Para tanto, foram obtidos 4 ejaculados de 6 cachaços. Em seguida o sêmen in natura foi avaliado quanto às características da motilidade pelo sistema computadorizado de análise do sêmen, morfologia espermática por contraste de interferência diferencial e concentração espermática. Após essa primeira avaliação, os ejaculados foram acondicionados em tubos cônicos de 50 mL para serem divididos em três tratamentos, a saber: não centrifugado (NC), centrifugado e com o plasma seminal retirado pós-centrifugação (CS) e centrifugado resuspendido (CR). A força de centrifugação utilizada foi de 500xg por 10 minutos. Todos os tratamentos foram submetidos à diluição em meio BTS para que se obtenha uma concentração de 30 x 106 espermatozoides por mililitro (mL). Em seguida, as amostras permaneceram por 90 minutos em temperatura ambiente e protegidas da luz antes de serem armazenadas. As doses com os diferentes tratamentos foram acondicionadas à temperatura de 17°C e foram avaliadas nos intervalos 0 (90 min pós-diluição), 24, 48 e 72 horas para os seguintes parâmetros: características da motilidade (CASA), integridade das membranas plasmática e acrossomal, estabilidade da membrana plasmática e peroxidação das membranas espermáticas (citometria de fluxo). Os tratamentos foram submetidos à análise de variância (PROC GLM), empregando-se o programa SAS (1998). Quando o principal efeito foi significativo, as médias foram comparadas pelo teste de Tukey-kramer ao nível de 5% de significância. Os resultados do presente estudo mostram que a ausência do plasma seminal foi deletéria para algumas características de motilidade, o mesmo ocorreu para a integridade das membranas plasmática e acrossomal uma vez que houve diminuição na percentagem de celulás espermáticas com membrana plasmatica integra e acrossomo integro no tratamento sem plasma seminal. A peroxidação lipídica das membranas e a manutenção da estabilidade da membrana plasmática não foram influenciadas pelo tratamento. Assim, conclui-se que a presença do plasma seminal em doses inseminantes refrigeradas por 72 h é importante para a manutenção das características de motilidade e para a integridade das membranas plasmáticas e acrossomal
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Artificial insemination is routinely used in the swine industry to reduce the costs of production through to increase the efficiency of the refrigerated boar semen process. The objective of this study was to evaluate the effect of different levels of cysteine (CYS) added to the Beltsville Thawing Solution (BTS) extender semen during cooling for up to 72 hours. Ejaculated from three boars were collected with the gloved-hand technique and semen aliquots were diluted in BTS as follow: BTS only (BTS), BTS + 0.1mM cysteine (CYS0.1), BTS + 0.5mM cysteine (CYS0.5), BTS + 1.0mM cysteine (CYS1.0), BTS + 2.5mM cysteine (CYS2.5), BTS + 5.0mM cysteine (CYS5.0), BTS + 10.0mM cysteine (CYS10.0), and BTS + 20.0mM cysteine (CYS20.0). Evaluation of sperm integrity were analyzed using 0.5mg/ml propidium iodide (plasma membrane), 100µg/ml isothiocynate-conjugated Pisum sativun agglutinin (acrosomal membrane) and 153µM 5,5',6,6'-tetrachloro-1,1',3,3'-tetraethylbenzimidazolyl carbocyanine iodide (mitochondria potential) after semen dilution at specific times (0, 24, 48 and 72 hours). Additionally, we also evaluated the effects of 5.0 mM CYS addition in the BTS extender on the maintenance of sperm quality and their influence on fertility in the swine production. After artificial insemination, animals were evaluated based on the estrous return and the number of piglet's born. Cysteine at concentrations of 10.0 and 20.0mM resulted in more pronounced reductions even at the time zero. Semen viability decreased to levels below 10% at these high levels of CYS in the first 24 hour of storage at 17ºC. At the end of the storage time, less than 65% of sperm cells had intact plasma membrane in all groups. The sperm viability decreased significantly when the semen was added at high concentrations of CYS (time "0"; CYS10.0 and CYS20.0; p<0.05), when compared to the other CYS concentrations. The BTS (10.20±0.39) treated group showed a lower rate of estrus return when compared to other (BTSCYS; 86.05±039), and it showed also the highest total number of piglets borne per treatment (12.71±3.38 vs. 9.00±3.38, respectively). In conclusion, the addition of CYS in the BTS semen extender did not maintain spermatic viability of boar cooled spermatozoa and it results in a higher percentage of return to estrus and lower number of piglets borne.
