Use of fluorescent probes to assess membrane integrity in mammalian spermatozoa
TLDR
The technique appeared to provide more reliable estimations of the percentage of functional cells than did motility estimations or assessments of acrosomal integrity, and demonstrated the sensitivity of the sperm plasma membrane to cold shock: virtually all cells rapidly became permeable to the stains after such stress.Abstract:
Carboxyfluorescein diacetate and propidium iodide were used as fluorescent stains to assess membrane integrity in sperm populations from ram and boar. The living spermatozoa were immobilized with low concentrations of formaldehyde so that individual stained cells could be observed in a suspension with the aid of a fluorescence microscope. Intracellular esterases liberated impermeant-free carboxyfluorescein from the permeant carboxyfluorescein diacetate and caused the product to accumulate and fluoresce green within the acrosome and the mitochondria as well as within the cytoplasm. Most of the spermatozoa (the intact ones) accumulated carboxyfluorescein in all compartments; however, a few cells (those with damaged plasma membranes) accumulated the stain only in the acrosome and/or the mitochondria, while others (all of whose membranes were damaged) remained entirely unstained. The impermeant propidium iodide did not stain any of the (intact) spermatozoa that accumulated carboxyfluorescein throughout their length, but stained all the others (the heads fluoresced red). The technique appeared to provide more reliable estimations of the percentage of functional cells than did motility estimations or assessments of acrosomal integrity (presence of normal apical ridge). The technique also demonstrated the sensitivity of the sperm plasma membrane to cold shock: virtually all cells rapidly became permeable to the stains after such stress. Assessments of boar sperm samples during preparative incubation for in-vitro fertilization indicated a considerable increase in the percentage of cells with damaged plasma membranes as incubation proceeded, in advance of the increase in the percentage of cells with discharged acrosomes.read more
Citations
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Basic aspects of frozen storage of semen
TL;DR: The possible roles of cryoprotectants and additives are considered in the context of their putative interactions with the sperm plasma membrane and modern approaches to the laboratory assessment of spermatozoa after freeze-thawing are discussed.
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Bicarbonate/CO2, an effector of capacitation, induces a rapid and reversible change in the lipid architecture of boar sperm plasma membranes
TL;DR: It is found that bicarbonate causes a rapid increase in the ability of live boar spermatozoa to bind merocyanine, apparently by perturbing enzymic control processes.
Journal ArticleDOI
Subtle membrane changes in cryopreserved bull semen in relation with sperm viability, chromatin structure, and field fertility
TL;DR: The results indicate a certain proportion of bull spermatozoa express PS on their surface after thawing, and that the incidence of such cells is inversely correlated to sperm viability, and positively correlated to abnormal sperm chromatin condensation since they eventually undergo necrosis.
Journal ArticleDOI
Flow cytometric evaluation of sperm parameters in relation to fertility potential.
TL;DR: Flow cytometry is a tool that may be used in the future to monitor many new potential markers of sperm function and in conjunction with the flow cytometer, permit the evaluation of a large number of spermatozoa.
Journal ArticleDOI
Decrease in glutathione content in boar sperm after cryopreservation: Effect of the addition of reduced glutathione to the freezing and thawing extenders
Joaquín Gadea,Elena Sellés,Marco Antonio Marco,Pilar Coy,Carmen Matás,Raquel Romar,Salvador Ruiz +6 more
TL;DR: There was a loss in GSH content after cryopreservation of boar semen, and addition of GSH to the freezing extender did not result in any improvement in either standard semen parameters or sperm fertilizing ability, which suggests that during the thawing process, GSH prevents damage of a sperm property that is critical in the fertilization process but that is not measured in the routine semen analysis.
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Assessment of spermatozoal function using dual fluorescent staining and flow cytometric analyses.
TL;DR: In this paper, a fluorogenic stain consisting of carboxyfluorescin diacetate (CFDA) and the relatively membrane-impermeant nuclear stain propidium iodide (PI) was used to distinguish three distinct populations of spermatozoa.
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Production, characterization, and use of ionophore‐induced, calcium‐dependent acrosome reaction in ram spermatozoa
TL;DR: Although the motile ionophore-treated spermatozoa were unsuccessful at penetrating normal mature sheep oocytes in vitro, they were able to penetrate zona-free oocytes, after which swelling and decondensation of the sperm head took place.