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© The Rockefeller University Press,
0021-9525/2000//783 $5.00
The Journal of Cell Biology, Volume 149, Number 4,
, 2000 783-792
Brief Report |
Intracellular Ca2+ and Ca2+/Calmodulin-Dependent Kinase II Mediate Acute Potentiation of Neurotransmitter Release by Neurotrophin-3
lub{at}codon.nih.gov
Neurotrophins have been shown to acutely modulate synaptic transmission in a variety of systems, but the underlying signaling mechanisms remain unclear. Here we provide evidence for an unusual mechanism that mediates synaptic potentiation at the neuromuscular junction (NMJ) induced by neurotrophin-3 (NT3), using Xenopus nerve–muscle co-culture. Unlike brain-derived neurotrophic factor (BDNF), which requires Ca2+ influx for its acute effect, NT3 rapidly enhances spontaneous transmitter release at the developing NMJ even when Ca2+ influx is completely blocked, suggesting that the NT3 effect is independent of extracellular Ca2+. Depletion of intracellular Ca2+ stores, or blockade of inositol 1, 4, 5-trisphosphate (IP3) or ryanodine receptors, prevents the NT3-induced synaptic potentiation. Blockade of IP3 receptors can not prevent BDNF-induced potentiation, suggesting that BDNF and NT3 use different mechanisms to potentiate transmitter release. Inhibition of Ca2+/calmodulin-dependent kinase II (CaMKII) completely blocks the acute effect of NT3. Furthermore, the NT3-induced potentiation requires a continuous activation of CaMKII, because application of the CaMKII inhibitor KN62 reverses the previously established NT3 effect. Thus, NT3 potentiates neurotransmitter secretion by stimulating Ca2+ release from intracellular stores through IP3 and/or ryanodine receptors, leading to an activation of CaMKII.
Key Words: ryanodine receptors • inositol 1, 4, • 5-trisphosphate receptors • acetylcholine • neuromuscular junction • synaptic transmission
© 2000 The Rockefeller University Press
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Introduction |
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Due to the complexity of CNS synapses, the mechanisms underlying the synaptic actions of neurotrophins are difficult to study. The neuromuscular junction (NMJ) offers a simple and easily accessible model to study the role and the mechanisms of neurotrophins in synaptic development and function in great detail. Two modes of neurotrophic regulation have been identified using the Xenopus nerve–muscle co-cultures: acute potentiation of neurotransmitter release and long-term regulation of synapse maturation. In the long-term mode, the spontaneous synaptic currents (SSCs) and impulse–evoked synaptic currents exhibit more mature properties after a prolonged treatment with NT3, and to a lesser extent, with BDNF (Wang et al. 1995; Liou and Fu 1997; Liou et al. 1997). The neurotrophins induce an increase in the expression of synaptic vesicle proteins, and in the number of synaptic varicosities in the presynaptic site (Wang et al. 1995), as well as changes in the acetylcholine (ACh) receptors in the postsynaptic site (Wang and Poo 1997; Gonzalez et al. 1999). In the acute mode, application of BDNF or NT3 rapidly enhances synaptic transmission at the NMJ (Lohof et al. 1993). The acute effect of neurotrophins is due strictly to an enhancement of transmitter release probability in the presynaptic site (Lohof et al. 1993; Stoop and Poo 1995). The SSC frequency is markedly increased, whereas the quantal sizes are not affected. The expression of NT3, but not BDNF or NT4, in the postsynaptic muscle cells is activity-dependent (Xie et al. 1997). Further, the secretion of NT4 in muscle cells seems to be induced by repetitive stimulation of presynaptic neurons (Wang and Poo 1997). These results suggest that neurotrophins may serve as target-derived, retrograde messengers that acutely modulate transmitter release at the developing neuromuscular synapses (Xie et al. 1997).
