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-subunits
MS 10807 Received 6 March 2000; accepted after revision 13 June 2000.
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ABSTRACT |
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 TopAbstract IntroductionMethodsResultsDiscussionReferences |
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-subunit modulation of slow inactivation of class A calcium (Ca2+) channels was studied with two-microlectrode voltage clamp after expression of the 
1A- (BI-2) together with 1a-, 2a-, 3- or 4-subunits in Xenopus oocytes.
1A/-subunit composition inducing the slower rate of fast inactivation displayed the faster rate of slow inactivation. The corresponding order of slow inactivation time constants (
onset) was: 1A/2a, 33 ± 3 s; 1A/4, 42 ± 4 s; 1A/1a, 59 ± 4 s; 1A/3, 67 ± 5 s (n 
7).
-subunits.
1A/IF-AA/3) in a similar manner as coexpression of the 2a-subunit. Recovery from slow inactivation was slightly slowed in the double mutant.
-subunits.
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INTRODUCTION |
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TopAbstractIntroductionMethodsResultsDiscussionReferences |
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Ca2+ entry through voltage-gated Ca2+ channels modulates a variety of neuronal functions such as: release of neurotransmitters, generation and propagation of action potentials and gene expression. Nine classes of voltage-gated Ca2+ channels that are coded by at least nine different genes (classes A, B, C, D, E, F, G, H, I) have been identified in neuronal cells (Birnbaumer et al. 1994; Perez-Reyes et al. 1999; Lee et al. 1999).
A hallmark of class A Ca2+ channels is their sensitivity to the funnel web spider venom 
-Aga-IVA (Mintz et al. 1992b). This channel type is widely distributed in the central and peripheral nervous system (Mintz et al. 1992a, b; Stea et al. 1994; Westenbroek et al. 1995) and there is evidence that Ca2+ entry through the 1A-subunit mediates the release of neurotransmitters more efficiently than other neuronal Ca2+ channels (Wu et al. 1999).
Class A Ca2+ channels are hetero-oligomeric protein complexes consisting of a pore-forming 1A-subunit, at least one of four -subunits (1-4) and an 2
-subunit. The auxiliary -subunits modulate expression density as well as voltage dependence of channel activation and inactivation kinetics (Stea et al. 1994; Olcese et al. 1994; De Waard & Campbell, 1995). Multiple -subunits are associated with the 1A-subunit to different extents in different parts of the mammalian brain (Liu et al. 1996; Pichler et al. 1997) suggesting that class A Ca2+ channel properties are modulated by tissue-specific expression of different -subunits (Tanaka et al. 1995). Missense mutations in 1A are associated with the aetiology of familial hemiplegic migraine (Ophoff et al. 1996; Kraus et al. 1998; Hans et al. 1999), ataxia (Zhuchenko et al. 1997) and epilepsy (Fletcher et al. 1996). Ca2+ influx through class A channels and the sensitivities to the -agatoxin IVA are modulated by alternative splicing of the 1A-subunit (see splice variants 1A-a and 1A-b in Bourinet et al. 1999).
Class A Ca2+ channel currents decay under voltage clamp with a biexponential time course suggesting two mechanisms of inactivation. Fast inactivation (corresponding to the transient current decay) is affected by point mutations in different parts of the 1A-subunit (see Hering et al. 1998 for review; Bourinet et al. 1999). The additional slow inactivation is much less understood.
We have, therefore, expressed a neuronal 1A-subunit (BI-2, Mori et al. 1991) together with 1a-, 2a-, 3- or 4-subunits in Xenopus oocytes and analysed the individual effects of various -subunits on slow inactivation.
We report here that a reduction of fast inactivation by coexpression of 1A- with the 2a-subunit simultaneously accelerates the channel state transitions into the slow inactivated state. Alternatively, slowing fast inactivation of 1A/3 channels by mutating two inactivation determinants in segment IIIS6 to alanine (IF1612/1613AA) accelerated the onset of slow inactivation in a similar manner. Our data suggest that open class A Ca2+ channels are more willing to enter the slow inactivated state than channels in the fast inactivated conformation. The tissue-specific expression patterns of different -subunits appear, therefore, as an indirect determinant of slow inactivation in class A Ca2+ channels.
