ABSTRACT
The aim of the present study was to report the occurrence of members of the Mollicutesclass in the reproductive system of dairy cattle in Brazil. Five farms containing dairy cattle were visited in January of 2012. In total, 100 cows of different ages, breeds and stages of lactation were examined in the present study. The cows were part of intensive or semi-intensive management systems and were submitted to mechanical milking or hand milking. The samples were collected after washing the vulvar region with water and soap, and then drying it with paper towels and disinfecting the area with alcohol (70°GL). Vaginal mucous was collected using a sterile alginate cotton swab, which was rubbed on the vagina, as well as the lateral and internal walls. Vulvovaginal mucous samples were cultured in both liquid and solid modified Hayflick´s medium, for mycoplasmas, and UB medium, for ureaplasmas. The PCR assays for Mollicutesand Ureaplasmaspp. were performed according to the standard protocols described in the current literature. During isolation, the frequency of Mycoplasmaspp. was of 13.0% (13/100) and for Ureaplasmaspp. was of 6.0% (6/100). In the PCR assays the frequency of Mollicuteswas of 26.0% (26/100) and for Ureaplasmaspp. was of 13.0% (13/100) in the dairy cattle studied. This is the first report of these agents in reproductive system of bovine of the Pernambuco state. Further studies are necessary to determine the pathogenic potential and species of these field isolates.
O presente estudo relata a ocorrência de membros da Classe Mollicutesno sistema reprodutivo de bovinos leiteiros no Brasil. Foram visitadas em janeiros de 2012 cinco fazendas de bovinos leiteiros. Um total de 100 vacas de diferentes idades, raças e estágios de lactação foram examinadas. Os animais foram mantidos em sistema de manejo intensivo e/ou semi-intensivo, sendo submetidos aos sistemas de ordenha manual ou mecânica. As amostras de muco foram colhidas após a lavagem da região vulvar com água e sabão, com posterior desinfecção com álcool (70°GL). O muco vaginal foi colhido com suabe alginado estéril que foi friccionado nas paredes internas da vagina. Em seguida, as amostras foram cultivadas em meio Hayflick´s modificado, para micoplasmas, e em meio UB, para ureaplasmas, ambos caldo e placa. Os ensaios da PCR para Mollicutese Ureaplasmaspp. foram realizados de acordo com protocolo padrão descrito na literatura. No isolamento, a frequência de Mycoplasmaspp. foi de 13% (13/100) e para Ureaplasmaspp. foi de 6% (6/100). Nas reações da PCR a frequência para Mollicutesfoi de 26% (26/100) e para Ureaplasmas spp. foi de 13% (13/100) nos rebanhos bovinos leiteiros estudados. Este é o primeiro relato destes agentes no trato reprodutivo de bovinos no Estado de Pernambuco. Estudos adicionais são necessários para determinar as espécies e o potencial patogênico destes isolados de campo.
Subject(s)
Animals , Female , Cattle , Reproductive Tract Infections/diagnosis , Reproductive Tract Infections/veterinary , Cervix Mucus , Tenericutes/virology , Vaginal Smears/veterinary , Mycoplasma Infections/veterinary , Ureaplasma Infections/veterinary , Polymerase Chain Reaction/veterinaryABSTRACT
O objetivo deste estudo foi monitorar o ciclo estral em cutias (Dasyprocta leporina) criadas em cativeiro no semiárido brasileiro. Durante 70 dias, cinco cutias foram diariamente submetidas a citologia esfoliativa vaginal, e o monitoramento ultrassonográfico ovariano foi realizado a cada três dias. Um total de 8 ciclos estrais foi completamente monitorado, com duração de 28,2±0,7 dias, variando de 24 a 31 dias. Pela citologia esfoliativa vaginal, houve uma predominância de células superficiais nas fases de proestro e estro (P<0,05), seguida da predominância de células intermediárias no metaestro (P<0,05) e de células parabasais no diestro (P<0,05). Por ultrassonografia, não houve diferenças na morfologia ovariana durante as diferentes fases do ciclo estral (P>0,05). Os folículos foram identificados durante as fases estrogênicas (proestro e estro), com diâmetro médio de 1±0,5mm. Em apenas 12,5% das fases luteais, corpos lúteos medindo 1,4±0,9mm foram identificados. Conclui-se que a associação da citologia vaginal e da ultrassonografia ovariana constitui uma alternativa viável para o monitoramento de ciclos estrais e identificação das fases estrogênicas em cutias da espécie Dasyprocta leporina.
