When unfertilized Xenopus eggs were treated by Cynops sperm extract in 10% Steinberg's solution (SB), egg's membranes hyperpolarized to about −37 mV and then depolarized to elicit a positive-going potential amounting to about 34 mV. The eggs underwent cortical contraction and resumption of meiosis. Activation of eggs in various external solutions indicates that the hyperpolarization is due mainly to opening of Na channels, but the positive-going potential is due to Cl channels on the egg's plasma membranes. Since the activation was inhibited by CdCl2, CoCl2, or NiCl2 as well as by amiloride, Ca influx through Ca channels is necessary for the activation by the sperm extract. A propagative intracellular Ca release was induced not only by Cynops sperm, but also by their sperm extract. Injection of BAPTA or heparin into the eggs completely inhibited activation, indicating that egg activation requires an intracellular Ca release dependent upon receptors for inositol 1,4,5-trisphosphate.
INTRODUCTION
The sperm induces egg activation to initiate embryonic development at fertilization. The mechanism how the initiation of egg activation is regulated remained unclear. In the invertebrate Urechis, the egg activation, including elicitation of a positive ferilization potential, can be induced by a protein isolated from the sperm acrosome [6–8]. In sea urchin eggs, a transmembrane glycoprotein on egg plasma membrane was characterized as a receptor for sperm-binding [5] and treatment with antiserum against a fragment of the receptor induces egg activation [4]. Recently, we have demonstrated that Xenopus eggs can be activated by the extract of Cynops sperm and its active component is a protease localized in the sperm acrosome [10].
Xenopus sperm triggers a transient, propagative increase in intracellular Ca2+ [1, 17] which is an indispensable signal for egg activation [2, 11]. In Xenopus eggs, the sperm initiates hydrolysis of phosphatidyl inositol 4,5-bisphosphate (PIP2) to produce inositol 1,4,5-trisphosphate (IP3), which is necessary for generation of the wave of Ca2+ at fertilization [17, 20]. The stimulation of exogenously introduced receptors can activate Xenopus eggs via coupling with G-protein [11], but it has not yet been determined the mechanism how the sperm triggers the production of IP3 to generate the intracellular increase of Ca2+. We have demonstrated that the voltage dependence is sensitive to extracellular Ca2+ activity in the activation of Xenopus egg by Cynops sperm or by their extract [10].
In order to understand the mechanism of egg activation that operates at the initial phase of amphibian fertilization, we attempted to clarify how the extract of Cynops sperm causes the egg activation in Xenopus, in particular, for role of both extra- and intra-cellular Ca2+ activities. We have demonstrated in this study that Ca influx through Ca channels on the egg plasma membrane induces a local increase in Ca2+ to cause the propagative Ca2+ wave in egg cytoplasm.
MATERIALS AND METHODS
Chemicals and solutions
De Boer's solution (DB) whose final composition in mM was, 110 NaCl, 1.3 KCl, 1.3 CaCl2, 5.7 Tris-HCl (pH 7.4); Steinberg's solution (SB), 58 NaCl, 0.67 KCl, 0.34 Ca(NO3)2, 0.85 MgSO4, and 4.6 Tris-HCl (pH 7.4); 3×NKP solution, 120 NaCl, 7.5 KCl, 4 NaH2PO4, 6 Na2HPO4 (pH 7.2); Ca-free phosphate buffer (Ca-free PB), 1 EGTA, 50 Na2HPO4, 50 NaH2PO4, 5 KCl (pH 7.0); Cacontaining phosphate buffer (Ca-PB), 1 CaCl2 50 Na2HPO4, 50 NaH2PO4, 5 KCl (pH 7.0).
Gametes
Sexually mature newts, Cynops pyrrhogaster, were collected near Yamaguchi, Japan. The clawed frogs, Xenopus laevis, were purchased from dealers and maintained in our laboratory. To obtain mature Xenopus eggs, females were injected with 500 IU of human chorionic gonadotropin (HCG; Teikoku Zoki, Tokyo) in the dorsal lymph sac and were kept at 18°C for 12 hr. Ovulation in Cynops was induced by two injections of 100 IU each of HCG at intervals of 48 hr at 23°C. Mature eggs were obtained from the lowest portion of oviducts by squeezing females. Jelly coats of Xenopus eggs were removed by immersion in 2% cysteine-HCl (pH 7.8), which was followed by thorough washing with 100 mM NaCl and 50 mM Tris-HCl (pH 7.0). The dejellied eggs were kept in DB at 18°C and used within 2 hr. The sperm of Cynops were obtained from sperm ducts by squeezing males or by dissection. In Xenopus, the sperm were obtained by mincing a piece of testis.
