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Molecular & Cellular Proteomics 7:2188-2198, 2008.
© 2008 by The American Society for Biochemistry and Molecular Biology, Inc.

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Research

Profiling the Phospho-status of the BK_Ca Channel Subunit in Rat Brain Reveals Unexpected Patterns and Complexity^*,S

Jiusheng Yan^,, Jesper V. Olsen^¶, Kang-Sik Park, Weiyan Li, Wolfgang Bildl^||, Uwe Schulte^**, Richard W. Aldrich, Bernd Fakler^||, and James S. Trimmer^,,¶¶

From the Department of Neurobiology, Physiology and Behavior, College of Biological Sciences, University of California, Davis, California 95616, Section of Neurobiology, School of Biological Sciences, University of Texas, Austin, Texas 78712, ^¶ Department of Proteomics and Signal Transduction, Max Planck Institute for Biochemistry, D-82152 Martinsried, Germany, ^|| Institute of Physiology, University of Freiburg, Hermann-Herder-Strasse 7, 79104 Freiburg, Germany, ^** Logopharm GmbH, Hermann-Herder-Strasse 7, 79104 Freiburg, Germany, Department of Physiology and Membrane Biology, School of Medicine, University of California, Davis, California 95616

	ABSTRACT

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Molecular diversity of ion channel structure and function underlies variability in electrical signaling in nerve, muscle, and non-excitable cells. Protein phosphorylation and alternative splicing of pre-mRNA are two important mechanisms to generate structural and functional diversity of ion channels. However, systematic mass spectrometric analyses of in vivo phosphorylation and splice variants of ion channels in native tissues are largely lacking. Mammalian large-conductance calcium-activated potassium (BK_Ca) channels are tetramers of subunits (BK) either alone or together with β subunits, exhibit exceptionally large single channel conductance, and are dually activated by membrane depolarization and intracellular Ca²⁺. The cytoplasmic C terminus of BK is subjected to extensive pre-mRNA splicing and, as predicted by several algorithms, offers numerous phospho-acceptor amino acids. Here we use nanoflow liquid chromatography tandem mass spectrometry on BK_Ca channels affinity-purified from rat brain to analyze in vivo BK phosphorylation and splicing. We found 7 splice variations and identified as many as 30 Ser/Thr in vivo phosphorylation sites; most of which were not predicted by commonly used algorithms. Of the identified phosphosites 23 are located in the C terminus, four were found on splice insertions. Electrophysiological analyses of phospho- and dephosphomimetic mutants transiently expressed in HEK-293 cells suggest that phosphorylation of BK differentially modulates the voltage- and Ca²⁺-dependence of channel activation. These results demonstrate that the pore-forming subunit of BK_Ca channels is extensively phosphorylated in the mammalian brain providing a molecular basis for the regulation of firing pattern and excitability through dynamic modification of BK structure and function.

Mammalian BK_Ca (large-conductance calcium-activated potassium, also termed K_Ca1.1, Maxi-K, or Slo1)¹ channels are unique potassium-selective channels that are dually activated by two independent physiological signals: intracellular Ca²⁺ concentration and transmembrane voltage (9–12); thereby playing a powerful integrative role in the regulation of electrical excitability through coupling of calcium signaling and cellular excitability. In mammalian central neurons, BK_Ca channels underlie the repolarization and fast after-hyperpolarization of action potentials (13, 14), shape dendritic Ca²⁺ spikes (15), and control neurotransmitter release at presynaptic terminals (16, 17). BK_Ca channels also play key roles in other diverse physiological processes such as contractile tone of various types of smooth muscle cells, frequency tuning of auditory hair cells, hormone secretion, and innate immunity (9–11).

BK_Ca channels are robustly expressed in central neurons throughout most regions of the mammalian brain (18). Unlike many mammalian potassium channels, a single gene (Slo1, KCNMA1) encodes all BK_Ca channel subunits (BK). However, native BK_Ca channels display a broad range of functional properties that differ between different cells (9, 10), at different stages of development (19, 20), and under different physiological conditions (21). In addition to assembly with tissue-specific auxiliary β subunits (β1-β4), diversity in the physiological properties of BK_Ca channels can be generated by extensive pre-mRNA splicing and phosphorylation of BK.

BK_Ca channels are tetramers of the pore-forming, voltage-, and Ca²⁺-sensing BK either alone or in association with regulatory β subunits. BKs are 125–140 kDa polypeptides containing seven transmembrane segments (S0–S6), a short extracellular N-terminal domain, and a large cytoplasmic C terminus (22) (Fig. 1). This C-terminal domain comprises >70% of the total protein and contains four hydrophobic segments (S7–S10) and sequences similar to RCK (Regulating Conductance of K⁺) domains (23–25), and a string of Asp residues known as the "Ca²⁺ bowl" (26).

View larger version (37K): [in this window] [in a new window]   FIG. 1. Affinity purification of BK from plasma membrane-enriched protein fractions prepared from total rat brain. A, SDS-PAGE separation of eluates from affinity purifications with three antibodies targeting different epitopes in the C terminus of BK. The gel was silver-stained; arrowhead denotes the band containing BK. B, immunoblot of input (appropriately solubilized membrane preparations), flow through (unbound), and eluate of affinity purifications of BK with the indicated antibodies after SDS-PAGE separation. The source and unbound lanes were loaded with samples normalized to equivalent amount of raw material. Note the complete depletion of the source material of BK.

To help understand the molecular structure and diversity of BK_Ca channels in the central nervous system, we have immunopurified BK from rat brain and taken an unbiased approach using nanoflow tandem mass spectrometry (nano-LC MS/MS) to systematically analyze their in vivo phosphorylation sites and splice variants. We have identified extensive in vivo phosphorylation of native BK and examined the functional consequence of phosphorylation at a number of identified sites by electrophysiological analyses of phospho- and dephosphomimetic BK mutants transiently expressed in HEK-293 cells.

