Your search keyword '"SPINACI, MARCELLA"' showing total 25 results

1. Epigallocatechin-3-gallate added after thawing to frozen dog semen: Effect on sperm parameters and ability to bind to oocytes’ zona pellucida

Author

Bucci, Diego, Cunto, Marco, Gadani, Beatrice, Spinaci, Marcella, Zambelli, Daniele, and Galeati, Giovanna

Published

2019

2. Seminal extracellular vesicles alter porcine in vitro fertilization outcome by modulating sperm metabolism.

Author

Barranco, Isabel, Spinaci, Marcella, Nesci, Salvatore, Mateo-Otero, Yentel, Baldassarro, Vito Antonio, Algieri, Cristina, Bucci, Diego, and Roca, Jordi

Subjects

*FERTILIZATION in vitro, *SEMINAL vesicles, *EXTRACELLULAR vesicles, *SPERMATOZOA, *FROZEN semen, *ATMOSPHERIC carbon dioxide, *ZONA pellucida

Abstract

Porcine seminal plasma (SP) is loaded with a heterogeneous population of extracellular vesicles (sEVs) that modulate several reproductive-related processes. This study investigated the effect of two sEV subsets, small (S-sEVs) and large (L-sEVs), on porcine in vitro fertilization (IVF). The sEVs were isolated from nine SP pools (five ejaculates/pool) using a size-exclusion chromatography-based procedure and characterized for quantity (total protein), morphology (cryogenic electron microscopy), size distribution (dynamic light scattering), purity and EV-protein markers (flow cytometry; albumin, CD81, HSP90β). The characterization confirmed the existence of two subsets of high purity (low albumin content) sEVs that differed in size (S- and L-sEVs). In vitro fertilization was performed with in vitro matured oocytes and frozen-thawed spermatozoa and the IVF medium was supplemented during gamete coincubation (1 h at 38.5 °C, 5 % CO 2 in a humidified atmosphere) with three different concentrations of each sEV subset: 0 (control, without sEVs), 0.1, and 0.2 mg/mL. The first experiment showed that sEVs, regardless of subset and concentration, decreased penetration rates and total IVF efficiency (P < 0.0001). In a subsequent experiment, it was shown that sEVs, regardless of subset and concentration, impaired the ability of spermatozoa to bind to the zona pellucida of oocytes (P < 0.0001). The following experiment showed that sEVs, regardless of the subset, bound to frozen-thawed sperm but not to in vitro matured oocytes, indicating that sEVs would affect sperm functionality but not oocyte functionality. The lack of effect on oocytes was confirmed by incubating sEVs with oocytes prior to IVF, achieving sperm-zona pellucida binding results similar to those of control. In the last experiment, conducted under IVF conditions, sperm functionality was analyzed in terms of tyrosine phosphorylation, acrosome integrity and metabolism. The sEVs, regardless of the subset, did not affect sperm tyrosine phosphorylation or acrosome integrity, but did influence sperm metabolism by decreasing sperm ATP production under capacitating conditions. In conclusion, this study demonstrated that the presence of sEVs on IVF medium impairs IVF outcomes, most likely by altering sperm metabolism. • Seminal extracellular vesicles decrease sperm-zona pellucida binding during porcine IVF. • Seminal extracellular vesicles impair IVF process during gamete co incubation. • Seminal extracellular vesicles can interact with pig frozen thawed spermatozoa. • Sperm metabolism can be modulated by seminal extracellular vesicles. [ABSTRACT FROM AUTHOR]

Published

2024

3. Impact of glyphosate and its formulation Roundup® on stallion spermatozoa.

Author

Spinaci, Marcella, Nerozzi, Chiara, Mislei, Beatrice, Blanco-Prieto, Olga, Mari, Gaetano, Galeati, Giovanna, and Bucci, Diego

Subjects

*STALLIONS, *SPERMATOZOA, *GLYPHOSATE, *GERM cells, *SPERM motility, *MITOCHONDRIAL membranes

Abstract

The growing and widespread use of glyphosate-based herbicides (GBHs) has raised an intense public debate about the impact of environmental contamination on animal and human health, including male fertility. The aim of this study was to deepen the impact of glyphosate (Gly) and GBHs on mammalian sperm investigating the effect of in vitro exposure of stallion spermatozoa to Gly and to its commercial formulation Roundup® (R). Spermatozoa were incubated at 37 °C with different Gly or R concentrations (from 0.5 to 720 μg/mL Gly or R at the same Gly-equivalent concentrations). After 1 h of incubation motility, viability, acrosome integrity, mitochondrial activity and ROS production were assessed. Gly, at all the concentrations tested, did not induce any detrimental impact on the sperm quality parameters evaluated. Conversely, R starting from 360 μg/mL (Gly-equivalent dose) significantly (P < 0.05) decreased total and progressive motility, viability, acrosome integrity, mitochondrial activity and the percentage of live spermatozoa with intact mitochondria not producing ROS. Our results indicate that the commercial formulation R is more toxic than its active molecule Gly and that the negative impact on stallion sperm motility might be likely due to a detrimental effect mainly at membrane and mitochondrial level and, at least in part, to redox unbalance. Moreover, based on the data obtained, it can be hypothesized a species-specificity in sperm sensitivity to Gly and GBHs as horse spermatozoa were negatively influenced at higher concentrations of R compared to those reported in literature to be toxic for human and swine male germ cells. • The effect of in vitro exposure of stallion spermatozoa to glyphosate (Gly) and to its commercial formulation Roundup (R) was evaluated. • Gly, at all the concentrations tested, did not induce any detrimental impact on the sperm quality parameters evaluated. • R ≥ 360 μg/mL decreased total and progressive motility, viability, acrosome integrity, mitochondrial activity and the percentage of spermatozoa not producing ROS. • The commercial formulation R is more toxic than its active molecule Gly. • The impact of R on stallion sperm motility might be due to a detrimental effect at membrane and mitochondrial level and, in part, to redox unbalance. [ABSTRACT FROM AUTHOR]

Published

2022

4. Sperm function and mitochondrial activity: An insight on boar sperm metabolism.

Author

Nesci, Salvatore, Spinaci, Marcella, Galeati, Giovanna, Nerozzi, Chiara, Pagliarani, Alessandra, Algieri, Cristina, Tamanini, Carlo, and Bucci, Diego

Subjects

*SPERMATOZOA, *BOARS, *METABOLISM, *ADENOSINE triphosphatase, *DIMETHYL sulfoxide, *RESPIRATION, *SEMEN