A critical and yet unresolved question is: what are the intracellular signaling mechanisms that mediate such rapid synaptic effects of neurotrophins? In the hippocampus, BDNF-induced enhancement of high frequency transmission at CA1 synapses appears to be mediated through the activation of mitogen-associated protein kinase and phosphatidylinositol-3 kinase pathways, but not phospholipase C-
pathway (Gottschalk et al. 1999). The acute modulation of synaptic transmission by BDNF at NMJ appears to require Ca2+ influx into the presynaptic terminals, but signaling events downstream of Ca2+ influx are not known (Stoop and Poo 1996). Do neurotrophins share similar mechanisms in modulating synapses in the CNS and at the NMJ? Do BDNF and NT3 use the same signaling pathway to potentiate the neuromuscular synapses? In this report, we address the role of the nerve terminal Ca2+ in the acute regulation of neurotransmitter release at the NMJ by NT3. Specifically, we focus on the intracellular Ca2+ stores and the presynaptic Ca2+/calmodulin-dependent kinase II (CaMKII). A number of recent studies have suggested the involvement of intracellular Ca2+ stores in synaptic transmission (for review see Berridge 1998). Although extensive studies have revealed diverse effects of CaMKII in postsynaptic functions (Chapman et al. 1995), the only clearly defined presynaptic effects of CaMKII is to regulate the availability of readily releasable synaptic vesicles at the nerve terminals (Llinas et al. 1985; Greengard et al. 1993). We have now provided evidence that the acute potentiation of transmitter release by NT3 depends on a rise of Ca2+ concentrations ([Ca2+]i) in the presynaptic terminals. Surprisingly, the increase in [Ca2+]i was due to Ca2+ released from intracellular stores, but not to Ca2+ influx from extracellular sources. Furthermore, the continuous activation of CaMKII, which is triggered by the increase in [Ca2+]i, appears to be required for the effect of NT3. These results may help understand how neurotrophins acutely modulate neurotransmitter release.
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Materials and Methods |
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12.5 µM. 1 d after injection, the neural tube and the associated myotomal tissues were dissected and used to prepare nerve–muscle cultures. Cells containing CaMKII-pep were identified by rhodamine fluorescence.
Culture Preparation
Xenopus nerve–muscle cultures were prepared according to the procedure described previously (Lu et al. 1992). In brief, the neural tube and the associated myotomal tissue of Xenopus embryos at stage 20 to 22 were dissociated in Ca2+-Mg2+–free saline supplemented with EDTA (58.2 mM NaCl, 0.7 mM KCl, 0.3 mM EDTA, pH 7.4) for 15–20 min. The cells were grown on glass coverslips for 24 h at room temperature (20–22°C). The culture medium consisted (vol/vol) of 50% Leibovitz L-15 medium (Sigma), 1% FCS (Life Technologies), and 49% Ringer's solution (115 mM NaCl, 2 mM CaCl2, 2.5 mM KCl, 10 mM Hepes, pH 7.6). NT3 (2–5 x 10–9 M; kindly provided by Regeneron Pharmaceuticals, Inc.) and various inhibitors were applied directly to the culture media at the time of recording.
Electrophysiology
Synaptic currents were recorded at room temperature in culture medium from myocytes innervated by spinal motoneurons using whole cell, voltage-clamp recording techniques (Lu et al. 1992). The solution inside the recording pipette contained: 150 mM KCl, 1 mM NaCl, 1 mM MgCl2, and 10 mM Hepes buffer, pH 7.2. Membrane currents in all recordings were monitored by a patch clamp amplifier (EPC-7), with a current signal filter at 3 kHz. The membrane potentials of the muscle cells were generally in the range of –55––75 mV and were voltage clamped at –70 mV after measuring the membrane potentials. For experiments performed in the absence of external Ca2+, the culture medium was replaced with a Ca2+-free extracellular solution containing 115 mM NaCl, 2 mM MgCl2, 10 mM Hepes, 3 mM EGTA, and 0.1% BSA. All data were stored on a videotape recorder for later playback on a storage oscilloscope (Tektronix TDS 420) and a chart recorder (Gould EasyGraf 240), or analysis using the SCAN program. To quantitatively measure the changes in neurotransmitter release, a time course of SSC frequency was first constructed on a minute-to-minute basis. The SSC frequencies in a 10-min period right before drug application were averaged as control. The changes in SSC frequency were measured by averaging a 10-min period recording starting from the highest number after drug application.
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Results |
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We then tested whether BDNF, which requires Ca2+ influx to enhance transmitter release (Stoop and Poo 1996), also depends on Ca2+ release from intracellular stores. Application of BDNF (50 ng/ml) elicited a fivefold increase in SSC frequency in normal Ca2+-containing medium (Fig. 3 D). In cultures pretreated with XeC (1 µM) to block IP3 receptors, BDNF elicited the same magnitude of synaptic potentiation (Fig. 3 D), suggesting that the Ca2+ release from intracellular stores is not required for BDNF-induced synaptic potentiation. Thus, BDNF and NT3, two proteins from the same neurotrophin family, can both potentiate neurotransmitter release, but they use totally different intracellular mechanisms.
