Metabolomics of Human Semen: A Review of Different Analytical Methods to Unravel Biomarkers for Male Fertility Disorders

Blaurock, Janet, Baumann, Sven, Grunewald, Sonja, Schiller, Jürgen, M. Engel, Kathrin

05 December 2023

Background: Human life without sperm is not possible. Therefore, it is alarming that the fertilizing ability of human spermatozoa is continuously decreasing. The reasons for that are widely unknown, but there is hope that metabolomics-based investigations may be able to contribute to overcoming this problem. This review summarizes the attempts made so far. Methods: We will discuss liquid chromatography–mass spectrometry (LC-MS), gas chromatography (GC), infrared (IR) and Raman as well as nuclear magnetic resonance (NMR) spectroscopy. Almost all available studies apply one of these methods. Results: Depending on the methodology used, different compounds can be detected, which is (in combination with sophisticated methods of bioinformatics) helpful to estimate the state of the sperm. Often, but not in all cases, there is a correlation with clinical parameters such as the sperm mobility. Conclusions: LC-MS detects the highest number of metabolites and can be considered as the method of choice. Unfortunately, the reproducibility of some studies is poor, and, thus, further improvements of the study designs are needed to overcome this problem. Additionally, a stronger focus on the biochemical consequences of the altered metabolite concentrations is also required

info:eu-repo/classification/ddc/571.8

ddc:571.8

Cell of Origin Identification Using Methylation Signatures from Seminal Cell-Free DNA and Heterogenous Cellular Mixtures

Barney, Ryan

13 November 2023

Infertility is an issue for approximately 12% of couples attempting to have a child. Of this group, 50% of the cases are due to male factor infertility. There are many reasons for decreased fecundity in men, but there remains 10% to 15% of infertile men that are diagnosed with the most severe form of infertility, non-obstructive azoospermia (NOA). A diagnosis of NOA implies the lack of sperm cells in the ejaculate with no physiological reason. The current diagnostic test and treatment consist of microscopic examination of seminal fluid and a biopsy to extract any viable sperm from the testis. This treatment is known to be problematic because of the destructive nature of surgery as well as expense. A non-invasive diagnostic test that could identify the presence of sperm in the testis at the beginning of fertility treatment would inform the patient and the physician about the functionality of the testis and thus lead to more informed decisions about treatment and potentially a decrease in cost. The ability to identify the tissue source of DNA present in the reproductive tract could facilitate a fertility diagnostic tool. Tissue specific epigenetic mechanisms are known to play a role in an organism's development. The identification of an epigenetic signature unique to sperm DNA would allow for the identification of sperm DNA in a heterologous mixture. Our lab has been able to identify a methylation signature that can consistently differentiate between sperm DNA and somatic DNA. We compared the sperm DNA signature with that of blood and testicular tissue and found that there was no overlap in epigenetic markers. To create an assay that could evaluate the presence of sperm DNA we used an Oxford Nanopore next-generation sequencing platform. Sequencing bisulfite converted DNA; we were able to retrieve the methylation status at locations of interest. A bioinformatic tool was created to analyze the thousands of reads obtained and analyze the individual methylation points within single molecules of DNA. To create a more accessible fertility test, we used the sperm DNA analysis tool to evaluate seminal cell-free DNA (cfDNA). The presence of sperm cfDNA in a patient's seminal fluid may indicate that there is sperm somewhere in the male reproductive tract even if the cells are not intact. A clinician could use this information to better advise the patient about treatment and potentially decrease cost of care.

DNA methylation

cell-free DNA

sperm epigenetics

seminal cfDNA assay

Life Sciences

Cultivo in vitro e desenvolvimento pós-seminal de espécies de Bromeliaceae com potencial ornamental / In vitro culture and post-seminal development of Bromeliaceae with ornamental potential

Kievitsbosch, Talitha Joana

30 August 2011

As bromélias são valorizadas por suas características ornamentais, sendo o gênero Vriesea representativo neste setor. O aprimoramento de métodos de propagação in vitro destas plantas é altamente necessário a fim de suprir as necessidades do mercado, e evitar o extrativismo ilegal. Nesse contexto, o presente trabalho objetivou aprimorar o protocolo de propagação in vitro de espécies do gênero Vriesea, bem como aumentar o conhecimento global das espécies em estudo. Para tanto, sementes das espécies V. carinata, V. friburgensis, V. paraibica e V. simplex foram submetidas a processos de assepsia e introduzidas in vitro sob três temperaturas: 22 °C, 27 °C e 32 °C. Paralelamente, sementes das mesmas espécies foram semeadas em bandejas e mantidas em casa de vegetação. Através da microscopia eletrônica de varredura e ótica foi realizada a descrição morfo-anatômica do desenvolvimento pós-seminal das plântulas das mesmas espécies. Além disso, procurou-se adequar o meio de cultura às necessidades das mesmas espécies e de V. hieroglyphica, sendo testadas 3 doses de nitrogênio e 3 doses de magnésio. Também procurou-se avaliar a taxa de sobrevivência durante o processo de aclimatização de plântulas das espécies de Vriesea mencionadas (com exceção de V. hieroglyphica). Objetivou-se comparar características anatômicas e morfológicas de folhas das referidas espécies cultivadas in vitro e em casa de vegetação. Por fim, com o objetivo de estabelecer um protocolo de micropropagação para as espécies Vriesea carinata, V. paraibica, V. phillipo-coburgii; V. simplex e Aechmea nudicaulis, foram introduzidos in vitro explantes somáticos, após testes de assepsia. A partir dos experimentos citados foi verificado que a temperatura exerce uma forte influência nas taxas de germinação e mortalidade das sementes de Vrieseas in vitro, sendo que a temperatura de 32°C proporcionou as maiores taxas de mortalidade, mostrando-se prejudicial ao sucesso reprodutivo. A germinação em casa de vegetação apresentou altas taxas de mortalidade e taxas de germinação mais baixas do que in vitro. A descrição morfo-anatômica do desenvolvimento pós-seminal permitiu a caracterização de cinco estágios de desenvolvimento. Com relação ao experimento de nutrição mineral, foi evidenciado que as doses de nitrogênio e magnésio testadas acarretaram em menor acúmulo de cálcio e de potássio nas plantas, sendo que esse fato resultou em menor acúmulo de massa fresca. O experimento de aclimatização ficou inviabilizado devido ao ataque às plântulas por praga Fungus Gnats. Com a análise morfo-anatômica das folhas de plantas cultivadas in vitro e em casa de vegetação foi possível observar a presença de estruturas típicas de Bromeliaceae nas plantas cultivadas em ambas as condições: estômatos, tricomas escamiformes, mesofilo com epiderme unisseriada, parênquima aqüífero, feixes colaterais fechados e canais de aeração. Com relação à introdução in vitro a partir de explantes somáticos, pode-se afirmar que o uso de cefotaxima apresentou uma boa eficiência no combate à contaminação bacteriana em cultura de ápices caulinares. A escolha de ápice vegetativo de brotos laterais como explantes iniciais para a cultura das referidas espécies in vitro é uma boa opção. A otimização da propagação destas espécies in vitro poderá diminuir a pressão extrativista que estas vêm sofrendo e, ao mesmo tempo, abastecer o mercado ornamental / Bromeliads are valued for their ornamental characteristics and the genus Vriesea is representative in this sector. The improvement of in vitro propagation of these plants is highly necessary in order to meet market needs, and, at the same time, to prevent illegal extraction of this plants from their natural habitat. In this context, this study aimed to improve the protocol for in vitro propagation of species of Vriesea and increase the global knowledge of these by morpho-anatomical characterization of the development of the seedling and leaf. Seeds of V. carinata, V. friburgensis, V.paraiba and V. simplex were submitted to aseptic procedures and introduced in vitro under three temperatures: 22 ° C, 27 ° C and 32 ° C. Additionaly, seeds of these species were sown in trays and maintained in a greenhouse. The post-seminal development was described by light and scanning electron microscopy. In addition, the adjustment of the culture medium for these four species and V. hieroglyphica was tested, by testing three doses of nitrogen combined with three doses of magnesium. The acclimatization efficiency of these Vriesea species, except for V. hieroglyphica, after a prior culture in the presence and absence of IBA was done, in three commercial substrates to verify IBA effect in rooting and seedling survival. This study also aimed to compare anatomical and morphological characteristics of leaves of the species cultivated in vitro and in the greenhouse. Finally, in order to establish a micropropagation protocol for the species Vriesea carinata, V. paraiba, V. phillipo-coburgii; V. simplex and Aechmea nudicaulis, somatic explants were introduced in vitro after sterilization tests. From all the experiments cited it was observed that the temperature strongly influences germination and mortality rates of Vriesea germinating seeds in vitro. The temperature of 32 ° C provided the highest mortality rates, being harmful to the reproductive success of this species. The germination in the greenhouse showed higher mortality and lower germination rates than in vitro germination. The morpho-anatomical description of the post-seminal development allowed for the characterization of five stages of development. With regard to the mineral nutrition experiment, the doses of nitrogen and magnesium tested resulted in less accumulation of calcium and potassium in plants, resulting in less accumulation of fresh weight. The acclimatization experiment was lost by the attack of Fungus gnats. With the morpho-anatomical analysis of leaves of plants grown in vitro and in the greenhouse it was possible to observe the presence of typical structures of Bromeliaceae such as stomata, scales, mesophyll with uniseriate epidermis, water storage tissue, collateral vascular bundles and air channels. Finally, the use of cefotaxime proved efficient against bacterial contamination in in vitro establishment of shoot apex explants in vitro. The choice of shoot apices from lateral buds as initial explants for in vitro establishment of those species was a good alternative. Optimization of in vitro propagation of bromeliad species can reduce their extractivism pressure and, at the same time, supply the ornamental plant market

