| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
RESEARCH |
Centre of Reproductive Medicine and Andrology of the University, Domagkstrasse 11, D-48129 Münster, Germany
Correspondence should be addressed to T G Cooper; Email: trevorg.cooper{at}ukmuenster.de
 |
Abstract |
|---|
 Top Abstract IntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
|
Introduction |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
Water cannot pass through occupied K+ channels, as the water of hydration is stripped off the ions before they enter the selectivity filter (Armstrong 2003, Saparov & Pohl 2004) and as the water can only diffuse slowly across the lipid bilayers, its transport across plasma membranes occurs mainly through aquaporins (AQPs) at 10- to 100-fold higher rates (see Agre et al. 2002). Among mammalian cells, 13 members of the AQP family have so far been identified; each being dominantly present in different tissues with most individual cell types having more than one isoform (see Castle 2005, Verkman 2005). Isoforms of AQPs used by spermatozoa for water transport have not been identified, although the presence of some proteins has been reported (Table 1).
|
Besides AQPs, there are other membrane proteins that participate in osmotic water transport; although they are present at lower densities than AQPs, their biological importance relative to AQPs has not been studied in most tissues (Verkman & Mitra 2000, see Table 1). Inhibitors of facilitative glucose transport, cytochalasin B and phloretin, decrease reversibly the osmotic water transport across the plasma membranes of several cell types (Table 1), but they are not entirely specific in their action. Nevertheless, the observation that phloretin inhibits water transport in ovine and human spermatozoa (Curry et al. 1995) and phloridzin, an inhibitor of sodium-coupled solute transporters, may block water influx into murine spermatozoa (Barfield et al. 2005) suggests that the approach of using transport inhibitors may throw light on the water channels employed by spermatozoa during regulatory volume decrease (RVD).
In the present work, the types of water channels involved in physiological sperm volume regulation were probed using various inhibitors of water transport. The volume of viable spermatozoa, ascertained from their forward scatter of a laser beam, was measured by a flow cytometer, since this permits the simultaneous determintation of cell vitality. Transfer to a hypotonic medium within the physiological range should trigger osmotic water influx and a related increase in cell volume which will induce RVD. Quinine, an effective inhibitor of sperm RVD, causes unopposed influx of water into the cell by blocking the K+ efflux responsible for driving water outwards for RVD. This swelling will be hampered if water transport is prohibited by co- or pre-incubation with putative water transport inhibitors. Therefore, failure of quinine to swell the treated sperm will provide clear evidence of inhibition of water influx.
|
Results |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
|
|
|
Initial time-course protocol
Control and quinine-treated spermatozoa
When murine epididymal spermatozoa were first pre-incubated for 10 min in isotonic medium (430 mmol/kg) and then transferred to hypotonic medium, the cells maintained their volume, first measured at 20 s, for the entire 5 min with a slight increase in size during the last 3 min. In the presence of quinine, cells were far larger than controls at the first time point and maintained this volume over the 5 min studied (Figs 3–5
).
|
|
|
Silver-treated cells
At the concentration tested (30 µmol/l), Ag+ had no effect on cell viability (Table 2). At 20 s, cells treated with silver and quinine were significantly smaller than those incubated in quinine alone and this was maintained during incubation until 305 s (Fig. 4). Spermatozoa incubated with Ag+ before hypotonic challenge swelled to volumes between those of the control and quinine-treated spermatozoa; but the variability was such that they were not significantly different from either group (Fig. 4).
Phloretin-treated cells
The viability of phloretin- and quinine-treated spermatozoa was not depressed below that of the controls (Table 2). At the first (20 s) time point, cells treated with phloretin and transferred to quinine were as large as untreated cells in quinine alone, but their size diminished during incubation so that by 305 s they were significantly smaller than both those incubated in quinine alone and the controls. Cells incubated in phloretin alone were smaller than the controls (Fig. 5).
Cytochalasin B-treated cells
Another glucose transporter inhibitor, cytochalasin B, at 5, 20, 40 µmol/l, with or without 800 µmol/l quinine, had no effect on sperm viability (Table 2). Unlike the other facilitative glucose transporter inhibitor phloretin, none of the concentrations tested had an influence on sperm volume or their response to quinine (data not shown).
