anti kv3 1b  (Alomone Labs)


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    Alomone Labs anti kv3 1b
    Anti Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    anti kv3 1b  (Alomone Labs)


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    Alomone Labs anti kv3 1b
    Anti Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    anti kv3 1b  (Alomone Labs)


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    Alomone Labs anti kv3 1b

    Anti Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse"

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    Journal: eLife

    doi: 10.7554/eLife.75219


    Figure Legend Snippet:

    Techniques Used: Knock-Out, Software

    apc 014  (Alomone Labs)


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    Alomone Labs apc 014
    Apc 014, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    kv3 1b  (Alomone Labs)


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    Alomone Labs kv3 1b
    ( A ) <t>Kv3.1</t> in the cochlear nucleus (outlined) of WT mouse at 1 month of age. ( B ) Kv3.3 in the same section of cochlear nucleus (outlined). ( C ) Overlay of Kv3.1 (green) and Kv3.3 (magenta) with DAPI (blue). ( D–F ) magnified section of cochlear nucleus showing Kv3.1 ( D ) and Kv3.3 ( E ) immunoreactivity. Images are overlayed in F. All scale bars = 100 µm. Antibodies and conditions have been independently validated previously using Kv3.1KO and Kv3.3KO tissues .
    Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/kv3 1b/product/Alomone Labs
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    kv3 1b - by Bioz Stars, 2023-09
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    1) Product Images from "Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse"

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    Journal: eLife

    doi: 10.7554/eLife.75219

    ( A ) Kv3.1 in the cochlear nucleus (outlined) of WT mouse at 1 month of age. ( B ) Kv3.3 in the same section of cochlear nucleus (outlined). ( C ) Overlay of Kv3.1 (green) and Kv3.3 (magenta) with DAPI (blue). ( D–F ) magnified section of cochlear nucleus showing Kv3.1 ( D ) and Kv3.3 ( E ) immunoreactivity. Images are overlayed in F. All scale bars = 100 µm. Antibodies and conditions have been independently validated previously using Kv3.1KO and Kv3.3KO tissues .
    Figure Legend Snippet: ( A ) Kv3.1 in the cochlear nucleus (outlined) of WT mouse at 1 month of age. ( B ) Kv3.3 in the same section of cochlear nucleus (outlined). ( C ) Overlay of Kv3.1 (green) and Kv3.3 (magenta) with DAPI (blue). ( D–F ) magnified section of cochlear nucleus showing Kv3.1 ( D ) and Kv3.3 ( E ) immunoreactivity. Images are overlayed in F. All scale bars = 100 µm. Antibodies and conditions have been independently validated previously using Kv3.1KO and Kv3.3KO tissues .

    Techniques Used:

    ( A–B ) Kv3.1 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. In addition to the spiral ganglion cell membranes, Kv3.1 was also present at the nodes of Ranvier (B, arrows). ( C ) No Kv3.1 staining was observed in the spiral ganglion cell bodies of Kv3.1KO mice. Non-specific signal was associated with the bony tissues of the modiolus, and assumed to be autofluorescence from the collagen fibers. ( D–E ) Kv3.3 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. Strong immunoreactivity was observed in the cell bodies. ( F ) Faint non-specific signal was observed in Kv3.3KO tissues, but did not appear to be associated with the spiral ganglion neurons. All scale bars = 100 µm.
    Figure Legend Snippet: ( A–B ) Kv3.1 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. In addition to the spiral ganglion cell membranes, Kv3.1 was also present at the nodes of Ranvier (B, arrows). ( C ) No Kv3.1 staining was observed in the spiral ganglion cell bodies of Kv3.1KO mice. Non-specific signal was associated with the bony tissues of the modiolus, and assumed to be autofluorescence from the collagen fibers. ( D–E ) Kv3.3 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. Strong immunoreactivity was observed in the cell bodies. ( F ) Faint non-specific signal was observed in Kv3.3KO tissues, but did not appear to be associated with the spiral ganglion neurons. All scale bars = 100 µm.

    Techniques Used: Staining

    ( A ) Current-Voltage (I–V) relationship for potassium currents in the calyx of Held terminal of WT mice (P10–P12) in control (black; n=7 terminals, 4 mice) and TEA, 1 mM (red, n=6 terminals, 5 mice; HP = –70 mV). Inset (top): Example current traces in response to voltage command of +10 mV step (grey box in IV) in WT (black) and WT +1 mM TEA (red). Scale bars = 5 nA and 20ms. Inset (lower): Bar graph of mean currents ± SD, measured on step depolarisation to +10 mV (from HP –70 mV) ±1 mM TEA. Outward Currents are significantly reduced by TEA (student’s t-test, unpaired, P =0.0386). ( B ) WT calyx AP (black trace) evoked by 100 pA step current injection; inset - diagram of recording configuration. ( C ) WT calyx AP in the presence of TEA (1 mM, red trace); inset – overlaid WT APs ±TEA (red) as indicated by dotted box (grey) around APs in B and C. ( D ) Representative AP traces from calyx terminals of WT (black), Kv3.3KO (blue), and Kv3.1KO (orange); double arrows indicate the half-width of WT AP. AP threshold is indicated by the grey dashed line. ( E ) AP half-width measured as time difference between rise and decay phases at 50% maximal amplitude. Half-width is significantly increased in TEA and in Kv3.3KO; N is individual terminals: WT N=9 from 6 animals; TEA = 7 from 5 mice; Kv3.3KO = 6 from 3 mice and Kv3.1KO = 5 from 3 mice. ( F ) AP amplitude, ( G ) AP Decay slope, ( H ) AP rise slope (10–90%) and ( I ) membrane resistance for calyceal recordings. Average data presented as mean ± SD. Statistical test (parts E-I) were one-way ANOVAs and Tukey’s post hoc for multiple comparisons, with significant Ps indicated on the graph. Figure 1—source data 1. Relates to .
    Figure Legend Snippet: ( A ) Current-Voltage (I–V) relationship for potassium currents in the calyx of Held terminal of WT mice (P10–P12) in control (black; n=7 terminals, 4 mice) and TEA, 1 mM (red, n=6 terminals, 5 mice; HP = –70 mV). Inset (top): Example current traces in response to voltage command of +10 mV step (grey box in IV) in WT (black) and WT +1 mM TEA (red). Scale bars = 5 nA and 20ms. Inset (lower): Bar graph of mean currents ± SD, measured on step depolarisation to +10 mV (from HP –70 mV) ±1 mM TEA. Outward Currents are significantly reduced by TEA (student’s t-test, unpaired, P =0.0386). ( B ) WT calyx AP (black trace) evoked by 100 pA step current injection; inset - diagram of recording configuration. ( C ) WT calyx AP in the presence of TEA (1 mM, red trace); inset – overlaid WT APs ±TEA (red) as indicated by dotted box (grey) around APs in B and C. ( D ) Representative AP traces from calyx terminals of WT (black), Kv3.3KO (blue), and Kv3.1KO (orange); double arrows indicate the half-width of WT AP. AP threshold is indicated by the grey dashed line. ( E ) AP half-width measured as time difference between rise and decay phases at 50% maximal amplitude. Half-width is significantly increased in TEA and in Kv3.3KO; N is individual terminals: WT N=9 from 6 animals; TEA = 7 from 5 mice; Kv3.3KO = 6 from 3 mice and Kv3.1KO = 5 from 3 mice. ( F ) AP amplitude, ( G ) AP Decay slope, ( H ) AP rise slope (10–90%) and ( I ) membrane resistance for calyceal recordings. Average data presented as mean ± SD. Statistical test (parts E-I) were one-way ANOVAs and Tukey’s post hoc for multiple comparisons, with significant Ps indicated on the graph. Figure 1—source data 1. Relates to .