Ápice caulinar

Bromélia

Bromeliad

Desenvolvimento pós-seminal

Germinação

Germination

In vitro nutrition

Light microscopy

Microscopia de luz

Microscopia eletrônica de varredura

Morfo-anatomia

Morpho-anatomy

Nutrição in vitro

Post-seminal development

Scanning electron microscopy

Shoot apices

Cultivo in vitro e desenvolvimento pós-seminal de espécies de Bromeliaceae com potencial ornamental / In vitro culture and post-seminal development of Bromeliaceae with ornamental potential

Talitha Joana Kievitsbosch

30 August 2011

As bromélias são valorizadas por suas características ornamentais, sendo o gênero Vriesea representativo neste setor. O aprimoramento de métodos de propagação in vitro destas plantas é altamente necessário a fim de suprir as necessidades do mercado, e evitar o extrativismo ilegal. Nesse contexto, o presente trabalho objetivou aprimorar o protocolo de propagação in vitro de espécies do gênero Vriesea, bem como aumentar o conhecimento global das espécies em estudo. Para tanto, sementes das espécies V. carinata, V. friburgensis, V. paraibica e V. simplex foram submetidas a processos de assepsia e introduzidas in vitro sob três temperaturas: 22 °C, 27 °C e 32 °C. Paralelamente, sementes das mesmas espécies foram semeadas em bandejas e mantidas em casa de vegetação. Através da microscopia eletrônica de varredura e ótica foi realizada a descrição morfo-anatômica do desenvolvimento pós-seminal das plântulas das mesmas espécies. Além disso, procurou-se adequar o meio de cultura às necessidades das mesmas espécies e de V. hieroglyphica, sendo testadas 3 doses de nitrogênio e 3 doses de magnésio. Também procurou-se avaliar a taxa de sobrevivência durante o processo de aclimatização de plântulas das espécies de Vriesea mencionadas (com exceção de V. hieroglyphica). Objetivou-se comparar características anatômicas e morfológicas de folhas das referidas espécies cultivadas in vitro e em casa de vegetação. Por fim, com o objetivo de estabelecer um protocolo de micropropagação para as espécies Vriesea carinata, V. paraibica, V. phillipo-coburgii; V. simplex e Aechmea nudicaulis, foram introduzidos in vitro explantes somáticos, após testes de assepsia. A partir dos experimentos citados foi verificado que a temperatura exerce uma forte influência nas taxas de germinação e mortalidade das sementes de Vrieseas in vitro, sendo que a temperatura de 32°C proporcionou as maiores taxas de mortalidade, mostrando-se prejudicial ao sucesso reprodutivo. A germinação em casa de vegetação apresentou altas taxas de mortalidade e taxas de germinação mais baixas do que in vitro. A descrição morfo-anatômica do desenvolvimento pós-seminal permitiu a caracterização de cinco estágios de desenvolvimento. Com relação ao experimento de nutrição mineral, foi evidenciado que as doses de nitrogênio e magnésio testadas acarretaram em menor acúmulo de cálcio e de potássio nas plantas, sendo que esse fato resultou em menor acúmulo de massa fresca. O experimento de aclimatização ficou inviabilizado devido ao ataque às plântulas por praga Fungus Gnats. Com a análise morfo-anatômica das folhas de plantas cultivadas in vitro e em casa de vegetação foi possível observar a presença de estruturas típicas de Bromeliaceae nas plantas cultivadas em ambas as condições: estômatos, tricomas escamiformes, mesofilo com epiderme unisseriada, parênquima aqüífero, feixes colaterais fechados e canais de aeração. Com relação à introdução in vitro a partir de explantes somáticos, pode-se afirmar que o uso de cefotaxima apresentou uma boa eficiência no combate à contaminação bacteriana em cultura de ápices caulinares. A escolha de ápice vegetativo de brotos laterais como explantes iniciais para a cultura das referidas espécies in vitro é uma boa opção. A otimização da propagação destas espécies in vitro poderá diminuir a pressão extrativista que estas vêm sofrendo e, ao mesmo tempo, abastecer o mercado ornamental / Bromeliads are valued for their ornamental characteristics and the genus Vriesea is representative in this sector. The improvement of in vitro propagation of these plants is highly necessary in order to meet market needs, and, at the same time, to prevent illegal extraction of this plants from their natural habitat. In this context, this study aimed to improve the protocol for in vitro propagation of species of Vriesea and increase the global knowledge of these by morpho-anatomical characterization of the development of the seedling and leaf. Seeds of V. carinata, V. friburgensis, V.paraiba and V. simplex were submitted to aseptic procedures and introduced in vitro under three temperatures: 22 ° C, 27 ° C and 32 ° C. Additionaly, seeds of these species were sown in trays and maintained in a greenhouse. The post-seminal development was described by light and scanning electron microscopy. In addition, the adjustment of the culture medium for these four species and V. hieroglyphica was tested, by testing three doses of nitrogen combined with three doses of magnesium. The acclimatization efficiency of these Vriesea species, except for V. hieroglyphica, after a prior culture in the presence and absence of IBA was done, in three commercial substrates to verify IBA effect in rooting and seedling survival. This study also aimed to compare anatomical and morphological characteristics of leaves of the species cultivated in vitro and in the greenhouse. Finally, in order to establish a micropropagation protocol for the species Vriesea carinata, V. paraiba, V. phillipo-coburgii; V. simplex and Aechmea nudicaulis, somatic explants were introduced in vitro after sterilization tests. From all the experiments cited it was observed that the temperature strongly influences germination and mortality rates of Vriesea germinating seeds in vitro. The temperature of 32 ° C provided the highest mortality rates, being harmful to the reproductive success of this species. The germination in the greenhouse showed higher mortality and lower germination rates than in vitro germination. The morpho-anatomical description of the post-seminal development allowed for the characterization of five stages of development. With regard to the mineral nutrition experiment, the doses of nitrogen and magnesium tested resulted in less accumulation of calcium and potassium in plants, resulting in less accumulation of fresh weight. The acclimatization experiment was lost by the attack of Fungus gnats. With the morpho-anatomical analysis of leaves of plants grown in vitro and in the greenhouse it was possible to observe the presence of typical structures of Bromeliaceae such as stomata, scales, mesophyll with uniseriate epidermis, water storage tissue, collateral vascular bundles and air channels. Finally, the use of cefotaxime proved efficient against bacterial contamination in in vitro establishment of shoot apex explants in vitro. The choice of shoot apices from lateral buds as initial explants for in vitro establishment of those species was a good alternative. Optimization of in vitro propagation of bromeliad species can reduce their extractivism pressure and, at the same time, supply the ornamental plant market