Artificial insemination and microinjection
For insemination of fully jellied Xenopus eggs, some drops of the sperm suspension in 50% SB or in appropriate solutions were placed on a petri dish. Unfertilized eggs were then directly dropped after squeezing the females. About 15 min after insemination, sufficient amount of 10% SB was added and incubated at 18°C. To avoid artificial activation of Xenopus eggs at the time of insertion of a micropipet for microinjection, the dejellied eggs were placed in Ca-free PB containing 4% polyvinylpyrrolidinone (PVP) and injected with a glass micropipet with a tip diameter of 20–30 μm. The injected eggs were incubated in Ca-PB for several minutes, and then stored in 3 × NKP containing 4% PVP until use.
Preparation of sperm extract
Sperm extracts were prepared according to the method described previously [10]. The sperm of Cynops were collected from sperm ducts and suspended in 10% SB at a concentration of about 5×106 cells/ml. After rapid freezing at −80°C, the thawed suspension of sperm was centrifuged at 10,000×g for 20 min at 2°C. The supernatant was again centrifuged at 100,000×g for 1 hr at 2°C. The supernatant was collected as the sperm extract and stored at − 80°C. One unit of the activity was for convenience defined as the amount of activity in 1 μl of the sperm extract. In some cases, the extract was desalted by a PD-10 column ("Pharmacia"), and then concentrated by lyophilization.
Electrical recordings
To record a fertilization potential or an activation potential, one electrode (10–20 M Ω with 3 M KCl) was inserted into the animal hemisphere of an egg, by increasing the capacitance compensation to produce oscillation. Recordings were made with a microelectrode amplifier (MEZ-7101 or MEZ-8301; Nihonkohden), a digital storageoscilloscope (DS-6612; Iwatsu), a voltage clamp amplifier (CEZ1100; Nihonkohden), and a chart recorder (WR-3701; Graphtec). Currents were measured with a converter between ground and an Ag-AgCl reference electrode, which was connected to the bath via an agar bridge. All the experiments were carried out at 18–23°C.
Activation of Xenopus eggs can be detected in the live egg by movement of pigments, cortical contraction, and formation of fertilization coat. Sections of Xenopus eggs were examined in order to confirm breakdown of cortical granules, as well as emission of the second polar body. Eggs were fixed in Smith's solution, and embedded in paraffin. The 10-μm-thick serial sections were stained with Feulgen's reaction and fast green for observation of nuclei or by the PAS reaction for observation of cortical granules.
Measurements for intracellular Ca ions
Measurements of activities of intracellular Ca2+ in Xenopus eggs were performed by the methods described previously [13]. The dejellied Xenopus eggs were placed in 100% SB, and their vitelline coats were removed by fine watchmarker's forceps. Aequorin used in the present study was a gift from Dr. Osamu Shimomura (MBL, Woods Hole). Aequorin was dissolved at a concentration of 10 mg/ml in water containing 100 μM EGTA and 10 mM Pipes at pH 7.0. The denuded eggs were immersed in 0.05 M phosphate buffer (pH7.0) for 10 min, and then 25–50 nl of the aequorin solution was injected. Final concentration of aequorin and EGTA was approximately 0.2–0.4 mg/ml and 2–4 μM, respectively. About 10 min after injection, the eggs were transferred to 100% SB. An image of the luminescence emitted from aequorin in the presence of Ca2+ was obtained by a two-dimensional photon-counting system (ARGUS100/VIM, Hamamatu Photonics). Technical details were reported previously [22, 23].