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Switzerland is currently porcine reproductive and respiratory syndrome virus (PRRSV) free, but semen imports from PRRSV-infected European countries are increasing. As the virus can be transmitted via semen, for example, when a free boar stud becomes infected, and the risk of its import in terms of PRRSV introduction is unknown, the annual probability to accidentally import the virus into Switzerland was estimated in a risk assessment. A quantitative stochastic model was set up with data comprised by import figures of 2010, interviews with boar stud owners and expert opinion. It resulted in an annual median number of 0.18 imported ejaculates (= imported semen doses from one collection from one donor) from PRRSV-infected boars. Hence, one infected ejaculate would be imported every 6 years and infect a mean of 10 sows. These results suggest that under current circumstances, there is a substantial risk of PRRSV introduction into Switzerland via imported boar semen and that measures to enhance safety of imports should be taken. The time from infection of a previously negative boar stud to its detection had the highest impact on the number of imported 'positive' ejaculates. Therefore, emphasis should be placed on PRRSV monitoring protocols in boar studs. Results indicated that a substantial increase in safety could only be achieved with much tighter sampling protocols than currently performed. Generally, the model could easily be customized for other applications like other countries or regions or even sow farms that want to estimate their risk when purchasing semen from a particular boar stud.
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An outbreak of porcine reproductive and respiratory syndrome virus (PRRSV) occurred in November 2012 in Switzerland (CH), traditionally PRRSV-free. It was detected after a German boar stud informed a semen importer about the detection of PRRSV during routine monitoring. Tracing of semen deliveries revealed 26 Swiss sow herds that had used semen from this stud after its last negative routine monitoring and 62 further contact herds. All herds were put under movement restrictions and examined serologically and virologically. As a first measure, 59 sows from five herds that had previously been inseminated with suspicious semen were slaughtered and tested immediately. Investigations in the stud resulted in 8 positive boars with recent semen deliveries to CH (Seven with antibodies and virus, one with antibodies only). In one boar out of six tested, virus was detected in semen. Of the 59 slaughtered sows, five from three herds were virus-positive. In one herd, the virus had spread, and all pigs were slaughtered or non-marketable animals euthanized. In the remaining herds, no further infections were detected. After confirmatory testings in all herds 3 weeks after the first examination gave negative results, restrictions were lifted in January 2013, and Switzerland regained its PRRSV-free status. The events demonstrate that import of semen from non-PRRS-free countries - even from negative studs - poses a risk, because monitoring protocols in boar studs are often insufficient to timely detect an infection, and infections of sows/herds occur even with low numbers of semen doses. The outbreak was eradicated successfully mainly due to the high disease awareness of the importer and because immediate actions were taken before clinical or laboratory diagnosis of a single case in the country was made. To minimize the risk of an introduction of PRRSV in the future, stricter import guidelines for boar semen have been implemented.