	EXPERIMENTAL PROCEDURES

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Affinity Purification of BK_Ca Channels from Rat Brain—
Two different sets of affinity purifications of BK_Ca channels were used in this study. One set employed monoclonal antibody-based immunopurification from rat brain membranes prepared from freshly isolated adult whole rat brains as described (35) and solubilized by 1% Triton X-100 or 1% dodecyl-maltoside. BK was affinity-purified using the monoclonal antibody L6/60 (termed anti-BK_1) (36, 37) immobilized on protein G agarose beads. L6/60 binds within amino acid residues 729–930 of mouse BK (UniProt/Swiss Prot accession number Q08460). Phosphatase inhibitors (10 mM NaF, 1 mM sodium orthovanadate, 5 mM sodium pyrophosphate) and protease inhibitors were used throughout the procedure. The other set of affinity purifications used two polyclonal antibodies with plasma membrane-enriched protein fractions prepared from adult rat brains as described previously (38, 39). Almost complete solubilization (>95% as judged from densitometric estimates of Western-probed solubilisate versus pellet) was achieved with 1–1.25 ml of ComplexioLyte 48 (including protease inhibitors; Logopharm GmbH, Freiburg, Germany) per mg membrane protein. 1.5 ml of solubilisate was incubated with 20 µg immobilized rabbit polyclonal antibodies raised either against amino acid residues 1184–1203 (termed anti-BK_2, gift from Dr. Hans-Guenther Knaus, University of Innsbruck) or 1184–1200 (termed anti-BK_3, Alomone Labs, Jerusalem, Israel) of the mouse BK (UniProt accession number Q08460). Bound proteins were eluted with Laemmli buffer (dithiothreitol added after elution). Aliquots from each step were analyzed on Western blots with equivalent fractions (as in Fig. 1B, lanes 1, 2 of each affinity purification and supplemental Fig. S4) to ensure quantitative purification and recovery of intact BK protein.

In-gel Digestion and Enrichment of Phosphopeptides—
Affinity-purified proteins were separated by SDS-PAGE and either silver-stained (in the absence of cross-linkers) or visualized with Coomassie G-250. Bands containing BK (as validated by Western analysis) as well as complete lanes were separately excised and washed thoroughly with 50% acetonitrile in 25 mM ammonium bicarbonate. In-gel digestion was carried out essentially as described by (40). After reduction and alkylation of Cys residues using dithiothreitol and iodoacetamide, gel pieces were washed, dehydrated, and subsequently swollen with ammonium bicarbonate buffer containing 10 ng/µl trypsin (Promega, Madison, WI) and incubated for 16 h at 37 °C. Digested peptide mixtures were extracted, dried in a speed vacuum concentrator, and finally redissolved in 0.2–0.5% formic acid (protein samples obtained from anti-BK_1 eluates) or trifluoroacetic acid (protein samples obtained from anti-BK_2 and anti-BK_3 eluates).

The peptide mixtures were either directly used for MS analyses or further processed to enrich the phosphopeptides. Phosphopeptide enrichment and tandem mass spectrometric analysis were performed essentially as described previously (41, 42) with a few modifications. Briefly, a slurry of titanium dioxide beads precoated with 2,5-dihydrobenzoic acid was prepared by mixing 10 µg of titansphere TiO₂ beads (GL Sciences) with 20 µl of 30 mg/ml 2,5-dihydrobenzoic acid (Fluka) in 80% acetonitrile. 5 µl of this 2,5-dihydrobenzoic acid/TiO₂ slurry was added to the acidified peptide mixtures, extracted from in-gel digests. The peptide mixtures were shaken for 30 min at 1000 rpm at 4 °C, and then spun down in a microcentrifuge. The pelleted TiO₂ beads were washed twice with 30% acetonitrile in 3% trifluoroacetic acid, and peptides were eluted with 15% NH₄OH in 40% acetonitrile (pH > 10.5). Finally, the eluates were dried in a speed vacuum concentrator for 20 min at 45 °C and reconstituted in 8 µl of 2% acetonitrile in 0.1% trifluoroacetic acid to prepare them for LC-MS.

Mass Spectrometry, Data Processing, and Analysis—
BK affinity-purified with the monoclonal antibody anti-BK_1 was analyzed with an LTQ ion trap or LTQ-FT hybrid mass spectrometer (Thermo-Fisher, San Jose, CA) connected to a Waters UltraPerformance LC system (Waters, Milford, MA). Peptide samples were concentrated on a Waters Symmetry C18 280 µm x 20 mm nanoAcquity trap column at a loading flow rate of 15 µl/min. Peptides were then eluted from the trap and separated by a Waters 100 µm x 100 mm UltraPerformance LC column using a 90 min gradient of 2–80% buffer B (buffer A, 0.1% formic acid, buffer B, 95% acetonitrile, 0.1% formic acid), and sprayed into an LTQ or LTQ-FT ion trap mass spectrometer through a nanoelectrospray source. The MS survey scan was acquired using the LTQ or Fourier transform ion cyclotron resonance mass analyzer and then the top four ions in each survey scan were subjected to automatic low energy collision-induced dissociation for MS/MS scans.

MS/MS spectra were extracted using the program Extract_msn v.4.0 of the Bioworks software v.3.3 (Thermo Finnigan) with default parameters and interpreted with Mascot v.2.2 (Matrix Science, London, UK) and Sequest/Bioworks v.3.3 search engines by searching against UniProt/Swiss-Prot database (release 50.8, subset Rodents, 18284 protein entries) supplemented with all known and artificially spliced variants of rat BK (rSlo), based on the rat genomic sequence and known splicing variants from mRNA or expressed sequence tag sequence of other mammalian species. Database searches were performed with a peptide mass tolerance of 2 Da (LTQ) or 20 ppm (LTQ-FT), MS/MS tolerance of 0.4 Da, and strict tryptic specificity (cleavage after lysine and arginine) allowing one missed cleavage site; carbamidomethylation of Cys was set as fixed modification, whereas oxidation (Met), N-acetylation, N-pyroglutamine formation, and phosphorylation (Ser, Thr, Tyr) were considered as variable modifications. Peptide ions with a Mascot ion score of <20 were manually checked for validation. For database search with Sequest/Bioworks, peptide sequences from the search result were filtered out with criteria of correlation value (Xcorr) >1.5, 2.0, and 3.0 for singly, doubly, and triply charged peptide ions, respectively, and Cn (difference in correlation with the next higher Xcorr) >0.08. Each MS/MS spectrum exhibiting possible phosphorylation was manually checked and validated based on the existence of a 98 Da mass loss (H₃PO₄; phosphopeptide-specific collision-induced dissociation neutral loss) for both precursor and fragmented ions.

The peptide mixtures from BK affinity-purified with the polyclonal antibodies anti-BK_2 and anti-BK_3 were separated by online high pressure liquid chromatography and directly electrosprayed into an LTQ-Orbitrap hybrid mass spectrometer as described (41). The instrument was operated in data-dependent mode to automatically switch between full scan MS and MS/MS acquisition. All full scans were acquired with a resolution of 60,000 at m/z = 400 by the Orbitrap detector system using automatic internal lock-mass recalibration in real-time (43). From each full scan up to five peptide ions with charge states 2 were selected for fragmentation by multi-stage activation (multistage activation or pseudo MS³) (44). All fragment ion spectra were recorded with the LTQ detectors.