Phloretin+tetraethylammonium (TEA)- or phloretin+furosemide-treated cells
In attempts to determine the cause of the volume decline in the presence of phloretin and quinine, additional inhibitors were provided with phloretin in the pre- and post-incubation media; the voltage-gated K-channel inhibitor TEA and the potassium-chloride co-transporter (KCC, SLC12A) inhibitor furosemide. Murine spermatozoa incubated with TEA or furosemide, either alone or each with quinine, were significantly more viable than the control cells (Table 2). In the absence of phloretin, neither compound alone altered swelling in the presence of quinine (data not shown).
In half of the animals used, and in both epididymides of the same mice, both TEA and furosemide separately were partially able to delay the decline in volume occurring in the presence of quinine after pre-incubation in phloretin (responders; Fig. 6), whereas in another four mice (non-responders), the decline in volume in the phloretin- and quinine-treated spermatozoa still occurred in the presence of furosemide or TEA (Fig. 6). At the first (20 s) time point, there were no differences between volumes of cells incubated with any treatment; none was different from the phloretin plus quinine control. By 305 s, significant differences were observed between the responders and non-responders to either furosemide or TEA in the cells given phloretin with quinine.
|
|
|
Discussion |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
Under similar conditions, however, the effects of Hg2+ were difficult to interpret. Cells were initially larger than controls, but this was followed by a decrease in volume. These results are compatible with the concept that when RVD becomes activated by the hypo-osmotic challenge, which should be immediate as in the controls, Hg2+ first inhibits water efflux more than influx, perhaps related to the time it takes to penetrate the cell and to bind to and inhibit the sulphydryl groups of the channels. Cell swelling caused by the initial inhibitory activity may trigger other, Hg-insensitive, water transport mechanisms to allow water efflux driven by osmolyte efflux in RVD. These may include Cl–/anion channels that also allow water passage (Hasegawa et al. 1992, Pohl 2004). With this protocol, in the transfer from epididymal fluid (high osmolality, high K+) to the test medium, spermatozoa are subjected to both osmotic and ionic changes. Changes in membrane potential would activate ion pumps, as it occurs during copulation.
To eliminate the problematical interpretation related to an anticipated delay in the action of Hg, the metal ion was allowed to interact with the functional groups on the transport proteins before hypo-osmotic challenge. In this experimental design (termed the initial time-course protocol), spermatozoa were pre-incubated in a medium with the mean osmolality of epididymal fluid, i.e. close to isotonic conditions (Cooper et al. 2008), so that osmotic challenges would be minimised during pre-incubation with the putative inhibitors without quinine. Thereafter, they were subjected to a physiological osmotic challenge in the drug in the absence or presence of quinine. In this protocol, sperm membrane repolarisation would occur under isotonic conditions, so that the subsequent transfer to the test medium would largely reflect an osmotic response.
If the pre-incubation were long enough for the water channel inhibitor to become effective, any immediate effects on water entry into the cell would become apparent; therefore, the cell volume was monitored at the earliest time-point (20 s) and continuously for 5 min. Furthermore, as quinine blocks osmolyte efflux during RVD, resulting in cell swelling by unopposed entry of water, any blockade of water entry would be demonstrated by cell volumes similar to those of the controls even in the presence of quinine.
Indeed, after pre-incubation, Hg2+ was able to block the volume increase that normally occurs under hypotonic conditions when RVD is inhibited by quinine, which suggests that Hg2+ blocks water entry. Because both AQP8 and AQP7 proteins are present in rat spermatozoa (Calamita et al. 2001) and Hg2+ inhibits AQP8 (Nielsen et al. 2007), but not AQP7 (Ishibashi et al. 1997), AQP8 may be mediating the water influx into murine spermatozoa. In the presence of quinine, blockade of water influx was also blocked by Ag+ since the volume of the treated cells was no different from that of control cells. Since AQP8 is Ag+ sensitive (Biernert et al. 2007), this is further evidence that AQP8 may be involved in water influx in spermatozoa. However, in the absence of quinine, Ag+ alone allowed water influx to some extent, since cell volumes were intermediate between those of the controls and those with quinine. The water channel involved here is not known.
