Quantitative proteomics of the Cav2 channel nano-environments in the mammalian brain

Müller, Christoph Michael; Haupt, Alexander; Bildl, Wolfgang; Schindler, Jens; Knaus, Hans−Günther; Meissner, Marcel; Rammner, Burkhard; Striessnig, Jörg; Flockerzi, Veit; Fakler, Bernd; Schulte, Uwe

doi:10.1073/pnas.1005940107

Cited by 264 publications

(311 citation statements)

References 55 publications

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“…When the stargazer mouse was identified to have a mutation in a protein that was a homolog of γ1 (termed stargazin or γ2), it was classified as a neuronal calcium channel γ-subunit (15). However, in the study by Müller et al (6), no interactions with any γ-subunits were found, which agrees with the predominantly held view that these proteins are transmembrane AMPA receptor interacting proteins (16).…”

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confidence: 36%

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Age of quantitative proteomics hits voltage-gated calcium channels

Dolphin¹

2010

Proc. Natl. Acad. Sci. U.S.A.

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confidence: 36%

“…Müller et al (6) are dealing with ion channels that are primarily presynaptic, and this is confirmed by the absence of key PSD proteins from the interactome. In this study, complexes of Ca V 2 channels and associated β-subunits from brain have been isolated using affinity purification steps, and MS has been used to identify the copurified proteins.…”

mentioning

confidence: 86%

Age of quantitative proteomics hits voltage-gated calcium channels

Dolphin¹

2010

Proc. Natl. Acad. Sci. U.S.A.

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“…Regulation of Ca 2+ influx is the best-characterized role for Ca V 1.2, but voltage-gated Ca 2+ channels anchor large macromolecular complexes (19) and could therefore control cellular processes independent of Ca 2+ influx. Indeed, the Ca 2+ channel auxiliary subunit β4 controls epiboly in zebrafish through a Ca 2+ -independent manner (20).…”

Section: Discussionmentioning

confidence: 99%

Calcium influx through L-type CaV1.2 Ca2+ channels regulates mandibular development

Ramachandran

Hennessey²,

Barnett³

et al. 2013

J. Clin. Invest.

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The identification of a gain-of-function mutation in CACNA1C as the cause of Timothy Syndrome (TS), a rare disorder characterized by cardiac arrhythmias and syndactyly, highlighted unexpected roles for the L-type voltage-gated Ca 2+ The broad array of abnormalities within nonexcitable tissues in Timothy Syndrome (TS) patients (1), however, revealed that Ca V 1.2 controls critical, yet previously unknown, roles in multiple nonexcitable tissues. Identified as a novel cardiac arrhythmia syndrome associated with syndactyly and dysmorphic facial features (2), the TS defect was discovered to be a specific gain-of-function mutation (G406R) in CACNA1C, the gene encoding Ca V 1.2. The mutation greatly slows channel inactivation, and thereby prolongs cellular repolarization in cardiac myocytes, which provided a clear rationale for the cardiac arrhythmias. Yet how Ca V 1.2 affects nonexcitable cells, as indicated by additional phenotypes documented in TS, such as small teeth, baldness at birth, and dysmorphic facial features, is unclear. These phenotypes were not consistent with previously understood roles for Ca V 1.2. Here, we

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“…Alternatively, the region of amplification could extend beyond the Ca V itself, if augmented by diffusion-impeding assemblies of associated components. In this regard, it is interesting to note that Ca V subtypes interact with a tremendous variety of proteins in different cellular contexts (52,53). Indeed, the very same molecules that aggregate near Ca V channels to convey downstream signals could also act to restrict diffusion, thereby increasing the gain between Ca 2+ flux and biochemical response.…”

Section: Significancementioning

confidence: 99%

Ca ²⁺ channel nanodomains boost local Ca ²⁺ amplitude

Tadross

Tsien

Yue

2013

Proc. Natl. Acad. Sci. U.S.A.

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Local Ca 2+ signals through voltage-gated Ca 2+ channels (Ca V s) drive synaptic transmission, neural plasticity, and cardiac contraction. Despite the importance of these events, the fundamental relationship between flux through a single Ca V channel and the Ca 2+ signaling concentration within nanometers of its pore has resisted empirical determination, owing to limitations in the spatial resolution and specificity of fluorescence-based Ca 2+ measurements. Here, we exploited Ca 2+ -dependent inactivation of Ca V channels as a nanometer-range Ca 2+ indicator specific to active channels. We observed an unexpected and dramatic boost in nanodomain Ca 2+ amplitude, ten-fold higher than predicted on theoretical grounds. Our results uncover a striking feature of Ca V nanodomains, as diffusion-restricted environments that amplify small Ca 2+ fluxes into enormous local Ca 2+ concentrations. This Ca 2+ tuning by the physical composition of the nanodomain may represent an energy-efficient means of local amplification that maximizes information signaling capacity, while minimizing global Ca 2+ load.L ocal Ca 2+ signals increase the information capacity of signaling within a cell, by enabling short-range signals to operate independently of Ca 2+ events elsewhere throughout the cell (1, 2). These local Ca 2+ signals are the conduit that drives diverse activity-dependent events, such as synaptic transmission (3), neural plasticity (4-6), and cardiac excitation-contraction coupling (7). However, with regard to the Ca 2+ amplitude within nanometers of individual Ca 2+ channels, our knowledge is based predominantly on diffusion theory, which predicts ∼100 μM Ca 2+ signals per picoampere flux at a distance of ∼10 nm from the pore (8-11). Although often quoted, this theory has been difficult to verify experimentally because diffusible Ca 2+ indicators report space-averaged [Ca 2+ ], and thus lack the spatial resolution needed for selective nanodomain reporting. Two recent efforts to overcome this limitation used voltage-gated Ca 2+ channel (Ca V )-tethered fluorescent Ca 2+ indicators to isolate nanodomain signals (12, 13), but were met with unexpected difficulties: Ca V -tethered indicators were unresponsive in the presence of high concentrations of intracellular 1,2-bis(oaminophenoxy)ethane-N,N,N',N'-tetraacetic acid (BAPTA), a Ca 2+ buffer that preserves Ca 2+ elevations within tens of nanometers of active channels but eliminates it elsewhere (8-10). A lack of response under these conditions would arise if the majority of tethered channels were silent, raising the concern that fluorescence changes observed under milder Ca 2+ buffering (12, 13) may represent the response of indicators tethered to silent channels, which nonetheless eavesdrop on Ca 2+ from active channels nearby. To overcome this fundamental limitation, we used a reverse strategy, whereby Ca 2+ /calmodulin-dependent inactivation (CDI) of channels themselves serves as a nanometer-range indicator of [Ca 2+ ]; a sensitive ionic readout that is unaffected by the pres...

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Quantitative proteomics of the Cav2 channel nano-environments in the mammalian brain

Cited by 264 publications

References 55 publications

Age of quantitative proteomics hits voltage-gated calcium channels

Age of quantitative proteomics hits voltage-gated calcium channels

Calcium influx through L-type CaV1.2 Ca2+ channels regulates mandibular development

Ca ²⁺ channel nanodomains boost local Ca ²⁺ amplitude

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Quantitative proteomics of the Cav2 channel nano-environments in the mammalian brain

Cited by 264 publications

References 55 publications

Age of quantitative proteomics hits voltage-gated calcium channels

Age of quantitative proteomics hits voltage-gated calcium channels

Calcium influx through L-type CaV1.2 Ca2+ channels regulates mandibular development

Ca 2+ channel nanodomains boost local Ca 2+ amplitude

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Product

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Ca ²⁺ channel nanodomains boost local Ca ²⁺ amplitude