    Techniques Used: Injection

    Individual images are identified in rows 1–6 and columns A-F, as indicated by the central labels. Four quadrants of 9 images are shown, each 3 × 3 matrix is from the named genotype and stained as specified in the title of each quadrant. The top row of each quadrant (rows 1 and 4) are single optical sections from 3 different MNTB neurons, in which their calyceal synaptic profiles are labelled with bassoon (purple) and co-labelled with either Kv3.1 or Kv3.3 antibodies (yellow): from Kv3.1KO and stained for Kv3.3 ( A1-C1 ); the Kv3.3KO stained for Kv3.1 ( D1-F1 ); WT stained for Kv3.3 ( A4-C4 ); WT stained for Kv3.1 ( D4-F4 ). In each MNTB neuron (rows 1 & 4) two synaptic regions of interest (ROI) containing bassoon are indicated by the red and green arrowheads. These magnified ROIs are displayed below (in rows 2+3 or 5+6) bordered by the same colour, respectively. The neuronal compartments are labelled: ‘post’ – postsynaptic; ‘pre’ – presynaptic; ‘term’ – synaptic terminal. In each image, the dark grey arrows point to presynaptic Kv3 labelling, and the white arrows point to postsynaptic Kv3 labelling. Scale bars are indicated for each row in column A (5 µm in rows 1 and 4: 1 µm in rows 2,3,5, and 6). Tissue was used from mice aged P28-P30.
    Figure Legend Snippet: Individual images are identified in rows 1–6 and columns A-F, as indicated by the central labels. Four quadrants of 9 images are shown, each 3 × 3 matrix is from the named genotype and stained as specified in the title of each quadrant. The top row of each quadrant (rows 1 and 4) are single optical sections from 3 different MNTB neurons, in which their calyceal synaptic profiles are labelled with bassoon (purple) and co-labelled with either Kv3.1 or Kv3.3 antibodies (yellow): from Kv3.1KO and stained for Kv3.3 ( A1-C1 ); the Kv3.3KO stained for Kv3.1 ( D1-F1 ); WT stained for Kv3.3 ( A4-C4 ); WT stained for Kv3.1 ( D4-F4 ). In each MNTB neuron (rows 1 & 4) two synaptic regions of interest (ROI) containing bassoon are indicated by the red and green arrowheads. These magnified ROIs are displayed below (in rows 2+3 or 5+6) bordered by the same colour, respectively. The neuronal compartments are labelled: ‘post’ – postsynaptic; ‘pre’ – presynaptic; ‘term’ – synaptic terminal. In each image, the dark grey arrows point to presynaptic Kv3 labelling, and the white arrows point to postsynaptic Kv3 labelling. Scale bars are indicated for each row in column A (5 µm in rows 1 and 4: 1 µm in rows 2,3,5, and 6). Tissue was used from mice aged P28-P30.

    Techniques Used: Staining

    ( A ) Superimposed calyceal EPSCs generated from each genotype (age P21-P25): wildtype (WT; black), Kv3.3KO (blue), and Kv3.1KO mice (orange). Thin lines show traces from individual neurons (each is mean of 5 EPSCs) with thick line showing the population mean for each genotype. Grey dashed line indicates the average WT amplitude; N=WT, 22 neurons (11 mice); Kv3.3KO, 22 neurons (10 mice); Kv3.1KO, 17 neurons (8 mice). Inset shows recording and stimulation configuration. ( B ) EPSC amplitude increased in the Kv3.3KO. ( C ) EPSC rise time (10–90%) no difference was found between groups (one-way ANOVA, p=0.1576). ( D ) EPSC decay tau and ( E ) EPSC total charge were increased in the Kv3.3KO relative to WT. ( F ) EPSC traces from WT, Kv3.3KO, and Kv3.1KO mice, before and after the addition of 1 mM TEA. ( Centre): EPSC amplitudes recorded before and after perfusion of TEA (1 mM); n=WT, 9 neurons (7 mice); Kv3.3KO, 6 neurons (3 mice); Kv3.1KO, 5 neurons (3 mice). ( G ) Increase in EPSC amplitude by 1 mM TEA. ( H ). The amplitude increase induced by TEA was significantly reduced in Kv3.3KO mice compared to WT. Average data presented as mean ± SD; statistics was using one-way ANOVA with Tukey’s post hoc for multiple comparisons. Kruskal-Wallis ANOVA with Dunn’s multiple corrections was used to compare change to EPSC amplitude in TEA due to a non-gaussian distribution in WT. Figure 3—source data 1. Relates to .
    Figure Legend Snippet: ( A ) Superimposed calyceal EPSCs generated from each genotype (age P21-P25): wildtype (WT; black), Kv3.3KO (blue), and Kv3.1KO mice (orange). Thin lines show traces from individual neurons (each is mean of 5 EPSCs) with thick line showing the population mean for each genotype. Grey dashed line indicates the average WT amplitude; N=WT, 22 neurons (11 mice); Kv3.3KO, 22 neurons (10 mice); Kv3.1KO, 17 neurons (8 mice). Inset shows recording and stimulation configuration. ( B ) EPSC amplitude increased in the Kv3.3KO. ( C ) EPSC rise time (10–90%) no difference was found between groups (one-way ANOVA, p=0.1576). ( D ) EPSC decay tau and ( E ) EPSC total charge were increased in the Kv3.3KO relative to WT. ( F ) EPSC traces from WT, Kv3.3KO, and Kv3.1KO mice, before and after the addition of 1 mM TEA. ( Centre): EPSC amplitudes recorded before and after perfusion of TEA (1 mM); n=WT, 9 neurons (7 mice); Kv3.3KO, 6 neurons (3 mice); Kv3.1KO, 5 neurons (3 mice). ( G ) Increase in EPSC amplitude by 1 mM TEA. ( H ). The amplitude increase induced by TEA was significantly reduced in Kv3.3KO mice compared to WT. Average data presented as mean ± SD; statistics was using one-way ANOVA with Tukey’s post hoc for multiple comparisons. Kruskal-Wallis ANOVA with Dunn’s multiple corrections was used to compare change to EPSC amplitude in TEA due to a non-gaussian distribution in WT. Figure 3—source data 1. Relates to .