Abstract

In this study boar sperm mitochondrial activity was studied and deepened in order to delineate the main metabolic strategies used by boar sperm to obtain energy and to link them to sperm function. Boar spermatozoa were collected, diluted at 30 × 106 spz/mL and incubated for 1 h with: Rotenone (ROT), complex I inhibitor, Dimethyl-malonate (DMM), complex II inhibitor, antimycin A (ANTI), complex III inhibitor, oligomycin (OLIGO), ATP synthase inhibitor, Carbonyl cyanide m-chlorophenyl hydrazone (CCCP), uncoupling agent, 2-deoxy-glucose (2DG), glucose agonist, and Dimethyl sulphoxide (DMSO) as control vehicle. Viability and mitochondrial membrane potential (Sybr14/PI/JC1 staining) and sperm motility (using CASA system) were assayed after incubation. ROT, ANTI, OLIGO and CCCP significantly reduced total and progressive motility as well as cell velocities; ANTI and CCCP depressed mitochondrial membrane potential but did not affect cell viability. Cluster analysis of kinematic parameters showed some interesting features of sperm subpopulations: ANTI and CCCP caused a shift in sperm subpopulation towards "slow non progressive" cells, OLIGO and ROT caused a shift towards "average" and "slow non progressive" cells, while DMM and 2DG increased the "fast progressive" cells subpopulation. Sperm mitochondrial respiration and substrate oxidation, assayed polographically and spectrofluorimetrically, respectively pointed out a high ATP turnover and a low spare respiratory capacity, mainly linked to the NADH-O 2 oxidase activity. Therefore, boar spermatozoa heavily rely on mitochondrial oxidative phosphorylation, and especially on Complex I activity, to produce ATP and fuel motility. • Boar sperm metabolism and function is not yet fully understood. • Assessment of mitochondrial complex I, II, III and V function and membrane potential with specific inhibitors. • Respiration study using polarographic method. • Boar spermatozoa prefer using complex I and are dependant on mitochondrial intactness for motility. • Different inhibitors modify sperm subpopulation kinematics. [ABSTRACT FROM AUTHOR]

Published

2020

5. A polyphenol-rich extract from an oenological oak-derived tannin influences in vitro maturation of porcine oocytes.

Author

Spinaci, Marcella, Bucci, Diego, Muccilli, Vera, Cardullo, Nunzio, Nerozzi, Chiara, and Galeati, Giovanna

Subjects

*OVUM, *TANNINS, *ENGLISH oak, *EXTRACTS

Abstract

Abstract Tannins have been demonstrated to have antioxidant and various health benefit properties. The aim of this study was to determine the effect of an ethanol extract (TRE) of a commercial oenological tannin (Quercus robur toasted oak wood, Tan'Activ R®) on female gamete using an in vitro model of pig oocyte maturation (IVM) and examining nuclear maturation, cytoplasmic maturation, intracellular GSH and ROS levels and cumulus cell steroidogenesis. To this aim, during IVM performed in medium either supplemented (IVM A) or not supplemented (IVM B) with cysteine and β-mercaptoethanol, TRE was added at different concentrations (0, 1, 5, 10, 20 μg/ml). The addition of TRE at all the concentration tested to either IVM A or IVM B, did not influence oocyte nuclear maturation. When IVM was performed in IVM A, no effect was induced on cytoplasmic maturation by TRE at the concentration of 1, 5 and 10 μg/ml, while TRE 20 μg/ml significantly reduced the penetration rate after IVF (p < 0.05) and the blastocyst rate after parthenogenetic activation (p < 0.01). Oocyte maturation in IVM B, compared to IVM A group, decreased GSH (p < 0.001) and increased ROS (p < 0.01) intracellular levels and in turn impaired oocyte cytoplasmic maturation reducing the ability to sustain male pronuclear formation after IVM (p < 0.001) and the developmental competence after parthenogenetic activation (p < 0.001). TRE supplementation to IVM B significantly reduced ROS production (5, 10, 20 μg/ml TRE) to levels similar to IVM A group, and increased GSH levels (10, 20 μg/ml TRE) compared to IVM B (p < 0.05) without reaching those of IVM A group. TRE supplementation to IVM B at the concentrations of 1, 5 and 10 μg/ml significantly improved (p < 0.001) oocyte cytoplasmic maturation enhancing the ability to sustain male pronuclear formation without reaching, however, IVM A group levels. TRE addition at all the concentration tested to both IVM A and IVM B, did not induce any effect on E2 and P4 secretion by cumulus cells suggesting that the biological effect of the ethanol extract is not exerted thought a modulation of cumulus cell steroidogenesis. In conclusion, TRE, thanks to its antioxidant activity, was partially able to reduce the negative effect of the absence of cysteine and β-mercaptoethanol in IVM B, while TRE at high concentration in IVM A was detrimental for oocyte cytoplasmic maturation underlying the importance of maintaining a balanced redox environment during oocyte maturation. Highlights • The effect of the ethanol extract (TRE) of a commercial oenological tannin (Tan'Activ R®) on pig IVM was investigated. • In absence of cysteine and ß-mercaptoethanol TRE reduced ROS levels, increased GSH levels and improved cytoplasmic maturation. • TRE at high concentration in presence of cysteine and ß-mercaptoethanol was detrimental for oocyte cytoplasmic maturation. [ABSTRACT FROM AUTHOR]

Published

2019

6. Sex-sorting of boar spermatozoa does not influence the localization of glucose transporters

Author

Bucci, Diego, Galeati, Giovanna, Giaretta, Elisa, Tamanini, Carlo, and Spinaci, Marcella

Published

2013

7. Combined effects of resveratrol and epigallocatechin-3-gallate on post thaw boar sperm and IVF parameters.

Author

Bucci, Diego, Spinaci, Marcella, Yeste, Marc, Mislei, Beatrice, Gadani, Beatrice, Prieto Martinez, Noelia, Love, Charles, Mari, Gaetano, Tamanini, Carlo, and Galeati, Giovanna

Subjects

*FERTILIZATION in vitro, *RESVERATROL, *EPIGALLOCATECHIN gallate, *SPERMATOZOA, *BOARS