MS/MS peak lists were extracted from the raw MS files by in-house written software Raw2msm v.1.10 (43) using default parameters (intensity-weighing the parent ion m/z over the LC elution profile and keeping top 6 most intense fragment ions per 100 m/z units), and searched by Mascot v.2.2 against a concatenated forward (target) and reversed (decoy) version of the IPI rat database v.3.25 supplemented with standard observed contaminants such as porcine trypsin and human keratins (total number of protein sequences: 82886). Carbamidomethylation of cysteine residues was set as a fixed modification, whereas oxidation (Met), N-pyroglutamine formation, and phosphorylation (Ser, Thr, Tyr) were considered as variable modifications. Full tryptic specificity (cleavage after lysine and arginine) was required and up to three missed cleavages were allowed. The initial mass tolerance in MS mode was set to 5 ppm and MS/MS mass tolerance was 0.5 Da. The resulting Mascot html-output file was linked to the raw MS files and loaded into the MSQuant software only accepting the highest-scoring peptide sequence for each MS/MS spectrum and requiring a minimum Mascot score of at least 10. To minimize the false discovery rate all peptide identifications were filtered by thresholds on peptide length, mass error, and Mascot score. We fixed the thresholds and accepted peptides based on the criteria that the number of forward hits were at least 200-fold higher than the number of reversed hits, which gives an estimated false discovery rate of less than 1% (p < 0.01). To pinpoint the actual phosphorylated amino acid residue within the identified phosphopeptides in an unbiased manner, we calculated the localization probabilities of all Ser and Thr phosphorylation sites using the post-translational modification score algorithm as described (41).

Site-directed Mutagenesis and Heterologous Expression in Culture Cells—
Phosphorylation site mutants were constructed with the recombinant cDNA plasmid, HF1-hSlo (45) encoding c-Myc-tagged human BK (EMBL-Bank accession number AAB65837). HEK-293 cells were cultured in Dulbecco's modified Eagle's medium (Invitrogen) with 10% fetal bovine serum (Hyclone, Logan, UT), 50 units/ml penicillin, 50 mg/ml streptomycin, and GlutaMAX^TM (Invitrogen). Cells were maintained in a humidified atmosphere of 5% CO₂ at 37 °C and transiently transfected with HF1-hSlo1 plasmid together with pEGFP-C1 using Lipofectamine (Invitrogen). All cells were used within 16–72 h after transfection for electrophysiological assays.

Electrophysiological Recordings and Data Analysis—
All recordings were performed at room temperature in the inside-out patch-clamp configuration. Data were acquired with an Axopatch 200A patch-clamp amplifier (Axon Instruments, Inc.) in resistive feedback mode and were low pass filtered at 10 kHz with its 4-pole Bessel filter. An ITC-16 hardware interface (Instrutech) and Pulse acquisition software (HEKA Elektronik) were used to sample the records at 20-µs intervals. Capacitive transients and leak currents were subtracted by a P/5 protocol at holding potentials of –120 mV or –150 mV (for recordings with 103 µM intracellular Ca²⁺). Four to eight consecutive current series were averaged to increase the signal to noise ratio. Normalized conductance-voltage relationships were fitted with single Boltzmann functions: G/G_max = 1/(1 + e^{(V1/2–Vm)*zF/RT}), with V_1/2 the half-maximal voltage of activation, and z the equivalent gating charge.

Pipette (external) solution contained (in mM): 140 KMeSO₃, 20 HEPES, 2 KCl, and 2 MgCl₂, pH 7.20. Bath (internal) solution: 136 KMeSO₃, 20 HEPES, 6 KCl, pH 7.20. Internal solutions with defined concentrations of free Ca²⁺ ([Ca²⁺]_i) were obtained by adding Ca²⁺ chelators EGTA, HEDTA, or nitrilotriacetic acid and CaCl₂ to the bath solution as calculated with the WEBMAXC v2.22; the final [Ca²⁺]_i was measured with a Ca²⁺-sensitive electrode (Orion Research, Inc.). To chelate contaminant Ba²⁺, 40 µM fresh (+)-18-crown-6-tetracarboxylic acid (18C6TA) was added to the internal solution just before recording. Inside-out patches were continuously perfused with internal solution using a sewer pipe flow system (DAD-12; Adams and List Assoc., Ltd.); computer-controlled switches allowed for complete solution exchange at excised patches in <1 s.

	RESULTS

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
MS Analyses of Rat Brain BK: Primary Sequence Coverage and Splice Variations—
Two independent proteomic analyses of BK affinity-purified from membrane preparations of total rat brain form the basis of this study. One set of analyses used BK immunopurified with a BK-specific mouse monoclonal antibody binding near the S9 region (anti-BK_1) (37), the other used BK immunopurified with two different rabbit polyclonal antibodies (anti-BK_2, anti-BK_3) recognizing short peptide sequences within the C-terminal tail region (38). All three antibodies were highly effective in affinity purifications fully depleting the source material of BK (Fig. 1). After separation on SDS gels, BK proteins were in-gel digested with trypsin, and the resultant tryptic peptides were analyzed by nanoflow liquid chromatography tandem MS (nano-LC MS/MS) using a linear ion trap or high resolution hybrid mass spectrometers (LTQ, LTQ-FT, or LTQ-Orbitrap).

Based on the high yield of our affinity purifications, mass spectrometry retrieved 60 BK-specific peptides, which is almost the complete set obtainable under our experimental conditions. Together, these peptide fragments cover 70% of the BK amino acid sequence as encoded by the 27 exons considered constitutive (34) (Fig. 2A). The non-covered regions are hydrophobic segments of the transmembrane core, and a short segment of the cytoplasmic C terminus for which no peptides could be detected because of the unfavorable mass of the resultant tryptic peptides (molecular weight of detectable peptide fragments between 740 and 3000). In addition, MS analysis retrieved a number of peptides that correspond to entries in a custom database of BK splice variants, and demonstrate expression of these isoforms of BK in the rat brain (supplemental Table S2). Fig. 2B illustrates the amino acid sequences of the peptide fragments that define these variations from the constitutive BK primary sequence. Together, MS analyses identified seven insertions at three distinct splice sites in the C terminus of BK as well as an extension at the N terminus. At the first site, insertions of either three (IYF, one letter code) or 61 amino acids (termed Strex) (46) were found (corresponding to the alternative usage of exons 22 or 23). At the second site, immediately proximal to a domain termed "Ca²⁺ bowl", an additional stretch of 27 residues encoded by exon 29 (AKPGKLPLVSVNQEKNSGTHILMITEL) was identified. At the C terminus, MS analyses determined four different termini ranging from 8 to 61 residues (resulting from alternative usage of the 3' part of constitutive exon 33 and the non-constitutive exons 34 and 35 (34)), whereas at the N terminus it was an extension of 65 amino acids resulting from alternative starts of translation. Together, these results verified alternative splicing of BK at the protein level and determined which splicing events were used in rat brain.

