mea plate Search Results


six-well mea plates coreplatetm  (3Brain GmbH)
90
3Brain GmbH six-well mea plates coreplatetm
Six Well Mea Plates Coreplatetm, supplied by 3Brain GmbH, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pmc11744402-40-0-7?v=3Brain+GmbH
Average 90 stars, based on 1 article reviews
six-well mea plates coreplatetm - by Bioz Stars, 2026-06
90/100 stars
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twenty-four-well multiwell-mea-plates 24w300/ 30g-288  (Mcs GmbH)
90
Mcs GmbH twenty-four-well multiwell-mea-plates 24w300/ 30g-288
Twenty Four Well Multiwell Mea Plates 24w300/ 30g 288, supplied by Mcs GmbH, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pm36868403-54-3-10?v=Mcs+GmbH
Average 90 stars, based on 1 article reviews
twenty-four-well multiwell-mea-plates 24w300/ 30g-288 - by Bioz Stars, 2026-06
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mea plate med probe  (Alpha MED Scientific)
90
Alpha MED Scientific mea plate med probe
Mea Plate Med Probe, supplied by Alpha MED Scientific, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/10__15761_slash_tim__1000145-36-13-17?v=Alpha+MED+Scientific
Average 90 stars, based on 1 article reviews
mea plate med probe - by Bioz Stars, 2026-06
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12-well ld-mea plate  (Axion BioSystems)
90
Axion BioSystems 12-well ld-mea plate
Comparison of functional assays for hiPSC-based disease study.
12 Well Ld Mea Plate, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pmc11750789-37-18-20?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
12-well ld-mea plate - by Bioz Stars, 2026-06
90/100 stars
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multielectrode array (mea)  (Axion BioSystems)
90
Axion BioSystems multielectrode array (mea)
Comparison of functional assays for hiPSC-based disease study.
Multielectrode Array (Mea), supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/us10444227-122-5-3?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
multielectrode array (mea) - by Bioz Stars, 2026-06
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48-well lumos mea plate  (Axion BioSystems)
90
Axion BioSystems 48-well lumos mea plate
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
48 Well Lumos Mea Plate, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/bio_rxiv__2020__09__02__276535-416-2-19?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
48-well lumos mea plate - by Bioz Stars, 2026-06
90/100 stars
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six-well mea plate m384-tmea-6w  (Axion BioSystems)
90
Axion BioSystems six-well mea plate m384-tmea-6w
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
Six Well Mea Plate M384 Tmea 6w, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pmc07525187-118-11-14?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
six-well mea plate m384-tmea-6w - by Bioz Stars, 2026-06
90/100 stars
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24-well cytoview mea plate axion biosystems  (Axion BioSystems)
90
Axion BioSystems 24-well cytoview mea plate axion biosystems
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
24 Well Cytoview Mea Plate Axion Biosystems, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pm35442931-112-28-31?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
24-well cytoview mea plate axion biosystems - by Bioz Stars, 2026-06
90/100 stars
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low-density 24-well mea plates axion biosystems  (Axion BioSystems)
90
Axion BioSystems low-density 24-well mea plates axion biosystems
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
Low Density 24 Well Mea Plates Axion Biosystems, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pm40540399-332-7-11?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
low-density 24-well mea plates axion biosystems - by Bioz Stars, 2026-06
90/100 stars
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mea plates  (Axion BioSystems)
90
Axion BioSystems mea plates
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
Mea Plates, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/pm37814815-71-1-9?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
mea plates - by Bioz Stars, 2026-06
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mea plate lumos 48  (Axion BioSystems)
90
Axion BioSystems mea plate lumos 48
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
Mea Plate Lumos 48, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/10__7554_slash_elife__50712-409-15-19?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
mea plate lumos 48 - by Bioz Stars, 2026-06
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dry mea plates  (Axion BioSystems)
90
Axion BioSystems dry mea plates
A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well <t>MEA</t> plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light <t>(Lumos)</t> at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.
Dry Mea Plates, supplied by Axion BioSystems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/mea+plate/ppr0826053-230-12-14?v=Axion+BioSystems
Average 90 stars, based on 1 article reviews
dry mea plates - by Bioz Stars, 2026-06
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Image Search Results


Comparison of functional assays for hiPSC-based disease study.

Journal: Frontiers in Neuroscience

Article Title: Harnessing the potential of human induced pluripotent stem cells, functional assays and machine learning for neurodevelopmental disorders

doi: 10.3389/fnins.2024.1524577

Figure Lengend Snippet: Comparison of functional assays for hiPSC-based disease study.

Article Snippet: KCNQ2-associated epilepsy (R581Q variation) , , 2D cortical excitatory neurons (NGN2 transduction + dual SMAD inhibition) , 12-well LD-MEA plate (Axion Biosystems) , Daily recording from days 15 to 31 , Neurobasal media with supplement , Patch clamping , Number of bursts, number of spikes per burst, % of spikes that occur within a burst, MFR, ISI, burst frequency, burst duration, IBI , KCNQ2-mutated neurons started exhibiting spontaneous activity earlier than the isogenic control cells, while showing an increasingly phasic bursting pattern with more and higher percentage of spikes per burst and shorter interval between spikes. Applying apamin (a SK channel antagonist) and paxilline (a BK antagonist) to KCNQ2-mutated neurons rescued the network activity to the same level as the control neurons, while the control neurons with chronic XE-991 treatment, M-current inhibitor, suggesting the role of reduced M-current and ion channel dysfunction in altered network behavior in KCNQ2-mutated neurons..