    Techniques Used: Generated

    Short-term depression was accelerated and enhanced in mice lacking Kv3.3. Values shown are for parameters measured from data presented in <xref ref-type= Figure 3 for WT, Kv3.3KO and Kv3.1KO genotypes at 100 Hz to 600 Hz range. Paired pulse depression of EPSC responses recorded in MNTB neurons (EPSC 2 /EPSC 1 ) was increased in Kv3.3 KO animals during high frequency stimulation of the calyx. The increased depression was maintained throughout the stimulation train (EPSC 80 /EPSC 1 ) across all frequencies. The rate of short term-depression in EPSC amplitudes during EPSC trains (duration 800ms), measured as short-term depression (STD) decay tau was significantly increased in Kv3.3 KOs at 100 and 200 Hz compared to WT. This STD was more severe in mice lacking Kv3.3, as shown by decreased normalized steady-state EPSC amplitudes compared to WT. STD tau and steady state amplitudes were measured using a single exponential fit to normalized EPSC amplitudes throughout the 800ms stimulation trains. n=number of neurons. Values in bold are significantly different to WT (see statistics table for more detail). Data represented as mean ± SD." title="... Figure 3 for WT, Kv3.3KO and Kv3.1KO genotypes at 100 Hz ..." property="contentUrl" width="100%" height="100%"/>
    Figure Legend Snippet: Short-term depression was accelerated and enhanced in mice lacking Kv3.3. Values shown are for parameters measured from data presented in Figure 3 for WT, Kv3.3KO and Kv3.1KO genotypes at 100 Hz to 600 Hz range. Paired pulse depression of EPSC responses recorded in MNTB neurons (EPSC 2 /EPSC 1 ) was increased in Kv3.3 KO animals during high frequency stimulation of the calyx. The increased depression was maintained throughout the stimulation train (EPSC 80 /EPSC 1 ) across all frequencies. The rate of short term-depression in EPSC amplitudes during EPSC trains (duration 800ms), measured as short-term depression (STD) decay tau was significantly increased in Kv3.3 KOs at 100 and 200 Hz compared to WT. This STD was more severe in mice lacking Kv3.3, as shown by decreased normalized steady-state EPSC amplitudes compared to WT. STD tau and steady state amplitudes were measured using a single exponential fit to normalized EPSC amplitudes throughout the 800ms stimulation trains. n=number of neurons. Values in bold are significantly different to WT (see statistics table for more detail). Data represented as mean ± SD.

    Techniques Used:


    Figure Legend Snippet:

    Techniques Used: Knock-Out, Software

    kv3 1b  (Alomone Labs)


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    Alomone Labs kv3 1b
    Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    kv3 1b  (Alomone Labs)


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    Alomone Labs kv3 1b
    ( A, B ) Immunostaining of 1-month-old somatosensory cortex for AnkR (red) and <t>Kv3.1b</t> (green). Low-magnification images are shown in ( A ) and high-magnification images in ( B ). The genotypes analyzed are shown. Scalebars, 50 µm in ( A ) and 10 µm in ( B ). ( C ) Immunostaining of human cortical biopsies from two separate patients using antibodies against AnkR (red) and Kv3.1b (green), and DAPI (blue) to label nuclei (Nu). Scalebars, 10 µm. ( D ) Quantification of Kv3.1b immunofluorescence intensity in control and Ank1 F/F ;Dlx5/6-Cre mice. Error bars indicate mean ± SEM. N=3/group. ( E ) Immunoblots of brain homogenates from three one-month-old control and three 1-month-old AnkR-deficient brains using antibodies against Kv3.1b, AnkR, and NFM. ( F ) Quantification of Kv3.1b protein normalized to NFM. ( G, H ). Immunoblots of AnkR-GFP immunoprecipitations in cells co-expressing AnkR-GFP with Myc-tagged β1 spectrin, full length Flag-tagged Kv3.1b, or truncated versions of Flag-tagged Kv3.1b. The amino acids included in the Flag-tagged Kv3.1b truncation mutants are indicated. ( I ) The consensus AnkR-binding motif present in Kv3.1b and Kv3.3, but not Kv3.2. ( J ) Immunoblots of Kv3.1b, AnkR, and IgG immunoprecipitation reactions using antibodies against AnkR and Kv3.1b. ( K ) Immunostaining of ventral root nodes of Ranvier in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice using antibodies against AnkG (green), Kv7.2 (red), and neurofascin (NFasc, blue) on the left, and AnkR (green), Kv3.1b (red), and NFasc (blue) on the right. Scalebars, 1 μm. ( L ) Quantification of the percentage of nodes of Ranvier labeled for Kv7.2, Kv3.1b, AnkG, and AnkR in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice. Ank3 F/+ - Kv7 (N=two mice; n=217 nodes), Kv3.1b (N=three mice; n=301 nodes), AnkG (N=two mice; n=222 nodes), AnkR (N=three mice; n=286 nodes). Ank3 F/F ; Chat-Cre - Kv7 (N=three mice; n=252 nodes), Kv3.1b (N=three mice; n=244 nodes), AnkG (N=three mice; n=251 nodes), AnkR (N=three mice; n=249 nodes). Error bars indicate mean ± SEM.
    Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/kv3 1b/product/Alomone Labs
    Average 93 stars, based on 1 article reviews
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    Images

    1) Product Images from "Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels"

