ABSTRACT
Developing effective cooled semen protocols is essential to increase pregnancy rates and reproductive efficiency in donkeys. This study aimed to evaluate the effect on sperm kinetic parameters and membrane integrity in cooled donkey semen diluted with defined milk proteins extender with 1% or 2% of egg yolk and the removal of seminal plasma. Twenty-four ejaculates from six jackasses were collected. Each ejaculate was divided into four aliquots that were diluted in extender with 1% (EY1) or 2% (EY2) egg yolk. One sample from each group was centrifuged, seminal plasma was removed (CEY1, CEY2 groups, respectively), and the samples were then refrigerated at 5 °C for 24 h. Fresh and cooled semen samples were assessed for sperm motility, morphology, and plasma membrane integrity. Total motility, progressive motility, sperm kinetic parameters, or live sperm cells were not statistically different when semen was cooled with an extender supplemented with 1% or 2% of egg yolk. Seminal plasma removal does not affect total motility or sperm kinetic parameters. However, progressive motility decreased (P<0.05) when semen was extended with 2% of egg yolk and seminal plasma was removed. Membrane integrity was affected (P<0.05) in centrifuged samples. In conclusion, the obtained results suggest that there is no difference in sperm kinetics and membrane integrity when 1% or 2% of egg yolk was added to the Equiplusï extender. Also, the removal of seminal plasma by centrifugation did not have any beneficial effect on cooled donkey semen. Further studies are needed to relate these results with in vivo fertility tests with cooled donkey semen.(AU)
O desenvolvimento de protocolos de sêmen resfriado eficazes é essencial para aumentar as taxas de prenhez e eficiência reprodutiva em jumentos. O objetivo desse estudo foi avaliar o efeito do diluente à base de proteínas do leite com 1 ou 2% de gema de ovo sobre os parâmetros cinéticos do sêmen e integridade da membrana em sêmen resfriado de jumento, com ou sem a remoção do plasma seminal. Vinte e quatro ejaculados de seis jumentos foram coletados. Cada ejaculado foi dividido em quatro alíquotas e diluído em diluente com 1% (EY1) ou 2% (EY2) de gema de ovo. Uma amostra por grupo foi centrifugada e o plasma seminal removido (grupos CEY1 e CEY2, respectivamente). Os pellets foram novamente ressuspendidos nas mesmas concentrações e diluentes. Em seguida, as quatro alíquotas foram refrigeradas a 5°C por 24 horas. Amostras de sêmen fresco e refrigerado foram avaliadas quanto à motilidade espermática e integridade da membrana plasmática. Motilidade total, motilidade progressiva, parâmetros de cinética espermática ou células espermáticas vivas não apresentaram diferença significativa quando o sêmen foi resfriado com diluente suplementado com 1% ou 2% de gema de ovo. A remoção do plasma seminal não afetou a motilidade total ou os parâmetros de cinética espermática; entretanto, a motilidade progressiva diminuiu (P<0,05) quando o sêmen foi diluído com 2% de gema de ovo e o plasma seminal removido. Nas amostras centrifugadas, a integridade da membrana foi afetada (P<0,05). Em conclusão, os resultados sugerem que não há diferença na cinética espermática e na integridade da membrana quando 1% ou 2% de gema de ovo são adicionados ao diluente Equiplusï e a remoção do plasma seminal por centrifugação não teve nenhum efeito benéfico no resfriamento de sêmen de jumento. Mais estudos são necessários para relacionar esses resultados com testes de fertilidade in vivo com sêmen resfriado em jumentos.(AU)