Abstract

Frozen-thawed boar semen suffer a fertility decrease that negatively affects its widespread use. In recent years supplementing frozen-thawed boar sperm with different antioxidants gave interesting and promising results; the aim of the present work was to study the effect of supplementing boar sperm thawing medium for 1 h with combination of epigallocatechin-3-gallate (EGCG, 50 μM) and Resveratrol (R, 2 mM), on boar sperm motility (assessed by CASA), viability, acrosome integrity, mitochondrial function, lipid peroxidation and DNA integrity (assessed by flow cytometry), protein tyrosine phosphorylation (assessed by immunofluorescence) and on in vitro fertilization (IVF). Our results demonstrate that sperm motility is negatively affected by R (alone or associated with EGCG, p < 0.05) in comparison to control and EGCG groups both at 1 h and 4 h; this effect is evident both in average motility parameters and in single cells kinematics, studied by cluster analysis, that showed the presence of a specific cell population with simil-hyperactivated features in R group (p < 0.01). Viability, acrosome integrity, mitochondrial functionality and lipid peroxidation are not influenced by the addition of the antioxidants; finally, DNA integrity is negatively influenced by R (both alone or associated with EGCG) both at 1 h and 4 h incubation (p < 0.05). Finally, tyrosine phosphorylated protein immunolocalization, used as capacitation parameter, is not affected by the different treatments. Penetration rate is strongly enhanced by R, both alone or associated with EGCG (p < 0.05); EGCG increases penetration rate as well but to a lower extent. Our findings demonstrate that the combination of R and EGCG could positively affect frozen-thawed boar sperm fertility in vitro; the effect is evident also in R groups, thus demonstrating that this antioxidant is predominant, and no synergic effect is present. Some insights are needed to understand if, in particular R (that showed the strongest effect) could be profitably used for artificial insemination in vivo, given the detrimental effect of this molecule on both sperm motility and DNA integrity. [ABSTRACT FROM AUTHOR]

Published

2018

8. Influence of secretome obtained from preovulatory follicular fluid on energy metabolism and meiotic competence of equine cumulus–oocyte complexes.

Author

Ortiz-Rodriguez, Jose M, Fernández-Hernández, Pablo, Luis-Calero, Marcos, Spinaci, Marcella, Bucci, Diego, Macías-García, Beatriz, and González-Fernández, Lauro

Abstract

Secretome is composed by proteins and microvesicles secreted by the granulosa cells that line the follicular wall. These bioactive compounds promote follicular growth and oocyte maturation, influencing oocyte metabolism. Hence, we hypothesized that addition of secretome from preovulatory follicular fluid (FF) to maturation medium may influence the meiotic competence and metabolism of cumulus-oocyte-complexes (COCs) obtained post mortem. FF was retrieved from preovulatory follicles (2 mares) after 32h of hCG administration. Three ml of FF from both mares were pooled, diluted 1:1 in PBS and centrifuged (4000g, 1h at 4°C) using a 10K Amicon® Ultra-15 Centrifugal Filter Unit and protein concentration was measured. A total of 186 COCs were retrieved from post mortem ovaries and were subjected to in vitro maturation (IVM) in TCM-199 medium, 10% of FBS and 5 mU/ml of FSH (Control; 59 oocytes) or with 20 µg/ml of secretome (Secretome20; 66 oocytes) or with 40 µg/ml of secretome (Secretome40; 61 oocytes) for 28 h in 5% CO 2 /95% air at 38.2°C. Oocytes were denuded, fixed in 4% formaldehyde and stained with Hoechst 33342 to assess chromatin conformation by fluorescence microscopy. Also, selected metabolites of the maturation medium prior to andafter IVM were assessed by magnetic proton nuclear resonance spectroscopy. After IVM, a trend towards glucose consumption and pyruvic acid production was observed compared to their controls prior IVM; a significant increase in lactic acid production in all treatments was observed (Table 1; p < 0.05). Our results show a tendency for quicker meiosis resumption in COCs incubated with Secretome40 (Table 2). In conclusion, secretome obtained from preovulatory follicular fluid added during IVM does not change COCs' energy metabolism nor maturation rate of equine cumulus-oocyte complexes in our in vitro culture system. Funding: MCCIN/AEI (PID2020-112723RB-I00; RYC-2017-21545; RYC2020-028915-I), Junta de Extremadura-FEDER (IB20005). [ABSTRACT FROM AUTHOR]

Published

2023

9. Mitochondrial calcium intake through Mitochondrial Calcium Uniporter is essential to modulate tail protein phosphorylation during boar sperm "in vitro" capacitation.

Author

Blanco-Prieto, Olga, Spinaci, Marcella, Galeati, Giovanna, Tamanini, Carlo, Rodriguez-Gil, Joan Enric, and Bucci, Diego

Subjects

*BOARS, *CALCIUM, *PHOSPHORYLATION, *MITOCHONDRIA, *INTRACELLULAR calcium, *SPERMATOZOA, *SEMEN

Abstract

Capacitation of mammalian spermatozoa involves numerous sperm function changes, from modification of energy metabolism to acquisition of hyperactivated motility, that are modulated through the activation of various molecular pathways including protein phosphorylation and intracellular calcium trafficking. This research was aimed at assessing the involvement of mitochondrial calcium uniporter (MCU) in capacitation regulation in boar sperm. Freshly ejaculated sperm (30 ×106 spz/ml) from 6 boars was incubated at 38.5°C under various conditions: Non- Capacitating Medium (NCM): 20 mM HEPES buffer (pH 7.4) added with 112 mM NaCl, 3.1 mM KCl, 5 mM glucose, 21.7 mM L-lactate, 1 mM sodium pyruvate, 0.3 mM Na 2 HPO 4 , 0.4 mM MgSO 4 , 4.5 mM CaCl 2 ; and Capacitating Medium (CM): NCM with 5 mg/ml BSA. Both CM and NCM were split into 4 subgroups: Control media (CM and NCM); EGTA media (CM-EGTA and NCM-EGTA) without 4.5 mM CaCl2 added with 5 µM EGTA; RU media (CM-RU and NCM-RU) added with 5 µM RU360, a specific inhibitor of MCU; EGTA-RU media (CM-EGTA-RU and NCM-EGTA-RU) EGTA media added with 5 µM RU360. At 0 and 4 h of incubation, Total and Progressive motility (TM, PM) were evaluated by CASA system and protein tyrosine phosphorylation by indirect immunofluorescence. Data were analysed using the R statistical environment v. 3.6.2 (The R Foundation for Statistical Computing, Vienna, Austria). Results are presented as the mean ± SD and level of significance was p<0.05. Differences were calculated by a linear mixed effects model using treatment and time as fixed factors and boar as a random factor; a Tukey post hoc test was applied. Tail sperm protein phosphorylation was not significantly different at 0 h but increased (p<0.05) in sperm incubated in CM for 4 h when compared to all other media (44.1%±19.1% CM vs 24.3%±9.3% CM-EGTA; 26.13%±4.1% CM-RU; 23.0%±11.6% CM-EGTA-RU; 10.0%±4.1% NCM; 10.5%±4.9% NCM-EGTA; 9.5%±4.7% NCM-EGTA-RU; 15.9%±4.1% NCM-RU respectively). Significant (p<0.05) differences were observed in both TM and PM between samples in NCM and those in CM-EGTA-RU (TM: 9.8%±7.7% NCM vs 32.7%±13.9% CM-EGTA-RU; PM: 4.0%±2.5% NCM vs 13.0%±3.1% CM-EGTA-RU); no differences were shown in the other media. In conclusion, intramitochondrial calcium intake through MCU is a key step for increasing phosphorylation of boar sperm tail proteins during in vitro capacitation process. [ABSTRACT FROM AUTHOR]

