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Measurement of intracellular calcium concentration and plasma membrane potential in human spermatozoa using flow cytometry
We report 2 novel approaches using flow cytometry to measure intracellular calcium concentration and plasma membrane potential in human spermatozoa. Both approaches have the potential to measure different responses in subpopulations of cells, which is particularly useful when studying heterogeneous...
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| Published in: | Journal of andrology 2000-03, Vol.21 (2), p.238-249 |
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| Main Authors: | , , , , |
| Format: | Article |
| Language: | English |
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| cited_by | cdi_FETCH-LOGICAL-c4831-1380ce9125ef5892d066558aeb7db9da8518cffdafb350028f7ae00aa3bf26703 |
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| cites | cdi_FETCH-LOGICAL-c4831-1380ce9125ef5892d066558aeb7db9da8518cffdafb350028f7ae00aa3bf26703 |
| container_end_page | 249 |
| container_issue | 2 |
| container_start_page | 238 |
| container_title | Journal of andrology |
| container_volume | 21 |
| creator | Brewis, I. A Morton, I. E Mohammad, S. N Browes, C. E Moore, H. D |
| description | We report 2 novel approaches using flow cytometry to measure intracellular calcium concentration and plasma membrane potential in human spermatozoa. Both approaches have the potential to measure different responses in subpopulations of cells, which is particularly useful when studying heterogeneous populations such as human spermatozoa. Intracellular calcium concentration ([Ca2+],) was measured using the probe indo‐1/AM. This allowed measurements to be made that were independent of variation in cell size and dye loading. It also enabled dead cells to be directly identified and excluded from the analyses without the need for counter‐staining. Mean basal [Ca2+], was determined as 50 nM (25–75 μM range) and, in response to the agonist progesterone (20 μM), this increased transiently to 195 nM (125–285 nM range) before declining to approximately half the maximal level within 2 minutes (values in parentheses correspond to the range of values typically found within a sperm population from 1 sample). These results are comparable with previously published data on whole sperm populations. Sperm membrane potential (VM) was assayed using the probe DiOC6(3). In carefully controlled experiments, a marked depolarization of the plasma membrane potential of capacitated spermatozoa was observed in response to progesterone (20 μM). Following in vitro capacitation, the sperm plasma membrane potential became hyperpolarized compared with the noncapacitated state. Therefore, this technique may be used to assay for sperm capacitation in vitro. |
| doi_str_mv | 10.1002/j.1939-4640.2000.tb02101.x |
| format | article |
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Mean basal [Ca2+], was determined as 50 nM (25–75 μM range) and, in response to the agonist progesterone (20 μM), this increased transiently to 195 nM (125–285 nM range) before declining to approximately half the maximal level within 2 minutes (values in parentheses correspond to the range of values typically found within a sperm population from 1 sample). These results are comparable with previously published data on whole sperm populations. Sperm membrane potential (VM) was assayed using the probe DiOC6(3). In carefully controlled experiments, a marked depolarization of the plasma membrane potential of capacitated spermatozoa was observed in response to progesterone (20 μM). Following in vitro capacitation, the sperm plasma membrane potential became hyperpolarized compared with the noncapacitated state. 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A</creatorcontrib><creatorcontrib>Morton, I. E</creatorcontrib><creatorcontrib>Mohammad, S. N</creatorcontrib><creatorcontrib>Browes, C. E</creatorcontrib><creatorcontrib>Moore, H. D</creatorcontrib><title>Measurement of intracellular calcium concentration and plasma membrane potential in human spermatozoa using flow cytometry</title><title>Journal of andrology</title><addtitle>J Androl</addtitle><description>We report 2 novel approaches using flow cytometry to measure intracellular calcium concentration and plasma membrane potential in human spermatozoa. Both approaches have the potential to measure different responses in subpopulations of cells, which is particularly useful when studying heterogeneous populations such as human spermatozoa. Intracellular calcium concentration ([Ca2+],) was measured using the probe indo‐1/AM. This allowed measurements to be made that were independent of variation in cell size and dye loading. It also enabled dead cells to be directly identified and excluded from the analyses without the need for counter‐staining. Mean basal [Ca2+], was determined as 50 nM (25–75 μM range) and, in response to the agonist progesterone (20 μM), this increased transiently to 195 nM (125–285 nM range) before declining to approximately half the maximal level within 2 minutes (values in parentheses correspond to the range of values typically found within a sperm population from 1 sample). These results are comparable with previously published data on whole sperm populations. Sperm membrane potential (VM) was assayed using the probe DiOC6(3). In carefully controlled experiments, a marked depolarization of the plasma membrane potential of capacitated spermatozoa was observed in response to progesterone (20 μM). Following in vitro capacitation, the sperm plasma membrane potential became hyperpolarized compared with the noncapacitated state. Therefore, this technique may be used to assay for sperm capacitation in vitro.