View larger version (31K): [in this window] [in a new window]   FIG. 2. In vivo phosphorylation sites and splice inserts of rat brain BK identified by MS analysis. A, amino acid sequence of the constitutive form of BK (Swiss-Prot accession number Q62976–2; last 8 residues from splice insert are not included) together with the identified phospho-Ser/Thr residues (highlighted in blue) and the splice insertion sites (marked by colored triangles). Dot-free Ser/Thr residues denote unambiguous phosphorylation sites, whereas dots underneath Ser/Thr residues mark ambiguous sites. B, amino acid sequence of the identified N-terminal extension and splice variants. Peptides identified by MS analysis are shown in red, those not identified in MS analyses are in gray. Name of each splice insert is given in bracket on the right side of the amino acid sequence. Horizontal bars denote hydrophobic segments S0–S10.

Extensive Phosphorylation of BK in Rat Brain—

View larger version (30K): [in this window] [in a new window]   FIG. 4. Localization of identified phosphosites and splice variants on rat brain BK. Membrane topology of BK together with localization of the identified phosphosites and splice insertions. The constitutive form of BK contains the transmembrane core (S0–S6), the pore region, the hydrophobic intracellular segments S7–S10, the Ca2+ bowl, and the RCK domains (25, 65, 66). Insertion sites of sequence stretches generated by alternative splicing or alternative start of translation are indicated by triangles with the same color coding and names as in Fig. 2. Phosphosite Ser(P)-855 exhibiting a marked effect on channel gating is highlighted in red.

View larger version (38K): [in this window] [in a new window]   FIG. 3. Representative MS/MS spectra of two phosphopeptides harboring either one phosphothreonine (Thr(P)-965, upper panel) or three phosphoserines (Ser(P)-854/Ser(P)-855/Ser(P)-859, lower panel). Spectra were obtained on an LTQ-Orbitrap mass spectrometer with multistage activation (pseudo-MS3) of the precursor ions shown in the insets.

The majority of the identified phosphosites were detected on peptides harboring single phosphorylated Ser/Thr residues, whereas the others were found on either doubly phosphorylated peptides (Ser(P)-655, Ser(P)-659, and Ser(P)-843) or triply phosphorylated peptides (Ser(P)-854, Ser(P)-855, Ser(P)-859, Ser(P)-1080, Ser(P)-1082, Ser(P)-1088, and Thr(P)-1089).

Differential Modulation of BK_Ca Channel Gating by Phosphorylation—
Next we individually mutated 16 of the identified phospho-Ser/Thr residues on BK to Ala and Asp attempting to mimic phospho and dephospho states, respectively (48). These mutations were made in the hSlo-HF1 plasmid (45) encoding the constitutive human BK (accession AAB65837) with the C-terminal splice insert C-ERL; hSlo1 is identical to rat BK except for five residues (human versus rat: A86V, I619V, K631R, S639P, and Q1093P).

Electrophysiological properties of wild type and mutant BK_Ca channels were determined in transfected HEK-293 cells under basal conditions (i.e. in the absence of any further stimulus) by patch-clamp recordings in inside-out configuration at different values for [Ca²⁺]_i. Similar to previous studies (45), activation of WT hSlo-HF1 channels was strongly dependent on [Ca²⁺]_i with half-maximal activation (V) occurring at a membrane potential of 149 ± 3 mV (mean ± S.E.) at Ca²⁺-free conditions (n = 9), 97 ± 2 mV at 1.1 µM Ca²⁺ (n = 11), 14 ± 2 mV at 10.1 µM Ca²⁺ (n = 12), and –35 ± 2 mV at 103 µM Ca²⁺ (n = 12; Fig. 5 and Table I). Similar to WT channels, all phosphosite mutants gave rise to robust BK_Ca currents, suggesting that none of the phosphosite mutations appreciably affected assembly and trafficking of channels in our heterologous expressions. Alterations in activation gating resulting from introduction of a phosphomimetic negatively charged Asp residue was observed for Ser(P)-855 (Fig. 5B and Table I). Compared with the dephospho-mimicking S855A mutant, the V value of S855D displayed a 28 mV shift toward hyperpolarizing potentials, from 152 ± 2 mV (n = 8) to 124 ± 3 mV (n = 9) under Ca²⁺-free conditions and of 24 mV, from 102 ± 1 mV (n = 8) to 78 ± 2 mV (n = 9) at 1.1 µM Ca²⁺. Smaller shifts (13 and 15 mV) were observed at higher [Ca²⁺]_i (10.1 and 103 µM, respectively). All other Ala/Asp mutants failed to exert significant changes on channel activation (i.e. shifts of V were smaller than 10 mV) (Table I). However, a role of these sites in modulating channel activity in other BK backbones, or in response to specific signaling events, cannot be excluded. Thus, previous studies on bovine BK showed that mutating the site corresponding to Ser-869 (identified here as Ser(P)-869) eliminated the 35 mV hyperpolarizing shift in channel activation observed upon treatment of excised patches with purified PKA (49). Moreover, it should be kept in mind that aspartate mutations may fail to mimic the phosphorylated state because of fundamental differences between the carboxylate anion and the phosphate di-anion and trigonal planar versus tetrahedral geometry, respectively (50–53).

View larger version (29K): [in this window] [in a new window]   FIG. 5. Functional characterization of the Ser-855 phosphorylation site. Macroscopic currents recorded in inside-out patches excised from HEK-293 cells transiently expressing wild type or mutant (S855A and S855D) BKCa channels. A, representative current traces through WT channels recorded at the indicated values for [Ca2+]i, current scaling is 1 nA, time scaling as indicated. B, activation curves of WT, S855A, and S855D channels. Lines represent fits of single Boltzmann functions to the data points (mean ± S.E., numbers given in Table I).