Published

2022

10. Cell bioenergetics and ATP production of boar spermatozoa.

Author

Prieto, Olga Blanco, Algieri, Cristina, Spinaci, Marcella, Trombetti, Fabiana, Nesci, Salvatore, and Bucci, Diego

Subjects

*RESPIRATION, *BIOENERGETICS, *SPERMATOZOA, *BOARS, *CELL metabolism, *OXIDATION of glucose

Abstract

Cellular metabolism is an important feature of spermatozoa that deserves more insights to be fully understood, in particular in porcine semen physiology. The present study aims to characterize the balance between glycolytic and oxidative metabolism in boar sperm cells. Agilent Seahorse technology was used to assess both oxygen consumption rate (OCR), as an oxidative metabolism index, and extracellular acidification rate (ECAR), as a glycolytic index. Different metabolic parameters were studied on freshly ejaculated sperm cells (identified as day zero sample, d0) and after one day of storage at 17 °C in Androhep extender (d1). Mitochondrial ATP production rate (MitoATP) was higher than the glycolytic ATP production rate (glycoATP) at both d0 and d1 while at d1 the amount of ATP production decreased, in particular, due to OXPHOS reduction. Conversely, glycoATP was not significantly different between d0 and d1. Interestingly, OCR profile showed no different bioenergetic parameters (i.e. ATP turnover, basal or maximal respiration, and spare respiration) between d0 and d1, thus indicating that sperm cell metabolism was reversibly decreased by preservation conditions. Other metabolic parameters showed the same trend, irrespective of the storage time: under stressed conditions (oligomycin plus FCCP), spermatozoa showed an increase in mitochondrial respiration while the metabolic potential of glycolysis did not undergo variations when compared to baseline metabolism. The rate of oxidation of fuel substrates – glucose, fatty acids, and glutamine – showed that sperm reliance on glucose oxidation to maintain baseline respiration was higher than fatty acids or glutamine. Interestingly spermatozoa demonstrated to have a low "capacity" parameter, which indicates that they cannot use only a single fuel substrate to produce energy. This feature of sperm metabolism to be unable to increase oxidation of a particular fuel to compensate for inhibition of alternative fuel pathway(s) was demonstrated by the negative value of "flexibility". Our results showed that ATP production in boar sperm cells relied on mitochondrial oxidative metabolism in freshly ejaculated cells, while, under liquid storage conditions, their oxidative metabolism decreased while the glycolysis remained constant. These results open new fields of research in the preservation techniques of boar sperm cells. • Oxidative cell metabolism of boar spermatozoa was storage time dependent. • The glycolysis activity was irrespective of the storage time. • In freshly ejaculated sperm cells, ATP was predominantly synthesized in mitochondria. • In sperm cells, the primary substrate for ATP production is likely glucose rather than glutamine or fatty acids. [ABSTRACT FROM AUTHOR]

Published

2023

11. Is Resveratrol Effective in Protecting Stallion Cooled Semen?

Author

Giaretta, Elisa, Bucci, Diego, Mari, Gaetano, Galeati, Giovanna, Love, Charles C., Tamanini, Carlo, and Spinaci, Marcella

Abstract

The aim of this work was to evaluate the effect of resveratrol (RSV) during liquid storage of stallion sperm for 24 hours at either 10°C or 4°C. The antioxidant RSV was added to reduce the oxidative damage that occurs during cold storage. Aliquots of 2 mL of diluted semen were stored either at 4°C or 10°C under anaerobic conditions, in the absence (control group) or presence of RSV at different concentrations (10, 20, 40, and 80 μM). Sperm quality parameters were assessed at 0 hours and after 24 hours of storage. Resveratrol treatment did not affect sperm quality parameters at 0 hours. At 24-hour storage, a significant ( P < .01) decrease of sperm quality was observed independently from RSV supplementation and storage temperature. A significant decrease of viable spermatozoa with high mitochondrial membrane potential (SYBR+/PI−/JC-1+) was evident at 24-hour storage in 40- and 80-μM RSV groups compared with control group. Moreover, a decline of total motility in 80-μM RSV group compared with the control group and a decrease of progressive motility and average path velocity in 80-μM RSV group compared with control and 20-μM RSV groups were observed. In conclusion, our findings demonstrate that RSV supplementation does not enhance sperm quality of stallion semen after 24 hours of storage. Moreover, 40- and 80-μM RSV concentrations could damage sperm functional status, probably acting as pro-oxidant. Finally, although 24-hour storage significantly affected most of the sperm quality parameters, no significant differences were found in groups maintained at 4°C or 10°C, suggesting that stallion semen could be equally preserved at these different temperatures. [ABSTRACT FROM AUTHOR]

Published

2014

12. Encapsulation of sex sorted boar semen: Sperm membrane status and oocyte penetration parameters

Author

Spinaci, Marcella, Chlapanidas, Theodora, Bucci, Diego, Vallorani, Claudia, Perteghella, Sara, Lucconi, Giulia, Communod, Ricardo, Vigo, Daniele, Galeati, Giovanna, Faustini, Massimo, and Torre, Maria Luisa

Subjects

*MICROENCAPSULATION, *ARTIFICIAL insemination, *SPERM sorting, *FERTILIZATION in vitro, *COMPARATIVE studies, *SPERM-ovum interactions

Abstract

Abstract: Although sorted semen is experimentally used for artificial, intrauterine, and intratubal insemination and in vitro fertilization, its commercial application in swine species is still far from a reality. This is because of the low sort rate and the large number of sperm required for routine artificial insemination in the pig, compared with other production animals, and the greater susceptibility of porcine spermatozoa to stress induced by the different sex sorting steps and the postsorting handling protocols. The encapsulation technology could overcome this limitation in vivo, protecting and allowing the slow release of low-dose sorted semen. The aim of this work was to evaluate the impact of the encapsulation process on viability, acrosome integrity, and on the in vitro fertilizing potential of sorted boar semen. Our results indicate that the encapsulation technique does not damage boar sorted semen; in fact, during a 72-hour storage, no differences were observed between liquid-stored sorted semen and encapsulated sorted semen in terms of plasma membrane (39.98 ± 14.38% vs. 44.32 ± 11.72%, respectively) and acrosome integrity (74.32 ± 12.17% vs. 66.07 ± 10.83%, respectively). Encapsulated sorted spermatozoa presented a lower penetration potential than nonencapsulated ones (47.02% vs. 24.57%, respectively, P < 0.0001), and a significant reduction of polyspermic fertilization (60.76% vs. 36.43%, respectively, polyspermic ova/total ova; P < 0.0001). However, no difference (P > 0.05) was observed in terms of total efficiency of fertilization expressed as normospermic oocytes/total oocytes (18.45% vs. 15.43% for sorted diluted and sorted encapsulated semen, respectively). The encapsulation could be an alternative method of storing of pig sex sorted spermatozoa and is potentially a promising technique in order to optimize the use of low dose of sexed spermatozoa in vivo. [Copyright &y& Elsevier]