The ability of murine spermatozoa to transport water during volume regulation in the presence of sodium azide and rotenone, at concentrations known to prevent sperm motility and mitochondrial activity (Aitken et al. 1997), suggests that the effects of Hg2+ and Ag+ on water transport were not due to any general toxic actions but more specific effects on water transport, most likely the binding of Hg2+ to the cysteine residue (cys-187) near to one of the two Asn-Pro-Ala (NPA) motifs that form the water pore of different AQP isoforms (Preston et al. 1993, see also Agre 2006).
Evidence for the involvement of glucose transporters in water transport includes the ability of specific inhibitors of glucose transport, cytochalasin B and phloretin to decrease reversibly the osmotic water transport across the plasma membranes of several cell types (Fischbarg et al. 1989, 1990). Previous studies have suggested that they may be involved in spermatozoa since water transport in ovine and human spermatozoa are sensitive to phloretin (Curry et al. 1995). Although glucose transporters have been detected in spermatozoa (Table 1), in this study neither phloretin nor cytochalasin B prevented water influx in the presence of quinine, making the glucose transporter an unlikely candidate as a water channel in murine spermatozoa.
In the presence of quinine and phloretin, cell volume was the same as that of cells incubated in quinine alone, indicating that water influx had not been inhibited by phloretin. Furthermore, neither was water efflux inhibited, since with time the spermatozoa shrank to volumes smaller than the controls. This suggests that phloretin promotes osmolyte efflux through channels insensitive to quinine. In the absence of quinine, phloretin reduced sperm volume below the level of the control cells. This implies that under the control experimental conditions, RVD was not efficient enough to prevent hypo-osmotic swelling completely and phloretin either inhibited water entry or was promoting water efflux. It is unlikely that these effects are due to abnormal metabolism through phloretin's inhibition of glucose transport via the glucose transporter, since the BWW medium contains the respiratory substrates lactate and pyuvuate. Although phloretin can inhibit AQP9 (Castle 2005), where antibodies have been used on epididymal sections, there are no reports of this AQP in luminal spermatozoa (Ruz et al. 2006, Da Silva et al. 2007).
Experiments designed to determine the possible alternative RVD mechanism in the presence of quinine and phloretin, leading to the observed water efflux, showed that both TEA and furosemide were able, in the same animals, to delay the onset of RVD. Unlike quinine, TEA itself has no effect on RVD of murine spermatozoa (Barfield et al. 2005), indicating that quinine-sensitive and TEA-insensitive voltage-sensitive K+ channels are preferentially utilised for K+ efflux in initial RVD. However, in the presence of quinine and phoretin in swollen cells, TEA-sensitive channels were clearly activated after a short delay. TEA blocks voltage-sensitive K+ channels, small conductance, Ca2+-sensitive K+ channels (SKCa: Coetzee et al. 1999) and large conductance K+ channels (BKCa: Rosenfeld et al. 2001), so it may be blocking K+ channels operating in swollen, but not normal, cells. Furosemide alone is capable of blocking RVD of murine spermatozoa with a delayed time course under long time-course conditions (Klein et al. 2006) and the K–Cl co-transporter it blocks in the present study is presumably operating earlier in swollen cells in the presence of quinine and phloretin in the responder animals.
That spermatozoa from only four of eight mice responded in this way reflects the between-male variability in osmotic responses. These responses may depend, among other things, on the ability of the spermatozoa to take up osmolytes, the ability of the epididymis to provide them, the osmolalities experienced within that epididymis, the length of time stored within the epididymis, which depends on sexual activity and nocturnal seminal emissions, and the expression of the osmolyte and water channels.