	DISCUSSION

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

Analysis of in Vivo Phosphorylation by Mass Spectrometry—
For investigation of in vivo phosphorylation of the BK polypeptide, we undertook a proteomic analysis based on a combination of affinity purification of appropriately solubilized BK with nano-LC MS/MS analyses (38, 48). Using this approach, we identified a total of 30 Ser/Thr phosphosites, a number that by far exceeds the average number of phosphosites detected in a recent proteomic study on proteins in the soluble fraction of culture cells (41) and even that found for affinity-purified Kv2.1 (48), another ion channel particularly known for its pronounced phospho-regulation (54). In addition both number and pattern of the MS-identified phosphosites markedly differed from the results obtained with computer algorithms, which were widely used in protein/ion channel research and were based on consensus sites of specific protein kinases. As illustrated in Fig. 6, although these algorithms predicted quite a number of phosphosites on the BK sequence, only a minor subset coincided with the Ser(P)/Thr(P) detected by mass spectrometry on BK_Ca channels isolated from native tissue. In other words, in this case prediction algorithms yielded a significant number of sites that were not phosphorylated under physiological conditions and failed to identify those actually targeted by cellular kinases (Fig. 6B). As further shown in Fig. 6B, the number of "false positives" may be reduced by combining the results of several computer algorithms. However, this strategy comes at the cost of losing many of the de-facto phosphorylation sites (Fig. 6B). Taken together the proteomic approach used here appears largely superior in providing comprehensive phospho-analysis of ion channel proteins to conventional (consensus-site based) strategies, although it may still underestimate the actual number of phosphosites present on BK.

View larger version (34K): [in this window] [in a new window]   FIG. 6. Comparison of MS-identified phosphosites on BK with sites predicted by computer algorithms. A, phosphorylation site predictions for all Ser/Thr residues of BK (including splice variations) by the indicated algorithms. Scores (given as relative values) considered significant by the individual algorithms are marked by the gray bar and by non-shaded symbols (for predictions by Scansite). Phosphorylation sites predicted by PhosphoSite are given as filled green circles; MS-identified sites are denoted by black (unambiguous sites) and gray rectangles (ambiguous sites). Ser/Thr residues inaccessible to our MS analyses are marked by horizontal dashes. B, overlap of phosphosites as predicted by at least three or four computer algorithms (left and middle panel; for details on the 7 algorithms used see Supplemental Material) or by phosphosite with the 30 sites identified by the MS analyses presented here. Predicted sites are depicted as blue circles, identified sites by red circles.

The striking extent of BK phosphorylation raises questions as to its physiological role in regulating neuronal BK_Ca channels. Obviously, phosphorylation at some sites is used to modify BK_Ca channel gating properties, as demonstrated by the significant V shift observed for certain phospho/dephospho-mimicking mutants, for example S855A/S855D (Fig. 5). Other properties of BK_Ca biology regulated through the phosphorylation state may include association with interacting proteins, trafficking to the cell surface, turnover/endocytosis of cell surface channels, targeting to distinct subcellular compartments, etc. (11). The significance of phosphorylation detected for the two residues in the extracellularly located N-terminal extension remains unclear at present.

Analysis of Alternative Splicing by Mass Spectrometry—
To date, expression of BK splice variants has been studied only at the mRNA level (2, 33, 34), and there are only a few reports using mass spectrometry to systematically analyze variants of extensively spliced proteins (56). The high yield of BK obtained from our affinity purifications allowed for comprehensive MS analysis of splice variations excluding, however, those variants with tryptic fragments too small for mass spectrometry, such as the four residue insert SRKR encoded by the 3'-truncated form of exon 19 or variants providing peptide fragments too low in mass for MS detection. By searching MS/MS spectra of immunopurified BK against a custom BK splice variant database, we have identified seven splicing inserts at three different C-terminal sites as well as an N-terminal extension. To our knowledge, this is the first evidence to show that the IYF splice variant and the three C-terminal variants, C-ERL, C-SSP, and C-DEC are present in the mammalian brain.

Alternative inclusion and exclusion of the seven identified splice inserts at three splice sites can form as many as 24 different splicing variants with distinct biophysical properties, or that are altered in other aspects of BK_Ca channel biology. For example, expression of Strex-containing BK_Ca channels is under hormonal control (46), yielding channels more sensitive to hypoxia (57), and that display a significant hyperpolarizing shift (20 mV) in V and considerably slower rates of deactivation when compared with the insertless form (58). The Ca27 splice variant yields channels with an increased activation rate and modified Ca²⁺ cooperativity (59). The C-DEC splice variant generates an extended C terminus resulting in BK with enhanced retention of newly synthesized BK_Ca channels in the endoplasmic reticulum, which finally results in decreased cell surface expression (60, 61). BK_Ca channels are robustly expressed in mammalian central neurons (62, 63) and are predominantly localized to axons and presynaptic terminals (17, 37) but are also present in certain neuronal somata and dendrites (18, 64). In rat brain, BK splice variants may be differentially expressed in distinct cell types or different compartments of the same neuron. A region-specific distribution of the insertless counterpart of Ca27 splice variant has been observed in rat brain, mRNA is predominantly enriched in cerebellum, whereas Ca27 is abundant in all brain regions (59).

	FOOTNOTES

 
Received, February 11, 2008, and in revised form, June 18, 2008.

Published, MCP Papers in Press, June 23, 2008, DOI 10.1074/mcp.M800063-MCP200

¹ The abbreviations used are: BK_Ca, large conductance calcium- and voltage-activated potassium channel; BK, BK channel subunit; WT, wild type; LC-MS/MS, liquid chromatography tandem mass spectrometry; RCK, regulating conductance of K⁺; HEDTA, N-(2-hydroxyethyl)ethylenediaminetriacetic acid; PKA, protein kinase A.

^* This work was supported, in whole or in part, by National Institutes of Health Grant NS34383 (to J. S. T.). This work was also supported by the Deutsche Forschungsgemeinschaft Grant SFB 746, TP16 (to B. F.). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

^S The on-line version of this article (available at http://www.mcponline.org) contains supplemental material, supplemental Figs. S1–S4, and supplemental Tables S1–S4.

