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Generation of reactive oxygen species by equine spermatozoa
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Abstract
Objective—To characterize generation of reactive
oxygen species (ROS) by equine spermatozoa.
Sample Population—Multiple semen samples collected
from 9 stallions.
Procedure—Equine spermatozoa were separated
from seminal plasma on a discontinuous
polyvinylpyrrolidone (PVP)-coated silica gradient and
resuspended in a modified Tyrode albumin-lactate-pyruvate
medium. Amount of hydrogen peroxide (H2O2)
generated was assayed by use of a 1-step fluorometric
assay, using 10-acetyl-3,7-dihydroxyphenoxazine as a
probe for detection of H2O2 in a microplate assay format.
Concentration of H2O2 was determined by use of
a fluorescence microplate reader.
Results—Amount of H2O2 generated increased significantly
with time and spermatozoa concentration for
live and flash-frozen spermatozoa, and amount of H2O2
generated was significantly greater for flash-frozen
than for live spermatozoa. Addition of the reduced form
of nicotinamide adenine dinucleotide phosphate
(NADPH) significantly increased generation of H2O2 by
live and flash-frozen spermatozoa. Addition of a calcium
ionophore also significantly increased the amount of
H2O2 generated by live spermatozoa but did not have
an effect on amount of H2O2 generated by flash-frozen
spermatozoa. Abnormal equine spermatozoa generated
significantly greater amounts of H2O2 than did normal
spermatozoa.
Conclusion and Clinical Relevance—Equine spermatozoa
generate ROS in vitro, possibly via a
NADPH-oxidase reaction. Spermatozoa damaged during
flash-freezing or morphologically abnormal spermatozoa
generated significantly greater amounts of
ROS than did live or morphologically normal spermatozoa.
Damaged and abnormal spermatozoa generate
greater amounts of ROS that may contribute to
reduced fertility or problems related to semen preservation.
(Am J Vet Res 2001;62:508–515)
American Veterinary Medical Association (AVMA)
Title: Generation of reactive oxygen species by equine spermatozoa
Description:
Abstract
Objective—To characterize generation of reactive
oxygen species (ROS) by equine spermatozoa.
Sample Population—Multiple semen samples collected
from 9 stallions.
Procedure—Equine spermatozoa were separated
from seminal plasma on a discontinuous
polyvinylpyrrolidone (PVP)-coated silica gradient and
resuspended in a modified Tyrode albumin-lactate-pyruvate
medium.
Amount of hydrogen peroxide (H2O2)
generated was assayed by use of a 1-step fluorometric
assay, using 10-acetyl-3,7-dihydroxyphenoxazine as a
probe for detection of H2O2 in a microplate assay format.
Concentration of H2O2 was determined by use of
a fluorescence microplate reader.
Results—Amount of H2O2 generated increased significantly
with time and spermatozoa concentration for
live and flash-frozen spermatozoa, and amount of H2O2
generated was significantly greater for flash-frozen
than for live spermatozoa.
Addition of the reduced form
of nicotinamide adenine dinucleotide phosphate
(NADPH) significantly increased generation of H2O2 by
live and flash-frozen spermatozoa.
Addition of a calcium
ionophore also significantly increased the amount of
H2O2 generated by live spermatozoa but did not have
an effect on amount of H2O2 generated by flash-frozen
spermatozoa.
Abnormal equine spermatozoa generated
significantly greater amounts of H2O2 than did normal
spermatozoa.
Conclusion and Clinical Relevance—Equine spermatozoa
generate ROS in vitro, possibly via a
NADPH-oxidase reaction.
Spermatozoa damaged during
flash-freezing or morphologically abnormal spermatozoa
generated significantly greater amounts of
ROS than did live or morphologically normal spermatozoa.
Damaged and abnormal spermatozoa generate
greater amounts of ROS that may contribute to
reduced fertility or problems related to semen preservation.
(Am J Vet Res 2001;62:508–515).
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