RESULTS
Ion channels which opened at activation of Xenopus eggs by Cynops sperm extract
When unfertilized Xenopus eggs were treated by Cynops sperm extract (1 unit/μl; 20 μl) in 10% SB ([Na+]o = 5.8 mM, [K+]o = 0.067 mM, [Cl]o = 6.3 mM), the egg underwent hyperpolarization to about −37 mV 2–3 min after treatment (Fig. 1A; Table 1). The egg membrane then deporlarized to reach a positive potential of about +38 mV 3–4 min after appearance of hyperpolarization. The egg underwent cortical contraction 2–3 min after eliciting the positive potential. The egg activation was confirmed by resumption of meiosis to form egg pronuclei (Fig. 2A) and by discharge of cortical granules (Fig. 2B). These potential changes were quite similar to those induced by Cynops sperm [9]. When the eggs were treated in 10% SB containing 52.2 mM NaCl to increase [Na+]o to 10-fold ([Na+]o = 5.8 mM, [K+]o = 0.067 mM, [Cl−]o = 58.5 mM), not only the amount of hyperpolarization, but the amount of positive potential (depolarization) decreased (Fig. 1B; Table 1). All the eggs underwent activation to show cortical contraction. In 10% SB containing 56.9 mM choline chloride to increase [Cl]o to 10-fold ([Na+]o] = 5.8 mM, [K+]o] = 0.067 mM, [Cl−]o = 63.2 mM), the amount of depolarization was reduced to −11 mV, but the hyperpolarization phase was almost unaffected (Fig. 1C; Table 1). Furthermore, an increase of [K+]o up to 6.7 mM did not affect the potential changes by the sperm extract at all (Table 1). These results indicate that the hyperpolarization is due to opening of Na channels, but the succeeding depolarization (the positive potential) is due to opening of Cl channels on egg plasma membrane, which is well consistent with the results obtained at cross-fertilization of Xenopus eggs by Cynops sperm [9].
Table 1
Electrical responses of Xenopus eggs to Cynops sperm extract under various conditions of external ions
Inhibition of egg activation by the sperm extract in the presence of Ca channel blockers
Since activation of Xenopus eggs by Cynops sperm extract did not occur in very low concentration of extracellular Ca2+; [Ca2+]o = 1.5 μM [10], it is worth to determine whether or not entry of extracellular Ca2+ through Ca channels is necessary for activation by the sperm extract. Unfertilized Xenopus eggs were treated by the sperm extract in various concentrations of CdCl2, CoCl2, or NiCl2 in 10% SB (Table 2). Egg activation was not affected in 0.1 μM CdCl2 at all. In 75% of eggs treated by the sperm extract in 0.5 μM CdCl2, small positive-going potentials were elicited (Fig. 3A; Table 2), but no cortical contraction was observed. Their egg nuclei stayed at the second meiotic metaphase (Fig. 2C) and their cortical granules remained intact (Fig. 2D). Finally, no positive-going potential was detected in the eggs treated in 1 μM CdCl2 (Fig. 3B). The hyperpolarization was, however, not affected at all. The egg activation was also inhibited either by 1 mM CoCl2 or by 5 mM NiCl2 (Table 2).
Table 2
Electrical responses of Xenopus eggs to Cynops sperm extract under various conditions of external ions
Unfertilized Xenopus eggs were treated by the sperm extract in various concentrations of amiloride which inhibits Ca channels as well as Na/Ca exchanger. The eggs elicited the positive-going potential and underwent cortical contraction in 0.5–1.0 mM amiloride, but appearance of positivegoing potential was delayed. In 2 mM amiloride, the egg activation was completely inhibited, so that neither a positivegoing potential nor cortical contraction was induced (Fig. 3C). When unfertilized eggs were treated by the sperm extract in various concentrations of verapamil; a Ca channel blocker, the egg activation was not inhibited, but the amount of positive-going potential significantly decreased when treated in 1 mM verapamil (Fig. 3D). These results suggest that an influx of Ca2+ through Ca channels on egg plasma membrane is involved in activation of Xenopus eggs by Cynops sperm extrat.