    Article Title: Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels

    Journal: eLife

    doi: 10.7554/eLife.66491

    ( A, B ) Immunostaining of 1-month-old somatosensory cortex for AnkR (red) and Kv3.1b (green). Low-magnification images are shown in ( A ) and high-magnification images in ( B ). The genotypes analyzed are shown. Scalebars, 50 µm in ( A ) and 10 µm in ( B ). ( C ) Immunostaining of human cortical biopsies from two separate patients using antibodies against AnkR (red) and Kv3.1b (green), and DAPI (blue) to label nuclei (Nu). Scalebars, 10 µm. ( D ) Quantification of Kv3.1b immunofluorescence intensity in control and Ank1 F/F ;Dlx5/6-Cre mice. Error bars indicate mean ± SEM. N=3/group. ( E ) Immunoblots of brain homogenates from three one-month-old control and three 1-month-old AnkR-deficient brains using antibodies against Kv3.1b, AnkR, and NFM. ( F ) Quantification of Kv3.1b protein normalized to NFM. ( G, H ). Immunoblots of AnkR-GFP immunoprecipitations in cells co-expressing AnkR-GFP with Myc-tagged β1 spectrin, full length Flag-tagged Kv3.1b, or truncated versions of Flag-tagged Kv3.1b. The amino acids included in the Flag-tagged Kv3.1b truncation mutants are indicated. ( I ) The consensus AnkR-binding motif present in Kv3.1b and Kv3.3, but not Kv3.2. ( J ) Immunoblots of Kv3.1b, AnkR, and IgG immunoprecipitation reactions using antibodies against AnkR and Kv3.1b. ( K ) Immunostaining of ventral root nodes of Ranvier in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice using antibodies against AnkG (green), Kv7.2 (red), and neurofascin (NFasc, blue) on the left, and AnkR (green), Kv3.1b (red), and NFasc (blue) on the right. Scalebars, 1 μm. ( L ) Quantification of the percentage of nodes of Ranvier labeled for Kv7.2, Kv3.1b, AnkG, and AnkR in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice. Ank3 F/+ - Kv7 (N=two mice; n=217 nodes), Kv3.1b (N=three mice; n=301 nodes), AnkG (N=two mice; n=222 nodes), AnkR (N=three mice; n=286 nodes). Ank3 F/F ; Chat-Cre - Kv7 (N=three mice; n=252 nodes), Kv3.1b (N=three mice; n=244 nodes), AnkG (N=three mice; n=251 nodes), AnkR (N=three mice; n=249 nodes). Error bars indicate mean ± SEM.
    Figure Legend Snippet: ( A, B ) Immunostaining of 1-month-old somatosensory cortex for AnkR (red) and Kv3.1b (green). Low-magnification images are shown in ( A ) and high-magnification images in ( B ). The genotypes analyzed are shown. Scalebars, 50 µm in ( A ) and 10 µm in ( B ). ( C ) Immunostaining of human cortical biopsies from two separate patients using antibodies against AnkR (red) and Kv3.1b (green), and DAPI (blue) to label nuclei (Nu). Scalebars, 10 µm. ( D ) Quantification of Kv3.1b immunofluorescence intensity in control and Ank1 F/F ;Dlx5/6-Cre mice. Error bars indicate mean ± SEM. N=3/group. ( E ) Immunoblots of brain homogenates from three one-month-old control and three 1-month-old AnkR-deficient brains using antibodies against Kv3.1b, AnkR, and NFM. ( F ) Quantification of Kv3.1b protein normalized to NFM. ( G, H ). Immunoblots of AnkR-GFP immunoprecipitations in cells co-expressing AnkR-GFP with Myc-tagged β1 spectrin, full length Flag-tagged Kv3.1b, or truncated versions of Flag-tagged Kv3.1b. The amino acids included in the Flag-tagged Kv3.1b truncation mutants are indicated. ( I ) The consensus AnkR-binding motif present in Kv3.1b and Kv3.3, but not Kv3.2. ( J ) Immunoblots of Kv3.1b, AnkR, and IgG immunoprecipitation reactions using antibodies against AnkR and Kv3.1b. ( K ) Immunostaining of ventral root nodes of Ranvier in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice using antibodies against AnkG (green), Kv7.2 (red), and neurofascin (NFasc, blue) on the left, and AnkR (green), Kv3.1b (red), and NFasc (blue) on the right. Scalebars, 1 μm. ( L ) Quantification of the percentage of nodes of Ranvier labeled for Kv7.2, Kv3.1b, AnkG, and AnkR in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice. Ank3 F/+ - Kv7 (N=two mice; n=217 nodes), Kv3.1b (N=three mice; n=301 nodes), AnkG (N=two mice; n=222 nodes), AnkR (N=three mice; n=286 nodes). Ank3 F/F ; Chat-Cre - Kv7 (N=three mice; n=252 nodes), Kv3.1b (N=three mice; n=244 nodes), AnkG (N=three mice; n=251 nodes), AnkR (N=three mice; n=249 nodes). Error bars indicate mean ± SEM.

    Techniques Used: Immunostaining, Immunofluorescence, Western Blot, Expressing, Binding Assay, Immunoprecipitation, Labeling

    AnkR is a scaffolding protein that binds to and stabilizes PNN-associated CAMs (including NrCAM and PlexinA4) and ion channels (including Kv3.1b) by linking them to the β1-α2 spectrin-based cytoskeleton. Loss of AnkR results in ( 1 ) altered PNN morphology including reduced WFA intensity and decreased compactness of the nets; ( 2 ) molecular changes including reduced β1 spectrin, PNN-associated NrCAM, and Kv3.1b; ( 3 ) behavioral changes including decreased anxiety-like behaviors in the open field and elevated plus maze; and ( 4 ) electrophysiological changes including decreased AP latency and threshold, broader APs with shallower and delayed AHP, and decreased firing rate during current injection.
    Figure Legend Snippet: AnkR is a scaffolding protein that binds to and stabilizes PNN-associated CAMs (including NrCAM and PlexinA4) and ion channels (including Kv3.1b) by linking them to the β1-α2 spectrin-based cytoskeleton. Loss of AnkR results in ( 1 ) altered PNN morphology including reduced WFA intensity and decreased compactness of the nets; ( 2 ) molecular changes including reduced β1 spectrin, PNN-associated NrCAM, and Kv3.1b; ( 3 ) behavioral changes including decreased anxiety-like behaviors in the open field and elevated plus maze; and ( 4 ) electrophysiological changes including decreased AP latency and threshold, broader APs with shallower and delayed AHP, and decreased firing rate during current injection.

