Journal Club

The Calcium Channel β4a Subunit: A Scaffolding Protein Between Voltage-Gated Calcium Channel and Presynaptic Vesicle-Release Machinery?

Norbert Weiss
Journal of Neuroscience 7 June 2006, 26 (23) 6117-6118; DOI: https://doi.org/10.1523/JNEUROSCI.1699-06.2006

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Neuronal voltage-gated calcium channels represent a major pathway for calcium entry into nerve termini, where they control neurotransmitter release. The channels are composed of a pore-forming subunit (Cav2.x) and auxiliary subunits (Cavβ1–4, α2Δ1–4 and γ1–8). The cytoplasmic Cavβ subunits belong to the membrane-associated guanylate kinase (GK) family of proteins and regulate trafficking to the plasma membrane and gating properties of Cav2.x channels. Their five domains (A–E), include hypervariable A, C, and E domains linked to the highly conserved Src homology 3 (SH3) (B) and GK (D) domains. The crystal structure of the core domains (B–D) of several β subunits was recently elucidated (Chen et al., 2004; Opatowsky et al., 2004; Van Petegem et al., 2004), but less is known about the structure of the A and E domains. A recent report published in The Journal of Neuroscience provides new information on the Cavβ4a subunit hypervariable A domain (Cavβ4a-A) (Vendel et al., 2006a). The authors previously showed that alternative splicing of the Cavβ4-A domain generates two distinct proteins, Cavβ4a and Cavβ4b (Helton and Horne, 2002), and they recently provided the solution structure of the Cavβ4a-A domain (Vendel et al., 2006b). Vendel et al. now address the expression pattern of the Cavβ4a splice variant and the functional importance of the Cavβ4a-A domain.

Using immunohistochemistry, the authors show that the Cavβ4a splice variant was expressed as punctuate structures throughout the molecular layer of the cerebellum [Vendel et al. (2006a), their Fig. 3D,E (http://www.jneurosci.org/cgi/content/full/26/10/2635/F3)]. In contrast, Cavβ4b was expressed in basket cells surrounding Purkinje cell bodies as well as in the Bergmann glia [Vendel et al. (2006a), their Fig. 3F (http://www.jneurosci.org/cgi/content/full/26/10/2635/F3)]. To determine the functional importance of the Cavβ4a-A domain, the authors performed two electrode voltage-clamp recording in Xenopus laevis oocytes expressing Cav2.1 channels (P/Q type currents) in combination with α2Δ and Cavβ4a subunits with (ABCDE) or without (BCDE) the N-terminal A domain. The Cavβ4a-A domain was not essential for the expression of the Cav2.1 channel at the plasma membrane and did not influence gating properties. Indeed, no difference was observed in current amplitude [Vendel et al. (2006a), their Fig. 2A (http://www.jneurosci.org/cgi/content/full/26/10/2635/F2)], nor in the voltage dependence of activation or inactivation [Vendel et al. (2006a), their Fig. 2C,D (http://www.jneurosci.org/cgi/content/full/26/10/2635/F2)]. These results are, however, in agreement with published studies (Bichet et al., 2000; Van Petegem et al., 2004) because (1) enhanced Cav2.x subunit trafficking to the plasma membrane occurs after binding of the Cavβ subunit to the channel (Bichet et al., 2000) via the α interaction domain (AID)-binding pocket within the GK domain (Van Petegem et al., 2004), and (2) the molecular determinants by which the Cavβ subunit modulates channel gating remain unclear but are probably carried by the conserved core domains because all Cavβ subtypes are able to modulate the biophysical properties of the channel. However, it is more surprising that channel inactivation kinetics was not influenced by deletion of the Cavβ4a-A domain [Vendel et al. (2006a), their Fig. 2B (http://www.jneurosci.org/cgi/content/full/26/10/2635/F2)]. Indeed, it is known that a deletion of the N-terminal of Cavβ subunits results in a drastic slowing of channel inactivation kinetics (Olcese et al., 1994). It seems not to be the case for the Cavβ4a splice variant. Thus, further investigations will provide interesting structural information on how the N-terminal of Cavβ subunits controls channel inactivation.