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Porcine circovirus infections are caused by the porcine circovirus 2 (PCV2). Among six different clinical manifestations involving respiratory, enteric, nervous and reproductive signs, the postweaning multisystemic wasting syndrome (PMWS) is the most important and studied disease. However, reproductive failures associated with PCV2 have been increasingly reported. Some studies have shown the possible contamination of sows by semen of PCV2 positive boars. In order to investigate the transmission of PCV2 by contaminated semen and its ability to infect the sow and piglets, 20 PCV2 negative sows were inseminated, 10 with negative boar semen and 10 with previously nested-PCR tested positive boar semen. The sows were weekly monitored and blood samples were collected. Based on the results, 4 out 20 sows were selected (1 sow was PCR negative and inseminated with a negative semen, 2 sows were PCR negative and inseminated with a positive semen and 1 sow was PCR negative and inseminated with a positive semen, but became PCR positive around the 30 days of pregnancy). After weaning, 12 male piglets, 3 of each sow, were selected and maintained under isolation. In order to investigate which organs harbored the virus, the young pigs were necropsied around 9 months of age. Samples of serum collected monthly were tested by immunocitochemistry (ICC), and all 12 pigs serum converted. Samples of lymphoid, systemic and reproductive organs were analyzed by nested-PCR and immunohistochemistry (IHC). Evaluation of the samples by nested-PCR, revealed that several tissues were positive in 10 of 12 pigs, mainly the lymph nodes, bone marrow and spleen. Various samples were positive by IHC in 8 of 12 piglets, being the lymph nodes, tonsils and bulbourethral glands the most frequently positive. Thus, the results of testing different samples, in the 3 tests (ICC, nested-PCR and IHC) were complementary. These results show that PCV2 transmission through semen to the sows and piglets may occur and may also represent a potential risk for the herd.
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It has been speculated that the homeopathic treatment of sperm cells in order to improve semen quality could be promising. However, few data is available and its use in spermatozoa requires investigation. It is well established that mitochondrial membrane potential is an important viability parameter of spermatozoa and it is intimately related to reproductive efficiency. In this manner, new technologies in order to improve the activity of sperm cells and, finally, the fecundity of swine herds are of extremely importance. Due to the lack of knowledge of homeopathic treatment effect on spermatozoa, the aim of the present study was to verify the effect of three different homeopathic treatments on viability of boar sperm cells. Three homeopathic treatments composed by Pulsatila CH6, Pulsatila and Avena CH6, Avena CH6 and one control treatment (sucrose) were added to diluted boar semen, which were cooled for 24 or 48 h. Interestingly, no positive effect of homeopathic treatments was observed over semen viability. However, it was demonstrated that the 24 h of cooling storage provided more viable sperm cells when compared to the 48-h period. This effect of storage period on sperm viability was assessed by intact plasmatic membrane, intact acrosome and mitochondrial membrane potential evaluation.
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Este estudo avaliou os efeitos de diferentes bimestres dentro da estação de monta sobre características reprodutivas de éguas. Foram utilizados 147 ciclos estrais de 100 éguas, por duas estações de monta consecutivas, com controle folicular por palpação retal diária e inseminação artificial com sêmen diluído, resfriado e transportado a 14ºC por 3,5 horas. Os grupos experimentais foram constituídos segundo cada bimestre da estação, a saber outubro/novembro, dezembro/janeiro e fevereiro/março, de acordo com a data de ovulação de cada ciclo estral. Os resultados demonstraram (na ordem citada dos bimestres) melhor taxa de concepção ao primeiro ciclo em dezembro/janeiro (42,9%; 70,0%, 28,6%), melhor taxa de concepção por ciclo também em dezembro/janeiro (45,6%; 63,5%; 29,6%), e melhor eficiência de prenhez em outubro/novembro e em dezembro/janeiro (4,4; 6,0; 2,3). Quanto às características ovulatórias, como tamanho do folículo à ovulação e tempo de crescimento folicular, não houve diferença entre os grupos. Conclui-se pela possibilidade de eliminação dos meses extremos da estação de monta sem prejuízo da eficiência reprodutiva do rebanho.