The Effect of NT3 Requires Continuous Activation of CaMKII
The release of Ca2+ from intracellular Ca2+ stores induced by NT3 may trigger the activation of the presynaptic CaMKII. CaMKII has been shown to enhance transmitter release in adult squid giant synapses and mammalian brain synaptosomes, presumably due to an increase in the availability of readily releasable synaptic vesicles at the nerve terminals (Llinas et al. 1985; Nichols et al. 1990). We first tested whether CaMKII is involved in modulating transmitter release at the developing NMJ in the Xenopus culture system using KN62, a frequently used inhibitor for CaMKII (Tokumitsu et al. 1990). We found that bath application of KN62 (3 µM) rapidly and reversibly reduced the amplitude of evoked synaptic currents. The average evoked synaptic current amplitudes before and 10 min after KN62 application were 1.77 + 0.36 nA and 1.01 + 0.24 nA, respectively (n = 8, P < 0.01, t test). In contrast, application of KN62 had little effect on the spontaneous release of neurotransmitters (Fig. 4A and Fig. B). These results are consistent with the idea that CaMKII may regulate transmitter release when the terminal [Ca2+]i is elevated, but may not be very effective at the quiescent level of [Ca2+]i. Since NT3 acts presynaptically at the NMJ and CaMKII is capable of regulating transmitter release, we determined whether CaMKII is involved in the synaptic action of NT3 at the developing NMJ. Pretreatment of the nerve–muscle cultures with KN62 completely prevented the increase of SSC frequency elicited by NT3 (Fig. 4). The average SSC frequencies before and 10 min after KN62 remained unchanged (before KN62; 5.9 ± 0.6 events/min; after KN62, 5.6 ± 0.6 events/min; n = 8, P > 0.1). These results suggest that CaMKII is necessary for the NT3 regulation of neurotransmitter release.
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Does the NT3-induced potentiation require a continuous activation of CaMKII? To address this question, we applied KN62 after synaptic transmission was potentiated by NT3. Fig. 6 A shows that within 20–30 min after NT3 application, the increase in SSC frequency reached the peak. Application of KN62 at the peak gradually suppressed the SSC frequency. Quantitative analysis indicated that KN62 virtually reversed the NT3 effect (Fig. 6 B). Thus, continuous activity of CaMKII appears to be necessary for NT3 modulation of transmitter release at the developing neuromuscular synapses.
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Discussion |
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In addition to extracellular Ca2+, the release of Ca2+ from intracellular stores could either modulate or contribute directly to transmitter release (Berridge 1998). Signals that result in the opening of either IP3 receptors or ryanodine receptors can generate local increases in [Ca2+]i, which in turn participates in the exocytotic process. Although still a fairly new concept, transmitter release triggered or modulated by the release of Ca2+ from intracellular stores has been shown in a number of systems such as the cholinergic synapse in Aplysia, reticulospinal synapse in lamprey, and sympathetic nerve terminals (Smith and Cunnane 1996; Cochilla and Alford 1998; Mothet et al. 1998). An important question then is whether neurotrophins, which are capable of eliciting an IP3 signal through the activation of phospholipase- pathway (Segal and Greenberg 1996), can serve as endogenous neuromodulators to regulate synaptic transmission under physiological conditions. In this study, we have provided strong evidence that NT3 potentiates transmitter release by stimulating Ca2+ release from intracellular stores. We have shown that NT3 increased transmitter release in Ca2+-free or Cd2+-containing medium, and that pretreatment with thapsigargin prevented the NT3 effect. Moreover, inhibition of IP3 receptors blocked the NT3 effect. Thus, NT3 induces the release of Ca2+ through IP3 receptors at the terminals of developing spinal neurons, leading to an increase in spontaneous transmitter secretion. It is conceivable that similar mechanisms are used for NT3 to enhance evoked synaptic transmission, although we could not test this possibility because most of our experiments have to be done in Ca2+-free medium. Consistent with our results, neurotrophins have been shown to induce an increase in [Ca2+]i in hippocampal neurons (Berninger and Garcia 1993; Marsh and Palfrey 1996), possibly by enhancing the release of Ca2+ from intracellular stores (Sakai et al. 1997; Li et al. 1998). The release of Ca2+ from IP3 receptors could further trigger Ca2+-induced Ca2+ release from ryanodine receptors (Berridge 1998). We found that the acute modulation of transmitter release by NT3 was blocked by the ryanodine receptor antagonist TMB-8 or a high concentration of ryanodine (100 µM). However, activation of the ryanodine receptor alone by low concentrations of ryanodine (2.5–5 µM) was not sufficient to enhance transmitter release, and application of NT3 on top of that still increased SSC frequency. Thus, both IP3 receptors and ryanodine receptors are involved in the acute effect of NT3, but the primary effect of NT3 is probably on the IP3 receptors. Although the electrophysiological analysis clearly indicates that NT3 potentiates neurotransmitter release through presynaptic mechanisms, our pharmacological experiments can not formally establish that NT3 acts on presynaptic terminals directly. We can not rule out the possibility that NT3 initially acts on postsynaptic muscle cells to trigger the release of Ca2+ from intracellular stores, leading to the secretion of some retrograde signal to activate presynaptic CaMKII.