In summary, there is no evidence that sodium-dependent glucose transporters, glucose transporters or AQP9 are involved in water transport during RVD of murine spermatozoa; but the Hg2+- and Ag+-sensitive AQP8 is a likely candidate as water channel.
|
Materials and Methods |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
In the second protocol (initial time-course), the tubule contents were transferred to an albumin (4 mg/ml)-containing BWW medium with osmolality raised with NaCl to 430 mmol/kg (BWW430; similar to that of epididymal fluid (Yeung et al. 1999) and close to isotonic with cauda epididymidal spermatozoa (Cooper et al. 2008)) for pre-incubation at 37 °C in the presence of water transport inhibitors but not quinine. After 10 min, the sample was transferred to BWW330 containing 6 µg/ml PI as well as the inhibitor with or without 800 µmol/l quinine and read immediately and continuously for 5 min in the flow cytometer. In this procedure, changes in membrane potential would occur in the 10-min pre-incubation period under isotonic conditions, but the subsequent challenge would be purely osmotic.
For each protocol, spermatozoa from the same mice were used for all conditions in a given replicate of an experiment.
Flow cytometry
The flow cytometer was a FACS 500 (Beckmann–Coulter Epics, Krefeld, Germany) using 488 nm laser as excitation source, a 19 °C for forward scatter detection and red PI fluorescence detection for gating of live cells. The machine alignment was checked on the day of use with fluorescent spheres (Fluorospheres, Beckmann–Coulter) in order to ensure that voltages and signals were reproducible between studies. For the long time-course protocol, samples were read from 5 min and then every 10 or 15 min for 45 min. For the initial time-course protocol, samples were read as soon as possible after sperm dispersion and 20 s after injection into the equipment (the time taken for the sample to load automatically and fill the dead space of sample tubing) in continuous reading mode for 5 min. Data were collected and displayed in sequential 15 s bins. Data presented here are solely from viable cells that excluded the vital dye PI. The volume of spermatozoa was calculated from a standard curve obtained from the forward scatter of fluorescent spheres of known diameter (3, 4 and 5 µm: Duke Scientific Corporation Palto Alto, CA, USA). A linear relationship between volume (fl: y) and forward scatter (mean channel number: x) was obtained (y=0.211x–41.336) with coefficients of correlation (r) of 0.980 and determination (r2) of 0.961. From this relationship, the mean (±S.E.M.) volume of 160 control spermatozoa in hypotonic medium was 73±1 fl and 82±1 fl in the absence and presence of quinine respectively. In order to determine changes with time, absolute cell volumes were expressed as ratios of the first control samples (5 min in the long time-course protocol and 20 s in the initial time-course procotol).
Inhibitors
All reagents were the purest grade from Sigma. Quinine–HCl, HgCl2 and AgNO3 were made up in water, whereas phoretin, cytochalasin B, phloridzin and furosemide were made up in DMSO. The final percentage of DMSO (0.2% v/v) had no effect on cell size (data not shown). Stock solutions of sodium azide (100 mM in water) and rotenone (20 mM in DMSO) were also prepared. In order to rule out the possibility that the metal ion effects were due to general toxicity, sperm volume and the response to quinine under hypotonic conditions were also measured when spermatozoa were pre-incubated (under initial time-course conditions) with the mitochondrial poisons at a final concentration of 20 µM.
Statistical analysis
Only the data from the long time-course experiments with phloridzin conformed to a normal distribution with equal variance and could be analysed by two-way ANOVA. No matter how transformed, the remaining data could not be made to meet the required assumptions; so the optimal statistical analysis (two-way ANOVA) could not be applied. One-way ANOVA on normally distributed data, otherwise Kruskall–Wallis one-way ANOVA on ranks, was applied at relevant time points to illustrate the trends observed. When significant changes were found (P<0.05), this was followed by all pair-wise comparisons or against the relevant controls as appropriate (with Dunn's test for non-Gaussian distributions and the Holm–Sidak method for Gaussian) with the statistical program SigmaStat (Systat Software, Version 3.5, Erkrath, Germany).
|
Declaration of interest |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
|
Funding |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
|
Footnotes |
|---|
Received 28 January 2008
First decision 19 March 2008
Revised manuscript received 30 June 2008
Accepted 9 July 2008
|
References |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and MethodsDeclaration of interestFundingReferences |
|---|
Agre P 2006 The aquaporin water channels. Proceedings of the American Thoracic Society 3 5–13.