Subject(s)
Animals , Plasma , Semen Preservation/veterinary , Sperm Motility , Cryopreservation , Equidae , Egg Yolk , Semen , ProteinsABSTRACT
RESUMEN El objetivo fue criopreservar semen de bagre rayado Pseudoplatystoma magdaleniatum con tres crioprotectores internos diferentes: dimetilsulfóxido (DMSO), dimetilacetamida (DMA) y etilenglicol (ETG) a dos porcentajes de inclusiones (5 y 10%), combinados con glucosa 6%, leche en polvo descremada 3% y vitamina E (0,4%). Cinco machos en fase de espermiación fueron inducidos con 0,4 ml de Ovaprim®/Kg. El semen fue diluido en la solución crioprotectora (1:3) en tubos de 2,5 ml, congelado en vapores de nitrógeno y descongelado a 35°C durante 90 segundos. El análisis estadístico incluyó un diseño factorial 3x2 y semen fresco (SF) como tratamiento testigo. En semen fresco, precongelado y descongelado se evaluó la movilidad total (Mt), tipos de movilidad, progresividad total y velocidades espermáticas con la ayuda de Sperm Class Analyzer SCA®. El SF registró volumen de 6,1±4,3 ml, Mt de 72,6±17,1%, activación de 31,2±2,1 segundos y concentración espermática de 54,7±22,9 millones/μl. En semen precongelado, el crioprotector (p<0,05) y porcentaje de inclusión (p<0,01), pero no su interacción, tuvieron un efecto significativo en la Mt, velocidad curvilínea (VCL) y velocidad lineal (VSL); mientras que en semen descongelado sólo la interacción de los factores (p<0,05) fue significativa en Mt, porcentajes de espermatozoide estáticos y VCL. La Mt cayó entre 36-67% en semen precongelado y entre 7486% en semen descongelado con relación a SF. Los resultados sugieren que DMSO, DMA y ETG incluidos a 5 o 10%, combinados con leche en polvo 3%, glucosa 6% y vitamina E 0,4% son alternativas viables de criopreservación del semen de bagre rayado.
ABSTRACT The objective of this study was to evaluate three internal cryoprotectants to preserve semen of striped catfish (Pseudoplatystoma magdaleniatum). The cryoprotectants tested were: dimethylsulfoxide (DMSO), dimethylacetamide (DMA) and ethylene glycol (ETG) at two inclusion percentages (5 and 10%), mixed with 6% glucose, 3% skim milk powder, and 0.4% vitamin E. Five males in the spermiation phase were induced with Ovaprim® (0.4 ml/kg). The semen was diluted in the cryoprotective solution (1: 3) in 2.5 ml tubes, frozen in nitrogen vapors and thawed at 35°C for 90 seconds. A 3x2 factorial design was used, and the control treatment was fresh semen (SF). Total motility (Mt), type of motility total progressivity, and spermatic velocities were evaluated in fresh, pre-frozen and post-thawed semen using the Sperm Class Analyzer (SCA®) software. The SF volume was 6.1 ± 4.3 ml, with Mt of 72.6 ± 17.1%, activation of 31.2 ± 2.1 seconds and sperm concentration of 54.7 ± 22.9 million/μl. In the pre-frozen semen, the cryoprotectant (p <0.05) and the percentage of inclusion (p <0.01) -but not their interaction- had a significant negative effect on Mt, curvilinear velocity (VCL), and linear velocity (VSL); whereas in thawed semen only the interaction of the factors (p <0.05) was significant for Mt, static sperm percentages and VCL. The Mt decreased between 36-67% in pre-frozen semen and between 74-86% in thawed semen compared to SF. These results suggest that 5 or 10% inclusion levels of DMSO, DMA, and ETG, in combination with 3% powdered milk, 6% glucose, and 0.4% vitamin E are viable alternatives to cryopreserve semen of striped catfish.