Because the Cavβ4a-A domain was not a key determinant in the regulation of Cav2.1 channel gating, Vendel et al. looked for a role of this domain in protein–protein interactions. Using the yeast two-hybrid system, the authors screened a human cerebellum cDNA library with the Cavβ4a-A domain (amino acids 1–58). Synaptotagmin I (Syt I) (amino acids 95–337 including the entire C2A domain and a half of the C2B domain) as well as the microtubule-associated protein 1A (MAP1A) (amino acids 2508–2775 corresponding to the complete LC2 domain) interacted specifically with the N-terminal A domain of the Cavβ4a splice variant but not with the Cavβ4b-A domain [Vendel et al. (2006a), their Fig. 4B (http://www.jneurosci.org/cgi/content/full/26/10/2635/F4)]. The authors then focused their study on Syt I and confirmed its interaction with the Cavβ4a-A domain by in vitro pull-down experiments. The interaction did not occur in the presence of 10 mm Ca2+ and could also be disrupted by adding Ca2+ to the medium [Vendel et al. (2006a), their Fig. 5C (http://www.jneurosci.org/cgi/content/full/26/10/2635/F5)]. These data certainly represent the most important findings of this study.

In conclusion, Vendel et al. (2006a) provide evidence that alternative splicing of the N-terminal A domain of the Cavβ4 auxiliary subunit confers functions other than modulations of channel gating and trafficking. Because Cavβ4a splicing variant can bind synaptotagmin I, an important protein for presynaptic vesicle release, the β subunit, could conceivably act as a scaffolding element to facilitate coupling of calcium signaling with neurotransmitter release (Fig. 1). However, the authors do not provide evidence that Cavβ4a can bind Cav2.1 channel and Syt I simultaneously. Pull-down experiments performed by preincubating the full-length Cavβ4a with the AID peptide (the molecular determinant of the Cav2.x channel, which interacts with the AID-binding pocket of the Cavβ subunit) before adding Syt I could partially answer this question. Finally, the fact that Cavβ4a–Syt I interaction is disrupted by Ca2+ is interesting. In this context, we speculate that at basal Ca2+ levels, Cavβ4a interacts both with Cav2.1 and Syt I to organize the vesicle-release machinery and that calcium entry into cells via voltage-gated calcium channels breaks this interaction, thus releasing the vesicle to allow fusion with the plasma membrane. FRET experiments using tagged Syt I and Cavβ4a in the presence of Cav2.1 channels before and during membrane depolarization might address such a possible mechanism.

Figure 1.
Figure 1.

A putative model of coupling between voltage-gated calcium channels, calcium signaling, and presynaptic vesicle-release machinery. A, In basal condition with a low Ca2+ level, Cavβ4a interacts both with Cav2.1 channel and Syt I to position the synaptic vesicle in front of the channel to better couple calcium signaling and neurotransmitter release. B, Calcium entry into the cell via voltage-gated calcium channels and after membrane depolarization disrupts Cavβ4a–Syt I interaction. The content of the synaptic vesicle is thus released by the fusion of the vesicle with the plasma membrane after soluble N-ethylmaleimide-sensitive factor attachment protein (SNAP) receptors v-SNAREs (synaptobrevin and synaptotagmin I) and t-SNAREs (syntaxin and SNAP 25) interactions. PM, Plasma membrane.

Footnotes

    • Received April 20, 2006.
    • Accepted April 27, 2006.

  • Review of Vendel et al. (http://www.jneurosci.org/cgi/content/full/26/10/2535)

  • Correspondence should be addressed to Norbert Weiss, Institut National de la Santé et de la Recherche Médicale U607, Laboratory Canaux Calciques, Fonctions et Pathologies, Commissariat à l'Energie Atomique/DRDC/Bâtiment C3, 17 Rue des Martyrs, 38054 Grenoble Cedex 09, France. Email: norbert.weiss{at}cea.fr

References

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