Propagative intracellular Ca2+ release during activation of Xenopus eggs by Cynops sperm extract
To determine whether or not activation of unfertilized Xenopus eggs is induced when the sperm extract is applied to a small area, about 2 μl of cocentrated sperm extract (10 units/μl) was applied to about 0.02 mm2 of egg surface with a small glass pipet. The eggs elicited a potential change which is quite similar to that induced by a large amount of extract (1 unit/μl; 20 μl) (Fig. 5A). All the eggs underwent activation, so that cortical contraction began at the site of extract treatment, suggesting propagation of activation stimuli, for example intracellular Ca release induced by the extract treatment.
To monitor potential changes concomitant with intracellular Ca2+ activities during cross-fertilization or egg activation, unfertilized Xenopus egg was injected with aequorin. The egg was inseminated with about 10 μl of Cynops sperm suspension (about 105 sperm/ml) in 50% SB (Fig. 4A). The luminescence for intracellular Ca2+ release was initiated at the site of an animal hemisphere and spread over the whole hemisphere. The luminescence was finally progressed to the vegetal hemisphere about 3 min after appearance of luminescence. The egg underwent a hyperpolarization followed by a positive-going potential (Fig. 4C). The luminescence was observed just after eliciting the positive-going potential. The amount of potential changes was small due to high [Na+]o and [Cl−]o in 50% SB. Thus, the pattern of propagative intracellular Ca release induced by Cynops sperm is quite similar to that induced by pricking [13].
When aequorin-injected Xenopus egg was locally treated by a small amount (1–5 μl) of concentrated sperm extract (10 units/μl) during recording the egg membrane potential in 50% SB (Fig. 4B), the egg underwent a hyperpolarization followed by a positive-going potential (Fig. 4D). The weak luminescence for intracellular Ca2+ release was detected at a site of an animal hemisphere after the peak of positive-going potential and spread over the whole egg surface. These results demonstrate that not only the sperm but also their extract induced the propagative intracellular Ca2+ release and that Ca2+ release occurs at eliciting a positive-going potential, but not during a hyperpolarization phase.
IP3-receptor dependent intracellular Ca2+ release is necessary for activation by the sperm extract
To determine whether or not the intracellular Ca2+ release is necessary for activation of Xenopus eggs by the sperm extract, unfertilized eggs were injected with BAPTA whose final concentration in cytoplasm was 2.5 mM. About 20 min after injection, the eggs were treated by the sperm extract (Fig. 5B; Table 3). The eggs underwent hyperpolarization from about −8 mV to about −38 mV, but neither a positive-going potential nor cortical contraction was observed. Egg activation was completely inhibited by BAPTA-injection because their cortical granules remained intact and their egg nuclei stayed at the second meiotic metaphase. The injection of distilled water did not affect egg activation at all.
Table 3
Electrical responses of Xenopus eggs which had been injected with BAPTA or heparin, to Cynops sperm extract in 10% SB
To know a role of inositol 1,4,5-trisphosphate (IP3) receptors in egg activation process, unfertilized eggs were injected with heparin in various concentrations (Figs. 5C and D; Table 3). The injection of heparin whose final concentration in egg cytoplasm was 75 μM did not affect egg activation by the sperm extract. When the eggs were injected with higher concentration of heparin (150 μM), the amount of hyperpolarization was not changed, but that of a positive-going potential was decreased (Fig. 5C). The injection of heparin whose final concentration was 300 μM completely inhibited egg activation by the sperm extract, so that a hyperpolarization was detected (Fig. 5D). The egg nuclei at the second meiotic metaphase and intact cortical granules were confirmed by cytological sections. Furthermore, unfertilized eggs injected with 0.5 μM thapsigargin, an inhibitor for Ca-ATPase, underwent activation by the treatment of a small amount (2 μl) of sperm extract (Table 3). These results suggest that the Ca2+ release dependent upon IP3 receptors in intracellular Ca2+ store is necessary for egg activation by the sperm extract, in particular eliciting the positive-going potential and undergoing cortical reactions, but the preceding hyperpolarization is independent of intracellular Ca2+ activity.