Ápice caulinar

Bromélia

Desenvolvimento pós-seminal

Germinação

Microscopia de luz

Microscopia eletrônica de varredura

Morfo-anatomia

Nutrição in vitro

Bromeliad

Germination

In vitro nutrition

Light microscopy

Morpho-anatomy

Post-seminal development

Scanning electron microscopy

Shoot apices

Sperm Quality and Cryopreservation in Teleost: Effect of Seminal Plasma Component and Climate Change

Padilla Sánchez, Malbelys

05 January 2024

[ES] La selección de gametos de alta calidad es un requisito indispensable a tener en cuenta en los programas de reproduccion asistida. El desarrollo de herramientas biotecnológicas como la criopreservación de gametos, juega un papel importante en la producción acuicola y en la formación de bancos de germoplasma, que contribuiran luego en la mejora genética de las poblaciónes de peces, principalmente aquellas en peligro y que pudieran estar más afectadas ante futuros cambios climáticos. En la primera fase de esta tesis realizada en la Unesp, se trabajó con una especie neotropical de elevada importancia económica para la region Suramericana. La segunda fase realizada en la UPV se trabajó con la Anguila europea (Anguilla anguilla), una especie clasificada en la Lista Roja de la (UICN) como especie "en peligro crítico de extinción". En la primera fase se buscó caracterizar la composición bioquímica del plasma y las características seminales de la especie para evaluar las posibles relaciones entre estos parámetros. El plasma seminal estuvo principalmente compuesto por iones de sodio (Na+) y dentro de los componentes orgánicos sobresalieron las proteínas totales y la glucosa. A través del análisis de componentes principales (PCA) se observó que la motilidad tenía una fuerte correlación positiva con el tiempo de motilidad, la concentración de espermatozoides y las proteínas totales. Estos análisis sirvieron de base para la creación de una solución diluyente utilizada posteriormente en la sustancia crioprotectora. Luego se determinó la influencia del plasma seminal como constituyente de la solución crioprotectora en la criopreservación de semen de P. reticulatum. Se utilizaron tres tratamientos: glucosa 5% + metanol 10% (T1), a este crioprotector se le agregó 30% de plasma seminal natural (T2) y 30% de plasma seminal artificial en base a los resultados de los componentes bioquímicos del plasma determinados para la especie en el experimento anterior (T3). Se evaluaron parámetros de motilidad espermática, capacidad fecundante del semen criopreservado, así como fragmentación del ADN. El tratamiento T1 resultó con los mejores valores de motilidad seguido del T2, y la capacidad fertilizante de estos dos tratamientos fue similar al control, sin embargo, el tratamiento T2 mostró menos daño en el ADN. Mediante el PCA se demostró que T1 tenía una mejor relación positiva con la fertilidad y la motilidad total y progresiva. Finalmente, evaluamos las estructuras de las subpoblaciones espermáticas en cada uno de los tratamientos utilizados. Mediante análisis multivariado en dos etapas, fue posible determinar tres subpoblaciones espermáticas en el semen crioconservado de la especie, SP1 (rápido-lineal), SP2 (rápido-no lineal) y SP3 (lento-lineal). T1 presentó el mayor porcentaje de SP1, siendo confirmado por la efectividad en la protección de las células de este tratamiento en el proceso de criopreservación de la especie. En la segunda fase que se está llevó a cabo en la UPV, el objetivo general fue determinar el efecto de la temperatura y el pH del agua de mar sobre la motilidad de los espermatozoides en la Anguila europea. Se determinó que el bajo pH del agua de mar (6.5-7.4) disminuyó la motilidad de los espermatozoides de anguila en comparación con el control (pH= 8.2). Cuando estudiamos el efecto combinado del pH del plasma seminal artificial y el pH de ASW (7.8 y 8.2), no encontramos diferencias estadísticas en la motilidad y cinética de los espermatozoides en relación con el pH del plasma seminal artificial, pero sí el pH del agua de mar. Se encontraron valores más altos de motilidad total (MOT), FA(rápidos) y ME (médios) con un pH de 8.2 que con un pH de 7.8. En contraste, la temperatura del agua de mar no afectó los parámetros de motilidad de los espermatozoides o la longevidad de los espermatozoides en el contexto del cambio climático. / [CA] La selecció de gàmetes d'alta qualitat és un requisit indispensable a tenir en compte en els programes de reproducció assistida. El desenvolupament d'eines biotecnològiques com la criopreservació de gàmetes, juga un paper important en la producció aqüicola i en la formació de bancs de germoplasma, que contribuiran després a la millora genètica de les població de peixos, principalment aquelles en perill i que poguessin estar més afectades davant de futurs canvis climàtics. A la primera fase d'aquesta tesi realitzada a la Unesp, es va treballar amb una espècie neotropical d'elevada importància econòmica per a la regió sud-americana. La segona fase realitzada a la UPV es va treballar amb l'Anguilla europea (Anguilla anguilla), una espècie classificada a la Llista Vermella de la (UICN) com a espècie "en perill crític d'extinció". A la primera fase es va buscar caracteritzar la composició bioquímica del plasma i les característiques seminals de l'espècie per avaluar les possibles relacions entre aquests paràmetres. El plasma seminal va estar principalment compost per ions de sodi (Na+) i dins dels components orgànics van sobresortir les proteïnes totals i la glucosa. A través de l'anàlisi de components principals (PCA), es va observar que la motilitat tenia una forta correlació positiva amb el temps de motilitat, la concentració d'espermatozoides i les proteïnes totals. Aquestes anàlisis van servir de base per a la creació d'una solució diluent utilitzada posteriorment a la substància crioprotectora. Després es va determinar la influència del plasma seminal com a constituent de la solució crioprotectora en la criopreservació de semen de P. reticulatum. Es van utilitzar tres tractaments: glucosa 5% + metanol 10% (T1), a aquest crioprotector se li va afegir 30% de plasma seminal natural (T2) i 30% de plasma seminal artificial sobre la base dels resultats dels components bioquímics del plasma determinats per a l'espècie a l'experiment anterior (T3). S'avaluaren paràmetres de motilitat espermàtica, capacitat fecundant del semen criopreservat, així