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A espécie Cebus apella (macaco-prego) é amplamente utilizada como modelo experimental na pesquisa biomédica. Entretanto, são escassos os estudos dedicados a avaliar o sêmen desses animais, que é composto por uma fração líquida e uma coagulada de difícil manipulação e alta concentração de espermatozóides imóveis. Portanto, objetivou-se I) avaliar o efeito de duas concentrações de cafeína (6 e 10 mM/mL) diluídas em TES-TRIS e água de coco in natura (ACIN) na ativação de espermatozóides de C. apella e II) testar um protocolo de criopreservação do sêmen comparando dois diluidores (TES-TRIS e ACIN) acrescidos de gema de ovo e glicerol. O sêmen de seis animais mantidos no Centro Nacional de Primatas foi coletado por eletroejaculação, diluído na fração-A de TES-TRIS ou ACIN, e incubado a 35°C até dissolução do coágulo seminal. O tempo de liquefação foi comparado. Posteriormente foi mensurado volume, concentração, morfologia espermática e percentual de espermatozóides vivos. No experimento I as amostras foram diluídas em TES-TRIS ou ACIN acrescidos de 6 e 10 mM de cafeína após o término da motilidade durante a liquefação e mantidas a 35°C. Motilidade e vigor foram avaliados por 5 h. Para o experimento II, após liquefação, o sêmen foi diluído na fração-B (fração-A + gema de ovo e glicerol) dos diluidores, envasado, resfriado a 4°C (2 h), em seguida a -60°C (20 min), antes de ser mergulhado em nitrogênio líquido. O sêmen foi descongelado a 35°C (5 min). Os resultados foram expressos como média ± EP. O efeito dos diluidores foi comparado pelo teste t Student e ANOVA (p _ 0,05). O coágulo liquefez em 4,5 ± 1,7 e 2,8 ± 1,1 horas (p < 0,05) em TES-TRIS e ACIN respectivamente. O volume médio, concentração, percentual de espermatozóides normais e vivos antes de congelação foi respectivamente 0,6 ± 0,2 mL; 1.806 ± 367 x 106 espermatozóides/mL; 81,3 ± 2, e 40,1 ± 3,3 (TES-TRIS) e 30,9 ± 4 (ACIN). A duração da motilidade em TES-TRIS e ACIN foi, respectivamente, 5 ± 1,4 e 1 ± 0,5 h. A motilidade média nesse período foi 38 ± 10% (TES-TRIS) e 18 ± 9% (ACIN). Foi verificado aumento da motilidade após adição de cafeína apenas nas amostras diluídas em ACIN 6 mM (21 ± 9%) e ACIN 10 mM (22 ± 11) (p > 0,05). O percentual de espermatozóides vivos após descongelação foi 26,2% em TES-TRIS e 13,2% em ACIN (p < 0,05). Para a criopreservação de sêmen de C. apella TES-TRIS é mais indicado e pode, assim como ACIN + cafeína, ser empregado na inseminação artificial com sêmen a fresco diluído.
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Liquid-chromatography (LC) high-resolution (HR) mass spectrometry (MS) analysis can record HR full scans, a technique of detection that shows comparable selectivity and sensitivity to ion transitions (SRM) performed with triple-quadrupole (TQ)-MS but that allows de facto determination of "all" ions including drug metabolites. This could be of potential utility in in vivo drug metabolism and pharmacovigilance studies in order to have a more comprehensive insight in drug biotransformation profile differences in patients. This simultaneous quantitative and qualitative (Quan/Qual) approach has been tested with 20 patients chronically treated with tamoxifen (TAM). The absolute quantification of TAM and three metabolites in plasma was realized using HR- and TQ-MS and compared. The same LC-HR-MS analysis allowed the identification and relative quantification of 37 additional TAM metabolites. A number of new metabolites were detected in patients' plasma including metabolites identified as didemethyl-trihydroxy-TAM-glucoside and didemethyl-tetrahydroxy-TAM-glucoside conjugates corresponding to TAM with six and seven biotransformation steps, respectively. Multivariate analysis allowed relevant patterns of metabolites and ratios to be associated with TAM administration and CYP2D6 genotype. Two hydroxylated metabolites, α-OH-TAM and 4'-OH-TAM, were newly identified as putative CYP2D6 substrates. The relative quantification was precise (<20 %), and the semiquantitative estimation suggests that metabolite levels are non-negligible. Metabolites could play an important role in drug toxicity, but their impact on drug-related side effects has been partially neglected due to the tremendous effort needed with previous MS technologies. Using present HR-MS, this situation should evolve with the straightforward determination of drug metabolites, enlarging the possibilities in studying inter- and intra-patients drug metabolism variability and related effects.
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We present a new phenomenological approach to nucleation, based on the combination of the extended modified liquid drop model and dynamical nucleation theory. The new model proposes a new cluster definition, which properly includes the effect of fluctuations, and it is consistent both thermodynamically and kinetically. The model is able to predict successfully the free energy of formation of the critical nucleus, using only macroscopic thermodynamic properties. It also accounts for the spinodal and provides excellent agreement with the result of recent simulations.