Agre P & Kozono D 2003 Aquaporin water channels: molecular mechanisms for human diseases. FEBS Letters 555 72–78.[CrossRef][Web of Science][Medline]
Agre P, King LS, Yasui M, Guggino WB, Ottersen OP, Fujiyoshi Y, Engel A & Nielsen S 2002 Aquaporin water channels – from atomic structure to clinical medicine. Journal of Physiology 542 3–16.
Aitken RJ, Fisher HM, Fulton N, Gomez E, Knox W, Lewis B & Irvine S 1997 Reactive oxygen species generation by human spermatozoa is induced by exogenous NADPH and inhibited by the flavoprotein inhibitors diphenylene iodonium and quinacrine. Molecular Reproduction and Development 47 468–482.[CrossRef][Web of Science][Medline]
Angulo C, Rauch MC, Droppelmann A, Reyes AM, Slebe JC, Delgado-Lopez F, Guaiquil VH, Vera JC & Concha II 1998 Hexose transporter expression and function in mammalian spermatozoa: cellular localization and transport of hexoses and vitamin C. Journal of Cellular Biochemistry 71 189–203.[CrossRef][Web of Science][Medline]
Armstrong CM 2003 Voltage-gated K channels. Science's STKE 2003 10.
Augustin R, Carayannopoulos MO, Dowd LO, Phay JE, Moley JF & Moley KH 2004 Identification and characterization of human glucose transporter-like protein-9 (GLUT9): alternative splicing alters trafficking. Journal of Biological Chemistry 279 16229–16236.
Barfield JP, Yeung CH & Cooper TG 2005 The effects of putative K+ channel blockers on volume regulation of murine spermatozoa. Biology of Reproduction 72 1275–1281.
Bienert GP, Moller AL, Kristiansen KA, Schulz A, Moller IM, Schjoerring JK & Jahn TP 2007 Specific aquaporins facilitate the diffusion of hydrogen peroxide across membranes. Journal of Biological Chemistry 282 1183–1192.
Biggers JD, Whittem WK & Whittingham DG1971The culture of mouse embryos in vitroJC DanielIn Methods in Mammalian Embryology San Francisco:Freeman:86–116.
Brooks HL, Regan JW & Yool AJ 2000 Inhibition of aquaporin-1 water permeability by tetraethylammonium: involvement of the loop E pore region. Molecular Pharmacology 57 1021–1026.
Burant CF & Davidson NO 1994 GLUT3 glucose transporter isoform in rat testis: localization, effect of diabetes mellitus, and comparison to human testis. American Journal of Physiology 267 R1488–R1495.[Web of Science][Medline]
Burant CF, Takeda J, Brot-Laroche E, Bell GI & Davidson NO 1992 Fructose transporter in human spermatozoa and small intestine is GLUT5. Journal of Biological Chemistry 267 14523–14526.
Calamita G, Mazzone A, Cho YS, Valenti G & Svelto M 2001 Expression and localization of the aquaporin-8 water channel in rat testis. Biology of Reproduction 64 1660–1666.
Castle NA 2005 Aquaporins as targets for drug discovery. Drug Discovery Today 10 485–493.[CrossRef][Web of Science][Medline]
Coetzee WA, Amarillo Y, Chiu J, Chow A, Lau D, McCormack T, Moreno H, Nadal MS, Ozaita A, Pountney D et al. 1999 Molecular diversity of K+ channels. Annals of the New York Academy of Sciences 868 233–285.[CrossRef][Web of Science][Medline]
Cooper TG & Barfield JP 2006 Utility of infertile male models for contraception and conservation. Molecular and Cellular Endocrinology 250 206–211.[CrossRef][Web of Science][Medline]
Cooper TG & Yeung CH 2007 Involvement of potassium and chloride channels and other transporters in volume regulation by spermatozoa. Current Pharmaceutical Design 13 3222–3230.[CrossRef][Web of Science][Medline]
Cooper TG, Barfield JP & Yeung CH 2008 The tonicity of murine epididymal spermatozoa and their permeability towards common cryoprotectants and epididymal osmolytes. Reproduction 135 625–633.