Although our results suggest a role of Ca2+ release from internal stores in NT3-induced synaptic potentiation, a previous study has shown that the acute potentiation by BDNF in the same preparation requires external Ca2+ (Stoop and Poo 1996). BDNF binds and interacts almost exclusively with the TrkB receptor, whereas NT3 binds primarily to the TrkC receptor (Kaplan and Stephens 1994). It is possible that the activation of TrkB triggers Ca2+ influx, whereas that of TrkC is coupled to internal Ca2+ stores in the developing spinal neurons. Indeed, we found that inhibition of Ca2+ release from internal stores can not block the BDNF-induced synaptic potentiation. Similarly, both BDNF and NT3 attract growth cone turning in these developing spinal neurons, but the intracellular mechanisms that mediate the turning responses to the two factors are completely different (Song et al. 1998). The BDNF effect requires Ca2+ influx into the terminals and elevation of [cAMP]i, whereas the NT3 effect is independent of extracellular Ca2+. In this study, we show that the activation of IP3 receptors is required for the synaptic effect of NT3, but not for that of BDNF. Thus, although both enhance synaptic transmission at developing neuromuscular synapses, the two factors may require Ca2+ from difference sources, one extracellular and one intracellular.
The potentiation of transmitter release usually occurs at least 5–10 min after NT3 application (Fig. 1, Fig. 2, and Fig. 6; see also Lohof et al. 1993; Xie et al. 1997). This time course implies that NT3-induced Ca2+ release modulates the transmitter release mechanisms, rather than contributing directly to the triggering of the exocytosis process. The NT3 modulation is known to be presynaptic in nature (Lohof et al. 1993). What are the presynaptic targets downstream of Ca2+ release induced by NT3? CaMKII may serve as an excellent candidate, because its role in transmitter release is relatively well-defined (Llinas et al. 1985; Lin et al. 1990; Nichols et al. 1990; Stanton and Gage 1996; Jin et al. 1998; for review see Greengard et al. 1993). Extensive studies indicate that the activation of CaMKII is triggered by Ca2+ influx through extracellular sources. An important finding in this study is that CaMKII can also be activated by Ca2+ released from internal stores through IP3 and ryanodine receptors. We showed that even in the complete absence of Ca2+ influx, the NT3-induced potentiation of transmitter release can be blocked by the CaMKII inhibitors CaMKII-pep or KN62. Furthermore, we found that KN62 can reverse established synaptic potentiation after NT3 application in Ca2+-free medium. These results not only provide a link between internal Ca2+ stores and CaMKII activation, but also point to CaMKII as a downstream signaling mediator for NT3-induced synaptic potentiation. Since it is difficult to test whether the activation of CaMKII alone is sufficient to mimic the NT3 effect, we can not rule out the possible involvement of other processes that may also contribute to the NT3-induced synaptic potentiation.
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Acknowledgments |
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Submitted: 16 February 2000
Revised: 11 April 2000
Accepted: 11 April 2000
Z.-P. Xie's current address is Department of Biology, Tsinghua University, Beijing, China.
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