PCR-based detection of Helicobacter spp. in animal facilities of a University in Rio de Janeiro, Brazil.

Pathogenic microbial detection and control in laboratory animal facilities is essential to guarantee animal welfare, data validity and reproducibility. Helicobacter spp. are known to affect mice health, what may interfere with experimental outcomes. This study aimed to screen for Helicobacter spp. in mice from animal facilities in Rio de Janeiro, Brazil using a PCR-based method. Primers designed to specifically identify Helicobacter spp. were used to amplify feces or intestine DNA extracted of mice from four different animal facilities. The expected 375 base pairs (bp) amplicon was purified, sequenced and a similarity of 95% was observed when compared to deposited sequences of H. hepaticus and H. bilis. In our screening, Helicobacter spp. was detected in ~59% of fecal and ~70% of intestine samples. Our study is the first to screen for Helicobacter spp. in mouse facilities of a Rio de Janeiro University using a low cost, rapid molecular diagnostic test. Although Helicobacter spp. screening is not mandatory according to Brazilian animal welfare regulation it is recommended by institutional animal health monitoring programs guidelines worldwide, including ARRIVE, AAALAC and FELASA.

Human Menstrual Blood-Derived Mesenchymal Cells Improve Mouse Embryonic Development.

There is a constant need for improving embryo culture conditions in assisted reproduction. One possibility is to use mesenchymal stem/stromal cells derived from menstrual blood (mbMSCs), with an endometrial origin. In this study, we sought to analyze the expansion of mouse embryos in a direct coculture model with mbMSCs. Our results showed that after five passages, mbMSCs presented a spindle-shaped morphology, with surface markers that were comparable with the normal mesenchymal cell phenotype. mbMSCs could differentiate into adipogenic and osteogenic lineages and secrete angiopoetin-2 and hepatocyte growth factor. The coculture experiments employed 103 two-cell-stage embryos that were randomly divided into two groups: control (n = 50), embryos cultured in GV-Blast medium, and cocultured mbMSCs (n = 53), embryos cocultured with GV-Blast and mbMSCs. Typically, two to three embryos were placed in a well with 200 µL of culture medium and observed until developmental day 5. After 5 days, the cocultured group had more embryos in the blastocyst stage (69.8%) when compared with the control group (30%) (p < 0.001). It was also found that nearly 57% of blastocysts in the cocultured group reached the hatching stage, while only 13% achieved this stage in the control group (p < 0.001). Analyses of cultured mbMSCs and growth media, in the presence or absence of an embryo, were also performed. Immunofluorescence detected similar levels of collagen I and III and fibronectin in both mbMSCs and cocultured mbMSCs, and similar amounts of growth factors, VEGF, PDGF-AA, and PDGF-BB, were also observed in the conditioned medium, regardless of embryo presence. The present study describes, for the first time, an easy, noninvasive, and autologous method that could potentially increase blastocyst growth rates during assisted reproductive procedures (i.e., in vitro fertilization). It is proposed that this mbMSC coculture strategy enriches the embryonic microenvironment and promotes embryo development. This technique may complement or replace existing assisted reproduction methods and is directly relevant to the field of personalized medicine. Impact statement The study demonstrates a novel and potentially personalized assisted reproduction approach. The search for alternative and autologous methods provides assisted reproduction patients with a better chance of a successful pregnancy. In this study, mesenchymal cells derived from menstrual blood resembled the outside uterine surface and could potentially be employed for improving embryo outgrowth. Our protocol enriches the embryonic microenvironment and facilitates high-quality single-embryo transfer.

Sperm Selection Using Three Semen Processing Techniques.

OBJECTIVE: This study aimed to assess the efficiency, in terms of recovered motile spermatozoa with normal morphology, of three sperm selection techniques: migration- sedimentation (SS), swim-up from fresh semen (SF), and swim-up from washed (SL) sperm. METHODS: Samples from 20 normozoospermic men were divided into three equal aliquots and processed in parallel. SS was performed in a Jondet tube, using 1 ml of semen and 2.5 ml of Human Tubal Fluid medium (HTF+10% Synthetic Serum Supplement, Irvine, USA). For SF, 1 ml of HTF was layered over 1 ml of fresh semen (SF). For SL, 1 ml of sperm was first centrifuged (300 g, 10 min) and the pellet resuspended in 1 ml of HTF; a second layer of HTF was placed on top. Migration time was 1h (SF and SL) and 1h30' for SS at 37°C. After migration, 200 µl were removed from the top layer (SF, SL) and from the central cone (SS). Concentration, morphology and motility were determined. RESULTS: Recovery rates were 25% for SS, 10.1% for SF and 4.5% for SL. SS recovery rate was significantly higher (P<0.01) than the two swim-up techniques. Total motility was statistically different (P<0.001), with 93.6% for SS, 91.2% for SF, and 77% for SL. Sperm morphology was similar between the three techniques (P= 0.12). CONCLUSION: SS is an efficient technique for the recovery of motile spermatozoa from native semen preparations and yielded better results than SF and SL. Routine use for assisted reproduction remains to be evaluated.