To whom correspondence may be addressed: Inst. of Physiology, University of Freiburg, Hermann-Herder-Strasse 7, 79104 Freiburg, Germany. E-mail: bernd.fakler{at}physiologie.uni-freiburg.de

^¶¶ To whom correspondence may be addressed: Section of Neurobiology, Physiology and Behavior, College of Biological Sciences, 196 Briggs Hall, University of California, One Shields Ave., Davis, CA 95616-8519. E-mail: jtrimmer{at}ucdavis.edu

	REFERENCES

TOP ABSTRACT EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 

1. Hille, B. (2001 ) Ionic channels of excitable membranes, 3rd Ed., Sinauer, Sunderland, MA

2. Shipston, M. J. (2001 ) Alternative splicing of potassium channels: a dynamic switch of cellular excitability. Trends Cell Biol. 11, 353 –358[CrossRef][Medline]

3. Cantrell, A. R., and Catterall, W. A. (2001 ) Neuromodulation of Na⁺ channels: an unexpected form of cellular plasticity. Nat. Rev. Neurosci. 2, 397 –407[Medline]

4. Coetzee, W. A., Amarillo, Y., Chiu, J., Chow, A., Lau, D., McCormack, T., Moreno, H., Nadal, M. S., Ozaita, A., Pountney, D., Saganich, M., Vega-Saenz de Miera, E., and Rudy, B. (1999 ) Molecular diversity of K⁺ channels. Ann. N. Y. Acad. Sci. 868, 233 –285[CrossRef][Medline]

5. Fury, M., Marx, S. O., and Marks, A. R. (2002 ) Molecular BKology: the study of splicing and dicing. Sci STKE 2002, PE12

6. Gray, A. C., Raingo, J., and Lipscombe, D. (2007 ) Neuronal calcium channels: splicing for optimal performance. Cell Calcium 42, 409 –417[CrossRef][Medline]

7. Park, K. S., Yang, J. W., Seikel, E., and Trimmer, J. S. (2008 ) Potassium channel phosphorylation in excitable cells: providing dynamic functional variability to a diverse family of ion channels. Physiology 23, 49 –57[Abstract/Free Full Text]

8. Schubert, R., and Nelson, M. T. (2001 ) Protein kinases: tuners of the BKCa channel in smooth muscle. Trends Pharmacol. Sci. 22, 505 –512[CrossRef][Medline]

9. Ghatta, S., Nimmagadda, D., Xu, X., and O'Rourke, S. T. (2006 ) Large-conductance, calcium-activated potassium channels: structural and functional implications. Pharmacol. Ther. 110, 103 –116[CrossRef][Medline]

10. Gribkoff, V. K., Starrett, J. E., Jr., and Dworetzky, S. I. (2001 ) Maxi-K potassium channels: form, function, and modulation of a class of endogenous regulators of intracellular calcium. Neuroscientist 7, 166 –177[Abstract/Free Full Text]

11. Lu, R., Alioua, A., Kumar, Y., Eghbali, M., Stefani, E., and Toro, L. (2006 ) MaxiK channel partners: physiological impact. J. Physiol. 570, 65 –72[Abstract/Free Full Text]

12. Salkoff, L., Butler, A., Ferreira, G., Santi, C., and Wei, A. (2006 ) High-conductance potassium channels of the SLO family. Nat. Rev. Neurosci. 7, 921 –931[CrossRef][Medline]

13. Shao, L. R., Halvorsrud, R., Borg-Graham, L., and Storm, J. F. (1999 ) The role of BK-type Ca²⁺-dependent K⁺ channels in spike broadening during repetitive firing in rat hippocampal pyramidal cells. J. Physiol. 521, 135 –146[Abstract/Free Full Text]

14. Womack, M. D., and Khodakhah, K. (2002 ) Characterization of large conductance Ca²⁺-activated K⁺ channels in cerebellar Purkinje neurons. Eur. J. Neurosci. 16, 1214 –1222[CrossRef][Medline]

15. Golding, N. L., Jung, H. Y., Mickus, T., and Spruston, N. (1999 ) Dendritic calcium spike initiation and repolarization are controlled by distinct potassium channel subtypes in CA1 pyramidal neurons. J. Neurosci. 19, 8789 –8798[Abstract/Free Full Text]

16. Raffaelli, G., Saviane, C., Mohajerani, M. H., Pedarzani, P., and Cherubini, E. (2004 ) BK potassium channels control transmitter release at CA3-CA3 synapses in the rat hippocampus. J. Physiol. 557, 147 –157[Abstract/Free Full Text]

17. Hu, H., Shao, L. R., Chavoshy, S., Gu, N., Trieb, M., Behrens, R., Laake, P., Pongs, O., Knaus, H. G., Ottersen, O. P., and Storm, J. F. (2001 ) Presynaptic Ca²⁺-activated K⁺ channels in glutamatergic hippocampal terminals and their role in spike repolarization and regulation of transmitter release. J. Neurosci. 21, 9585 –9597[Abstract/Free Full Text]

18. Sausbier, U., Sausbier, M., Sailer, C. A., Arntz, C., Knaus, H. G., Neuhuber, W., and Ruth, P. (2006 ) Ca²⁺-activated K⁺ channels of the BK-type in the mouse brain. Histochem. Cell Biol. 125, 725 –741[CrossRef][Medline]

19. Lin, M. T., Hessinger, D. A., Pearce, W. J., and Longo, L. D. (2006 ) Modulation of BK channel calcium affinity by differential phosphorylation in developing ovine basilar artery myocytes. Am. J. Physiol. Heart Circ. Physiol. 291, H732 –H740[Abstract/Free Full Text]

20. MacDonald, S. H., Ruth, P., Knaus, H. G., and Shipston, M. J. (2006 ) Increased large conductance calcium-activated potassium (BK) channel expression accompanied by STREX variant down-regulation in the developing mouse CNS. BMC Dev. Biol. 6, 37[CrossRef][Medline]

21. Khan, R. N., Smith, S. K., Morrison, J. J., and Ashford, M. L. (1993 ) Properties of large-conductance K⁺ channels in human myometrium during pregnancy and labour. Proc. Biol. Sci. 251, 9 –15[Abstract/Free Full Text]

22. Fodor, A. A., and Aldrich, R. W. (2006 ) Statistical limits to the identification of ion channel domains by sequence similarity. J. Gen. Physiol. 127, 755 –766[Abstract/Free Full Text]

23. Jiang, Y., Lee, A., Chen, J., Cadene, M., Chait, B. T., and MacKinnon, R. (2002 ) Crystal structure and mechanism of a calcium-gated potassium channel. Nature 417, 515 –522[CrossRef][Medline]

