Silicon-based microelectrode arrays for stimulation and signal recording of in vitro cultured neurons

Microelectrode arrays (MEAs) for stimulation and signal recording of in vitro cultured neurons are presented. Each MEA is composed of 60 independent electrodes with 59 working ones and one reference one. These electrodes are divided into 30 pairs. Through each pair of electrodes, four independent st...

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Published inScience China. Information sciences Vol. 54; no. 10; pp. 2199 - 2208
Main Authors Pan, HaiXian, Lü, XiaoYing, Wang, ZhiGong, Ren, TianLing, Fang, Tao, Zhang, Jie, Zhou, ChangJian, Wang, LiGang
Format Journal Article
LanguageEnglish
Published Heidelberg SP Science China Press 01.10.2011
Springer Nature B.V
Subjects
Arrays
Biocompatibility
Circuit boards
Circuit design
Computer Science
Culture
Electrodes
Impedance measurement
In vitro testing
Information Systems and Communication Service
Microelectrodes
Neurons
PC12细胞
Printed circuits
Recording
Research Papers
Semiconductors
Silicon
Stimulation
体外培养
信号记录
半导体工艺
微电极阵列
神经元
细胞培养
extracellular recording
microelectrode arrays (MEAs)
stimulation and recording
neurons network
in vitro
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Summary:Microelectrode arrays (MEAs) for stimulation and signal recording of in vitro cultured neurons are presented. Each MEA is composed of 60 independent electrodes with 59 working ones and one reference one. These electrodes are divided into 30 pairs. Through each pair of electrodes, four independent states can be realized to define the accessing modes of neurons cultured on the surface of the electrodes. A total MEA covers an area of 10 mmx 10 mm. MEAs are fabricated in a silicon-based semiconductor process. An implemented MEA is bonded on a specially designed printed-circuit-board (PCB) and surrounded by a culture chamber. An impedance measurement has been made to verify the electrical characteristics of MEAs. The surface was modified to enhance the biocompatibility. A series of PC12 cells culture experiments validates the effectiveness of the modification. An extracellular signal recording experiment with acetylcholine (Ach) as a stimulant has been carried out, and the results show the feasibility of MEAs for extracellular action potential recording. Extracellular electrical stimulation and recording experiments have been carried out too. They indicate that MEAs can be used for extracellular stimulation, recording, simultaneous stimulation and recording, and isolation of PC12 cells network cultured in vitro.
Bibliography:microelectrode arrays (MEAs), extracellular recording, stimulation and recording, neurons network, in vitro
11-5847/TP
Microelectrode arrays (MEAs) for stimulation and signal recording of in vitro cultured neurons are presented. Each MEA is composed of 60 independent electrodes with 59 working ones and one reference one. These electrodes are divided into 30 pairs. Through each pair of electrodes, four independent states can be realized to define the accessing modes of neurons cultured on the surface of the electrodes. A total MEA covers an area of 10 mmx 10 mm. MEAs are fabricated in a silicon-based semiconductor process. An implemented MEA is bonded on a specially designed printed-circuit-board (PCB) and surrounded by a culture chamber. An impedance measurement has been made to verify the electrical characteristics of MEAs. The surface was modified to enhance the biocompatibility. A series of PC12 cells culture experiments validates the effectiveness of the modification. An extracellular signal recording experiment with acetylcholine (Ach) as a stimulant has been carried out, and the results show the feasibility of MEAs for extracellular action potential recording. Extracellular electrical stimulation and recording experiments have been carried out too. They indicate that MEAs can be used for extracellular stimulation, recording, simultaneous stimulation and recording, and isolation of PC12 cells network cultured in vitro.
ObjectType-Article-2
SourceType-Scholarly Journals-1
ObjectType-Feature-1
content type line 23
ISSN:1674-733X
1869-1919
DOI:10.1007/s11432-011-4384-7