com fragmentació de l'ADN. El tractament T1 va resultar amb els millors valors de motilitat seguit del T2, i la capacitat fertilitzant d'aquests dos tractaments va ser similar al control, però el tractament T2 va mostrar menys mal a l'ADN. Mitjançant el PCA es va demostrar que T1 tenia una millor relació positiva amb la fertilitat i la motilitat total i progressiva. Finalment, avaluem les estructures de les subpoblacions espermàtiques a cadascun dels tractaments utilitzats. Mitjançant anàlisi multivariada en dues etapes, va ser possible determinar tres subpoblacions espermàtiques en el semen crioconservat de l'espècie, SP1 (ràpid-lineal), SP2 (ràpid-no lineal) i SP3 (lent-lineal). T1 va presentar el percentatge més gran de SP1, i va ser confirmat per l'efectivitat en la protecció de les cèl·lules d'aquest tractament en el procés de criopreservació de l'espècie. A la segona fase que es va dur a terme a la UPV, l'objectiu general va ser determinar l'efecte de la temperatura i el pH de l'aigua de mar sobre la motilitat dels espermatozoides a l'Anguila europea. Es va determinar que el pH baix de l'aigua de mar (6.5-7.4) va disminuir la motilitat dels espermatozoides d'anguila en comparació del control (pH= 8.2). Quan estudiem l'efecte combinat del pH del plasma seminal artificial i el pH d'ASW (7.8 i 8.2), no trobem diferències estadístiques en la motilitat i la cinètica dels espermatozoides en relació amb el pH del plasma seminal artificial, però sí el pH de l'aigua de mar. Es van trobar valors més alts de motilitat total (MOT), FA(ràpids) i ME (metges) amb un pH de 8.2 que amb un pH de 7.8. En contrast, la temperatura de l'aigua de mar no va afectar els paràmetres de motilitat dels espermatozous o la longevitat dels espermatozous en el context del canvi climàtic. / [EN] The selection of high-quality gametes is an essential requirement to take into account in assisted reproduction programs. The development of biotechnological tools such as cryopreservation of gametes plays an important role in aquaculture production and in the formation of germplasm banks, which will later contribute to the genetic improvement of fish populations, mainly those in danger and that could be more affected by future climate changes. In the first phase of this thesis carried out at Unesp, we worked with a neotropical species of high economic importance for the South American region. The second phase carried out at the UPV worked with the European Eel (Anguilla anguilla), a species classified on the (IUCN) Red List as a "critically endangered" species. In the first phase, we sought to characterize the biochemical composition of the plasma and the seminal characteristics of the species to evaluate the possible relationships between these parameters. The seminal plasma was mainly composed of sodium ions (Na+) and within the organic components, total proteins and glucose stood out. Through principal component analysis (PCA) it was observed that motility had a strong positive correlation with motility time, sperm concentration and total proteins. These analyzes served as the basis for the creation of a diluent solution later used in the cryoprotective substance. Then the influence of seminal plasma as a constituent of the cryoprotectant solution in the cryopreservation of P. reticulatum semen was determined. Three treatments were used: 5% glucose + 10% methanol (T1), 30% natural seminal plasma (T2) and 30% artificial seminal plasma were added to this cryoprotectant based on the results of the determined biochemical components of the plasma. for the species in the previous experiment (T3). Parameters of sperm motility, fertilizing capacity of cryopreserved semen, as well as DNA fragmentation were evaluated. Treatment T1 resulted with the best motility values followed by T2, and the fertilizing capacity of these two treatments was similar to the control, however, treatment T2 showed less DNA damage. Using PCA, it was shown that T1 had a better positive relationship with fertility and total and progressive motility. Finally, we evaluated the structures of the sperm subpopulations in each of the treatments used. Through two-stage multivariate analysis, it was possible to determine three sperm subpopulations in the cryopreserved semen of the species, SP1 (fast-linear), SP2 (fast-nonlinear) and SP3 (slow-linear). T1 presented the highest percentage of SP1, being confirmed by the effectiveness in protecting the cells of this treatment in the cryopreservation process of the species. In the second phase that is being carried out at the UPV, the general objective was to determine the effect of temperature and pH of seawater on sperm motility in the European Eel. It was determined that the low pH of seawater (6.5-7.4) decreased the motility of eel sperm compared to the control (pH= 8.2). When we studied the combined effect of the pH of the artificial seminal plasma and the pH of ASW (7.8 and 8.2), we did not find statistical differences in the motility and kinetics of the sperm in relation to the pH of the artificial seminal plasma, but we did find the pH of the water of sea Higher values of total motility (MOT), FA (fast) and ME (medium) were found at a pH of 8.2 than at a pH of 7.8. In contrast, seawater temperature did not affect sperm motility parameters or sperm longevity in the context of climate change. / I also thank the Coordination for the Improvement of Higher Education Personnel (CAPES/PROEX) (N° 88887.302629/2018-00), National Council for Scientific, Technological Development CNPq (N° 200452/2022-3) and the Brazilian fostering agencies Foundation for Research Support of the State of Sao Paulo FAPESP (N° 2020/15020-0), for its financial support in Brazil. In Spain, the ThinkInAzul programme, supported by the Spanish Ministry of Science and Innovation (MCIN) with funding from the European Union NextGenerationEU (PRTR-C17.I1) and the Generalitat Valenciana (THINKINAZUL/2021/012) to SEASPERM, which has made it possible the preparation of this work. To the AUIP (Ibero-American Postgraduate University Association) for the Academic Mobility scholarship between Institutions Associated with the AUIP 2022 / Padilla Sánchez, M. (2023). Sperm Quality and Cryopreservation in Teleost: Effect of Seminal Plasma Component and Climate Change [Tesis doctoral]. Universitat Politècnica de València. https://doi.org/10.4995/Thesis/10251/201549