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METHODS |
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Generation of the 1A mutant
The class A Ca2+ channel mutant 1A/IF-AA was constructed by introducing two point mutations (I1612A and F1613A) into 1A cDNA (BI-2 accession number X57477, Mori et al. 1991) by the 'gene SOEing' technique (Horton et al. 1989). The point mutations were verified by sequence analysis. All constructs were inserted into the polyadenylating transcription plasmids pNKS2 (a kind gift of Dr O. Pongs, Zentrum für Neurale Signalverarbeitung, Hamburg, Germany).
Electrophysiology
In accordance with national guidelines, female Xenopus laevis (NASCO, USA) were anaesthetized by exposing them for 15 min to a 0·2 % MS-222 (methane sulfonate salt of 3-aminobenzoic acid ethyl ester; Sandoz) solution before surgically removing parts of the ovaries. The frogs were then allowed to recover and returned to their tank. Each frog was reused up to two times and subsequently killed by decapitation under anaesthesia. The interval between the operations was longer than 4 months. Follicle membranes from isolated oocytes were enzymatically digested with 2 mg ml-1 collagenase (Type 1A, Sigma). Preparation of stage V-VI oocytes from Xenopus laevis, synthesis of capped off run-off poly(A+) cRNA transcripts from linearized cDNA templates and injection of cRNA were performed as previously described in detail by Grabner et al. (1996).
Calcium channel currents (IBa) were studied 2-7 days after microinjection of approximately equimolar cRNA mixtures of 1A or 1A/IF-AA (0·3 ng (50 nl)-1) with 1a (2a, 3, 4) (0·1 ng (50 nl)-1) with two-microelectrode voltage clamp in Xenopus oocytes with 40 mM Ba2+ as charge carrier in a bath solution containing (mM): 40 Ba(OH)2, 40 N-methyl-D-glucamine, 10 Hepes, 10 glucose; adjusted to pH 7·4 with methanesulfonic acid as previously described (Grabner et al. 1996). Endogenous chloride currents of the oocytes were suppressed by injecting 20-40 nl of a 0·1 M BAPTA solution 30-240 min before the voltage clamp measurements. Voltage-recording and current-injecting microelectrodes were filled with 2·8 M CsCl, 0·2 M CsOH, 10 mM EGTA and 10 mM Hepes (pH 7·4) and had resistances of 0·3-2 M
. The maximum of the activation curve of all 1A/-subunit combinations studied was in the range of 10 ± 5 mV (n > 5). Only IBa with amplitudes in the range between 0·3 and 1·5 µA were included in the analysis.
Data analysis
Recovery of class A Ca2+ channels from inactivation is sufficiently well described by the equation:
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IN = 1 - Afast exp(-t/fast) - Aslowexp(-t/slow),
| (1) |
where IN represents the normalized current amplitude, t the recovery time, Afast the fraction of channels that are fast inactivated and Aslow the fraction of channels that are slow inactivated at the end of the inactivating prepulse. 1/fast gives the rate constant of recovery from the fast inactivated state and 1/slow the rate constant of recovery from the slow inactivated state (see Appendix for details).
The time constant of IBa recovery from fast inactivation (fast) was estimated by means of a conventional double pulse protocol (Fig. 1B, top panel) and the normalized peak current amplitudes were fitted to eqn (1). To enable complete recovery from fast and slow inactivated states we introduced a 1·5 min rest at a holding potential of -120 mV between the subsequently applied double pulses.
The onset of slow inactivation (onset) can be estimated by relating IS, the fraction of channels in the slow inactivated state at the end of a conditioning prepulse, to the prepulse duration (tpre):
IS  1 - const × exp(-tpre/onset)
| (2) |
(see Appendix for details), which on a logarithmic scale turns to:
-KStpre - C,
where KS = 1/onset, and C is a constant.
In the experiments described in Fig. 2, the fraction IS and the time constant of recovery from slow inactivation slow were estimated by fitting the time course of IBa recovery to:
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IN = 1 - ISexp (-t/slow),
| (3) |
where IN is the normalized current amplitude and t the recovery time.
The pCLAMP software package (version 6.0, Axon Instruments, Inc.) was used for data acquisition and preliminary analysis. Microcal Origin 5.0 was employed for analysis and curve fitting. Data are given as means ± S.E.M. Statistical significance was calculated according to Student's unpaired t test (P < 0·05).