Curry MR, Millar JD & Watson PF 1995 The presence of water channel proteins in ram and human sperm membranes. Journal of Reproduction and Fertility 104 297–303.
Detmers FJ, de Groot BL, Muller EM, Hinton A, Konings IB, Sze M, Flitsch SL, Grubmuller H & Deen PM 2006 Quaternary ammonium compounds as water channel blockers. Specificity, potency, and site of action. Journal of Biological Chemistry 281 14207–14214.
Doege H, Bocianski A, Joost HG & Schurmann A 2000 Activity and genomic organization of human glucose transporter 9 (GLUT9), a novel member of the family of sugar-transport facilitators predominantly expressed in brain and leucocytes. Biochemical Journal 350 771–776.[CrossRef][Web of Science][Medline]
Van Dop C, Hutson SM & Lardy HA 1977 Pyruvate metabolism in bovine epididymal spermatozoa. Journal of Biological Chemistry 252 1303–1308.
Fischbarg J, Kuang KY, Hirsch J, Lecuona S, Rogozinski L, Silverstein SC & Loike J 1989 Evidence that the glucose transporter serves as a water channel in J774 macrophages. PNAS 86 8397–8401.
Fischbarg J, Kuang KY, Vera JC, Arant S, Silverstein SC, Loike J & Rosen OM 1990 Glucose transporters serve as water channels. PNAS 87 3244–3247.
Gomez O, Romero A, Terrado J & Mesonero JE 2006 Differential expression of glucose transporter GLUT8 during mouse spermatogenesis. Reproduction 131 63–70.
Gorelick DA, Praetorius J, Tsunenari T, Nielsen S & Agre P 2006 Aquaporin-11: a channel protein lacking apparent transport function expressed in brain. BMC Biochemistry 7 14.[CrossRef][Medline]
Haber RS, Weinstein SP, O'Boyle E & Morgello S 1993 Tissue distribution of the human GLUT3 glucose transporter. Endocrinology 132 2538–2543.
Hasegawa H, Skach W, Baker O, Calayag MC, Lingappa V & Verkman AS 1992 A multifunctional aqueous channel formed by CFTR. Science 258 1477–1479.
Helliwell PA, Richardson M, Affleck J & Kellett GL 2000 Stimulation of fructose transport across the intestinal brush-border membrane by PMA is mediated by GLUT2 and dynamically regulated by protein kinase C. Biochemical Journal 350 149–154.[CrossRef][Web of Science][Medline]
Ishibashi K 2006 Aquaporin superfamily with unusual npa boxes: S-aquaporins (superfamily, sip-like and subcellular-aquaporins). Cellular and Molecular Biology 52 20–27.[Medline]
Ishibashi K, Kuwahara M, Gu Y, Kageyama Y, Tohsaka A, Suzuki F, Marumo F & Sasaki S 1997 Cloning and functional expression of a new water channel abundantly epressed in the testis permeable to water, glycerol, urea. Journal of Biological Chemistry 272 20782–20786.
Kasahara T & Kasahara M 1997 Characterization of rat Glut4 glucose transporter expressed in the yeast Saccharomyces cerevisiae: comparison with Glut1 glucose transporter. Biochimica et Biophysica Acta 1324 111–119.[Medline]
Kim ST & Moley KH 2007 The expression of GLUT8, GLUT9a and GLUT9b in the mouse testis and sperm. Reproductive Sciences 14 445–455.
Klein T, Cooper TG & Yeung CH 2006 The role of potassium chloride cotransporters in murine and human sperm volume regulation. Biology of Reproduction 75 853–858.
Kuwahara M, Gu Y, Ishibashi K, Marumo F & Sasaki S 1997 Mercury-sensitive residues and pore site in AQP3 water channel. Biochemistry 36 13973–13978.[CrossRef][Web of Science][Medline]
Liu C, Gao D, Preston GM, McGann LE, Benson CT, Critser ES & Critser JK 1995 High water permeability of human spermatozoa is mercury-resistant and not mediated by CHIP28. Biology of Reproduction 52 913–919.[Abstract]
Loo DD, Zeuthen T, Chandy G & Wright EM 1996 Cotransport of water by the Na+/glucose cotransporter. PNAS 93 13367–13370.