Plasma seminal

Calidad del esperma

Bagre

Anguila europea

Reproducción de peces

Temperatura

Seminal plasma

Sperm quality

Catfish

European eel

Fish reprodution

Temperature

pH

Principal Component Analysis (PCA)

PRODUCCION ANIMAL

Novas percepções sobre o uso de lecitina de soja na criopreservação e fertilidade de espermatozoide bovino / New insights on the use of soybean lecithin on bovine sperm cryopreservation and fertility

Rodrigues, Mariana de Paula

21 February 2014

A grande demanda por proteína animal e a importância que a criação bovina exerce sobre a economia nacional, vêm exigindo eficientes sistemas de produção. A preservação e disseminação da genética do rebanho bovino dependem de biotecnologias como a criopreservação espermática, inseminação artificial e fertilização in vitro. No entanto, atualmente muito tem sido discutido sobre o uso da gema de ovo nos diluidores seminais. Pois apresentam variabilidade em sua composição e risco de contaminação microbiológica. Em contrapartida, apesar dos diluidores sintetizados com lecitina de soja não fornecerem esses riscos, seus resultados não são muito satisfatórios na criopreservação espermática bovina. Com base na hipótese de que a suplementação do diluidor seminal à base de lecitina de soja com antioxidantes, preserve as características das células espermáticas de maneira tão eficiente quanto à gema de ovo, o objetivo do presente experimento foi comparar o efeito do diluidor à base de gema de ovo com o diluidor à base de lecitina de soja (com e sem antioxidantes), sobre a manutenção da funcionalidade e fertilidade de amostras espermáticas bovinas criopreservadas. Para tal, foram utilizadas amostras seminais de 20 touros Brangus, cujas colheitas foram realizadas pelo método de eletroejaculação e as amostras foram diluídas em 4 grupos de diluidores: LElecitina de soja (sem a adição de antioxidantes); LAlecitina de soja suplementada com ácido ascórbico (AA, 4,5mM); LS lecitina de soja suplementada com superóxido dismutase (SOD, 60UI/mL) e GOgema de ovo (sem adição de antioxidantes). O sêmen foi então, criopreservado de maneira automatizada. As amostras foram descongeladas e analisadas quanto aos testes laboratoriais de motilidade computadorizada do espermatozóide (CASA); integridade de membrana plasmática (eosina/nigrosina); integridade de membrana acrossomal (fast Green/ rosa bengala); atividade citoquímica mitocondrial (DAB); susceptibilidade do DNA à desnaturação (SCSA); índice de estresse oxidativo induzido (TBARS). Além disso, foram realizados testes para verificar o potencial de fertilidade das amostras espermáticas criopreservadas. A fertilidade in vivo foi realizada pela técnica de inseminação artificial em tempo fixo (IATF), utilizando 450 fêmeas bovinas, seguido de exame ultrassonográfico para avaliação de prenhez. Teste de fertilidade in vitro, foi realizado pela técnica de produção in vitro de embriões (PIV) com o uso de ovários de frigoríficos, a classificação do desenvolvimento embrionário e a avaliação da motilidade espermática foram promovidas no decorrer do processo. Os resultados demonstraram que o diluidor LE apresentou efeito na proteção espermática de maneira semelhante ao diluidor GO. No entanto a suplementação desse primeiro com antioxidantes é uma alternativa para melhorar ainda mais esse processo, já que a taxa de prenhez obtida nos grupos LA e LS é satisfatória em um programa de IATF. Ainda o grupo LS foi o que apresentou melhores resultados no processo de PIV. Concluindo que o diluidor à base de lecitina de soja suplementado com o antioxidante superóxido dismutase seria uma opção para a substituição definitiva dos diluidores sintetizados com gema de ovo. / Due to the great demand for animal protein and the importance that bovine breeding exert on national economy, efficient production systems have been required. Cattle genetics preservation and dissemination depend on reproductive biotechnologies such as sperm cryopreservation, artificial insemination and in vitro fertilization. However, the use of egg yolk-based extender is under discussion nowadays, once there is great variability in its composition and risks of bacteriological contamination. On the other hand, despite soybean lecithin-based extenders do not present these risks, satisfactory results, after bovine sperm cryopreservation, have not been reached yet. Based on the hypothesis that soybean lecithinbased extender supplemented with antioxidants, preserve the sperm cell characteristics so efficient as egg yolk does, the aim of the present experiment was to compare the effects of egg yolk-based extender and soybean lecithin-based extender (with and without antioxidants), on functionality and fertility maintenance of bovine cryopreserved sperm samples. For this, seminal samples from 20 Brangus bulls were used, collects were realized by eletroejaculation method and samples were diluted in 4 extenders group: LE-soybean lecithin-based extender (without antioxidant supplementation); LA- soybean lecithin supplemented with ascorbic acid (AA, 4,5mM); LS- soybean lecithin supplemented with superoxide dismutase (SOD, 60UI/mL) and GO-egg yolk-based extender (without antioxidant supplementation). Then, semen was cryopreserved by automatic method. Samples were thawed and analyzed by laboratorial tests such as computer assisted semen analysis (CASA); plasma membrane integrity (eosin/nigrosin); acrosome membrane integrity (fast green/ rose bengal); mitochondrial cytochemical activity (DAB); susceptibility of chromatin denaturation (SCSA); induced oxidative stress index (TBARS). Furthermore, tests for fertility potential of cryopreserved semen samples were performed. In vivo fertility was accessed by timed artificial insemination (TAI), 450 bovine females were inseminated, and ultrasonographical exam was realized for pregnancy detection. In vitro fertility test was accessed by embryo in vitro production (IVP), ovaries from slaughterhouses were used, embryo development classification and sperm motility were promoted during the process. Results indicate that sperm protection is similar between LE and GO extenders. However the antioxidant supplementation of soybean lecithin-based extender is a great alternative to improve the process of sperm protection, since pregnancy rate of LA and LS groups was satisfactory for a TAI program. Besides, LS group presented the best results on IVP process. In conclusion, soybean lecithin-based extender supplemented with superoxide dismutase would be a better option for a definite replacement of egg yolk-based extender for sperm bovine cryopreservation.