24. Jiang, Y., Pico, A., Cadene, M., Chait, B. T., and MacKinnon, R. (2001 ) Structure of the RCK domain from the E. coli K⁺ channel and demonstration of its presence in the human BK channel. Neuron 29, 593 –601[CrossRef][Medline]

25. Kim, H. J., Lim, H. H., Rho, S. H., Eom, S. H., and Park, C. S. (2006 ) Hydrophobic interface between two regulators of K+ conductance domains critical for calcium-dependent activation of large conductance Ca²⁺-activated K⁺ channels. J. Biol. Chem. 281, 38573 –38581[Abstract/Free Full Text]

26. Schreiber, M., and Salkoff, L. (1997 ) A novel calcium-sensing domain in the BK channel. Biophys. J. 73, 1355 –1363[Medline]

27. White, R. E., Schonbrunn, A., and Armstrong, D. L. (1991 ) Somatostatin stimulates Ca²⁺-activated K⁺ channels through protein dephosphorylation. Nature 351, 570 –573[CrossRef][Medline]

28. Reinhart, P. H., Chung, S., Martin, B. L., Brautigan, D. L., and Levitan, I. B. (1991 ) Modulation of calcium-activated potassium channels from rat brain by protein kinase A and phosphatase 2A. J. Neurosci. 11, 1627 –1635[Abstract]

29. White, R. E., Lee, A. B., Shcherbatko, A. D., Lincoln, T. M., Schonbrunn, A., and Armstrong, D. L. (1993 ) Potassium channel stimulation by natriuretic peptides through cGMP-dependent dephosphorylation. Nature 361, 263 –266[CrossRef][Medline]

30. Esguerra, M., Wang, J., Foster, C. D., Adelman, J. P., North, R. A., and Levitan, I. B. (1994 ) Cloned Ca²⁺-dependent K⁺ channel modulated by a functionally associated protein kinase. Nature 369, 563 –565[CrossRef][Medline]

31. Lee, K., Rowe, I. C., and Ashford, M. L. (1995 ) Characterization of an ATP-modulated large conductance Ca²⁺-dependent K⁺ channel present in rat cortical neurons. J. Physiol. (Lond.) 488, 319 –337[Abstract/Free Full Text]

32. Widmer, H. A., Rowe, I. C., and Shipston, M. J. (2003 ) Conditional protein phosphorylation regulates BK channel activity in rat cerebellar Purkinje neurons. J. Physiol. 552, 379 –391[Abstract/Free Full Text]

33. Tseng-Crank, J., Foster, C. D., Krause, J. D., Mertz, R., Godinot, N., DiChiara, T. J., and Reinhart, P. H. (1994 ) Cloning, expression, and distribution of functionally distinct Ca²⁺-dependent K⁺ channel isoforms from human brain. Neuron 13, 1315 –1330[CrossRef][Medline]

34. Beisel, K. W., Rocha-Sanchez, S. M., Ziegenbein, S. J., Morris, K. A., Kai, C., Kawai, J., Carninci, P., Hayashizaki, Y., and Davis, R. L. (2007 ) Diversity of Ca²⁺-dependent K⁺ channel transcripts in inner ear hair cells. Gene 386, 11 –23[CrossRef][Medline]

35. Trimmer, J. S. (1991 ) Immunological identification and characterization of a delayed rectifier K⁺ channel polypeptide in rat brain. Proc. Natl. Acad. Sci. U. S. A. 88, 10764 –10768[Abstract/Free Full Text]

36. Pyott, S. J., Glowatzki, E., Trimmer, J. S., and Aldrich, R. W. (2004 ) Extrasynaptic localization of inactivating calcium-activated potassium channels in mouse inner hair cells. J. Neurosci. 24, 9469 –9474[Abstract/Free Full Text]

37. Misonou, H., Menegola, M., Buchwalder, L., Park, E. W., Meredith, A., Rhodes, K. J., Aldrich, R. W., and Trimmer, J. S. (2006 ) Immunolocalization of the Ca²⁺-dependent K⁺ channel Slo1 in axons and nerve terminals of mammalian brain and cultured neurons. J. Comp. Neurol. 496, 289 –302[CrossRef][Medline]

38. Berkefeld, H., Sailer, C. A., Bildl, W., Rohde, V., Thumfart, J. O., Eble, S., Klugbauer, N., Reisinger, E., Bischofberger, J., Oliver, D., Knaus, H. G., Schulte, U., and Fakler, B. (2006 ) BKCa-Cav channel complexes mediate rapid and localized Ca²⁺-dependent K⁺ signaling. Science 314, 615 –620[Abstract/Free Full Text]

39. Schulte, U., Thumfart, J. O., Klocker, N., Sailer, C. A., Bildl, W., Biniossek, M., Dehn, D., Deller, T., Eble, S., Abbass, K., Wangler, T., Knaus, H. G., and Fakler, B. (2006 ) The epilepsy-linked Lgi1 protein assembles into presynaptic Kv1 channels and inhibits inactivation by Kvbeta1. Neuron 49, 697 –706[CrossRef][Medline]

40. Pandey, A., Andersen, J. S., and Mann, M. (2000 ) Use of mass spectrometry to study signaling pathways. Sci. STKE 2000, PL1

41. Olsen, J. V., Blagoev, B., Gnad, F., Macek, B., Kumar, C., Mortensen, P., and Mann, M. (2006 ) Global, in vivo, and site-specific phosphorylation dynamics in signaling networks. Cell 127, 635 –648[CrossRef][Medline]

42. Thingholm, T. E., Jorgensen, T. J., Jensen, O. N., and Larsen, M. R. (2006 ) Highly selective enrichment of phosphorylated peptides using titanium dioxide. Nat. Protoc. 1, 1929 –1935[CrossRef][Medline]

43. Olsen, J. V., de Godoy, L. M., Li, G., Macek, B., Mortensen, P., Pesch, R., Makarov, A., Lange, O., Horning, S., and Mann, M. (2005 ) Parts per million mass accuracy on an Orbitrap mass spectrometer via lock mass injection into a C-trap. Mol. Cell. Proteomics 4, 2010 –2021[Abstract/Free Full Text]

44. Schroeder, M. J., Shabanowitz, J., Schwartz, J. C., Hunt, D. F., and Coon, J. J. (2004 ) A neutral loss activation method for improved phosphopeptide sequence analysis by quadrupole ion trap mass spectrometry. Anal. Chem. 76, 3590 –3598[Medline]