DISCUSSION
We showed in this study that the hyperpolarization is due to the opening of Na channels, and the succeeding depolarization (a positive-going potential) is due to the opening of Cl channels on the egg plasma membrane during the activation of Xenopus eggs by Cynops sperm extract. Properties of these potential changes are quite similar to those in crossfertilization of Xenopus eggs with Cynops sperm [9]. These potential changes are probably caused by a sperm protease localized in an acrosomal region [10]. When a protease activity in the sperm extract was abolished by protease inhibitors or by competitive substrates, not only the positivegoing potential, but also the hyperpolarization was inhibited [10]. In contrast, we observed in this study that inhibition of Ca channels does not affect the hyperpolarization phase. Furthermore, an increase in intracellular Ca2+ occurs after eliciting the positive-going potential. Thus, Ca2+ influx through Ca channels seems to be necessary for elevation of intracellular Ca2+ level, rather than for the initial interactions between the sperm protease and their putative receptors on egg plasma membrane.
The opening of Cl channels to produce a fertilization potential is dependent upon intracellular Ca2+ activity at normal fertilization in Xenopus [11, 12], but the opening of Na channels has not yet been determined. However, it has been recently reported that an ATP-activated Na+ channels is involved in sperm-induced fertilization [15]. Furthermore, treatment of Xenopus oocytes with trypsin induces Ca2+-activated Cl− currents [3]. These results suggest that a sperm protease of Xenopus which is similar to that of Cynops sperm is involved in activation of normal fertilization in Xenopus.
The propagative intracellular Ca2+ release induced by the sperm extract is quite similar to that induced by Xenopus sperm [17] or by pricking [13]. The requirement of an intracellular Ca release dependent upon inositol 1,4,5trisphosphate (IP3) receptors is also well consistent with the results obtained in normal fertilization of Xenopus eggs [17]. Injection of IP3 into unfertilized eggs induces egg activation, whereas injection of heparin inhibits egg activation by sperm [20]. IP3 mass increases after fertilization of Xenopus eggs preinjected with BAPTA or heparin [20]. Furthermore, IP3 receptors are localized in cortical endoplasmic reticulum in Xenopus eggs [14]. These suggest that the sperm extract induces the propagative Ca release by producing IP3. The opening of Cl channels is probably caused by increase in intracellular Ca2+. However, the opening of Na channels seems to be independent of an increase in intracellular Ca2+, because the hyperpolarization was induced even after inhibition of intracellular Ca2+ activities by BAPTA or by heparin.
We found in this study that Ca influx through egg plasma membrane is indispensable for egg activation. Although amiloride is also known as an inhibitor for Na/Ca exchanger which causes Ca influx in low [Na+]o condition [18], CdCl2 inhibits Ca channels in less than 100 μM, but does not affect Na/Ca exchanger in cardiac muscles [19]. These results suggest that the opening of Ca channels rather than stimulation of Na/Ca exchanger causes Ca entry during egg activation.
Although the mechanism how the stimulation by sperm entry induces the intracellular Ca2+ release is still controversial between species, there are several possibilities [16]: (1) a sperm agonist binds to a receptor molecule on egg plasma membrane to produce IP3, which results in Ca2+ release from Ca2+ store in egg cytoplasm, (2) a sperm agonist induces Ca influx through egg plasma membrane to produce a local increase in intracellular Ca2+ level, which causes the propagative Ca2+ release, and (3) a substance from sperm is introduced through the connection between the sperm and the egg after their membrane fusion. Our results obtained here seems to support the possibility that the sperm opens Ca channels to increase Ca influx during egg activation. How does local increase in intracellular Ca2+ cause the Ca wave? The local increase in Ca2+ may stimulate phospholipase C to produce IP3 (IP3-induced Ca release, IICR), because heparin which is known as an inhibitor for IP3 receptors inhibited egg activation by the sperm extract. Alternatively, the local increase in Ca2+ may stimulate directly Ca store to release Ca2+ (Ca-induced Ca-release, CICR). In this case, Ca may stimulate IP3 receptors to induce Ca2+ release [17], rather than causes an overload of Ca stores to undergo Ca2+ release through Ca-ATPase, because thapsigargin which is known as an inhibitor for Ca-ATPase [21] did not inhibit egg activation by the sperm extract.
Acknowledgments
We thank Dr. Osamu Shimomura for kindly providing us with purified aequorin. This work was supported in part by a Grant-inAid for Scientific Research from Ministry of Education, Science and Culture, Japan to Y.I., and by the foundation of Kato Memorial Bioscience to Y. I.