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RESULTS |
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Estimation of slow inactivation in class A Ca2+ channels
To evaluate the effects of different -subunits on slow inactivation of class A Ca2+ channels we expressed the 1A-subunit together with 1a-, 2a-, 3- or 4-subunits in Xenopus oocytes for later voltage clamp experiments with the two-microelectrode technique. Negligible run-down during two-microelectrode voltage clamp makes this channel type particular suitable for long-lasting experiments as required for kinetic studies of slow inactivation.
As shown in Fig. 1A, each subunit combination produced Ca2+ channels with distinct kinetic phenotypes (see also Stea et al. 1994; De Waard & Campbell, 1995). Since slow inactivation in class A Ca2+ channels with different -subunit composition (except the 1A/2a channel) is masked by fast inactivation, this process is difficult to observe from the kinetics of IBa decay.
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-subunit composition
A, IBa through | ||
However, as illustrated in Fig. 1B, IBa of class A Ca2+ channels recovered from inactivation with a biexponential time course. The fraction of channels in the slow inactivated state can be estimated by extrapolating the slow recovery component to the end of the inactivating prepulse (Khodorov et al. 1976; see Appendix).
This approach facilitated the estimation of the on-rate of slow inactivation by means of a 'back-extrapolation technique' illustrated in Fig. 2. Conditioning pulses ranging from 3 to 30 s were applied from a holding potential of -80 mV to 10 mV and recovery from slow inactivation was observed at the same holding potential (-80 mV) during a series of short (60 ms) test pulses to 10 mV (Fig. 2A). A 5 s rest between the end of the inactivating prepulse and the first test pulse enabled complete recovery from fast inactivation (see Fig. 4C and Table 1 for corresponding time constants of recovery from fast inactivation). The recovery time constant from slow inactivation (slow) was estimated by fitting IBa recovery to a mono-exponential function. The fraction of Ca2+ channels in the slow inactivated state (IS, see eqn (3) in Data analysis) was subsequently calculated by extrapolating the exponential function to the end of the inactivating prepulse (Fig. 2A). A conventional double pulse protocol, where single test pulses were applied at various intervals after the conditioning pulse, yielded similar results ensuring that inactivation during the 60 ms test pulse train did not affect the time course of recovery from slow inactivation (data not shown).
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A, recovery from slow inactivation was observed at a holding potential of -80 mV during eight 60 ms test pulses to 10 mV applied 5, 10, 20, 30, 60, 90, 120 and 180 s after conditioning pulses of either 3, 7, 10, 20 or 30 s. Channels recovered completely from fast inactivation during the 5 s rest between the end of the conditioning pulse and the first test pulse (see Fig. 4C for | ||
As demonstrated in Fig. 2A, the fraction of channels in the slow inactivated state increased with the prolongation of the conditioning prepulse. On a logarithmic scale the time course of the onset of slow inactivation could be approximated by a linear function:
(Fig. 2B) with the slope KS = 1/onset representing the on-rate of slow inactivation, tpre the length of the inactivating prepulse, IS the fraction of channels in the slow inactivated state and C the y-intercept. The interpretation of the y-intercept is given in Discussion.
Slow inactivation of class A Ca2+ channels with different -subunit composition
The 'back-extrapolation' technique described above enabled the estimation of the on- and off-rates of slow inactivation in class A Ca2+ channels with different -subunit composition. In line with previous observations, the 3-subunit induced the fastest, 2a- the slowest and the 1a- and 4-subunits intermediate rates of fast inactivation (see also Stea et al. 1994; De Waard & Campbell, 1995; Fig. 1A). The reversed order was, however, observed for the kinetics of slow inactivation. During a test pulse to 10 mV 1A/2a channels entered the slow inactivated state at an about 2-fold higher rate than rapidly inactivating 1A/3 channels (Fig. 3A, see Fig. 3B for a comparison of the slow inactivation rates of all -subunit combinations).
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-subunit composition
A, slow inactivation was estimated by using conditioning pulses of different length (Fig. 2A). The rate constants were calculated as described in Fig. 2B. A comparison of IBa inactivation in | ||
Recovery of class A Ca2+ channels from the slow inactivated state was voltage dependent and occurred in all four 1/-subunit combinations at a significantly faster rate if the membrane was held at more negative voltages (Fig. 4D). However, at a given holding potential (-120, -80 or -60 mV) channels with different -subunit composition recovered from slow inactivation with similar kinetics.
