Sperm cell capacitation status of ram semen after cooling

Detalhes bibliográficos
Autor(a) principal: Bartmer, Monica Elisa
Data de Publicação: 2022
Outros Autores: Sanguinet, Eduardo de Oliveira, Pinzón Osorio, César Augusto, Cunha, Thomaz Kranen, Ferreira, Higor da Silva, Kohler, Louise Fontoura, Rodrigues, José Luiz Rigo, Bertolini, Marcelo
Tipo de documento: Artigo
Idioma: eng
Título da fonte: Repositório Institucional da UFRGS
Texto Completo: http://hdl.handle.net/10183/254591
Resumo: Background: The use of conventional artificial insemination (AI) in sheep production is usually associated with lower fertility rates when frozen semen is used. Cooled ram semen has been an alternative over frozen semen due to the higher viability, seminal quality and fertility rates following AI. The semen preservation process promotes sperm cell modifica¬tions similar to capacitation (capacitation-like) that causes cell damage affecting viability and seminal quality, but such effects are unclear for cooled semen. The aim of this study was to determine the status of sperm cell capacitation (CA) and acrosome reaction (AR) during ram semen processing and cooling under different extenders, dilution factors, and aerobiosis conditions as a function of storage time at 5oC. Materials, Methods & Results: Two consecutive ejaculates per day per male were collected from 2 adult rams by artifi¬cial vagina at 48-72 h intervals, in three replications. After macro- and microscopic evaluations, semen was segregated into groups under 3 extenders (Tris-egg yolk or TY, citrate-egg yolk or CY, skimmed milk or SM), 2 dilution factors (1 x 109 or Bi, 100 x 106 or Mi cells/mL), and 2 aerobiosis conditions (aerobic or A, semi-anaerobic or SA). Diluted semen was cooled to 5ºC and stored for up to 72 h, with evaluations every 24 h. Aliquots of fresh ejaculates and of each cooled diluted subgroup, according to extender, dilution, and aerobiosis, were collected at times T0 and T72 for determination of acrosome status and membrane integrity by the chlortetracycline (CTC) and trypan blue-Giemsa stainings, respectively. No differences were detected in sperm cell motility (M) and motility vigor (V) between fresh and diluted semen. After cooling, a significant decrease in M was observed after 48 h in CY and SM compared with fresh semen and 0 h of cool¬ing, while V started to decrease after 24 h in CY compared with TY. Likewise, M/V from different dilutions and aerobic conditions decreased more significantly after 48 and 24 h of cooling, respectively. The sperm capacitation status did not show differences in the proportion of non-capacitated (NCA), CA and AR sperm cells between TY, CY, and SM extend¬ers (NCA: 75.0%, 71.3%, 74.0%; CA: 15.7%, 17.2%, 15.9%; AR: 9.3%, 11.5%, 10.2%) or between Bi and Mi dilutions (NCA: 74.0%, 72.9%; CA: 15.9%, 16.6%; AR: 10.1%, 10.5%), respectively. However, differences (P < 0.05) were observed between A and SA aerobic conditions, with CA (17.0% vs. 15.5%) and AR (11.9% vs. 8.7%) rates being higher in A than SA, respectively, with no differences in NCA (71.1% vs. 75.8%), irrespective of the storage time. Sperm cell viability decreased after 48 h, especially in CY (P < 0.05). Discussion: Ram sperm cells can suffer irreversible damage due to thermal shock during cooling. Egg yolk-based extend¬ers provide phospholipids and cholesterol to protect the sperm cell membrane during the thermal shock caused by the change in temperature. In this study, sperm cells had irreversible decreases in M/V, with increase in acrosome and plasma membrane damage after cooling to 5ºC. The largest and smallest decreases in M and V over time were observed in the CY and TY extenders, respectively. In addition to the extender type, the semen preservation method and storage time promoted changes in the capacitation status, AR and in sperm cell viability, which per se were associated with a decrease in semen fertility. In fact, the proportions of CA and/or AR sperm cells gradually increased over time after dilution and storage at 5ºC, with a negative correlation between sperm cell viability and M/V over time. In summary, extender and cooling time affected mostly M/V, while aerobiosis condition and dilution factor were more associated with acrosome status and sperm survival, with the extender having less impact on the acrosome status as a function of time.