    Techniques Used: Scaffolding, Injection


    Figure Legend Snippet:

    Techniques Used: Sequencing, Transfection, Construct, Plasmid Preparation, Immunoprecipitation, Software

    ls c322374 rrid ab 2891125  (Alomone Labs)


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    Alomone Labs ls c322374 rrid ab 2891125

    Ls C322374 Rrid Ab 2891125, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels"

    Article Title: Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels

    Journal: eLife

    doi: 10.7554/eLife.66491


    Figure Legend Snippet:

    Techniques Used: Sequencing, Transfection, Construct, Plasmid Preparation, Immunoprecipitation, Software

    apc 014 rrid ab  (Alomone Labs)


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    kv3 1b  (Alomone Labs)


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    Alomone Labs kv3 1b
    ( A, B ) Immunostaining of 1-month-old somatosensory cortex for AnkR (red) and <t>Kv3.1b</t> (green). Low-magnification images are shown in ( A ) and high-magnification images in ( B ). The genotypes analyzed are shown. Scalebars, 50 µm in ( A ) and 10 µm in ( B ). ( C ) Immunostaining of human cortical biopsies from two separate patients using antibodies against AnkR (red) and Kv3.1b (green), and DAPI (blue) to label nuclei (Nu). Scalebars, 10 µm. ( D ) Quantification of Kv3.1b immunofluorescence intensity in control and Ank1 F/F ;Dlx5/6-Cre mice. Error bars indicate mean ± SEM. N=3/group. ( E ) Immunoblots of brain homogenates from three one-month-old control and three 1-month-old AnkR-deficient brains using antibodies against Kv3.1b, AnkR, and NFM. ( F ) Quantification of Kv3.1b protein normalized to NFM. ( G, H ). Immunoblots of AnkR-GFP immunoprecipitations in cells co-expressing AnkR-GFP with Myc-tagged β1 spectrin, full length Flag-tagged Kv3.1b, or truncated versions of Flag-tagged Kv3.1b. The amino acids included in the Flag-tagged Kv3.1b truncation mutants are indicated. ( I ) The consensus AnkR-binding motif present in Kv3.1b and Kv3.3, but not Kv3.2. ( J ) Immunoblots of Kv3.1b, AnkR, and IgG immunoprecipitation reactions using antibodies against AnkR and Kv3.1b. ( K ) Immunostaining of ventral root nodes of Ranvier in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice using antibodies against AnkG (green), Kv7.2 (red), and neurofascin (NFasc, blue) on the left, and AnkR (green), Kv3.1b (red), and NFasc (blue) on the right. Scalebars, 1 μm. ( L ) Quantification of the percentage of nodes of Ranvier labeled for Kv7.2, Kv3.1b, AnkG, and AnkR in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice. Ank3 F/+ - Kv7 (N=two mice; n=217 nodes), Kv3.1b (N=three mice; n=301 nodes), AnkG (N=two mice; n=222 nodes), AnkR (N=three mice; n=286 nodes). Ank3 F/F ; Chat-Cre - Kv7 (N=three mice; n=252 nodes), Kv3.1b (N=three mice; n=244 nodes), AnkG (N=three mice; n=251 nodes), AnkR (N=three mice; n=249 nodes). Error bars indicate mean ± SEM.
    Kv3 1b, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Images

    1) Product Images from "Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels"

    Article Title: Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels

    Journal: eLife

    doi: 10.7554/eLife.66491

    ( A, B ) Immunostaining of 1-month-old somatosensory cortex for AnkR (red) and Kv3.1b (green). Low-magnification images are shown in ( A ) and high-magnification images in ( B ). The genotypes analyzed are shown. Scalebars, 50 µm in ( A ) and 10 µm in ( B ). ( C ) Immunostaining of human cortical biopsies from two separate patients using antibodies against AnkR (red) and Kv3.1b (green), and DAPI (blue) to label nuclei (Nu). Scalebars, 10 µm. ( D ) Quantification of Kv3.1b immunofluorescence intensity in control and Ank1 F/F ;Dlx5/6-Cre mice. Error bars indicate mean ± SEM. N=3/group. ( E ) Immunoblots of brain homogenates from three one-month-old control and three 1-month-old AnkR-deficient brains using antibodies against Kv3.1b, AnkR, and NFM. ( F ) Quantification of Kv3.1b protein normalized to NFM. ( G, H ). Immunoblots of AnkR-GFP immunoprecipitations in cells co-expressing AnkR-GFP with Myc-tagged β1 spectrin, full length Flag-tagged Kv3.1b, or truncated versions of Flag-tagged Kv3.1b. The amino acids included in the Flag-tagged Kv3.1b truncation mutants are indicated. ( I ) The consensus AnkR-binding motif present in Kv3.1b and Kv3.3, but not Kv3.2. ( J ) Immunoblots of Kv3.1b, AnkR, and IgG immunoprecipitation reactions using antibodies against AnkR and Kv3.1b. ( K ) Immunostaining of ventral root nodes of Ranvier in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice using antibodies against AnkG (green), Kv7.2 (red), and neurofascin (NFasc, blue) on the left, and AnkR (green), Kv3.1b (red), and NFasc (blue) on the right. Scalebars, 1 μm. ( L ) Quantification of the percentage of nodes of Ranvier labeled for Kv7.2, Kv3.1b, AnkG, and AnkR in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice. Ank3 F/+ - Kv7 (N=two mice; n=217 nodes), Kv3.1b (N=three mice; n=301 nodes), AnkG (N=two mice; n=222 nodes), AnkR (N=three mice; n=286 nodes). Ank3 F/F ; Chat-Cre - Kv7 (N=three mice; n=252 nodes), Kv3.1b (N=three mice; n=244 nodes), AnkG (N=three mice; n=251 nodes), AnkR (N=three mice; n=249 nodes). Error bars indicate mean ± SEM.
    Figure Legend Snippet: ( A, B ) Immunostaining of 1-month-old somatosensory cortex for AnkR (red) and Kv3.1b (green). Low-magnification images are shown in ( A ) and high-magnification images in ( B ). The genotypes analyzed are shown. Scalebars, 50 µm in ( A ) and 10 µm in ( B ). ( C ) Immunostaining of human cortical biopsies from two separate patients using antibodies against AnkR (red) and Kv3.1b (green), and DAPI (blue) to label nuclei (Nu). Scalebars, 10 µm. ( D ) Quantification of Kv3.1b immunofluorescence intensity in control and Ank1 F/F ;Dlx5/6-Cre mice. Error bars indicate mean ± SEM. N=3/group. ( E ) Immunoblots of brain homogenates from three one-month-old control and three 1-month-old AnkR-deficient brains using antibodies against Kv3.1b, AnkR, and NFM. ( F ) Quantification of Kv3.1b protein normalized to NFM. ( G, H ). Immunoblots of AnkR-GFP immunoprecipitations in cells co-expressing AnkR-GFP with Myc-tagged β1 spectrin, full length Flag-tagged Kv3.1b, or truncated versions of Flag-tagged Kv3.1b. The amino acids included in the Flag-tagged Kv3.1b truncation mutants are indicated. ( I ) The consensus AnkR-binding motif present in Kv3.1b and Kv3.3, but not Kv3.2. ( J ) Immunoblots of Kv3.1b, AnkR, and IgG immunoprecipitation reactions using antibodies against AnkR and Kv3.1b. ( K ) Immunostaining of ventral root nodes of Ranvier in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice using antibodies against AnkG (green), Kv7.2 (red), and neurofascin (NFasc, blue) on the left, and AnkR (green), Kv3.1b (red), and NFasc (blue) on the right. Scalebars, 1 μm. ( L ) Quantification of the percentage of nodes of Ranvier labeled for Kv7.2, Kv3.1b, AnkG, and AnkR in Ank3 F/+ and Ank3 F/F ;Chat-Cre mice. Ank3 F/+ - Kv7 (N=two mice; n=217 nodes), Kv3.1b (N=three mice; n=301 nodes), AnkG (N=two mice; n=222 nodes), AnkR (N=three mice; n=286 nodes). Ank3 F/F ; Chat-Cre - Kv7 (N=three mice; n=252 nodes), Kv3.1b (N=three mice; n=244 nodes), AnkG (N=three mice; n=251 nodes), AnkR (N=three mice; n=249 nodes). Error bars indicate mean ± SEM.