Voltage dependence of recovery from fast inactivation in class A Ca2+ channels with different -subunit composition
IBa recovery from fast inactivation was examined by means of a conventional double pulse protocol (similar to Fig. 1B, top panel) over a period of 180 s at -120, -100, -80 and -60 mV. The holding potential was -120 mV in all experiments. As illustrated in Fig. 4A and B, recovery of rapidly inactivating channels (e.g. 1A/4) was dominated by recovery from fast inactivation whereas 1A/2a channels generally recovered at a slower rate and with an apparent smaller impact of fast inactivation. Coexpression of 1A with 2a did not totally prevent but substantially diminished the fast component of IBa inactivation. 1A/2a channels recovered with significantly slower kinetics from fast inactivation (e.g. at -60 mV: fast,1A/2a = 2·9 ± 0·3 s, n = 3 vs. fast,1A/1a = 1·3 ± 0·2 s, n = 4) suggesting a direct effect of the 2a-subunit on the 'fast inactivated' channel conformation.
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-subunit composition
A and B, IBa recovery from inactivation after 10 s conditioning pulses to 10 mV measured by a conventional double pulse protocol (similar to Fig. 1B, top panel). The recovery potentials were -120 mV ( | ||
The time constants of recovery from fast (fast) and slow (slow) inactivation of class A channels with different 1A/-subunit composition at different recovery potentials and corresponding amplitude coefficients are summarized in Fig. 4C and D, and Table 1. Recovery from both fast and slow inactivation was voltage dependent and occurred at a significantly faster rate at more negative voltages. Note that at -120 and -100 mV, where recovery from inactivation is complete, amplitude coefficients of fast and slow components in recovery represent the fractions of fast- and slow-inactivated channels at the end of the depolarizing pulse and are invariant of recovery voltage. However, at -80 and -60 mV normalized IBa did not recover to unity and amplitude coefficients of biexponential fit did not represent such fractions.
Table 1. Parameters of the biexponential fit to recovery from inactivation at various voltages
| Channel | Vh (mV) |
fast |
Afast (s) |
slow |
Aslow (s) |
Offset | n |
| 1A/1a |
-120 | 0·14 ± 0·01 | 0·81 ± 0·02 | 8·2 ± 0·7 | 0·18 ± 0·01 | 1·01 ± 0·01 | 4 |
| -100 | 0·24 ± 0·04 | 0·82 ± 0·03 | 16 ± 3 | 0·17 ± 0·03 | 0·99 ± 0·01 | 4 | |
| -80 | 0·32 ± 0·04 | 0·69 ± 0·03 | 21 ± 2 | 0·19 ± 0·02 | 0·95 ± 0·01 | 5 | |
| -60 | 1·3 ± 0·2 | 0·68 ± 0·02 | 45 ± 6 | 0·20 ± 0·01 | 0·87 ± 0·01 | 4 | |
| 1A/2a |
-120 | 0·7 ± 0·3 | 0·24 ± 0·03 | 16 ± 2 | 0·26 ± 0·02 | 1·00 ± 0·01 | 4 |
| -100 | 1·0 ± 0·4 | 0·21 ± 0·02 | 20 ± 3 | 0·29 ± 0·02 | 1·01 ± 0·01 | 4 | |
| -80 | 1·1 ± 0·3 | 0·23 ± 0·02 | 19 ± 3 | 0·25 ± 0·02 | 0·97 ± 0·01 | 5 | |
| -60 | 2·9 ± 0·3 | 0·19 ± 0·01 | 47 ± 9 | 0·21 ± 0·01 | 0·90 ± 0·01 | 3 | |
| 1A/3 |
-120 | 0·08 ± 0·01 | 0·86 ± 0·02 | 8 ± 1 | 0·12 ± 0·03 | 1·00 ± 0·01 | 5 |
| -100 | 0·20 ± 0·03 | 0·85 ± 0·04 | 10 ± 1 | 0·15 ± 0·03 | 1·01 ± 0·01 | 4 | |
| -80 | 0·5 ± 0·1 | 0·76 ± 0·06 | 19 ± 2 | 0·10 ± 0·01 | 0·93 ± 0·01 | 8 | |
| -60 | 1·1 ± 0·1 | 0·77 ± 0·02 | 35 ± 5 | 0·15 ± 0·01 | 0·69 ± 0·01 | 8 | |
| 1A/4 |
-120 | 0·12 ± 0·02 | 0·83 ± 0·02 | 14 ± 1 | 0·17 ± 0·01 | 1·01 ± 0·01 | 4 |
| -100 | 0·18 ± 0·02 | 0·83 ± 0·02 | 16 ± 2 | 0·16 ± 0·02 | 1·01 ± 0·01 | 4 | |