Published

2013

13. Coupling sperm mediated gene transfer and sperm sorting techniques: a new perspective for swine transgenesis

Author

De Cecco, Marco, Spinaci, Marcella, Zannoni, Augusta, Bernardini, Chiara, Seren, Eraldo, Forni, Monica, and Bacci, Maria Laura

Subjects

*GENETIC transformation, *TRANSGENE expression, *FERTILIZATION in vitro, *SEXING of animals, *LABORATORY swine, *SPERMATOZOA

Abstract

Abstract: Flow cytometric separation of X and Y chromosome-bearing spermatozoa has been demonstrated to be effective in pigs, allowing the use of boar sexed semen in in vitro trials. Sperm Mediated Gene Transfer (SMGT) is a widely used and efficient technique for the creation of transgenic animals. The present research intended to prove that it is possible to associate sperm sexing with the SMGT technique in order to speed up the assessment of homozygous lines of transgenic pigs. In the first experiment, the sorting protocol was modified in order to obtain the highest DNA uptake by sorted spermatozoa. In the second experiment, spermatozoa that had undergone only sperm sorting, only SMGT, or both procedures (Sorted-SMGT) were used for in in vitro fertilization of in vitro matured oocytes. In the third experiment, transformed blastocysts of the desired gender (male) were obtained with Sorted-SMGT in an in vitro fertilization trial. The method we developed here allowed us to produce transgenic swine blastocysts of pre-determined gender, giving a positive answer at the aim to couple SMGT and sperm sorting in swine, obtaining fertile spermatozoa able to produce transgenic embryos of pre-determined gender. [ABSTRACT FROM AUTHOR]

Published

2010

14. In vitro production of cat blastocysts of predetermined sex using flow cytometrically sorted semen

Author

Spinaci, Marcella, Merlo, Barbara, Zannoni, Augusta, Iacono, Eleonora, De Ambrogi, Marco, Turba, Maria Elena, and Zambelli, Daniele

Subjects

*CATS as laboratory animals, *BLASTOCYST, *SEMEN, *ANIMAL breeding

Abstract

Abstract: Sex preselection in cats can have applications for both breeding purposes and as an experimental model for endangered felids. The present study examined the ability to produce cat embryos from in vitro fertilization (IVF) of in vitro matured (IVM) cat oocytes with flow cytometrically sorted spermatozoa and to verify the sex of the embryos obtained from sexed spermatozoa by PCR. In the first experiment, a total of 224 oocytes were fertilized with spermatozoa from six ejaculates sorted without sex separation. The sorting process did not influence the cleavage rate (sorted 44.0% versus unsorted 46.1%), day 6 morula-blastocyst rate (sorted 26.6% versus unsorted 29.6%) and day 7 blastocyst rate (sorted 16.5% versus unsorted 16.5%). In the second experiment, a total of 84 IVM oocytes were fertilized with sorted X- and Y-chromosome bearing spermatozoa from four ejaculates in order to obtain embryos of preselected sex. Embryonic sex determination by PCR revealed that 21 out of 24 embryos reaching morula/blastocyst stage (87.5%) were of the desired sex. In particular 12 out of 14 embryos (85.7%) derived from X-bearing spermatozoa were female and 9 embryos out of 10 (90%) derived from Y-bearing spermatozoa were male. Our results show, for the first time, that X- and Y-chromosome bearing spermatozoa sorted by high-speed flow cytometry can be successfully used in an IVM-IVF system to obtain cat embryos of a predetermined sex. [Copyright &y& Elsevier]

Published

2007

15. Preliminary insights into Red LED Irradiation for thawing cryopreserved boar semen.

Author

Tovar, Laura, Bucci, Diego, Spinaci, Marcella, Mammi, Ludovica, Merlo, Barbara, Gil, Joan Enric Rodriguez, and Rodriguez, José Manuel Ortiz

Subjects

*FROZEN semen, *THAWING, *IRRADIATION

Published

2025

16. Study of mitochondrial function in thawed bull spermatozoa using selective electron transfer chain inhibitors.

Author

Blanco-Prieto, Olga, Mislei, Beatrice, Martínez-Pastor, Felipe, Spinaci, Marcella, Mari, Gaetano, and Bucci, Diego

Subjects

*CHARGE exchange, *SPERMATOZOA, *MITOCHONDRIA, *ADENOSINE triphosphatase, *BULLS, *PLANT mitochondria, *GLYCOLYSIS

Abstract

Bull spermatozoa depend equally on glycolysis and oxidative phosphorylation for the maintenance of the energy necessary for their proper functioning. The aim of the present work was to delineate the mitochondrial activity of bull spermatozoa after incubation with specific inhibitors of the different mitochondrial complexes and evaluate their ROS production. Thawed bull sperm cells (30 × 106 mL−1 in Tyrode's extender) were incubated 1 and 3h at 37 °C with rotenone 5 μM (ROT), complex I inhibitor; dimethyl-malonate 10 mM (DMM), complex II inhibitor; carbonyl cyanide m-chlorophenyl hydrazine 5 μM (CCCP), uncoupling agent; antimycin A 1 μg/mL (ANTI), complex III inhibitor; oligomycin 5 μM (OLIGO), ATP synthase inhibitor, and 0.5% DMSO, vehicle (CTR). Sperm motility and kinematics were assessed by Hamilton Thorn IVOS 12.0. Mitochondrial membrane potential, mitochondrial O 2 •– production and H 2 O 2 intracellular content were evaluated by BD FACSCalibur flow cytometer, and sperm viability (SYBR-14/PI) and mitochondrial activity (JC-1/SYBR-14/PI) were assessed by epifluorescence microscopy. A multivariate analysis was performed on the results. In addition, sperm kinematic features, registered for each motile spermatozoon, were studied by cluster analysis. The incubation during 1 or 3 h in presence of the inhibitors of mitochondrial functionality only had a minor effect on motility parameters, decreasing the proportion of the SP1 (fast progressive) subpopulation after 3 h of incubation with ROT, ANTI or OLIGO. The percentage of live spermatozoa with active mitochondria was reduced under the effect of ANTI and CCCP both at 1 and 3 h. In conclusion, mitochondrial function is somehow impaired in frozen thawed bull sperm as not all live cells showed active mitochondria. These results support the findings that bull spermatozoa can alternatively rely on oxidative phosphorylation or glycolysis for energy obtainment and that their mitochondria are less affected by ETC inhibitors. [Display omitted] • Bull spermatozoa are resilient to freezing-thawing thanks to their metabolism. • Sperm cells' mitochondrial function nis impaired by FT process. • Bull sperm strongly rely on glycolytic metabolism after thawing. [ABSTRACT FROM AUTHOR]