    Techniques Used: Immunostaining, Immunofluorescence, Western Blot, Expressing, Binding Assay, Immunoprecipitation, Labeling

    AnkR is a scaffolding protein that binds to and stabilizes PNN-associated CAMs (including NrCAM and PlexinA4) and ion channels (including Kv3.1b) by linking them to the β1-α2 spectrin-based cytoskeleton. Loss of AnkR results in ( 1 ) altered PNN morphology including reduced WFA intensity and decreased compactness of the nets; ( 2 ) molecular changes including reduced β1 spectrin, PNN-associated NrCAM, and Kv3.1b; ( 3 ) behavioral changes including decreased anxiety-like behaviors in the open field and elevated plus maze; and ( 4 ) electrophysiological changes including decreased AP latency and threshold, broader APs with shallower and delayed AHP, and decreased firing rate during current injection.
    Figure Legend Snippet: AnkR is a scaffolding protein that binds to and stabilizes PNN-associated CAMs (including NrCAM and PlexinA4) and ion channels (including Kv3.1b) by linking them to the β1-α2 spectrin-based cytoskeleton. Loss of AnkR results in ( 1 ) altered PNN morphology including reduced WFA intensity and decreased compactness of the nets; ( 2 ) molecular changes including reduced β1 spectrin, PNN-associated NrCAM, and Kv3.1b; ( 3 ) behavioral changes including decreased anxiety-like behaviors in the open field and elevated plus maze; and ( 4 ) electrophysiological changes including decreased AP latency and threshold, broader APs with shallower and delayed AHP, and decreased firing rate during current injection.

    Techniques Used: Scaffolding, Injection


    Figure Legend Snippet:

    Techniques Used: Sequencing, Transfection, Construct, Plasmid Preparation, Immunoprecipitation, Software

    apc 014  (Alomone Labs)


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    kv3 1b  (Alomone Labs)
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    ( A ) <t>Kv3.1</t> in the cochlear nucleus (outlined) of WT mouse at 1 month of age. ( B ) Kv3.3 in the same section of cochlear nucleus (outlined). ( C ) Overlay of Kv3.1 (green) and Kv3.3 (magenta) with DAPI (blue). ( D–F ) magnified section of cochlear nucleus showing Kv3.1 ( D ) and Kv3.3 ( E ) immunoreactivity. Images are overlayed in F. All scale bars = 100 µm. Antibodies and conditions have been independently validated previously using Kv3.1KO and Kv3.3KO tissues .
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    ls c322374 rrid ab 2891125  (Alomone Labs)
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    Alomone Labs ls c322374 rrid ab 2891125

    Ls C322374 Rrid Ab 2891125, supplied by Alomone Labs, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    ( A ) Kv3.1 in the cochlear nucleus (outlined) of WT mouse at 1 month of age. ( B ) Kv3.3 in the same section of cochlear nucleus (outlined). ( C ) Overlay of Kv3.1 (green) and Kv3.3 (magenta) with DAPI (blue). ( D–F ) magnified section of cochlear nucleus showing Kv3.1 ( D ) and Kv3.3 ( E ) immunoreactivity. Images are overlayed in F. All scale bars = 100 µm. Antibodies and conditions have been independently validated previously using Kv3.1KO and Kv3.3KO tissues .

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet: ( A ) Kv3.1 in the cochlear nucleus (outlined) of WT mouse at 1 month of age. ( B ) Kv3.3 in the same section of cochlear nucleus (outlined). ( C ) Overlay of Kv3.1 (green) and Kv3.3 (magenta) with DAPI (blue). ( D–F ) magnified section of cochlear nucleus showing Kv3.1 ( D ) and Kv3.3 ( E ) immunoreactivity. Images are overlayed in F. All scale bars = 100 µm. Antibodies and conditions have been independently validated previously using Kv3.1KO and Kv3.3KO tissues .

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques:

    ( A–B ) Kv3.1 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. In addition to the spiral ganglion cell membranes, Kv3.1 was also present at the nodes of Ranvier (B, arrows). ( C ) No Kv3.1 staining was observed in the spiral ganglion cell bodies of Kv3.1KO mice. Non-specific signal was associated with the bony tissues of the modiolus, and assumed to be autofluorescence from the collagen fibers. ( D–E ) Kv3.3 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. Strong immunoreactivity was observed in the cell bodies. ( F ) Faint non-specific signal was observed in Kv3.3KO tissues, but did not appear to be associated with the spiral ganglion neurons. All scale bars = 100 µm.

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet: ( A–B ) Kv3.1 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. In addition to the spiral ganglion cell membranes, Kv3.1 was also present at the nodes of Ranvier (B, arrows). ( C ) No Kv3.1 staining was observed in the spiral ganglion cell bodies of Kv3.1KO mice. Non-specific signal was associated with the bony tissues of the modiolus, and assumed to be autofluorescence from the collagen fibers. ( D–E ) Kv3.3 immunoreactivity spiral ganglion neurons in the WT mouse at 1 month of age. Strong immunoreactivity was observed in the cell bodies. ( F ) Faint non-specific signal was observed in Kv3.3KO tissues, but did not appear to be associated with the spiral ganglion neurons. All scale bars = 100 µm.