| -80 | 0·72 ± 0·13 | 0·64 ± 0·03 | 23 ± 5 | 0·19 ± 0·02 | 0·97 ± 0·01 | 4 | |
| -60 | 2·2 ± 0·2 | 0·57 ± 0·02 | 41 ± 11 | 0·12 ± 0·02 | 0·82 ± 0·01 | 4 |
Point mutations at the inner mouth of segment IIIS6 reduce fast inactivation and enhance the rate of slow inactivation
The data shown in Fig. 3 indicate that class A channels with 1A/-subunit composition inducing a slower rate of fast inactivation, enter the slow inactivated state at a significantly higher rate (KS: 1A/2a > 1A/4 > 1A/1a 1A/3). It was interesting to investigate if this correlation reflects a direct -subunit effect on the slow inactivated channel conformation or, instead, if the -subunit effect on slow inactivation is secondary to the changes in fast inactivation.
We have, therefore, constructed an 1A mutant with a slower rate of fast inactivation than wild-type by substituting two amino acids in IIIS6 of 1A by alanine (IF1612/1613AA, 1A numbering). Both amino acids at the inner mouth of segment IIIS6 have previously been shown to play an essential role in inactivation of class A/L-type channel chimeras (see IFV-motif in Hering et al. 1997, 1998). As illustrated in Fig. 5A, the resulting mutant (1A/IF-AA/3) displayed dramatically slower fast-inactivation kinetics. Furthermore, 1A/IF-AA/3 channels entered the slow inactivated state at a faster rate compared with 1A/3 channels (onset,1A/IF-AA/3 = 38 ± 5 s (n = 6) vs. onset,1A/3 = 67 ± 5 s, n = 10, P < 0·01; Fig. 5A).
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1A (IF1612,1613AA) affect the on-rate of slow inactivation and recovery
A, onset of slow inactivation in | ||
However, we also observed a small but significant difference in recovery of 1A/IF-AA/3 from slow inactivation (24 ± 1 s in 1A/IF-AA/3 vs. 19 ± 1 s in 1A/3 at -80 mV, P < 0·01, Fig. 5B).
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DISCUSSION |
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Class A Ca2+ channels affect synaptic function in the mammalian nervous system by mediating the release of neurotransmitters. It is believed that the fine tuning of voltage-dependent Ca2+ entry into neurons is mediated by the -subunit composition of class A Ca2+ channels. In the present study we expressed an 1A-subunit (BI-2) together with 1a-, 2a-, 3- or 4-subunits in Xenopus oocytes and estimated the on- and off-rate constants of slow inactivation in channels with different -subunit composition.
A back-extrapolation technique for estimation of slow inactivation
The 'back-extrapolation' technique described in Fig. 2 enabled the estimation of the on- and off-rate constants of slow inactivation in class A Ca2+ channels. The first detailed study of slow inactivation in Ca2+ channels was performed by Boyett et al. (1994) who focused on an analysis of the kinetics of current decay of L-type channels during long-lasting membrane depolarizations. Slow inactivation is, however, often masked by fast and/or Ca2+-dependent inactivation (see McMorn et al. 1995 for studies in L-type channels). A comparable picture was observed for class A Ca2+ channels where a transient component in IBa inactivation of 1A/1a, 1A/3 and 1A/4 channels prevented a straight estimation of transitions to the slow inactivated state from the current shape (Fig. 1A). Moreover, transitions from fast to slow inactivation cannot be observed from the kinetics of current decay.