Avaliação do comportamento de ratos alojados em caixas de cores diferentes / Evaluation of the behavior of rats housed in boxes of different colors

A adequação do ambiente físico quanto aos hábitos da espécie em relação ao bem-estar animal e o refinamento das pesquisas, ultimamente vem ganhando importância investigativa. Com o objetivo de avaliar o comportamento de ratos alojados em caixas de diferentes cores, utilizaram-se 48 animais machos com 3 meses de idade divididos em seis grupos, sendo que três grupos foram alojados em caixas brancas e outros três em caixas pretas, durante 4 semanas. Empregando-se o labirinto em cruz elevado (LCE), os resultados mostraram maior tempo de permanência nos braços fechados dos animais alojados nas caixas brancas. No teste do campo aberto (CA), houve maior ambulação do grupo mantido em caixas pretas, e na esquiva inibitória, os dados indicaram um aumento significativo no tempo de permanência na plataforma do grupo alojado em caixas pretas. Assim, os animais alojados em gaiolas de cor preta apresentaram maior tendência exploratória (menor ansiedade) e melhor aprendizado.

Lately, the adequacy of a physical ambient to the specie’s habits relating to their well being and refined researches is getting important for researchers. With the aim of evaluate the behavior of rats housed in boxes of different colors, it was used 48 male animals, with 3 months of age, divided in 6 groups, three groups in white boxes and the other three in black boxes, for 4 weeks. Observing on the elevated plus maze, the results showed that the animals from white boxes stayed more time in the closed arms. On the open field test, there was more walking of the group kept in Black boxes, and on the inhibitory avoidance, data indicated a significant increase on the time spent on the platform by the group housed in the black boxes. Thus, the animal housed in Black cages have shown a greater exploratory tendency (decreased anxiety), and better learning.

Vacuum-cooled liquid nitrogen increases the developmental ability of vitrified-warmed bovine oocytes

The objective of this study was to determine the effects of vacuum-cooled liquid nitrogen on the development of vitrified immature (germinal vesicle stage; GV) and mature (metaphase II; MII) bovine oocytes after re-warming. Liquid nitrogen was exposed to either atmospheric pressure or to a vacuum (300mm Hg for 45sec); the latter decreased the temperature of the liquid nitrogen to -200°C. Partially denuded oocytes were vitrified either just after selection (GV) or after 22 hours of in vitro maturation (MII) in TCM 199 medium + 10 percent of estrous mare serum. For vitrification, oocytes were firstly exposed to an intermediate solution (10 percent EG + 10 percent DMSO) for 30sec, followed by the vitrification solution (20 percent EG + 20 percent DMSO + 0.5M sucrose) for 20sec. Groups of three or four oocytes were loaded into an open-pulled-straw and directly plunged into liquid nitrogen. Oocytes were subsequently re-warmed by exposure to air (25°C) for 4sec, followed by 5 min exposure to decreasing concentrations (0.3 and 0.15M) of sucrose. Fertilization (Day 0) was done with 2 x 106 spermatozoa mL-1 (selected by a swim-up procedure) and incubated for 18 to 22 hours. Presumptive zygotes were cultured at 39°C in four-well dishes with SOFaaci medium, under 5 percent CO2 and saturated humidity. Cleavage (Day 2) and blastocyst rates (Day 8) were 33.9 and 4.2 percent, respectively, for GV stage oocytes at atmospheric pressure, 41.2 and 8.8 percent for GV oocytes under vacuum, 43.5 and 6.7 percent for MII oocytes at atmospheric pressure, and 53.6 and 10.6 percent for MII oocytes under vacuum. In conclusion, vacuum-cooled liquid nitrogen improved developmental rates of vitrified-thawed bovine oocytes.