Published

2023

17. Analysis of stallion spermatozoa metabolism using Agilent Seahorse XFp Technology.

Author

Ortiz-Rodriguez, Jose Manuel, Bucci, Diego, Tovar-Pascual, Laura, Granata, Silvia, Spinaci, Marcella, and Nesci, Salvatore

Subjects

*REPRODUCTIVE technology, *SPERMATOZOA analysis, *BIOENERGETICS, *FLUORESCENT probes, *SPERM motility, *SEMEN analysis

Abstract

Sperm metabolism consists of a sophisticated network of biochemical reactions and varies between species, resulting in different metabolic strategies for ATP production to maintain sperm functionality. ATP can be produced through glycolysis or in the mitochondria by oxidative phosphorylation (OXPHOS). Since OXPHOS is the predominant metabolic pathway in horses spermatozoa, various assessments of mitochondrial activity are used to evaluate fertility, utilizing techniques such as fluorescent probes analysed via microscopy or flow cytometry, and polarographic electrode assays to measure current flow in response to an applied voltage. Though, these methods are limited by low throughput, as they assess mitochondrial activity at a single time point under a specific treatment condition. This study explores, for the first time, the application of the Agilent Seahorse XFp Technology to evaluate metabolism in stallion spermatozoa. This method enables real-time measurement of cellular metabolism across multiple samples or experimental conditions simultaneously. Ejaculates from eight different stallions were collected, and pools were prepared from three of them. Sperm viability and mitochondrial activity were evaluated by fluorescence microscopy, sperm motility by a computer-assisted sperm analysis system, and sperm metabolism was analysed via the Seahorse XFp analyser. Results confirmed a preference for OXPHOS over glycolysis in ATP production in stallion sperm, with mitochondria contributing significantly to total ATP generation. The Seahorse XFp Technology proved effective in evaluating equine sperm bioenergetics, offering insights into metabolic pathways critical for sperm function. In conclusion, this technology grants a new method for high-throughput analysis of sperm metabolism and quality, which could be applied to future reproductive studies in male equine fertility. • Equine spermatozoa present preference for OXPHOS over glycolysis in ATP production. • The Seahorse XFp Technology is effective in evaluating equine sperm bioenergetics. • Seahorse XFp may aid in analysing sperm metabolism in assisted reproductive techniques. [ABSTRACT FROM AUTHOR]

Published

2024

18. Fasting influences steroidogenesis, vascular endothelial growth factor (VEGF) levels and mRNAs expression for VEGF, VEGF receptor type 2 (VEGFR-2), endothelin-1 (ET-1), endothelin receptor type A (ET-A) and endothelin converting enzyme-1 (ECE-1) in newly formed pig corpora lutea

Author

Galeati, Giovanna, Forni, Monica, Spinaci, Marcella, Zannoni, Augusta, Govoni, Nadia, Ribeiro, Luciana A., Seren, Eraldo, and Tamanini, Carlo

Subjects

*FASTING, *VASCULAR endothelial growth factors, *MESSENGER RNA, *ENDOTHELINS

Abstract

Abstract: This study was designed to verify whether fasting influences vascular endothelial growth factor (VEGF) production and VEGF, VEGF receptor-2 (VEGFR-2) as well as endothelin (ET) system members (endothelin converting enzyme-1, ECE-1; ET-1; endothelin receptor type A, ET-A) mRNA expression in pig corpora lutea; furthermore, we wanted to assess whether fasting affects steroidogenesis in luteal cells. Eight prepubertal gilts were induced to ovulate and were randomly assigned to two groups: (A) n =4, normally fed; and (B) n =4, fasted for 72h starting 3 days after ovulation. At the end of fasting, ovaries were removed from all the animals and corpora lutea (CLs) were collected. VEGF and steroid levels in luteal tissue were determined by ELISA and RIA, respectively; VEGF, VEGFR-2, ET-1, ET-A and ECE-1 mRNAs expression was measured by real-time PCR. VEGF protein levels were similar in the two groups, while all steroid (progesterone, testosterone, estradiol 17β) concentrations were significantly (P &#60;0.001) higher in CLs collected from fasted animals compared with those from normally fed gilts. VEGF, VEGFR-2, ET-1 and ECE-1 (but not ET-A) mRNA expression was significantly lower (P &#60;0.05) in fasted versus normally fed animals. The overall conclusion is that all the parameters studied are affected by feed restriction, but the mechanisms activated at luteal level are possibly not fully adequate to compensate for nutrient shortage. [Copyright &y& Elsevier]

Published

2005

19. Implementing an open-access CASA software for the assessment of stallion sperm motility: Relationship with other sperm quality parameters.

Author

Giaretta, Elisa, Munerato, Mauro, Yeste, Marc, Galeati, Giovanna, Spinaci, Marcella, Tamanini, Carlo, Mari, Gaetano, and Bucci, Diego

Subjects

*FISH spermatozoa motility, *SPERMATOZOA analysis, *MITOCHONDRIAL membranes, *MEMBRANE potential, *COMPUTER software, *ZEBRA danio, *FISHES

Abstract

Setting an open-access computer assisted sperm analysis (CASA) may benefit the evaluation of motility in mammalian sperm, especially when economic constraints do not allow the use of a commercial system. There have been successful attempts to develop such a device in Zebra fish sperm and the system has been used in very few studies on mammalian spermatozoa. Against this background, the present study aimed at developing an open-access CASA system for mammalian sperm using the horse as a model and based upon the Image J software previously established for Zebra fish sperm. Along with determining the sperm progressive motility and other kinetic parameters (such as amplitude of lateral head displacement), the “results” window was adjusted to simplify subsequent statistical analyses. The path window was enriched with colored sperm trajectories on the basis of the subpopulation they belong to and a number that allowed the sperm track to be associated to the sperm motility data shown in the “results” window. Data obtained from the novel plugin (named as CASA_bgm) were compared with those of the commercial CASA Hamilton-Thorn IVOS Vers.12, through Bland Altman’s plots. While the percentage of total and progressive motile sperm, VCL, VAP, VSL, LIN and STR and ALH were in agreement with those obtained with the commercial system, BCF significantly differed between the two systems probably due to their settings. Interestingly, a positive and significant correlation between the percentages of total motile sperm evaluated through CASA_bgm and those showing high mitochondrial membrane potential evaluated by JC-1 staining was found. In conclusion, CASA_bgm ImageJ plugin could be useful and reliable for stallion sperm motility analysis and it is our aim to apply this system to other mammalian species. [ABSTRACT FROM AUTHOR]