Loo DD, Hirayama BA, Meinild AK, Chandy G, Zeuthen T & Wright EM 1999 Passive water and ion transport by cotransporters. Journal of Physiology 518 195–202.
Loo DD, Wright EM & Zeuthen T 2002 Water pumps. Journal of Physiology 542 53–60.
Maher F, Davies-Hill TM & Simpson IA 1996 Substrate specificity and kinetic parameters of GLUT3 in rat cerebellar granule neurons. Biochemical Journal 315 827–831.[Web of Science][Medline]
Martin HJ, Kornmann F & Fuhrmann GF 2003 The inhibitory effects of flavonoids and antiestrogens on the Glut1 glucose transporter in human erythrocytes. Chemico-Biological Interactions 146 225–235.[CrossRef][Web of Science][Medline]
Meinild AK, Klaerke DA & Zeuthen T 1998 Bidirectional water fluxes and specificity for small hydrophilic molecules in aquaporins 0–5. Journal of Biological Chemistry 273 32446–32451.
Nielsen S, Kwon TH, Frokiaer J & Agre P 2007 Regulation and dysregulation of aquaporins in water balance disorders. Journal of Internal Medicine 261 53–64.[CrossRef][Web of Science][Medline]
Niemietz CM & Tyerman SD 2002 New potent inhibitors of aquaporins: silver and gold compounds inhibit aquaporins of plant and human origin. FEBS Letters 531 443–447.[CrossRef][Web of Science][Medline]
Nilius B 2004 Is the volume-regulated anion channel VRAC a ‘water-permeable’ channel? Neurochemistry Research 29 3–8.[CrossRef][Web of Science][Medline]
Pohl P 2004 Combined transport of water and ions through membrane channels. Biological Chemistry 385 921–926.[CrossRef][Web of Science][Medline]
Preston GM, Jung JS, Guggino WB & Agre P 1993 The mercury-sensitive residue at cysteine 189 in the CHIP28 water channel. Journal of Biological Chemistry 268 17–20.
Rigau T, Rivera M, Palomo MJ, Fernandez-Novell JM, Mogas T, Ballester J, Pena A, Otaegui PJ, Guinovart JJ & Rodriguez-Gil JE 2002 Differential effects of glucose and fructose on hexose metabolism in dog spermatozoa. Reproduction 123 579–591.[Abstract]
Rosenfeld CR, Cornfield DN & Roy T 2001 Ca2+-activated K+ channels modulate basal and E2-beta-induced rises in uterine blood flow in ovine pregnancy. American Journal of Physiology 281 H422–H431.[Web of Science]
Ruz R, Gregory M, Smith CE, Cyr DG, Lubahn DB, Hess RA & Hermo L 2006 Expression of aquaporins in the efferent ductules, sperm counts, and sperm motility in estrogen receptor-alpha deficient mice fed lab chow versus casein. Molecular Reproduction and Development 73 226–237.[CrossRef][Web of Science][Medline]
Saito K, Kageyama Y, Okada Y, Kawakami S, Kihara K, Ishibashi K & Sasaki S 2004 Localization of aquaporin-7 in human testis and ejaculated sperm: possible involvement in maintenance of sperm quality. Journal of Urology 172 2073–2076.[CrossRef][Web of Science][Medline]
Sancho S, Casas I, Ekwall H, Saravia F, Rodriguez-Martinez H, Rodriguez-Gil JE, Flores E, Pinart E, Briz M, Garcia-Cil N et al. 2007 Effects of cryopreservation on semen quality and the expression of sperm membrane hexose transporters in the spermatozoa of Iberian pigs. Reproduction 134 111–121.
Saparov SM & Pohl P 2004 Beyond the diffusion limit: water flow through the empty bacterial potassium channel. PNAS 101 4805–4809.