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Combining the data from conventional semen analysis with oocyte penetration assays should improve the assessment of the fertilizing ability of a semen sample. Thus, the objective of the present study was to evaluate the prognostic value of various semen parameters on the in vitro interactions between frozen-thawed canine sperm and homologous oocytes. Ten ejaculates from five stud dogs (two ejaculates/dog) were collected by digital manipulation. Semen samples were evaluated, extended in Tris-egg yolk-glycerol, frozen and stored in liquid nitrogen, and thawed several weeks later. Samples were evaluated for motility and sperm populations by computer-aided semen analysis (CASA), plasma membrane integrity (carboxy-fluorescein diacetate and propidium iodide), and sperm morphology (Bengal Rose). Thawed spermatozoa were also incubated with homologous oocytes for 18 h in an atmosphere of 5% CO2 and 95% air at 38 degrees C and sperm-oocyte interactions were evaluated. Simple linear regression models were calculated, with sperm parameters as independent variables and sperm-oocyte interactions as the dependent variable. There were significant associations between: percentage of oocytes bound to spermatozoa and beat cross frequency (BCF; R-2 = 63%); percentage of oocytes that interacted with spermatozoa and BCF (R-2 = 73%); and number of penetrated spermatozoa and velocity average pathway (VAP; R-2 = 64%) and velocity straight line (VSL; R-2 = 64%). Although plasma membrane integrity and sperm morphology had little prognostic value for in vitro interactions between canine frozen-thawed sperm and homologous oocytes, some motility patterns (evaluated by CASA) were predictive of in vitro sperm-oocyte interactions. (c) 2005 Elsevier B.V. All rights reserved.
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Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
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Presently AI in the koala has been based on the insemination of fresh undiluted semen collected with an artificial vagina (1). While this approach has been extremely successful, further refinement and implementation of AI for use with cryopreserved semen will require protocols that incorporate diluted semen collected by EE. Recent studies have shown that koala semen is likely to have an "ovulation factor" such that over-dilution may result in ovulation failure (2). The current study determined whether AI of EEed neat and/or diluted semen was capable of inducing a luteal phase and/or resulted in the production of pouch young. All koalas were inseminated in the breeding season between day 2 and 5 of oestrus and subsequently monitored for evidence of parturition (day 35) and return of oestrus. Successful induction of a luteal phase was based on evidence of an elevated progesterone concentration 28 days after insemination (2). All semen samples were collected by EE and seminal characteristics recorded (3). The diluent used for semen extension was Tris-citrate glucose (TCG) which contained antibiotics but no egg yolk (4). AI was conducted on conscious koalas using a "Cook koala insemination catheter" and a glass rod used to mimic penile thrusting (1). Three insemination treatments were used; (A) 1mL of undiluted semen (n = 9); (B) 2mL of 1:1 diluted semen (n = 9); and (C) 1 mL of 1:1 diluted semen (n = 9). The results of the AI trial are shown in Table 1. This study has shown that it is possible to use both neat and diluted semen (1:1; 1 or 2 mL) to successfully produce koala offspring at conception rates similar to those achieved following natural mating. Interestingly, dilution of semen had no apparent detrimental effect on induction of a luteal phase following AI.
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Plantaginis Semen is commonly used in traditional medicine to treat edema, hypertension, and diabetes. The commercially available Plantaginis Semen in China mainly comes from three species. To clarify the chemical composition and distinct different species of Plantaginis Semen, we established a metabolite profiling method based on ultra high performance liquid chromatography with electrospray ionization quadrupole time-of-flight tandem mass spectrometry coupled with elevated energy technique. A total of 108 compounds, including phenylethanoid glycosides, flavonoids, guanidine derivatives, terpenoids, organic acids, and fatty acids, were identified from Plantago asiatica L., P. depressa Willd., and P. major L. Results showed significant differences in chemical components among the three species, particularly flavonoids. This study is the first to provide a comprehensive chemical profile of Plantaginis Semen, which could be involved into the quality control, medication guide, and developing new drug of Plantago seeds.