O objetivo deste estudo foi determinar o efeito do nitrogênio liquido super resfriado por vácuo no desenvolvimento, após reaquecimento, de oócitos bovinos vitrificados imaturos ou maturados. O nitrogênio líquido foi mantido em atmosfera normal ou submetido ao vácuo (300mm Hg por 45s) este último reduzindo a temperatura do nitrogênio para -200°C. Oócitos parcialmente desnudos foram vitrificados logo após a seleção (estádio de vesícula germinativa; VG), ou após 22 horas de maturação (metáfase II; MII) em meio TCM 199 + 10 por cento de soro de égua em estro. Para a vitrificação, os oócitos foram inicialmente expostos a uma solução intermediária (10 por cento EG + 10 por cento DMSO) por 30s e a seguir a uma solução de vitrificação (20 por cento EG + 20 por cento DMSO + 0,5M sacarose) por 20s. Grupos de 3 ou 4 oócitos foram envasados em palhetas estiradas e abertas e mergulhados no nitrogênio líquido. Os oócitos foram então reaquecidos por exposição ao ar (25°C) por 4s, seguido de exposição a concentrações decrescentes de sacarose (0,3 e 0,15M - 5 minutos cada). A fecundação (dia 0) foi realizada com 2 x 106 espermatozóides mL-1 (selecionados por "swim-up") e incubação por 18 a 22 horas. Os presumíveis zigotos foram cultivados a 39°C, em placas de quatro poços, com meio SOFaaci, com 5 por cento de CO2 e umidade saturada. As taxas de clivagem (Dia 2) e de blastocistos (Dia 8) obtidas foram de 33,9 e de 4,2 por cento, respectivamente, para oócitos no estágio de VG / pressão normal, de 41,2 e 8,8 por cento para oócitos VG / vácuo, 43,5 e 6,7 por cento para oócitos MII / pressão normal e de de 53,6 e 10,6 por cento para oócitos MII / vácuo. Conclui-se que o emprego de nitrogênio líquido super resfriado pelo vácuo melhora as taxas de desenvolvimento de oócitos bovinos após a vitrificação.

Prevalence of endometritis and its effects on reproductive performance of dairy cows.

Hostein cows (n=141) in five commercial dairy herds in central New York were examined for endometritis by examination of endometrial aspirates for presence of inflammatory cells, principally neutrophils, by endometrial cytology at 40-60 days postpartum. The prevalence of cytologically-diagnosed endometritis was 53%; within herds the prevalence varied from 37 to 74% (P=0.02). There was excellent agreement between two examiners (Kappa=0.864; P<0.0001). Parity did not influence prevalence of endometritis (P=0.53). Cytologically diagnosed endometritis was associated with profoundly impaired reproductive performance; Kaplan-Meier survival analysis revealed lower overall pregnancy rate (P<0.0001). Median days open was 206 for cows with endometritis and 118 for cows free of the condition. Overall, 76% of cows in this study became pregnant by 300 days postpartum; 63% of cows with endometritis and 89% of cows without endometritis were confirmed pregnant by 300 days postpartum (P<0.003). (For these two groups, 69, and 90% respectively, became pregnant during the duration of the study). Pregnancy to first service percentage was lower (11 versus 36%; P=0.001) for cows with than without endometritis, and these cows required more services before 50% became pregnant (3 versus 2; P=0.006). In a second study using 22 cows in a university-owned herd, the prevalence of cytological evidence of inflammation was 100% at 2 weeks postpartum, and dropped to 89, 58, and 41% at 4, 6, and 8 weeks, respectively. Endometritis diagnosed by endometrial cytology late in the voluntary waiting period was highly prevalent and exerted a profoundly detrimental effect on subsequent reproductive performance, making this condition potentially extremely costly to the North American dairy industry.

Tritrichomonas foetus induces apoptotic cell death in bovine vaginal epithelial cells.

Tritrichomonas foetus is a serious veterinary pathogen, causing bovine trichomoniasis, a sexually transmitted disease leading to infertility and abortion. T. foetus infects the mucosal surfaces of the reproductive tract. Infection with T. foetus leads to apoptotic cell death of bovine vaginal epithelial cells (BVECs) in culture. An affinity-purified cysteine protease (CP) fraction yielding on sodium dodecyl sulfate-polyacrylamide gel electrophoresis a single band with an apparent molecular mass of 30 kDa (CP30) also induces BVEC apoptosis. Treatment of CP30 with the protease inhibitors TLCK (Nalpha-p-tosyl-l-lysine chloromethyl ketone) and E-64 [l-trans-epoxysuccinyl-leucylamide-(4-guanido)-butane] greatly reduces induction of BVEC apoptosis. Matrix-assisted laser desorption ionization-time-of-flight MALDI-TOF mass spectrometry analysis of CP30 reveals a single peak with a molecular mass of 23.7 kDa. Mass spectral peptide sequence analysis of proteolytically digested CP30 reveals homologies to a previously reported cDNA clone, CP8 (D. J. Mallinson, J. Livingstone, K. M. Appleton, S. J. Lees, G. H. Coombs, and M. J. North, Microbiology 141:3077-3085, 1995). Induction of apoptosis is highly species specific, since the related human parasite Trichomonas vaginalis and associated purified CPs did not induce BVEC death. Fluorescence microscopy along with the Cell Death Detection ELISA(PLUS) assay and flow cytometry analyses were used to detect apoptotic nuclear condensation, DNA fragmentation, and changes in plasma membrane asymmetry in host cells undergoing apoptosis in response to T. foetus infection or incubation with CP30. Additionally, the activation of caspase-3 and inhibition of cell death by caspase inhibitors indicates that caspases are involved in BVEC apoptosis. These results imply that apoptosis is involved in the pathogenesis of T. foetus infection in vivo, which may have important implications for therapeutic interference with host cell death that could alter the course of the pathology in vivo.