45. Meera, P., Wallner, M., Song, M., and Toro, L. (1997 ) Large conductance voltage- and calcium-dependent K⁺ channel, a distinct member of voltage-dependent ion channels with seven N-terminal transmembrane segments (S0–S6), an extracellular N terminus, and an intracellular (S9–S10) C terminus. Proc. Natl. Acad. Sci. U. S. A. 94, 14066 –14071[Abstract/Free Full Text]

46. Xie, J., and McCobb, D. P. (1998 ) Control of alternative splicing of potassium channels by stress hormones. Science 280, 443 –446[Abstract/Free Full Text]

47. Qian, X., Niu, X., and Magleby, K. L. (2006 ) Intra- and intersubunit cooperativity in activation of BK channels by Ca²⁺. J. Gen. Physiol. 128, 389 –404[Abstract/Free Full Text]

48. Park, K. S., Mohapatra, D. P., Misonou, H., and Trimmer, J. S. (2006 ) Graded regulation of the Kv2.1 potassium channel by variable phosphorylation. Science 313, 976 –979[Abstract/Free Full Text]

49. Zhou, X. B., Arntz, C., Kamm, S., Motejlek, K., Sausbier, U., Wang, G. X., Ruth, P., and Korth, M. (2001 ) A molecular switch for specific stimulation of the BKCa channel by cGMP and cAMP kinase. J. Biol. Chem. 276, 43239 –43245[Abstract/Free Full Text]

50. Caillaud, A., Hovanessian, A. G., Levy, D. E., and Marie, I. J. (2005 ) Regulatory serine residues mediate phosphorylation-dependent and phosphorylation-indepen-dent activation of interferon regulatory factor 7. J. Biol. Chem. 280, 17671 –17677[Abstract/Free Full Text]

51. Eldar-Finkelman, H., Argast, G. M., Foord, O., Fischer, E. H., and Krebs, E. G. (1996 ) Expression and characterization of glycogen synthase kinase-3 mutants and their effect on glycogen synthase activity in intact cells. Proc. Natl. Acad. Sci. U. S. A. 93, 10228 –10233[Abstract/Free Full Text]

52. Gunter, F. (2000 ) Chemical aspects of peptide bond isomerization. Chem. Soc. Rev. 29, 119 –127[CrossRef]

53. Shao, J., Prince, T., Hartson, S. D., and Matts, R. L. (2003 ) Phosphorylation of serine 13 is required for the proper function of the Hsp90 co-chaperone, Cdc37. J. Biol. Chem. 278, 38117 –38120[Abstract/Free Full Text]

54. Park, K. S., Mohapatra, D. P., and Trimmer, J. S. (2007 ) Proteomic analyses of Kv2.1 channel phosphorylation sites determining cell background-specific differences in function. Channels 1, 59 –61[Medline]

55. Fukao, M., Mason, H. S., Britton, F. C., Kenyon, J. L., Horowitz, B., and Keef, K. D. (1999 ) Cyclic GMP-dependent protein kinase activates cloned BKCa channels expressed in mammalian cells by direct phosphorylation at serine 1072. J. Biol. Chem. 274, 10927 –10935[Abstract/Free Full Text]

56. Paarmann, I., Schmitt, B., Meyer, B., Karas, M., and Betz, H. (2006 ) Mass spectrometric analysis of glycine receptor-associated gephyrin splice variants. J. Biol. Chem. 281, 34918 –34925[Abstract/Free Full Text]

57. McCartney, C. E., McClafferty, H., Huibant, J. M., Rowan, E. G., Shipston, M. J., and Rowe, I. C. (2005 ) A cysteine-rich motif confers hypoxia sensitivity to mammalian large conductance voltage- and Ca²⁺-activated K⁺ (BK) channel subunits. Proc. Natl. Acad. Sci. U. S. A. 102, 17870 –17876[Abstract/Free Full Text]

58. Chen, L., Tian, L., MacDonald, S. H., McClafferty, H., Hammond, M. S., Huibant, J. M., Ruth, P., Knaus, H. G., and Shipston, M. J. (2005 ) Functionally diverse complement of large conductance calcium- and voltage-activated potassium channel (BK) subunits generated from a single site of splicing. J. Biol. Chem. 280, 33599 –33609[Abstract/Free Full Text]

59. Ha, T. S., Jeong, S. Y., Cho, S. W., Jeon, H., Roh, G. S., Choi, W. S., and Park, C. S. (2000 ) Functional characteristics of two BKCa channel variants differentially expressed in rat brain tissues. Eur. J. Biochem. 267, 910 –918[Medline]

60. Ma, D., Nakata, T., Zhang, G., Hoshi, T., Li, M., and Shikano, S. (2007 ) Differential trafficking of carboxyl isoforms of Ca²⁺-gated (Slo1) potassium channels. FEBS Lett. 581, 1000 –1008[CrossRef][Medline]

61. Kim, E. Y., Ridgway, L. D., Zou, S., Chiu, Y. H., and Dryer, S. E. (2007 ) Alternatively spliced C-terminal domains regulate the surface expression of large conductance calcium-activated potassium channels. Neuroscience 146, 1652 –1661[CrossRef][Medline]

62. Chang, C. P., Dworetzky, S. I., Wang, J., and Goldstein, M. E. (1997 ) Differential expression of the and β subunits of the large-conductance calcium-activated potassium channel: implication for channel diversity. Brain Res. Mol. Brain Res. 45, 33 –40[Medline]

63. Sailer, C. A., Kaufmann, W. A., Kogler, M., Chen, L., Sausbier, U., Ottersen, O. P., Ruth, P., Shipston, M. J., and Knaus, H. G. (2006 ) Immunolocalization of BK channels in hippocampal pyramidal neurons. Eur. J. Neurosci. 24, 442 –454[CrossRef][Medline]

64. Grunnet, M., and Kaufmann, W. A. (2004 ) Coassembly of big conductance Ca²⁺-dependent K⁺ channels and L-type voltage-gated Ca²⁺ channels in rat brain. J. Biol. Chem. 279, 36445 –36453[Abstract/Free Full Text]

65. Xia, X. M., Zeng, X., and Lingle, C. J. (2002 ) Multiple regulatory sites in large-conductance calcium-activated potassium channels. Nature 418, 880 –884[CrossRef][Medline]

66. Yusifov, T., Savalli, N., Gandhi, C. S., Ottolia, M., and Olcese, R. (2008 ) The RCK2 domain of the human BKCa channel is a calcium sensor. Proc. Natl. Acad. Sci. U. S. A. 105, 376 –381[Abstract/Free Full Text]

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