Ácido ascórbico

Antioxidant

Antioxidante

Ascorbic acid

Diluidor seminal

Egg yolk

Gema de ovo

Semen extender

Superoxide dismutase

Superóxido dismutase

Estudo do efeito das condições de manipulação do sêmen de jaguatiricas (Leopardus pardalis, Linnaeus, 1758) sobre a capacitação e a integridade morfológica e funcional dos espermatozóides / Study of the effect of ocelot (Leopardus pardalis; Linnaeus, 1758) semen manipulation on capacitation and on morphological and functional integrity of spermatozoa

Queiroz, Vinicius de Seixas

28 November 2003

O presente estudo visou investigar o efeito da refrigeração do sêmen da jaguatirica sobre o Índice de Motilidade Espermática [IME=(%M+MPx5)/2; %M = proporção de espermatozóides móveis; MP = motilidade progressiva], integridade acrossomal (IA) e capacitação espermática; assim como avaliar a eficácia da técnica FITC-PNA/IP na avaliação simultânea da viabilidade espermática (VE) e IA. Sete jaguatiricas foram eletroejaculadas, sendo utilizados apenas ejaculados (n=16) apresentando %M>=60% e MP>=3. Avaliou-se a IA por meio da Coloração Simples. Os ejaculados foram diluídos 1:1 na Variante do Diluente de PLatz e submetidos aos Protocolos de Transporte: Temperatura Ambiente e Refrigeração, - 0,23ºC/min, (Experimento 1); ou apenas Temperatura Ambiente (Experimentos 2 e 3). Após 2h, as alíquotas foram reaquecidas, reavaliando-se os parâmetros observados antes do transporte. Os espermatozóides foram lavados por centrifugação em meio F10 de Ham, ressuspensos nesse meio e processados conforme o experimento: (1) após pré-incubação (38ºC; 5%CO2) durante 0, 1, 2 e 4 horas, foram retiradas alíquotas a cada intervalo para serem incubadas (30 min) na ausência e na presença do cálcio ionóforo A23187 (Ca2+Ion) (1mM), avaliando-se IA e IME; (2) após pré-incubação por 0, 1 e 2h, foram incubadas alíquotas na ausência e presença de 1 e 2mM de Ca2+Ion, avaliado-se IA e IME; (3) pré-incubados por 9h, sendo retiradas alíquotas a cada hora, para as avaliações da IA e VE, (a) separadamente através da Coloração Simples e do IME, ou (b) simultaneamente através da técnica FITC-PNA/IP. A refrigeração causou declínio (p<0,02) da IA (71,0%) e IME (67,1), em comparação aos valores observados antes do transporte (88,5%; 85,4), enquanto a manutenção das amostras à temperatura ambiente não afetou (p>0,1) essas variáveis (84,8%; 76,4). Dentre as amostras refrigeradas, aquelas expostas ao Ca2+Ion sofreram redução (p<0,01) na IA (52,4%) frente ao controle (55,56%). Já nas amostras transportadas à temperatura ambiente, não foi observada diferença (p>0,1) entre os grupos com e sem ionóforo (64,41% vs. 63,87%). Quando analisados os tempos separadamente, o único tratamento em que houve efeito (p<0,05) do Ca2+Ion sobre a IA foi aquele refrigerado e pré-incubado por 2h. Foi verificada redução (p<0,05) nos valores de IME e IA devida à simples incubação, mesmo na ausência do Ca2+Ion. A concentração de 2µM dessa substância foi mais efetiva na indução da reação acrossômica que 1µM. Apesar dos fluorocromos FITC-PNA/IP terem se ligado aos espermatozóides, nas regiões esperadas, a proporção de células marcadas variou aleatoriamente durante pré-incubação, sem correlação (p>0,1) com IME. A IA avaliada pela Coloração Simples apresentou correlação positiva (r=0,77; p<0,0001) com IME, decrescendo (p<0,0001) durante pré-incubação. A refrigeração mostrou-se desvantajosa frente à manutenção do sêmen à temperatura ambiente, pois foi deletéria à função e às membranas dos espermatozóides. A refrigeração tornou-os capazes de responder ao estímulo do Ca2+Ion, característica observada nos espermatozóides capacitados. O ensaio de reação acrossômica induzida pelo Ca2+Ion deve ser aperfeiçoado para permitir avaliação acurada da capacitação espermática na jaguatirica. A Coloração Simples associada à avaliação do IME foi mais eficiente e menos laboriosa, frente á técnica FITC-PNA/IP, na avaliação da IA e VE. / This study aimed to investigate the effect of ocelot semen refrigeration on Sperm Motility Index [SMI=(%M+PMx5)/2; %M = proportion of motile spermatozoa ; PM = Progressive Motility], acrossomal integrity (AI) and sperm capacitation. Another objective was to evaluate the FITC-PNA/IP technique efficacy on evaluating simultaneously sperm viability (SV) and AI. Five ocelots, were electroejaculated, the semen was evaluated and only ejaculates (n=16) presenting %M>=60% and PM>=3 were used. Sperm AI was evaluated using Fast Green / Rose Bengal staining (FGRB). The ejaculates were diluted 1:1 in Platz Diluent Variant and subjected to the transportation protocols: Room Temperature and Cooling, -0.23ºC/min, (experiment 1); or only Room Temperature (experiments 2 and 3). After 2 hours, the aliquots were rewarmed and samples were taken to re-evaluate the parameters observed before the transport. The spermatozoa were washed in Ham’s F10 medium, ressuspended in fresh medium and processed differently, according the experiment: (1) after pre-incubation (38ºC; 5%CO2) during 0, 1, 2 and 4 hours, samples were taken at each time point to be incubated in the absence and presence of 1mM calcium ionophore A23187 (Ca2+Ion), SMI and AI were evaluated; (2) after pre-incubation during 0, 1 and 2h, aliquots were incubated in the absence and presence of 1 and 2 mM Ca2+Ion; SMI and AI were evaluated; (3) after pre-incubation during 9h, aliquots were taken every hour to compare the evaluation of SV and AI (a) separately by the FGRB staining and SMI or (b) simultaneously by the FITC-PNA / IP technique. Cooling caused decline (p<0.02) on AI (71.0%) and SMI (67.1), when compared to values observed before transportation (88.5%; 85.4). Maintenance at room temperature didn’t affect (p>0.1) these variables (84.8%; 76.4). Among cooled samples, spermatozoa exposed to Ca2+Ion showed smaller (P<0.01) AI value (52.4%) compared to the group incubated without that substance (55.56%). For samples transported at room temperature, it wasn’t observed difference (P>0.05) between the groups with and without ionophore (64.41% vs. 63.87%). When time intervals were analysed separately, the only treatment in which there was effect (p<0,05) of Ca2+Ion on AI was the group refrigerated and pre-incubated for 2h. There was a reduction (p<0,05) on SMI and AI due simply to incubation, even in the absence of Ca2+Ion. The 2µM concentration of this substance was more effective to induce acrosome reaction than 1µM. FITC-PNA and IP fluorocromes bound spermatozoa at the expected sites. However, proportion of marked cells varied randomly during pre-incubation, and didn’t correlate (p>0,1) with SMI. IA evaluated by FGRB staining showed positive correlation (r=0,77; p<0,0001) with SMI, decreasing (p<0,0001) during incubation. Cooling was disadvantageous compared to maintaining semen at room temperature, since it was deleterious to spermatozoa membranes and function, and made those cells capable to answer the Ca2+Ion challenge, a characteristic observed in capacitated spermatozoa. Ca2+Ion induced acrosome reaction assay must be improved to allow accurate evaluation of sperm capacitation on ocelots. FGRB staining associated to SMI evaluation was more efficient and easier to perform, than FITC-PNA/IP technique, for AI and SV investigation.