Published

2017

20. Alkaline phosphatase added to capacitating medium enhances horse sperm-zona pellucida binding.

Author

Bucci, Diego, Giaretta, Elisa, Merlo, Barbara, Iacono, Eleonora, Spinaci, Marcella, Gadani, Beatrice, Mari, Gaetano, Tamanini, Carlo, and Galeati, Giovanna

Subjects

*ALKALINE phosphatase, *SEMINAL proteins, *SPERMATOZOA, *STALLIONS, *ACROSOME reaction

Abstract

Alkaline phosphatase (AP) is present in equine seminal plasma and spermatozoa, but its functional role is not fully understood yet. Being that, sperm-oocyte interaction in equine species has been reported to be enhanced at a slightly basic pH, this work aimed at verifying whether exogenous alkaline phosphatase exerts any role on stallion spermatozoa and sperm-oocyte interaction at different pHs (7.4; 8.0; 9.0). Stallion spermatozoa were capacitated in Tyrode's medium at pH 7.4, 8.0, and 9.0 for 4 hours at 38 °C, 5% CO 2 with 2.5-IU AP (AP group) or without AP (capacitated spermatozoa group); viability with mitochondrial activity, motility, and acrosome integrity were measured. In addition, a homologous binding assay was carried out: stallion spermatozoa were capacitated 1 hour at 38 °C, 5% CO 2 with 2.5-IU AP (AP group) or without AP (capacitated spermatozoa group). Oocytes were then added to sperm suspensions and coincubated for 1 hour. Our results indicate that AP at pH 9.0 significantly increases the percentage of living cells with active mitochondria, whereas it significantly reduces the percentage of acrosome-damaged cells at pH 8.0. No significant differences were registered in motility parameters. The homologous binding assay showed a strong effect of AP, that increased the number of sperm bound to the oocyte's zona pellucida at all pHs tested. In conclusion, AP can induce some modifications on sperm membranes thus enhancing their capacity to bind to the zona pellucida of equine oocytes. [ABSTRACT FROM AUTHOR]

Published

2017

21. The feature of boar sperm energy metabolism and evidence on time-dependent ATP production.

Author

Nesci, Salvatore, Algieri, Cristina, Prieto, Olga Blanco, Spinaci, Marcella, and Bucci, Diego

Subjects

*ENERGY metabolism, *RESPIRATION, *SPERMATOZOA, *BOARS, *ENERGY consumption, *ALTERNATIVE fuels

Abstract

Cellular metabolism is a flexible network allowing spermatozoa to meet demands for homeostasis and motility. This study aimed to deepen the knowledge of sperm metabolism. Oxygen consumption rate (OCR) was used to assess oxidative phosphorylation (OXPHOS), whereas extracellular acidification rate (ECAR) measured glycolysis. The amount of ATP produced by mitochondria (mitoATP) or glycolysis (glycoATP) was detected the day of sperm collection (d0) and after 1 d (d1). MitoATP production rate was four and seven-times higher than the glycoATP production rate at d0 and d1, respectively. Total ATP production calculated was 430.2±127.1 pmol/min at d0 and 173.7±22.5 pmol/min at d1; the difference was due to a decrease of oxidative metabolism in mitochondria (d0=365.4±135.7 pmol/min vs d1=116.6±20.2 pmol/min). This trend was confirmed by functional sperm analysis (JC1/PI/SYBR green staining evaluated by epifluorescence microscopy) for live sperm with active mitochondria (d0=81.26±6.19 and d1=60.72±8.72) and live cells with inactive mitochondria (d0=1.49±1.87, d1=12.81±10.26). However, the OCR profile had no different bioenergetic parameters (i.e. ATP turnover, basal or maximal respiration, and spare respiration) between d0 and d1. Irrespective of the storage time, spermatozoa had increased mitochondrial respiration under stressed conditions (oligomycin plus FCCP) to meet energy demands (metabolic potential of OCR increased by 200%). The metabolic potential of glycolysis did not undergo variations when compared to baseline metabolism. Furthermore, the rate of oxidation of fuel substrates – glucose (Glu), fatty acids (FA), and glutamine (Gln) – was not time-dependent. Sperm reliance on Glu oxidative pathway to maintain baseline respiration was higher than FA or Gln. Interestingly, even if the "dependence" on Glu was higher, the metabolism of spermatozoa had a low "capacity" parameter. In other words, spermatozoa cannot use only a fuel substrate to produce energy. Indeed, sperm inability to increase oxidation of a particular fuel to compensate for inhibition of alternative fuel pathway(s) was demonstrated by the negative value of "flexibility". Our results showed that ATP production in sperm cells relied on mitochondrial oxidative metabolism; consistently, the difference in ATP production at d0 and d1 was caused by a different number of active mitochondria-dependent on the storage time. [ABSTRACT FROM AUTHOR]

Published

2022

22. Characterization of alkaline phosphatase activity in seminal plasma and in fresh and frozen–thawed stallion spermatozoa.

Author

Bucci, Diego, Giaretta, Elisa, Spinaci, Marcella, Rizzato, Giovanni, Isani, Gloria, Mislei, Beatrice, Mari, Gaetano, Tamanini, Carlo, and Galeati, Giovanna

Subjects

*HORSE reproduction, *ALKALINE phosphatase, *SEMINAL proteins, *SPERMATOZOA, *MALE ejaculation, *THERIOGENOLOGY