The objective of the study was to monitor the estrous cycle in agoutis (Dasyprocta leporina) bred in captivity in Brazilian semiarid. During 70 days, five agoutis were daily subjected to vaginal exfoliative cytology, and the ovarian ultrasound monitoring was conducted every three days. A total of 8 estrous cycles were completely monitored, lasting 28.2±0.7 days, ranging from 24 to 31 days. By vaginal exfoliative cytology, there was predominance of superficial cells at proestrus and estrus phases (P<0.05), followed by the predominance of intermediate cells in the metestrus (P<0.05) and parabasal cells in diestrus (P<0.05). By ultrasound, there were no differences in ovarian morphology during the different phases of the estrous cycle (P>0.05). Follicles during the estrogenic phases (proestrus and estrus) were identified, with an average diameter of 1±0.5mm. In only 12.5% of luteal phases, corpora lutea measuring 1.4±0.9mm were identified. We conclude that the association of vaginal cytology and ovarian ultrasonography is a useful alternative for monitoring the estrous cycle and identifying the estrogenic phases in Dasyprocta leporina.
Subject(s)
Animals , Female , Estrous Cycle/physiology , Dasyproctidae/physiology , Vaginal Smears/veterinary , Ultrasonography/veterinary , Ovarian Follicle , Ovary/physiologyABSTRACT
Se utilizó el Análisis Automatizado de la Morfometría Espermática (ASMA) con el fin de determinar las dimensiones de la cabeza del espermatozoide (DCE) en semen de cerdos domésticos según la edad, además de agrupar las medidas obtenidas en subpoblaciones espermáticas (SP). Se evaluaron 36 muestras de semen fresco y diluido de 20 cerdos los cuales se clasificaron en dos categorías. A: menores de 18 meses de edad y B: mayores de 18 meses de edad. Las DCE (Largo, µm/ Ancho, µm/ Área, µm 2 y Perímetro, µm) se analizaron en frotis teñidos con Hemacolor ® mediante Sperm-Class Analyser ® (SCA) y los valores obtenidos guardados en una base de datos. El procedimiento GLM fue utilizado para evaluar el efecto de la edad del cerdo sobre las DCE y el análisis de agrupamiento (FASTCLUS) para identificar las SP. Los espermatozoides provenientes de cerdos mayores de 18 meses de edad presentaron mayor longitud (8,84 vs. 8,95 µm) que los cerdos menores de 18 meses de edad, sin embargo, las medias correspondientes al ancho (4,44 vs. 4,32 µm), área (33,33 vs. 32,39µm 2) y perímetro (27,65 vs. 26,3 µm) fueron más pequeñas en los cerdos de mayor edad. Dos SP fueron obtenidas con el fin de ratificar las diferencias observadas entre las 2 categorías de edades evaluadas (P<0,001). La población que incluyó los espermatozoides con las mayores dimensiones disminuyó de 41,61 por ciento en cerdos menores de 18 meses a 20,78 por ciento en cerdos mayores de 18 meses. Contrariamente, la SP que contenía los espermatozoides de menor tamaño incrementó de un 58,39 por ciento en cerdos menores de 18 meses a 79,22 por ciento en cerdos mayores de 18 meses. En conclusión, la edad de los cerdos influye significativamente sobre las DCE. Los cerdos de mayor edad tienen 20 por ciento más de espermatozoides de menor tamaño que los cerdos más jóvenes.
Assisted Sperm Morphometry Analysis (ASMA) was used to determine the sperm head dimensions (DCE) of boar by age, and then the data set clustered in sperm subpopulations (SP). To this purpose were evaluated 36 fresh and diluted semen samples of 20 Dalland domestic pigs, which were classified in 2 categories: under 18 months old and over 18 months old. The DCE (Length, µm/ Width, µm/, Area, µm 2 / and Perimeter, µm) were analyzed in slides stained by Hemacolor ® by the Sperm-Class Analyser ® (SCA), and the mean measurements recorded. A GLM procedure was performed to evaluate the effects of boar age on sperm head dimensions and clustering analysis (FAST-CLUS procedure) to separate in SP. Spermatozoa collected from older boar (over 18 months old) had head length larger (8.84 vs. 8.95 µm) than younger boar (under 18 months old), however, the width (4.44 vs. 4.32 µm), area (33.33 vs. 32.39 µm 2) and perimeter (27.65 to 26.3 µm) were smaller in older boar than younger boar. Two SP were clustered in this trial toratify the differences between younger and older pigs. The mean values of each DCE among the SP were significantly dif-ferent (P<0.001). Thus, the percentage of representation of the subpopulation that includes those spermatozoa whose dimensions are the largest decreased from 41.61 percent in pigs under 18 months old to 20.78 percent in pigs over 18 months old. Whereas, the percent of representation of the SP containing the smallest sper-matozoa increased from 58.39 percent in pigs under 18 months old to 153 79.22 percent in pigs over 18 months old. In conclusion, the age of sexually mature domestic male pig had a significant effect on the morphometric traits of their spermatozoa. Older boar had 20 percent more of smaller spermatozoa than younger boar.