acrosome reaction

assisted reproduction

capacitação espermática

felidae

felidae

jaguatirica

ocelot

reação acrossômica

refrigeração seminal

reprodução assistida

semen cooling

sperm capacitation

Novas percepções sobre o uso de lecitina de soja na criopreservação e fertilidade de espermatozoide bovino / New insights on the use of soybean lecithin on bovine sperm cryopreservation and fertility

Mariana de Paula Rodrigues

21 February 2014

A grande demanda por proteína animal e a importância que a criação bovina exerce sobre a economia nacional, vêm exigindo eficientes sistemas de produção. A preservação e disseminação da genética do rebanho bovino dependem de biotecnologias como a criopreservação espermática, inseminação artificial e fertilização in vitro. No entanto, atualmente muito tem sido discutido sobre o uso da gema de ovo nos diluidores seminais. Pois apresentam variabilidade em sua composição e risco de contaminação microbiológica. Em contrapartida, apesar dos diluidores sintetizados com lecitina de soja não fornecerem esses riscos, seus resultados não são muito satisfatórios na criopreservação espermática bovina. Com base na hipótese de que a suplementação do diluidor seminal à base de lecitina de soja com antioxidantes, preserve as características das células espermáticas de maneira tão eficiente quanto à gema de ovo, o objetivo do presente experimento foi comparar o efeito do diluidor à base de gema de ovo com o diluidor à base de lecitina de soja (com e sem antioxidantes), sobre a manutenção da funcionalidade e fertilidade de amostras espermáticas bovinas criopreservadas. Para tal, foram utilizadas amostras seminais de 20 touros Brangus, cujas colheitas foram realizadas pelo método de eletroejaculação e as amostras foram diluídas em 4 grupos de diluidores: LElecitina de soja (sem a adição de antioxidantes); LAlecitina de soja suplementada com ácido ascórbico (AA, 4,5mM); LS lecitina de soja suplementada com superóxido dismutase (SOD, 60UI/mL) e GOgema de ovo (sem adição de antioxidantes). O sêmen foi então, criopreservado de maneira automatizada. As amostras foram descongeladas e analisadas quanto aos testes laboratoriais de motilidade computadorizada do espermatozóide (CASA); integridade de membrana plasmática (eosina/nigrosina); integridade de membrana acrossomal (fast Green/ rosa bengala); atividade citoquímica mitocondrial (DAB); susceptibilidade do DNA à desnaturação (SCSA); índice de estresse oxidativo induzido (TBARS). Além disso, foram realizados testes para verificar o potencial de fertilidade das amostras espermáticas criopreservadas. A fertilidade in vivo foi realizada pela técnica de inseminação artificial em tempo fixo (IATF), utilizando 450 fêmeas bovinas, seguido de exame ultrassonográfico para avaliação de prenhez. Teste de fertilidade in vitro, foi realizado pela técnica de produção in vitro de embriões (PIV) com o uso de ovários de frigoríficos, a classificação do desenvolvimento embrionário e a avaliação da motilidade espermática foram promovidas no decorrer do processo. Os resultados demonstraram que o diluidor LE apresentou efeito na proteção espermática de maneira semelhante ao diluidor GO. No entanto a suplementação desse primeiro com antioxidantes é uma alternativa para melhorar ainda mais esse processo, já que a taxa de prenhez obtida nos grupos LA e LS é satisfatória em um programa de IATF. Ainda o grupo LS foi o que apresentou melhores resultados no processo de PIV. Concluindo que o diluidor à base de lecitina de soja suplementado com o antioxidante superóxido dismutase seria uma opção para a substituição definitiva dos diluidores sintetizados com gema de ovo. / Due to the great demand for animal protein and the importance that bovine breeding exert on national economy, efficient production systems have been required. Cattle genetics preservation and dissemination depend on reproductive biotechnologies such as sperm cryopreservation, artificial insemination and in vitro fertilization. However, the use of egg yolk-based extender is under discussion nowadays, once there is great variability in its composition and risks of bacteriological contamination. On the other hand, despite soybean lecithin-based extenders do not present these risks, satisfactory results, after bovine sperm cryopreservation, have not been reached yet. Based on the hypothesis that soybean lecithinbased extender supplemented with antioxidants, preserve the sperm cell characteristics so efficient as egg yolk does, the aim of the present experiment was to compare the effects of egg yolk-based extender and soybean lecithin-based extender (with and without antioxidants), on functionality and fertility maintenance of bovine cryopreserved sperm samples. For this, seminal samples from 20 Brangus bulls were used, collects were realized by eletroejaculation method and samples were diluted in 4 extenders group: LE-soybean lecithin-based extender (without antioxidant supplementation); LA- soybean lecithin supplemented with ascorbic acid (AA, 4,5mM); LS- soybean lecithin supplemented with superoxide dismutase (SOD, 60UI/mL) and GO-egg yolk-based extender (without antioxidant supplementation). Then, semen was cryopreserved by automatic method. Samples were thawed and analyzed by laboratorial tests such as computer assisted semen analysis (CASA); plasma membrane integrity (eosin/nigrosin); acrosome membrane integrity (fast green/ rose bengal); mitochondrial cytochemical activity (DAB); susceptibility of chromatin denaturation (SCSA); induced oxidative stress index (TBARS). Furthermore, tests for fertility potential of cryopreserved semen samples were performed. In vivo fertility was accessed by timed artificial insemination (TAI), 450 bovine females were inseminated, and ultrasonographical exam was realized for pregnancy detection. In vitro fertility test was accessed by embryo in vitro production (IVP), ovaries from slaughterhouses were used, embryo development classification and sperm motility were promoted during the process. Results indicate that sperm protection is similar between LE and GO extenders. However the antioxidant supplementation of soybean lecithin-based extender is a great alternative to improve the process of sperm protection, since pregnancy rate of LA and LS groups was satisfactory for a TAI program. Besides, LS group presented the best results on IVP process. In conclusion, soybean lecithin-based extender supplemented with superoxide dismutase would be a better option for a definite replacement of egg yolk-based extender for sperm bovine cryopreservation.

Ácido ascórbico

Antioxidante

Diluidor seminal

Gema de ovo

Superóxido dismutase

Antioxidant

Ascorbic acid

Egg yolk

Semen extender

Superoxide dismutase

Actions of seminal fluid signalling factors in the female reproductive tract and on pregnancy outcome.