The 'back-extrapolation' technique accounts for all channel state transitions to the slow inactivated state including those that are camouflaged by fast or Ca2+-dependent inactivation and requires shorter depolarizing pulses.
Role of -subunits in slow inactivation of class A Ca2+ channels
The rate of slow inactivation is crucially dependent on subunit composition. Slowly inactivating 1A/2a channels (Fig. 1A) displayed the fastest rate of slow inactivation. Our results demonstrate that a 2a-subunit-induced reduction in fast inactivation does not prevent but even accelerates state transitions to the slow inactivated state (Fig. 3). There is evidence that the properties of 1A proteins are regulated by interaction with more than a single -subunit (Burgess et al. 1999). Tissue-specific expression patterns of different -subunits or changes in the subunit assembly during development (Tanaka et al. 1995) appear, therefore, as significant determinants of slow inactivation in class A Ca2+ channels.
The kinetics of class A channel recovery from the slow inactivated state were independent of the length of the applied prepulses (Fig. 2A). The latter finding indicates that class A Ca2+ channels recover, unlike NaII and NaIIA channels (Toib et al. 1998), in a non-duration-of-activity-dependent manner.
Class A Ca2+ channels are more willing to enter slow inactivation from the open state
To answer the question if enhanced slow inactivation in 1A/2a channels (Fig. 3) reflects a specific -subunit effect or, alternatively, occurs at a higher rate from the open state, we designed a class A Ca2+ channel mutant with slower inactivation kinetics. In previous studies on class A/L-type chimeras we have identified a hot spot of inactivation determinants at the inner channel mouth in segment IIIS6 (IFV-motif, Hering et al. 1998) and suggested an inactivation model where fast inactivation is substantially determined by non-covalent interaction of S6 segements (Hering et al. 1996, 1998). Here we demonstrate for the first time that two amino acids of a homologous motif at the inner mouth of segment IIIS6 in 1A (I1612, F1613) play an essential role in fast inactivation of class A Ca2+ channels (Fig. 5). The faster on-rate of slow inactivation in the slowly inactivating double mutant 1A/IF-AA/3 supports the hypothesis that the faster rate of slow inactivation in 1A/IF-AA/3 and 1A/2a channels is more probably caused by reduced fast inactivation than by a direct -subunit effect on the 'slow inactivated' state. However, a small but significant increase of the slow recovery time constant in 1A/IF-AA/3 compared with 1A/3 channels (Fig. 5B) does not allow an unequivocal conclusion. Hence, the apparent faster on-rate demonstrated in Fig. 5A could also partially result from an additional stabilization of the slow inactivated conformation by mutations IF1612/1613AA.
A higher rate of slow inactivation from the open to the slow inactivated state is also suggested by the y-intercept of the linear function fitted to the log of slow inactivation in 1A/3 channels compared with 1A/2a (Fig. 3A). 1A/3 channels enter the slow inactivated state during the first few seconds of the inactivating prepulse predominantly from the open state and later exclusively from the 'fast inactivated' state. Due to the much slower current decay 1A/2a channels enter the slow inactivated state during the prepulse from both open and 'fast inactivated' states. The y-intercept in 1A/3 channels can, therefore, be explained by an initially higher transition rate of open channels to the slow inactivated state causing a somewhat steeper slope during the first few seconds whereas later during the pulse the slope is determined mainly by the slower rate of redistribution between fast and slow inactivation. 1A/2a channels enter the slow inactivated state during the conditioning pulse from both states with an obviously smaller impact of the redistribution rate between fast and the slow inactivated state resulting in the smaller y-intercept. For a detailed mathematical description of the y-intercept see Appendix.
Possible implications for synaptic function
Ca2+ channels that have opened during an action potential appear to be more willing to enter the slow inactivated state than channels in the fast inactivated conformation. It is tempting to speculate, that, due to slow recovery (Fig. 4D), a certain fraction of class A Ca2+ channels will inevitably accumulate in the slow inactivated state during action potential trains. Such a mechanism would be particularly important for the slowly inactivating 1A-b splice variant (Bourinet et al. 1999). Slow inactivation in class A channels could, therefore, play an important role in regulating the voltage-dependent Ca2+ entry into neurons.