ABSTRACT
PURPOSE: Sperm cryopreservation before cancer treatment is the most effective method to preserve the fertility of male patients. We present our 21 years experience with sperm cryopreservation for cancer patients, including an examination of semen quality, the current status of cryopreserved sperm, and the rate of sperm use for assisted reproductive technology (ART). MATERIALS AND METHODS: A total of 721 cancer patients at Fertility Center of CHA Gangnam Medical Center successfully performed sperm cryopreservation for fertility preservation from January 1996 to December 2016. Medical chart review was used to analyze patient age, marital status, cancer type, semen volume, sperm counts and motility, length of storage, and current banking status. RESULTS: The major cancers of the 721 patients were leukemia (28.4%), lymphoma (18.3%), testis cancer (10.0%). The mean age at cryopreservation was 27.0 years, and 111 patients (15.4%) performed sperm cryopreservation during or after cancer treatment. The mean sperm concentration was 66.7±66.3 ×106/mL and the mean sperm motility was 33.8%±16.3%. During median follow-up duration of 75 months (range, 1–226 months), 44 patients (6.1%) used their banked sperm at our fertility center for ART and 9 patients (1.2%) transferred their banked sperm to another center. The median duration from cryopreservation to use was 51 months (range, 1–158 months). CONCLUSIONS: Sperm cryopreservation before gonadotoxic treatment is the most reliable method to preserve the fertility of male cancer patients. Sperm cryopreservation should be offered as a standard of care for all men planning cancer therapy.
Subject(s)
Humans , Male , Cryopreservation , Fertility Preservation , Fertility , Follow-Up Studies , Leukemia , Lymphoma , Marital Status , Methods , Reproductive Techniques, Assisted , Semen , Semen Analysis , Semen Preservation , Sperm Count , Sperm Motility , Spermatozoa , Standard of Care , Testicular NeoplasmsABSTRACT
This study investigated the correlation between oxidative stress status and key canine sperm parameters and the effect of addition of a superoxide dismutase (SOD), catalase (CAT), and glutathione peroxidase (GPx) combination in egg yolk tris-citrate glucose (EYT-G) extender on semen during 10 days of storage at 4℃. Ten Boxer dogs were divided into two groups, fertile (F) and hypofertile (H), depending on pregnancy and live birth rate status in the previous year. Semen evaluation was performed on the day of collection (D0) and after 5 (D5) and 10 (D10) days of cooled storage. Sperm motility, kinetic parameters, and DNA integrity were assessed. A correlation between oxidative status and key semen parameters in both F and H groups was observed. Total and progressive motilities were significantly higher in the treated (SOD, CAT, and GPx addition) versus control groups at D10 in both F and H groups, and at D5 in the H group. DNA integrity was significantly higher in both treated groups (H and F) at D5 and D10. In conclusion, the addition of SOD, CAT, and GPx in the extender allows preservation of semen quality for up to 10 days of storage at 4℃ in both fertile and hypofertile dogs.
Subject(s)
Animals , Cats , Dogs , Pregnancy , Antioxidants , Catalase , DNA , Egg Yolk , Fertility , Glucose , Glutathione Peroxidase , Glutathione , Live Birth , Oxidative Stress , Semen Analysis , Semen Preservation , Semen , Sperm Motility , Spermatozoa , Superoxide Dismutase , SuperoxidesABSTRACT
Since the first successful pregnancy from a frozen human oocyte was reported, remarkable technological progress has been made in the area of cryopreservation of human oocytes. We report a successful delivery of two healthy babies after transfer of vitrified-warmed embryos derived from intracytoplasmic sperm injection (ICSI) with vitrified-warmed oocytes and frozen-thawed sperm. A female patient and her husband with severe oligoasthenspermia are reported. At the day of oocyte collection, very few inactive sperms were found in her husband semen. Multiple site open testicular biopsy was performed on her husband, but no sperm was retrieved. The patient did not become pregnant after transferring two embryos coming from half of oocytes and inactive sperms. The patient got pregnant and delivered two healthy babies after receiving a transfer of vitrified-warmed embryos from vitrified-warmed oocytes and frozen-thawed sperm.
La criopreservación de oocitos humanos ha progresado mucho desde que el primer embarazo exitoso desde un oocito congelado fue informado. Nosotros informamos el parto de dos bebés sanos después de transferir embriones vitrificados y recalentados y espermios descongelados. Se trata de una mujer y su marido con una oligoastenoespermia severa. En el día de la recolección de oocitos, se encontraron muy pocos espermios inactivos en el semen del marido. Se tomaron biopsias testiculares pero se encontraron muy pocos espermios inactivos. La mujer logró quedar embarazada y dio luz a dos bebés sanos después de recibir una trasferencia de embriones vitrificados y recalentados, y de espermios descongelados.