Glynn, Danielle Jannette

January 2008

The cytokine environment of early pregnancy is known to be a key determinant of the development of the pre-implantation embryo, and its subsequent implantation and growth. Factors in male seminal fluid have been identified as regulators of the expression of cytokines in the female tract of mice, humans and other mammalian species, with insemination eliciting a cascade of molecular and cellular events, reminiscent of a classic inflammatory response. In humans, perturbations in seminal fluid signalling have been proposed to predispose to pathologies of pregnancy including implantation failure, recurrent miscarriage and pre-eclampsia. Seminal transforming growth factor-beta (TGFβ) is identified as one key molecule present in seminal fluid responsible for inducing the female post-mating cytokine response in mice. Research in humans however, has shown the seminal TGFβ content of fertile versus infertile couples to be similar, while the content of other known seminal constituents such as interferon-gamma (IFNγ), correlate with reproductive success. This project aimed to investigate the nature of active factors present in seminal fluid in mice, and their interactions in regulating the uterine cytokine environment during early pregnancy, utilising a variety of in vitro and in vivo experimental strategies. Further, the effect of perturbation in the peri-conception cytokine environment on short and long term pregnancy and postnatal outcomes was investigated. Evaluation of uterine fluids from estrous and mated mice showed a marked upregulation of a number of cytokines following mating, including granulocyte macrophage colony stimulating factor (GM-CSF), interleukin-6 (IL-6) and the chemokine KC (rodent IL-8 homologue). Increased production of factors such as GM-CSF and subsequent generation of a receptive uterine environment is thought to be crucial for optimal embryo development and placentation. It has previously been shown that seminal factors such as TGFβ contribute to the uterine post-mating inflammatory response, however other moieties present in seminal fluid, for instance cytokines induced in response to infection such as IFNγ or products from the mucosal microflora, may also play a regulatory role. Using uterine epithelial cells cultured in vitro, it was shown that a variety of immune modulators including the cytokines TGFβ and IFNγ, as well as bacterial products, gram negative lipopolysaccharide (LPS) and gram positive lipoteichoic acid (LTA), can alter basal cytokine production. IFNγ, a pro-inflammatory cytokine secreted by activated natural killer cells and T-cells, is known to interfere with TGFβ signalling in other contexts. Independently TGFβ, LPS and LTA stimulate GM-CSF production while differentially regulating IL-6 and KC production. Conversely IFNγ inhibits GM-CSF production, without effecting IL-6 or KC. Pair wise combinations of TGFβ, LPS and LTA resulted in additive stimulation of GM-CSF, while addition of IFNγ to cultures in conjunction with any of these molecules downregulated GM-CSF and KC stimulation. These in vitro studies indicate factor-specific interactions between seminal fluid constituents and highlight the complex nature of seminal fluid signalling. Consequently we propose that the relative ratio of seminal signalling factors is likely to be more important than the absolute concentration of various regulators, in determining the optimal female reproductive tract response. Using the mouse as an in vivo model, I have in addition demonstrated that LPS and LTA instilled into an estrous uterus can elicit cytokine production comparable to that observed following insemination. Further, these studies have shown that IFNγ instilled into the uterus of a recently mated mouse can reduce the post-copulatory GM-CSF and KC surge. However administration of IFNγ had no effect on near term pregnancy outcomes including fetal or placental weights, fetal crown-rump length, or implantation or resorption rates. The ‘developmental origins of adult disease hypothesis’ proposes the idea that the early uterine environment encountered by the conceptus contributes toward the risk of metabolic disorders in adulthood, hence a long term study of progeny conceived after IFNγ administration was also undertaken. Neo-natal outcomes, such as birth weight, litter size and gestation length were unaltered, as was growth trajectory to 22 weeks of age. Adult metabolic markers, glucose tolerance, organ weight, muscle weight, adiposity and systolic blood pressure were not affected by the perturbation of peri-conceptual cytokine parameters. This work has examined the potential regulatory role of a number of seminal fluid signalling agents in directing the post-mating cytokine response, and has furthermore shown the relatively resilient nature of the early cytokine environment to subtle perturbation. Delineating the identity and roles of seminal fluid factors in early pregnancy brings us closer to an understanding of the key physiological events of early pregnancy and assists in identifying potential risk factors for human pregnancy pathologies. / Thesis (Ph.D.) -- University of Adelaide, School of Paediatrics and Reproductive Health, 2008

Generative organs, Female.

Pregnancy

Semen

Análisis, función y aplicaciones biotecnológicas de las proteínas del plasma seminal de porcino PSP-I y PSP-II

García Hernández, Eva María

04 December 2007

La aplicación de procesos biotecnológicos como la separación de espermatozoides X e Y mediante citometría de flujo, pueden generar la eliminación de determinados componentes del plasma seminal necesarios para conservar su funcionalidad. En este sentido, se ha observado que la adición de plasma seminal al medio espermático, protege a los espermatozoides cuando estos son sometidos a separación espermática mediante citometría de flujo. Sin embargo, diversos estudios demuestran que rel efecto beneficioso que ejerce el plasma seminal sobre los espermatozoides reside en determinadas proteínas. En el caso de la especie porcina, hay estudios previos que determinan que el efecto protector que ejerce el plasma seminal sobre los espermatozoides, se debe a una proteína denominada heterodímero PSP-I/PSP-II. El efecto beneficioso de dicha proteína sobre la funcionalidad espermática en espermatozoides de verraco altamente diluidos parece estar conservada, en su subunidad PSP-II y, concretamente, en la fracción peptídica de ésta. Estudiar, además, su localización a lo largo del tracto genital del verraco así como en las distintas fracciones del eyaculado, puede ser importante para llegar a conocer si la presencia de este heterodímero en el medio de recogida espermático de espermatozoides X e Y, es beneficioso tanto en la funcionalidad como en la capacidad fecundante de estos espermatozoides. / Biotechnological procedures of semen, such as sexing using flow cytometry/cell sorting procedures, causes high dilutions during sperm manipulation, linked with the wash away or high dilution of seminal plasma components. Thus, to develop strategies to extend the viability of treated spermatozoa are necessary. It is well known that add seminal plasma (SP) to the sperm media contributes to preserving the integrity and the fertilizing potential of sperm. Nevertheless, the beneficial effects of seminal plasma seem to be restricted to specific proteins of the SP. In porcine, previous studies have related this protective effect of the seminal plasma on the sperm cells to a protein called PSP-I/PSP-II heterodimer. The beneficial effect of this protein on the functionality of highly diluted boar spermatozoa is largely preserved in its PSP-II subunit and does not appear to require its glycan moiety. Moreover, study its localization along male reproductive tract and in different portions of the ejaculate could be important to know if the presence of PSP-I/PSP-II heterodimer in the collection medium for sex sorted spermatozoa is beneficial on the in vitro function and in vivo fertilizing ability.

reproductive tract

sex-sorted spermatozoa

boar seminal plasma

PSP-II

PSP-I

Reproducción y obstetricia

6

60

612

619