Abstract

Alkaline phosphatase (AP) has been studied in several situations to elucidate its role in reproductive biology of the male from different mammalian species; at present, its role in horse sperm physiology is not clear. The aim of the present work was to measure AP activity in seminal plasma and sperm extracts from freshly ejaculated as well as in frozen–thawed stallion spermatozoa and to verify whether relationship exists between AP activity and sperm quality parameters. Our data on 40 freshly ejaculated samples from 10 different stallions demonstrate that the main source of AP activity is seminal plasma, whereas sperm extracts contribution is very low. In addition, we found that AP activity at physiological pH (7.0) is significantly lower than that observed at pH 8.0, including the optimal AP pH (pH 10.0). Alkaline phosphatase did not exert any effect on sperm–oocyte interaction assessed by heterologous oocyte binding assay. Additionally, we observed a thermal stability of seminal plasma AP, concluding that it is similar to that of bone isoforms. Positive correlations were found between seminal plasma AP activity and sperm concentration, whereas a negative correlation was present between both spermatozoa extracts and seminal plasma AP activity and seminal plasma protein content. A significant decrease in sperm extract AP activity was found in frozen–thawed samples compared with freshly ejaculated ones (n = 21), concomitantly with the decrease in sperm quality parameters. The positive correlation between seminal plasma AP activity measured at pH 10 and viability of frozen–thawed spermatozoa suggests that seminal plasma AP activity could be used as an additional predictive parameter for stallion sperm freezability. In conclusion, we provide some insights into AP activity in both seminal plasma and sperm extracts and describe a decrease in AP after freezing and thawing. [ABSTRACT FROM AUTHOR]

Published

2016

23. Sex-sorted canine sperm cryopreservation: Limits and procedural considerations.

Author

Merlo, Barbara, Zambelli, Daniele, Cunto, Marco, Iacono, Eleonora, Nasi, Ludovica, Giaretta, Elisa, Galeati, Giovanna, Bucci, Diego, and Spinaci, Marcella

Subjects

*SPERMATOZOA physiology, *CANIDAE, *DOG physiology, *ARTIFICIAL insemination, *CENTRIFUGATION, *ALBUMINS

Abstract

The aim of this study was to define a protocol to store dog sperm before and after sorting to obtain an insemination dose sufficient to allow the conception by artificial insemination. Experiment 1 and 2 were performed to evaluate the more appropriate extender for preserving at room temperature dog sperm before and after sorting. Four extenders were tested: (1) Tris-fructose-citrate (TFC), (2) Tris-glucose-citrate (TGC), (3) modified Tyrode's albumin lactate pyruvate medium (mTALP), and (4) third fraction of the ejaculate (after centrifugation at 5000× g for 10 minutes; III FRAC). Experiment 3 and 4 were performed to evaluate the ability of dog semen to withstand sex sorting and freezing/thawing. Modified Tyrode's albumin lactate pyruvate medium was the best extender for canine sperm storage at room temperature (20 °C–25 °C) before (total motility: TFC, 8.3 ± 1.7; TGC, 50.0 ± 11.5; mTALP, 70.0 ± 0.1; III FRAC, 25.0 ± 1 0.4; P < 0.05) and after sorting (total motility: TFC, 7.3 ± 1.5; TGC, 10.3 ± 1.5; mTALP, 33.3 ± 6.7; III FRAC, 8.7 ± 5.8; P < 0.05), even if at 24-hour sorted sperm quality was impaired in all extenders tested herein. Sperm quality decreased after sorting (total motility: control, 92.5 ± 0.9; sorted, 52.9 ± 6.0; P < 0.05) and, especially, after freezing/thawing (total motility: frozen control, 25.7 ± 4.1; frozen sorted, 2.4 ± 1.2; P < 0.05). In conclusion, mTALP is an appropriate medium for canine sperm storage before and soon after sorting (hours), but a long storage period of sexed sperm at room temperature is not adequate. Cryopreservation greatly impaired sperm quality, and further studies are needed to optimize the freezing protocol for sexed dog sperm. [ABSTRACT FROM AUTHOR]

Published

2015

24. Daidzein does affect progesterone secretion by pig cumulus cells but it does not impair oocytes IVM

Author

Galeati, Giovanna, Vallorani, Claudia, Bucci, Diego, Bernardini, Chiara, Tamanini, Carlo, Parmeggiani, Albamaria, and Spinaci, Marcella

Subjects

*PROGESTERONE, *EMBRYOLOGY, *ISOFLAVONES, *SWINE embryos, *ESTRADIOL, *OVUM, *FERTILIZATION in vitro

Abstract

Abstract: Daidzein, an isoflavone abundant in soybeans and other legumes, displays estrogen like properties. This study was aimed at evaluating the effect of daidzein (1 and 10 μM) on nuclear and cytoplasmic maturation of pig oocytes and on steroidogenic activity of cumulus cells. Daidzein supplementation during IVM had no effect on nuclear maturation and on fertilization traits. By contrast, both concentrations significantly (P < 0.05) inhibited progesterone production by cumulus cells after 24 and 48 h of culture while they did not induce any effect on estradiol production. Furthermore, daidzein did not exert any effect on the percentage of embryos that developed to blastocyst stage, on the number of blastomeres per blastocyst, or on the level of Hsp-70 and -90 gene transcript. Overall, our data demonstrate that daidzein added during oocyte maturation does not affect pig embryo development even if it markedly inhibits progesterone production by cumulus cells. Further studies are needed to evaluate the possible effect of daidzein during embryonic development. [Copyright &y& Elsevier]

Published

2010

25. Food deprivation stimulates the luteolytic capacity in the gilt

Author

Galeati, Giovanna, Forni, Monica, Govoni, Nadia, Spinaci, Marcella, Zannoni, Augusta, De Ambrogi, Marco, Volpe, Sara, Seren, Eraldo, and Tamanini, Carlo

Subjects

*LUTEAL phase, *PROGESTERONE, *MESSENGER RNA, *BIOLOGICAL transport

Abstract

Abstract: The aims of this study were to study the effects of fasting on progesterone (P4) production in the pig and to verify whether fasting influences luteal expression of PGF2α receptor (FPr) and prostaglandin secretion. Superovulated prepubertal gilts were used; half of them were fasted for 72h starting on day 2 (F2) or 9 (F9) of the induced estrous cycle, respectively, while two groups (C2 and C9) served as respective controls. Plasma P4 and PGFM concentrations were determined by RIA while FPr mRNA expression in CLs collected at the end of fasting period was measured by real-time PCR. In experiment 1, plasma P4 concentrations in fasted gilts were significantly (P <0.01) higher than in controls starting from day 3 (F2; n =6) and 10 (F9; n =6). FPr mRNA expression was similar in F2 and C2 (n =6) CLs while it was significantly (P <0.05) higher in F9 than in C9 (n =6) CLs. In experiment 2, cloprostenol administered on day 12 significantly (P <0.05) increased FPr mRNA expression in CLs from both F9 (n =6) and C9 (n =6) gilts. At the time of cloprostenol injection PGFM levels were significantly higher (P <0.05) in the fasted group and cloprostenol-induced luteolysis in fasted but not in normally fed gilts. Results from this study indicate that fasting in prepubertal gilts induced to ovulate stimulates luteal P4 and PGFM production as well as FPr mRNA expression, thus increasing luteolytic susceptibility. [Copyright &y& Elsevier]

Published

2007