Schurmann A, Axer H, Scheepers A, Doege H & Joost HG 2002 The glucose transport facilitator GLUT8 is predominantly associated with the acrosomal region of mature spermatozoa. Cell and Tissue Research 307 237–242.[CrossRef][Web of Science][Medline]
Da Silva N, Shum WW, El-Annan J, Paunescu TG, McKee M, Smith PJ, Brown D & Breton S 2007 Relocalization of the V-ATPase B2 subunit to the apical membrane of epididymal clear cells of mice deficient in the B1 subunit. American Journal of Physiology. Cell Physiology 293 C199–C210.[CrossRef]
Tsukaguchi H, Shayakul C, Berger UV, Mackenzie B, Devidas S, Guggino WB, van Hoek AN & Hediger MA 1998 Molecular characterization of a broad selectivity neutral solute channel. Journal of Biological Chemistry 273 24737–24743.
Tsukaguchi H, Weremowicz S, Morton CC & Hediger MA 1999 Functional and molecular characterization of the human neutral solute channel aquaporin-9. American Journal of Physiology 277 F685–F696.[Web of Science][Medline]
Urner F & Sakkas D 1999 A possible role for the pentose phosphate pathway of spermatozoa in gamete fusion in the mouse. Biology of Reproduction 60 733–739.
Verkman AS 2005 More than just water channels: unexpected cellular roles of aquaporins. Journal of Cell Science 118 3225–3232.
Verkman AS & Mitra AK 2000 Structure and function of aquaporin water channels. American Journal of Physiology. Renal Physiology 278 F13–F28.
Walker J, Jijon HB, Diaz H, Salehi P, Churchill T & Madsen KL 2005 5-Aminoimidazole-4-carboxamide riboside (AICAR) enhances GLUT2-dependent jejunal glucose transport: a possible role for AMPK. Biochemical Journal 385 485–491.[CrossRef][Web of Science][Medline]
Yakata K, Hiroaki Y, Ishibashi K, Sohara E, Sasaki S, Mitsuoka K & Fujiyoshi Y 2007 Aquaporin-11 containing a divergent NPA motif has normal water channel activity. Biochimica et Biophysica Acta 1768 688–693.
Yang B & Verkman AS 1998 Urea transporter UT3 functions as an efficient water channel. Direct evidence for a common water/urea pathway. Journal of Biological Chemistry 273 9369–9372.
Yang B & Verkman AS 2002 Analysis of double knockout mice lacking aquaporin-1 and urea transporter UT-B. Evidence for UT-B-facilitated water transport in erythrocytes. Journal of Biological Chemistry 277 36782–36786.
Yang B, Kim JK & Verkman AS 2006 Comparative efficacy of HgCl2 with candidate aquaporin-1 inhibitors DMSO, gold, TEA+ and acetazolamide. FEBS Letters 580 6679–6684.[CrossRef][Web of Science][Medline]
Yeung CH, Sonnenberg-Riethmacher E & Cooper TG 1999 Infertile spermatozoa of c-ros tyrosine kinase receptor knockout mice show flagellar angulation and maturational defects in cell volume regulatory mechanisms. Biology of Reproduction 61 1062–1069.
Yeung CH, Wagenfeld A, Nieschlag E & Cooper TG 2000 The cause of infertility of male c-ros tyrosine kinase receptor knockout mice. Biology of Reproduction 63 612–618.
Yeung CH, Barfield JP & Cooper TG 2005 The role of anion channels and Ca2+ in addition to K+ channels in the physiological volume regulation of murine spermatozoa. Molecular Reproduction and Development 71 368–379.[CrossRef][Web of Science][Medline]
Yeung CH, Barfield JP & Cooper TG 2006 Physiological volume regulation by spermatozoa. Molecular and Cellular Endocrinology 250 98–105.[CrossRef][Web of Science][Medline]
Zeuthen T, Meinild AK, Loo DD, Wright EM & Klaerke DA 2001 Isotonic transport by the Na+-glucose cotransporter SGLT1 from humans and rabbit. Journal of Physiology 531 631–644.
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
, between test and quinine treated at the same time point; P<0.05. At least 5000 spermatozoa were registered at each time point from each of eight epididymides. Spermatozoa from the same mice were used for all treatments.