Subject(s)
Humans , Female , Pregnancy , Infant, Newborn , Adult , Oocytes , Pregnancy Outcome , Cryopreservation , Sperm Injections, Intracytoplasmic , Embryo Transfer , Pregnancy, TwinABSTRACT
PURPOSE: To compare sperm recovery from slow versus rapid thawing technique using thirty-eight normozoospermic human sperm samples, as follows. Twenty-one samples from men taking part in routine infertility screening exams (infertile group) and seventeen from proven fertile volunteer men with at least one child (fertile group). MATERIALS AND METHODS: After analysis of motility, concentration, strict morphology and functional integrity of membranes, sperm was divided into two aliquots of 0.5 mL each and frozen in TyB-G medium. Samples were thawed at room temperature (25 ± 2º C) for 25 minutes (slow thaw) or in a water bath at 75º C for 20 seconds followed by water bath at 37º C for 3 minutes (rapid thaw). After thawing, motility, strict morphology and functional integrity of membranes were evaluated by a blinded investigator. The results were expressed as mean ± standard deviation for parametric variables and analyzed using Student's t-test. Data with unpaired non-parametric variables were expressed as median (interquartile range) and analyzed by the Mann-Whitney test. Wilcoxon test was used to analyze non-parametric paired variables. RESULTS: There was no significant difference between techniques for total and progressive motility, percentage of normal morphological forms, hypoosmotic swelling test. CONCLUSIONS: Although the rapid thawing protocol was completed in a shorter time (three minutes and 20 seconds versus 25 minutes, respectively), it wasn't harmful since both techniques showed comparable spermatozoa recovery. Additional research is needed to confirm its safety in clinical research before introducing this methodology in routine assisted reproduction.
Subject(s)
Adult , Humans , Male , Cryopreservation/standards , Fertility/physiology , Infertility, Male/physiopathology , Semen Preservation/standards , Sperm Motility/physiology , Spermatozoa/physiology , Cryopreservation/methods , Double-Blind Method , Sperm CountABSTRACT
Objective To compare clinical outcome of intracytoplasmic sperm injection(ICSI)cycle by using fresh and cryopreserved-thawed testicular and epididymal spermatozoa in azoospermic patients.Methods Between September 2006 and May 2007,208 azoospermic patients underwent in vitro fertilization(IVF)were treated in Center of Reproductive Medicine,Peking University Third Hospital.Those couples were divided into two groups based on their wishes,including 171 cases in fresh group and 37 cases in cryopreserved-thawed group.The cryopreserved testicular or epididymal spermatozoa were thawed and recovered before ICSI procedure iu thawed group.The outcomes of ICSI in each group were compared.including clinical outcomes(two pronuclear fertilization,high quality embryo,clinical pregnancy and embryo implantation)and pregnancy outcomes(spontaneous miscarriage,gestational weeks and neonatal birth weight).Results (1),The utilization rate were 92%(23/25)in cryopreserved-thawed testicular spermatozoa and 100%(12/12)in epididymal spermatozoa.(2)Between fresh and cryopreserved-thawed groups,no statistical difference was observed in two pronuclear fertilization rate[62.25%(973/1563)vs.64.53%(282/437),P=0.960],high quality embryo rate[78.9%(768/973)vs.79.1%(223/282),P=0.985],clinical pregnancy rate per embryo transfer[44.4%(60/135)vs.46.9%(15/32),P:0.688]and embryo implantation rate[29.3%(84/287)vs.33.3%(23/69),P=0.508].(3)No significant difference between flesh and cryopreserved group was found in spontaneous miscarriage rate (11%vs.7%,P=1.000),gestational weeks(single birth:39.0 weeks vs.38.7 weeks,P:0.538;twins:36.8 weeks vs.36.3 weeks,P=0.571)and birth weight(single birth:3409 g vs.3350 g,P=0.699;twins:2584 g vs.2635 g,P=0.703).Conclusion It suggested that tissue from the azoospermic patients who underwent diagnostic testieular and epididymal biopsy should be eryopreseved for IVF-ET.