Direct evidence for a role of class A Ca2+ channel inactivation in post-tetanic depression of excitatory postsynaptic currents was recently presented by Forsythe et al. (1998). Presynaptic P-type channels in a brainstem giant synapse (calyx of Held) recover with biexponential kinetics from inactivation. Forsythe et al. (1998) suggest that accumulation of the channels during high frequency stimulation in inactivation represents a fail safe mechanism that would reduce Ca2+ entry and thereby slow or prevent presynaptic vesicle depletion. The mean time constant of about 50 s for slow P-type channel recovery in the presynaptic membrane of the calyx of Held is comparable to the values of class A Ca2+ channel recovery from slow inactivation (Fig. 4D). The -subunit composition of class A Ca2+ channels may, therefore, represent a significant determinant of short-term synaptic plasticity.
This assumption is supported by our finding that only the on-rate was -subunit-modulated whereas recovery from slow inactivation at a given membrane potential was not affected. However, voltage clamp experiments with faster temporal resolution on mammalian cells are required to compare the relative impacts of slow inactivation, fast inactivation of open channels and closed-state inactivation (Patil et al. 1998) during trains of brief action potential waveforms.
Slow inactivation of class A Ca2+ channels may also represent an important mechanism to prevent Ca2+ overload during long-lasting depolarizations in neuronal tissue during hypoxic or ischaemic events (Kristián & Siesjö, 1996).
Taken together, we demonstrate a technique that enabled a detailed description of the on- and off-rate constants of slow inactivation in Ca2+ channels. Class A Ca2+ channels enter the 'slow inactivated' state from both open and 'fast inactivated' conformations. Open channels appear, however, to be more willing to enter the slow inactivated state.
The -subunit regulation of fast inactivation has an indirect effect on the rate of slow inactivation which may play an important role in fine tuning of voltage-dependent Ca2+ entry and help to maintain the neuronal Ca2+ homeostasis.
Our data are consistent with a state diagram where class A Ca2+ channels enter the slow inactivation state (S) either directly from the open (O) or via the fast inactivated state (F). Possible state transitions during a membrane depolarization are illustrated in the reaction scheme:
Index d indicates rate constants at a depolarizing potential.
The exact solution for this system of differential equations
incorporates the characteristic roots of the system:
Assuming that slow inactivation develops at a much slower rate than fast inactivation (
d,d << d,d), this process can be approximated by:
where s = -1/
1 and f = -1/2.
During the slow phase of onset of inactivation (when fast inactivation is completed):
If this function is extrapolated to zero time we obtain an expression for the experimentally observed y-intercept:
If transitions to the slow inactivated state occur predominantly via the fast inactivated state O 
F S, d < d and the y-intercept is expected to have a negative value whereas predominantly parallel transition (from O directly to S, i.e. d < d) will result in a positive y-intercept, as observed in our experiments.
Recovery from inactivation at negative membrane potentials occurs in accordance with the following scheme:
Index h indicates rate constants at a hyperpolarizing potential.
Solving this set of equations we obtain:
where slow = 1/(h + h) and fast = 1/(h + h).
Under the assumptions that the recovery from fast inactivation occurs at a much faster rate than recovery from slow inactivation (h >> h, h >> h, h >> h) this equation can be simplified to:
S0 exp(-t/slow) + F0 exp(-t/fast).This expression demonstrates that under conditions where the fast and slow kinetic components of recovery are well separated from each other, the amplitude coefficient of the slow component reflects the fraction of slow-inactivated Ca2+ channels at the end of the conditioning prepulse.
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We thank Professor H. Glossmann for continuous support of our work and Drs S. Berjukow and J. Mitterdorfer for comments on the manuscript. We also thank Drs Y. Mori and K. Imoto for the gift of the 1A cDNA, Dr Schwartz for providing the 2/ cDNA and Dr Birnbaumer for providing the 2a, 3 and 4 cDNAs. This work was supported by grants from the Fonds zur Förderung der Wissenschaftlichen Forschung P12649 (S.H.), a grant from the Else Kröner Fresenius Stiftung (S.H.) and a grant from the Austrian National Bank (S.H.) and is part of the thesis of S.S.
Corresponding author
S. Hering: Institut für Biochemische Pharmakologie, Peter-Mayr-Straße 1, A-6020 Innsbruck, Austria.
Email: steffen.hering{at}uibk.ac.at
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