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques: Staining

    ( A ) Current-Voltage (I–V) relationship for potassium currents in the calyx of Held terminal of WT mice (P10–P12) in control (black; n=7 terminals, 4 mice) and TEA, 1 mM (red, n=6 terminals, 5 mice; HP = –70 mV). Inset (top): Example current traces in response to voltage command of +10 mV step (grey box in IV) in WT (black) and WT +1 mM TEA (red). Scale bars = 5 nA and 20ms. Inset (lower): Bar graph of mean currents ± SD, measured on step depolarisation to +10 mV (from HP –70 mV) ±1 mM TEA. Outward Currents are significantly reduced by TEA (student’s t-test, unpaired, P =0.0386). ( B ) WT calyx AP (black trace) evoked by 100 pA step current injection; inset - diagram of recording configuration. ( C ) WT calyx AP in the presence of TEA (1 mM, red trace); inset – overlaid WT APs ±TEA (red) as indicated by dotted box (grey) around APs in B and C. ( D ) Representative AP traces from calyx terminals of WT (black), Kv3.3KO (blue), and Kv3.1KO (orange); double arrows indicate the half-width of WT AP. AP threshold is indicated by the grey dashed line. ( E ) AP half-width measured as time difference between rise and decay phases at 50% maximal amplitude. Half-width is significantly increased in TEA and in Kv3.3KO; N is individual terminals: WT N=9 from 6 animals; TEA = 7 from 5 mice; Kv3.3KO = 6 from 3 mice and Kv3.1KO = 5 from 3 mice. ( F ) AP amplitude, ( G ) AP Decay slope, ( H ) AP rise slope (10–90%) and ( I ) membrane resistance for calyceal recordings. Average data presented as mean ± SD. Statistical test (parts E-I) were one-way ANOVAs and Tukey’s post hoc for multiple comparisons, with significant Ps indicated on the graph. Figure 1—source data 1. Relates to .

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet: ( A ) Current-Voltage (I–V) relationship for potassium currents in the calyx of Held terminal of WT mice (P10–P12) in control (black; n=7 terminals, 4 mice) and TEA, 1 mM (red, n=6 terminals, 5 mice; HP = –70 mV). Inset (top): Example current traces in response to voltage command of +10 mV step (grey box in IV) in WT (black) and WT +1 mM TEA (red). Scale bars = 5 nA and 20ms. Inset (lower): Bar graph of mean currents ± SD, measured on step depolarisation to +10 mV (from HP –70 mV) ±1 mM TEA. Outward Currents are significantly reduced by TEA (student’s t-test, unpaired, P =0.0386). ( B ) WT calyx AP (black trace) evoked by 100 pA step current injection; inset - diagram of recording configuration. ( C ) WT calyx AP in the presence of TEA (1 mM, red trace); inset – overlaid WT APs ±TEA (red) as indicated by dotted box (grey) around APs in B and C. ( D ) Representative AP traces from calyx terminals of WT (black), Kv3.3KO (blue), and Kv3.1KO (orange); double arrows indicate the half-width of WT AP. AP threshold is indicated by the grey dashed line. ( E ) AP half-width measured as time difference between rise and decay phases at 50% maximal amplitude. Half-width is significantly increased in TEA and in Kv3.3KO; N is individual terminals: WT N=9 from 6 animals; TEA = 7 from 5 mice; Kv3.3KO = 6 from 3 mice and Kv3.1KO = 5 from 3 mice. ( F ) AP amplitude, ( G ) AP Decay slope, ( H ) AP rise slope (10–90%) and ( I ) membrane resistance for calyceal recordings. Average data presented as mean ± SD. Statistical test (parts E-I) were one-way ANOVAs and Tukey’s post hoc for multiple comparisons, with significant Ps indicated on the graph. Figure 1—source data 1. Relates to .

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques: Injection

    Individual images are identified in rows 1–6 and columns A-F, as indicated by the central labels. Four quadrants of 9 images are shown, each 3 × 3 matrix is from the named genotype and stained as specified in the title of each quadrant. The top row of each quadrant (rows 1 and 4) are single optical sections from 3 different MNTB neurons, in which their calyceal synaptic profiles are labelled with bassoon (purple) and co-labelled with either Kv3.1 or Kv3.3 antibodies (yellow): from Kv3.1KO and stained for Kv3.3 ( A1-C1 ); the Kv3.3KO stained for Kv3.1 ( D1-F1 ); WT stained for Kv3.3 ( A4-C4 ); WT stained for Kv3.1 ( D4-F4 ). In each MNTB neuron (rows 1 & 4) two synaptic regions of interest (ROI) containing bassoon are indicated by the red and green arrowheads. These magnified ROIs are displayed below (in rows 2+3 or 5+6) bordered by the same colour, respectively. The neuronal compartments are labelled: ‘post’ – postsynaptic; ‘pre’ – presynaptic; ‘term’ – synaptic terminal. In each image, the dark grey arrows point to presynaptic Kv3 labelling, and the white arrows point to postsynaptic Kv3 labelling. Scale bars are indicated for each row in column A (5 µm in rows 1 and 4: 1 µm in rows 2,3,5, and 6). Tissue was used from mice aged P28-P30.

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet: Individual images are identified in rows 1–6 and columns A-F, as indicated by the central labels. Four quadrants of 9 images are shown, each 3 × 3 matrix is from the named genotype and stained as specified in the title of each quadrant. The top row of each quadrant (rows 1 and 4) are single optical sections from 3 different MNTB neurons, in which their calyceal synaptic profiles are labelled with bassoon (purple) and co-labelled with either Kv3.1 or Kv3.3 antibodies (yellow): from Kv3.1KO and stained for Kv3.3 ( A1-C1 ); the Kv3.3KO stained for Kv3.1 ( D1-F1 ); WT stained for Kv3.3 ( A4-C4 ); WT stained for Kv3.1 ( D4-F4 ). In each MNTB neuron (rows 1 & 4) two synaptic regions of interest (ROI) containing bassoon are indicated by the red and green arrowheads. These magnified ROIs are displayed below (in rows 2+3 or 5+6) bordered by the same colour, respectively. The neuronal compartments are labelled: ‘post’ – postsynaptic; ‘pre’ – presynaptic; ‘term’ – synaptic terminal. In each image, the dark grey arrows point to presynaptic Kv3 labelling, and the white arrows point to postsynaptic Kv3 labelling. Scale bars are indicated for each row in column A (5 µm in rows 1 and 4: 1 µm in rows 2,3,5, and 6). Tissue was used from mice aged P28-P30.

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques: Staining

    ( A ) Superimposed calyceal EPSCs generated from each genotype (age P21-P25): wildtype (WT; black), Kv3.3KO (blue), and Kv3.1KO mice (orange). Thin lines show traces from individual neurons (each is mean of 5 EPSCs) with thick line showing the population mean for each genotype. Grey dashed line indicates the average WT amplitude; N=WT, 22 neurons (11 mice); Kv3.3KO, 22 neurons (10 mice); Kv3.1KO, 17 neurons (8 mice). Inset shows recording and stimulation configuration. ( B ) EPSC amplitude increased in the Kv3.3KO. ( C ) EPSC rise time (10–90%) no difference was found between groups (one-way ANOVA, p=0.1576). ( D ) EPSC decay tau and ( E ) EPSC total charge were increased in the Kv3.3KO relative to WT. ( F ) EPSC traces from WT, Kv3.3KO, and Kv3.1KO mice, before and after the addition of 1 mM TEA. ( Centre): EPSC amplitudes recorded before and after perfusion of TEA (1 mM); n=WT, 9 neurons (7 mice); Kv3.3KO, 6 neurons (3 mice); Kv3.1KO, 5 neurons (3 mice). ( G ) Increase in EPSC amplitude by 1 mM TEA. ( H ). The amplitude increase induced by TEA was significantly reduced in Kv3.3KO mice compared to WT. Average data presented as mean ± SD; statistics was using one-way ANOVA with Tukey’s post hoc for multiple comparisons. Kruskal-Wallis ANOVA with Dunn’s multiple corrections was used to compare change to EPSC amplitude in TEA due to a non-gaussian distribution in WT. Figure 3—source data 1. Relates to .