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spelling Bartmer, Monica ElisaSanguinet, Eduardo de OliveiraPinzón Osorio, César AugustoCunha, Thomaz KranenFerreira, Higor da SilvaKohler, Louise FontouraRodrigues, José Luiz RigoBertolini, Marcelo2023-02-10T04:56:32Z20221678-0345http://hdl.handle.net/10183/254591001161674Background: The use of conventional artificial insemination (AI) in sheep production is usually associated with lower fertility rates when frozen semen is used. Cooled ram semen has been an alternative over frozen semen due to the higher viability, seminal quality and fertility rates following AI. The semen preservation process promotes sperm cell modifica¬tions similar to capacitation (capacitation-like) that causes cell damage affecting viability and seminal quality, but such effects are unclear for cooled semen. The aim of this study was to determine the status of sperm cell capacitation (CA) and acrosome reaction (AR) during ram semen processing and cooling under different extenders, dilution factors, and aerobiosis conditions as a function of storage time at 5oC. Materials, Methods & Results: Two consecutive ejaculates per day per male were collected from 2 adult rams by artifi¬cial vagina at 48-72 h intervals, in three replications. After macro- and microscopic evaluations, semen was segregated into groups under 3 extenders (Tris-egg yolk or TY, citrate-egg yolk or CY, skimmed milk or SM), 2 dilution factors (1 x 109 or Bi, 100 x 106 or Mi cells/mL), and 2 aerobiosis conditions (aerobic or A, semi-anaerobic or SA). Diluted semen was cooled to 5ºC and stored for up to 72 h, with evaluations every 24 h. Aliquots of fresh ejaculates and of each cooled diluted subgroup, according to extender, dilution, and aerobiosis, were collected at times T0 and T72 for determination of acrosome status and membrane integrity by the chlortetracycline (CTC) and trypan blue-Giemsa stainings, respectively. No differences were detected in sperm cell motility (M) and motility vigor (V) between fresh and diluted semen. After cooling, a significant decrease in M was observed after 48 h in CY and SM compared with fresh semen and 0 h of cool¬ing, while V started to decrease after 24 h in CY compared with TY. Likewise, M/V from different dilutions and aerobic conditions decreased more significantly after 48 and 24 h of cooling, respectively. The sperm capacitation status did not show differences in the proportion of non-capacitated (NCA), CA and AR sperm cells between TY, CY, and SM extend¬ers (NCA: 75.0%, 71.3%, 74.0%; CA: 15.7%, 17.2%, 15.9%; AR: 9.3%, 11.5%, 10.2%) or between Bi and Mi dilutions (NCA: 74.0%, 72.9%; CA: 15.9%, 16.6%; AR: 10.1%, 10.5%), respectively. However, differences (P < 0.05) were observed between A and SA aerobic conditions, with CA (17.0% vs. 15.5%) and AR (11.9% vs. 8.7%) rates being higher in A than SA, respectively, with no differences in NCA (71.1% vs. 75.8%), irrespective of the storage time. Sperm cell viability decreased after 48 h, especially in CY (P < 0.05). Discussion: Ram sperm cells can suffer irreversible damage due to thermal shock during cooling. Egg yolk-based extend¬ers provide phospholipids and cholesterol to protect the sperm cell membrane during the thermal shock caused by the change in temperature. In this study, sperm cells had irreversible decreases in M/V, with increase in acrosome and plasma membrane damage after cooling to 5ºC. The largest and smallest decreases in M and V over time were observed in the CY and TY extenders, respectively. In addition to the extender type, the semen preservation method and storage time promoted changes in the capacitation status, AR and in sperm cell viability, which per se were associated with a decrease in semen fertility. In fact, the proportions of CA and/or AR sperm cells gradually increased over time after dilution and storage at 5ºC, with a negative correlation between