Techniques: Comparison, Functional Assay, Transferring, Microscopy, Imaging, Fluorescence

How MEA was used to study NDD with hiPSC model.

Journal: Frontiers in Neuroscience

Article Title: Harnessing the potential of human induced pluripotent stem cells, functional assays and machine learning for neurodevelopmental disorders

doi: 10.3389/fnins.2024.1524577

Figure Lengend Snippet: How MEA was used to study NDD with hiPSC model.

Article Snippet: KCNQ2-associated epilepsy (R581Q variation) , , 2D cortical excitatory neurons (NGN2 transduction + dual SMAD inhibition) , 12-well LD-MEA plate (Axion Biosystems) , Daily recording from days 15 to 31 , Neurobasal media with supplement , Patch clamping , Number of bursts, number of spikes per burst, % of spikes that occur within a burst, MFR, ISI, burst frequency, burst duration, IBI , KCNQ2-mutated neurons started exhibiting spontaneous activity earlier than the isogenic control cells, while showing an increasingly phasic bursting pattern with more and higher percentage of spikes per burst and shorter interval between spikes. Applying apamin (a SK channel antagonist) and paxilline (a BK antagonist) to KCNQ2-mutated neurons rescued the network activity to the same level as the control neurons, while the control neurons with chronic XE-991 treatment, M-current inhibitor, suggesting the role of reduced M-current and ion channel dysfunction in altered network behavior in KCNQ2-mutated neurons..

Techniques: Control, Transduction, Activity Assay, Disruption, Mutagenesis, Imaging, Inhibition, In Vitro

A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well MEA plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light (Lumos) at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.

Journal: bioRxiv

Article Title: BrainPhys neuronal medium optimized for imaging and optogenetics in vitro

doi: 10.1101/2020.09.02.276535

Figure Lengend Snippet: A-E, optogenetic testing of human iPSC-derived neurons with whole-cell patch-clamp recordings. A, live image of typical neurons expressing the optogene synapsin:ChETA-YFP and filled with rhodamine from the patch pipette. B, optogenetic responses of patch-clamped human neurons to blue LED stimuli. Whole-cell patch-clamped traces of example neurons stimulated with 0.4 mW 10 × 5 ms flashes of blue light at 10 Hz in BPI and ACSF. Top traces show ChR2-mediated currents recorded in voltage-clamp at −70 mV. Bottom traces show action potential evoked by ChR2-evoked membrane depolarization in current-clamp. Corresponding raster plots highlight consistent light-evoked firing over 10 sweeps. C, quantitative comparison shown in the graphs on the right were performed from a total of 8 neurons recorded in ACSF and BPI and tested with identical light stimulation parameters as shown in the trace-examples. Symbols represent human neurons tested first (triangles) or second (circle) in either medium. D , optogenetic responses from the same patch-clamped neuron under 0.1 mW of blue light while alternating perfusate from BPI to NEUMO and back to BPI for recovery. E, quantitative comparison shown on the graphs on the right were performed from a total of 22 neurons across four coverslips. The perfusate was alternated between BPI and NEUMO. The neurons were stimulated with 10 × 5 ms flashes of blue light at 10 Hz under three different blue LED power intensities (0.1, 0.2, 0.4 mW at 475 nm). F-I, optogenetically evoked and spontaneous firing rates of human iPSC-derived neurons expressing synapsin:ChETA-YFP were recorded in a 48-well multielectrode array (MEAs) plate at 37 °C with 5% CO 2 in either BP, BPI or NEUMO basal media with identical supplements. Spontaneous and light-evoked firing rates were recorded for 10 minutes after feeding. Neurons in this dataset were cultured in standard BP for 82 days before testing different media. 240 electrodes across 15 wells were recorded over 40 days during media testing. F-G, recordings collected from one 48-well MEA plate were split into two groups of wells represented in the graph by ‘circles’ (8 wells) and ‘triangles’ (7 wells); Both groups were maintained in BP from neural maturation until they were changed to BPI on day 0. Days 7-13 were the ‘test’ period in which half the wells (7) were switched to NEUMO. From day 14, both groups were cultured in BP to recover for one week and then were switched back to BPI. H-I, optogenetics responses of human iPSC-derived neurons recorded with MEAs. The wells in NEUMO and BPI were optically stimulated with blue light (Lumos) at increasing intensities while recording on MEA. Stimulation lasted 1.1s and consisted of 10 flashes of light, each lasting 10ms at 10 Hz. The cumulative number of spikes was summed in binning windows ( H ): 27.5 ms bins ; ( I ): 2s bins starting at the onset of the first light stimulus) over three replicates. In ( H) the cumulative number spikes were plotted with quadratic non-linear curves at various LED intensity (% of max power: 3.9mW/mm 2 ). Values are shown as mean ± SEM. Significance determined via two-tailed non-parametric unpaired (Mann Whitney) tests. P-values are annotated as follows: ns for P>0.05.

Article Snippet: The 48-well Lumos MEA plate was maintained at 37°C, 5% CO 2 environment within a Maestro Pro MEA system (Axion Biosystems).

Techniques: Derivative Assay, Patch Clamp, Expressing, Transferring, Cell Culture, Optogenetics, Two Tailed Test, MANN-WHITNEY