Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry

Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry

Neuropeptides are synthesized in and released from neurons and are involved in a wide range of physiological processes, including temperature homeostasis, learning, memory, and disease. When working with sparse neuronal networks, the ability to collect and characterize small sample volumes is import...

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Main Authors: Croushore C., Supharoek S., Lee C., Jakmunee J., Sweedler J.
Format: Journal
Published: 2017
Online Access:https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=84868599887&origin=inward
http://cmuir.cmu.ac.th/jspui/handle/6653943832/42732
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Institution: Chiang Mai University
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spelling th-cmuir.6653943832-427322017-09-28T06:38:09Z Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry Croushore C. Supharoek S. Lee C. Jakmunee J. Sweedler J. Neuropeptides are synthesized in and released from neurons and are involved in a wide range of physiological processes, including temperature homeostasis, learning, memory, and disease. When working with sparse neuronal networks, the ability to collect and characterize small sample volumes is important as neurons often release only a small proportion of their mass-limited content. Microfluidic systems are well suited for the study of neuropeptides. They offer the ability to control and manipulate the extracellular environment and small sample volumes, thereby reducing the dilution of peptides following release. We present an approach for the culture and stimulation of a neuronal network within a microfluidic device, subsequent collection of the released peptides, and their detection via mass spectrometry. The system employs microvalve-controlled stimulation channels to selectively stimulate a low-density neuronal culture, allowing us to determine the temporal onset of peptide release. Released peptides from the well-characterized, peptidergic bag cell neurons of Aplysia californica were collected and their temporal pattern of release was characterized with matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. We show a robust difference in the timing of release for chemical solutions containing elevated K + (7 ± 3 min), when compared to insulin (19 ± 7 min) (p < 0.000 01). © 2012 American Chemical Society. 2017-09-28T06:38:09Z 2017-09-28T06:38:09Z 2012-11-06 Journal 00032700 2-s2.0-84868599887 10.1021/ac302283u https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=84868599887&origin=inward http://cmuir.cmu.ac.th/jspui/handle/6653943832/42732
institution Chiang Mai University
building Chiang Mai University Library
country Thailand
collection CMU Intellectual Repository
description Neuropeptides are synthesized in and released from neurons and are involved in a wide range of physiological processes, including temperature homeostasis, learning, memory, and disease. When working with sparse neuronal networks, the ability to collect and characterize small sample volumes is important as neurons often release only a small proportion of their mass-limited content. Microfluidic systems are well suited for the study of neuropeptides. They offer the ability to control and manipulate the extracellular environment and small sample volumes, thereby reducing the dilution of peptides following release. We present an approach for the culture and stimulation of a neuronal network within a microfluidic device, subsequent collection of the released peptides, and their detection via mass spectrometry. The system employs microvalve-controlled stimulation channels to selectively stimulate a low-density neuronal culture, allowing us to determine the temporal onset of peptide release. Released peptides from the well-characterized, peptidergic bag cell neurons of Aplysia californica were collected and their temporal pattern of release was characterized with matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. We show a robust difference in the timing of release for chemical solutions containing elevated K + (7 ± 3 min), when compared to insulin (19 ± 7 min) (p < 0.000 01). © 2012 American Chemical Society.
format Journal
author Croushore C.
Supharoek S.
Lee C.
Jakmunee J.
Sweedler J.
spellingShingle Croushore C.
Supharoek S.
Lee C.
Jakmunee J.
Sweedler J.
Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
author_facet Croushore C.
Supharoek S.
Lee C.
Jakmunee J.
Sweedler J.
author_sort Croushore C.
title Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
title_short Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
title_full Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
title_fullStr Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
title_full_unstemmed Microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
title_sort microfluidic device for the selective chemical stimulation of neurons and characterization of peptide release with mass spectrometry
publishDate 2017
url https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=84868599887&origin=inward
http://cmuir.cmu.ac.th/jspui/handle/6653943832/42732
_version_ 1681422245098946560

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