sperm cell viability and M/V over time. In summary, extender and cooling time affected mostly M/V, while aerobiosis condition and dilution factor were more associated with acrosome status and sperm survival, with the extender having less impact on the acrosome status as a function of time.application/pdfengActa scientiae veterinariae. Porto Alegre, RS. Vol. 50 (2022), Pub. 1899, 14 p.ResfriamentoDiluente de espermaCapacitação espermáticaViabilidade espermáticaQualidade do sêmenOvinosCooled semenExtendersDilution factorAerobiosisAcrosome statusSperm cell viabilitySheepSperm cell capacitation status of ram semen after coolinginfo:eu-repo/semantics/articleinfo:eu-repo/semantics/otherinfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UFRGSinstname:Universidade Federal do Rio Grande do Sul (UFRGS)instacron:UFRGSTEXT001161674.pdf.txt001161674.pdf.txtExtracted Texttext/plain62643http://www.lume.ufrgs.br/bitstream/10183/254591/2/001161674.pdf.txtb770a118446496f676cd294e371585b3MD52ORIGINAL001161674.pdfTexto completo (inglês)application/pdf630206http://www.lume.ufrgs.br/bitstream/10183/254591/1/001161674.pdf68a9a28c2639915f9f278491485722c7MD5110183/2545912023-02-24 04:21:27.560321oai:www.lume.ufrgs.br:10183/254591Repositório InstitucionalPUBhttps://lume.ufrgs.br/oai/requestlume@ufrgs.bropendoar:2023-02-24T06:21:27Repositório Institucional da UFRGS - Universidade Federal do Rio Grande do Sul (UFRGS)false
dc.title.pt_BR.fl_str_mv Sperm cell capacitation status of ram semen after cooling
title Sperm cell capacitation status of ram semen after cooling
spellingShingle Sperm cell capacitation status of ram semen after cooling
Bartmer, Monica Elisa
Resfriamento
Diluente de esperma
Capacitação espermática
Viabilidade espermática
Qualidade do sêmen
Ovinos
Cooled semen
Extenders
Dilution factor
Aerobiosis
Acrosome status
Sperm cell viability
Sheep
title_short Sperm cell capacitation status of ram semen after cooling
title_full Sperm cell capacitation status of ram semen after cooling
title_fullStr Sperm cell capacitation status of ram semen after cooling
title_full_unstemmed Sperm cell capacitation status of ram semen after cooling
title_sort Sperm cell capacitation status of ram semen after cooling
author Bartmer, Monica Elisa
author_facet Bartmer, Monica Elisa
Sanguinet, Eduardo de Oliveira
Pinzón Osorio, César Augusto
Cunha, Thomaz Kranen
Ferreira, Higor da Silva
Kohler, Louise Fontoura
Rodrigues, José Luiz Rigo
Bertolini, Marcelo
author_role author
author2 Sanguinet, Eduardo de Oliveira
Pinzón Osorio, César Augusto
Cunha, Thomaz Kranen
Ferreira, Higor da Silva
Kohler, Louise Fontoura
Rodrigues, José Luiz Rigo
Bertolini, Marcelo
author2_role author
author
author
author
author
author
author
dc.contributor.author.fl_str_mv Bartmer, Monica Elisa
Sanguinet, Eduardo de Oliveira
Pinzón Osorio, César Augusto
Cunha, Thomaz Kranen
Ferreira, Higor da Silva
Kohler, Louise Fontoura
Rodrigues, José Luiz Rigo
Bertolini, Marcelo
dc.subject.por.fl_str_mv Resfriamento
Diluente de esperma
Capacitação espermática
Viabilidade espermática
Qualidade do sêmen
Ovinos
topic Resfriamento
Diluente de esperma
Capacitação espermática
Viabilidade espermática
Qualidade do sêmen
Ovinos
Cooled semen
Extenders
Dilution factor
Aerobiosis
Acrosome status
Sperm cell viability
Sheep
dc.subject.eng.fl_str_mv Cooled semen
Extenders
Dilution factor
Aerobiosis
Acrosome status
Sperm cell viability
Sheep