</description><subject>Biological and medical sciences</subject><subject>Calcium - metabolism</subject><subject>capacitation</subject><subject>Cell Membrane - physiology</subject><subject>cyanine</subject><subject>FACS</subject><subject>Flow Cytometry</subject><subject>Fundamental and applied biological sciences. Psychology</subject><subject>Humans</subject><subject>indo‐1</subject><subject>Male</subject><subject>Mammalian male genital system</subject><subject>Membrane Potentials</subject><subject>Morphology. Physiology</subject><subject>progesterone</subject><subject>Sperm</subject><subject>Spermatozoa - metabolism</subject><subject>Spermatozoa - physiology</subject><subject>Vertebrates: reproduction</subject><issn>0196-3635</issn><issn>1939-4640</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2000</creationdate><recordtype>article</recordtype><recordid>eNqVkUtv1DAUhS0EotPCX0AWAnYJdpyHw4qqlJcKbGBt3Th2xyM7Tu1E6fTX4ygjYMvKlu45x-d-RuglJTklpHh7yGnL2qysS5IXhJB86khBCc3vH6Hdn9FjtCO0rTNWs-oMncd4SF5CG_YUnVHS0JJTvkMP3xTEOSinhgl7jc0wBZDK2tlCwBKsNLPD0g9SrZPJ-AHD0OPRQnSAnXJdgEHh0U9JYMCmBLyfHQw4jio4mPyDBzxHM9xibf2C5XHyTk3h-Aw90WCjen46L9Cvj9c_rz5nNz8-fbm6vMlkyRnNKONEqpYWldIVb4ue1HVVcVBd03dtD7yiXGrdg-5YlVbkugFFCADrdFE3hF2gN1vuGPzdrOIknInriqm3n6NoSJtwtWUSvtuEMvgYg9JiDMZBOApKxEpeHMSKV6x4xUpenMiL-2R-cXpl7pzq_7FuqJPg1UkAMXHVCZs08a-OMbKVeL_JFmPV8T8aiK-X3z-s1xTxeovYm9v9YoIS6ausTcWoWJaloKIQBePsN7h5sNU</recordid><startdate>200003</startdate><enddate>200003</enddate><creator>Brewis, I. A</creator><creator>Morton, I. E</creator><creator>Mohammad, S. N</creator><creator>Browes, C. E</creator><creator>Moore, H. D</creator><general>Am Soc Andrology</general><general>Blackwell Publishing Ltd</general><general>American Society of Andrology</general><scope>IQODW</scope><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7X8</scope></search><sort><creationdate>200003</creationdate><title>Measurement of intracellular calcium concentration and plasma membrane potential in human spermatozoa using flow cytometry</title><author>Brewis, I. A ; Morton, I. E ; Mohammad, S. N ; Browes, C. E ; Moore, H. D</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c4831-1380ce9125ef5892d066558aeb7db9da8518cffdafb350028f7ae00aa3bf26703</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2000</creationdate><topic>Biological and medical sciences</topic><topic>Calcium - metabolism</topic><topic>capacitation</topic><topic>Cell Membrane - physiology</topic><topic>cyanine</topic><topic>FACS</topic><topic>Flow Cytometry</topic><topic>Fundamental and applied biological sciences. Psychology</topic><topic>Humans</topic><topic>indo‐1</topic><topic>Male</topic><topic>Mammalian male genital system</topic><topic>Membrane Potentials</topic><topic>Morphology. Physiology</topic><topic>progesterone</topic><topic>Sperm</topic><topic>Spermatozoa - metabolism</topic><topic>Spermatozoa - physiology</topic><topic>Vertebrates: reproduction</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Brewis, I. A</creatorcontrib><creatorcontrib>Morton, I. E</creatorcontrib><creatorcontrib>Mohammad, S. N</creatorcontrib><creatorcontrib>Browes, C. E</creatorcontrib><creatorcontrib>Moore, H. D</creatorcontrib><collection>Pascal-Francis</collection><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>MEDLINE - Academic</collection><jtitle>Journal of andrology</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Brewis, I. A</au><au>Morton, I. E</au><au>Mohammad, S. N</au><au>Browes, C. E</au><au>Moore, H. D</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Measurement of intracellular calcium concentration and plasma membrane potential in human spermatozoa using flow cytometry</atitle><jtitle>Journal of andrology</jtitle><addtitle>J Androl</addtitle><date>2000-03</date><risdate>2000</risdate><volume>21</volume><issue>2</issue><spage>238</spage><epage>249</epage><pages>238-249</pages><issn>0196-3635</issn><eissn>1939-4640</eissn><coden>JOAND3</coden><abstract>We report 2 novel approaches using flow cytometry to measure intracellular calcium concentration and plasma membrane potential in human spermatozoa. Both approaches have the potential to measure different responses in subpopulations of cells, which is particularly useful when studying heterogeneous populations such as human spermatozoa. Intracellular calcium concentration ([Ca2+],) was measured using the probe indo‐1/AM. This allowed measurements to be made that were independent of variation in cell size and dye loading. It also enabled dead cells to be directly identified and excluded from the analyses without the need for counter‐staining. Mean basal [Ca2+], was determined as 50 nM (25–75 μM range) and, in response to the agonist progesterone (20 μM), this increased transiently to 195 nM (125–285 nM range) before declining to approximately half the maximal level within 2 minutes (values in parentheses correspond to the range of values typically found within a sperm population from 1 sample). These results are comparable with previously published data on whole sperm populations. Sperm membrane potential (VM) was assayed using the probe DiOC6(3). In carefully controlled experiments, a marked depolarization of the plasma membrane potential of capacitated spermatozoa was observed in response to progesterone (20 μM). 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| ispartof | Journal of andrology, 2000-03, Vol.21 (2), p.238-249 |
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| language | eng |
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| source | Wiley |
| subjects | Biological and medical sciences Calcium - metabolism capacitation Cell Membrane - physiology cyanine FACS Flow Cytometry Fundamental and applied biological sciences. Psychology Humans indo‐1 Male Mammalian male genital system Membrane Potentials Morphology. Physiology progesterone Sperm Spermatozoa - metabolism Spermatozoa - physiology Vertebrates: reproduction |
| title | Measurement of intracellular calcium concentration and plasma membrane potential in human spermatozoa using flow cytometry |
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