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet: ( A ) Superimposed calyceal EPSCs generated from each genotype (age P21-P25): wildtype (WT; black), Kv3.3KO (blue), and Kv3.1KO mice (orange). Thin lines show traces from individual neurons (each is mean of 5 EPSCs) with thick line showing the population mean for each genotype. Grey dashed line indicates the average WT amplitude; N=WT, 22 neurons (11 mice); Kv3.3KO, 22 neurons (10 mice); Kv3.1KO, 17 neurons (8 mice). Inset shows recording and stimulation configuration. ( B ) EPSC amplitude increased in the Kv3.3KO. ( C ) EPSC rise time (10–90%) no difference was found between groups (one-way ANOVA, p=0.1576). ( D ) EPSC decay tau and ( E ) EPSC total charge were increased in the Kv3.3KO relative to WT. ( F ) EPSC traces from WT, Kv3.3KO, and Kv3.1KO mice, before and after the addition of 1 mM TEA. ( Centre): EPSC amplitudes recorded before and after perfusion of TEA (1 mM); n=WT, 9 neurons (7 mice); Kv3.3KO, 6 neurons (3 mice); Kv3.1KO, 5 neurons (3 mice). ( G ) Increase in EPSC amplitude by 1 mM TEA. ( H ). The amplitude increase induced by TEA was significantly reduced in Kv3.3KO mice compared to WT. Average data presented as mean ± SD; statistics was using one-way ANOVA with Tukey’s post hoc for multiple comparisons. Kruskal-Wallis ANOVA with Dunn’s multiple corrections was used to compare change to EPSC amplitude in TEA due to a non-gaussian distribution in WT. Figure 3—source data 1. Relates to .

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques: Generated

    Short-term depression was accelerated and enhanced in mice lacking Kv3.3. Values shown are for parameters measured from data presented in <xref ref-type= Figure 3 for WT, Kv3.3KO and Kv3.1KO genotypes at 100 Hz to 600 Hz range. Paired pulse depression of EPSC responses recorded in MNTB neurons (EPSC 2 /EPSC 1 ) was increased in Kv3.3 KO animals during high frequency stimulation of the calyx. The increased depression was maintained throughout the stimulation train (EPSC 80 /EPSC 1 ) across all frequencies. The rate of short term-depression in EPSC amplitudes during EPSC trains (duration 800ms), measured as short-term depression (STD) decay tau was significantly increased in Kv3.3 KOs at 100 and 200 Hz compared to WT. This STD was more severe in mice lacking Kv3.3, as shown by decreased normalized steady-state EPSC amplitudes compared to WT. STD tau and steady state amplitudes were measured using a single exponential fit to normalized EPSC amplitudes throughout the 800ms stimulation trains. n=number of neurons. Values in bold are significantly different to WT (see statistics table for more detail). Data represented as mean ± SD." width="100%" height="100%">

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet: Short-term depression was accelerated and enhanced in mice lacking Kv3.3. Values shown are for parameters measured from data presented in Figure 3 for WT, Kv3.3KO and Kv3.1KO genotypes at 100 Hz to 600 Hz range. Paired pulse depression of EPSC responses recorded in MNTB neurons (EPSC 2 /EPSC 1 ) was increased in Kv3.3 KO animals during high frequency stimulation of the calyx. The increased depression was maintained throughout the stimulation train (EPSC 80 /EPSC 1 ) across all frequencies. The rate of short term-depression in EPSC amplitudes during EPSC trains (duration 800ms), measured as short-term depression (STD) decay tau was significantly increased in Kv3.3 KOs at 100 and 200 Hz compared to WT. This STD was more severe in mice lacking Kv3.3, as shown by decreased normalized steady-state EPSC amplitudes compared to WT. STD tau and steady state amplitudes were measured using a single exponential fit to normalized EPSC amplitudes throughout the 800ms stimulation trains. n=number of neurons. Values in bold are significantly different to WT (see statistics table for more detail). Data represented as mean ± SD.

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques:

    Journal: eLife

    Article Title: Kv3.3 subunits control presynaptic action potential waveform and neurotransmitter release at a central excitatory synapse

    doi: 10.7554/eLife.75219

    Figure Lengend Snippet:

    Article Snippet: Afterwards primary antibodies for Kv3.1b (Rabbit, Alomone APC-014, 1:1000) and Kv3.3 (Mouse, Neuromab 75–354, 1:3000) were diluted in blocking solution and incubated overnight at 4 °C.

    Techniques: Knock-Out, Software

    Journal: eLife

    Article Title: Ankyrin-R regulates fast-spiking interneuron excitability through perineuronal nets and Kv3.1b K + channels

    doi: 10.7554/eLife.66491

    Figure Lengend Snippet:

    Article Snippet: Rabbit polyclonal antibodies against AnkR ( ) (RRID: AB_2833096 ), Ank1 (Thermo Fisher Scientific Cat# PA5-63372, RRID: AB_2638015 ), neurofilament M (Millipore Cat# AB1987, RRID: AB_91201 ), parvalbumin (Novus Cat# NB120-11427, RRID: AB_791498 ), somatostatin (Peninsula Laboratories Cat# T-4103.0050, RRID: AB_518614 ), versican (Millipore Cat# AB1032, RRID: AB_11213831 ), PlexinA4 (Abcam Cat# ab39350, RRID: AB_944890 ), neuropilin-1 (GeneTex Cat# GTX16786, RRID: AB_422398 ), Kv3.1 (LSBio (LifeSpan), Cat# LS-C322374, RRID: AB_2891125 ), Kv3.1b (Alomone Labs Cat# APC-014, RRID: AB_2040166 ), Kv3.3 (Alomone Labs Cat# APC-102, RRID: AB_2040170 ), GFP (Thermo Fisher Scientific, Cat# A-11122, RRID: AB_221569 ).

    Techniques: Sequencing, Transfection, Construct, Plasmid Preparation, Immunoprecipitation, Software