description Background: The use of conventional artificial insemination (AI) in sheep production is usually associated with lower fertility rates when frozen semen is used. Cooled ram semen has been an alternative over frozen semen due to the higher viability, seminal quality and fertility rates following AI. The semen preservation process promotes sperm cell modifica¬tions similar to capacitation (capacitation-like) that causes cell damage affecting viability and seminal quality, but such effects are unclear for cooled semen. The aim of this study was to determine the status of sperm cell capacitation (CA) and acrosome reaction (AR) during ram semen processing and cooling under different extenders, dilution factors, and aerobiosis conditions as a function of storage time at 5oC. Materials, Methods & Results: Two consecutive ejaculates per day per male were collected from 2 adult rams by artifi¬cial vagina at 48-72 h intervals, in three replications. After macro- and microscopic evaluations, semen was segregated into groups under 3 extenders (Tris-egg yolk or TY, citrate-egg yolk or CY, skimmed milk or SM), 2 dilution factors (1 x 109 or Bi, 100 x 106 or Mi cells/mL), and 2 aerobiosis conditions (aerobic or A, semi-anaerobic or SA). Diluted semen was cooled to 5ºC and stored for up to 72 h, with evaluations every 24 h. Aliquots of fresh ejaculates and of each cooled diluted subgroup, according to extender, dilution, and aerobiosis, were collected at times T0 and T72 for determination of acrosome status and membrane integrity by the chlortetracycline (CTC) and trypan blue-Giemsa stainings, respectively. No differences were detected in sperm cell motility (M) and motility vigor (V) between fresh and diluted semen. After cooling, a significant decrease in M was observed after 48 h in CY and SM compared with fresh semen and 0 h of cool¬ing, while V started to decrease after 24 h in CY compared with TY. Likewise, M/V from different dilutions and aerobic conditions decreased more significantly after 48 and 24 h of cooling, respectively. The sperm capacitation status did not show differences in the proportion of non-capacitated (NCA), CA and AR sperm cells between TY, CY, and SM extend¬ers (NCA: 75.0%, 71.3%, 74.0%; CA: 15.7%, 17.2%, 15.9%; AR: 9.3%, 11.5%, 10.2%) or between Bi and Mi dilutions (NCA: 74.0%, 72.9%; CA: 15.9%, 16.6%; AR: 10.1%, 10.5%), respectively. However, differences (P < 0.05) were observed between A and SA aerobic conditions, with CA (17.0% vs. 15.5%) and AR (11.9% vs. 8.7%) rates being higher in A than SA, respectively, with no differences in NCA (71.1% vs. 75.8%), irrespective of the storage time. Sperm cell viability decreased after 48 h, especially in CY (P < 0.05). Discussion: Ram sperm cells can suffer irreversible damage due to thermal shock during cooling. Egg yolk-based extend¬ers provide phospholipids and cholesterol to protect the sperm cell membrane during the thermal shock caused by the change in temperature. In this study, sperm cells had irreversible decreases in M/V, with increase in acrosome and plasma membrane damage after cooling to 5ºC. The largest and smallest decreases in M and V over time were observed in the CY and TY extenders, respectively. In addition to the extender type, the semen preservation method and storage time promoted changes in the capacitation status, AR and in sperm cell viability, which per se were associated with a decrease in semen fertility. In fact, the proportions of CA and/or AR sperm cells gradually increased over time after dilution and storage at 5ºC, with a negative correlation between sperm cell viability and M/V over time. In summary, extender and cooling time affected mostly M/V, while aerobiosis condition and dilution factor were more associated with acrosome status and sperm survival, with the extender having less impact on the acrosome status as a function of time.
publishDate 2022
dc.date.issued.fl_str_mv 2022
dc.date.accessioned.fl_str_mv 2023-02-10T04:56:32Z
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dc.identifier.issn.pt_BR.fl_str_mv 1678-0345
dc.identifier.nrb.pt_BR.fl_str_mv 001161674
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dc.language.iso.fl_str_mv eng
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dc.relation.ispartof.pt_BR.fl_str_mv Acta scientiae veterinariae. Porto Alegre, RS. Vol. 50 (2022), Pub. 1899, 14 p.
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