Profiling inflammatory responses with microfluidic immunoblotting.

Rapid profiling of signaling pathways has been a long sought after goal in biological sciences and clinical medicine. To understand these signaling pathways, their protein components must be profiled. The protein components of signaling pathways are typically profiled with protein immunoblotting. Pr...

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Main Authors: Huai-Ning Chang, Pascale R Leroueil, Katherine Selwa, C J Gasper, Ryan E Tsuchida, Jason J Wang, Walker M McHugh, Timothy T Cornell, James R Baker, Sascha N Goonewardena
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3842271?pdf=render
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spelling doaj-be7941900b654783804f80ec3176e1df2020-11-24T22:03:59ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-01811e8188910.1371/journal.pone.0081889Profiling inflammatory responses with microfluidic immunoblotting.Huai-Ning ChangPascale R LeroueilKatherine SelwaC J GasperRyan E TsuchidaJason J WangWalker M McHughTimothy T CornellJames R BakerSascha N GoonewardenaRapid profiling of signaling pathways has been a long sought after goal in biological sciences and clinical medicine. To understand these signaling pathways, their protein components must be profiled. The protein components of signaling pathways are typically profiled with protein immunoblotting. Protein immunoblotting is a powerful technique but has several limitations including the large sample requirements, high amounts of antibody, and limitations in assay throughput. To overcome some of these limitations, we have designed a microfluidic protein immunoblotting device to profile multiple signaling pathways simultaneously. We show the utility of this approach by profiling inflammatory signaling pathways (NFκB, JAK-STAT, and MAPK) in cell models and human samples. The microfluidic immunoblotting device can profile proteins and protein modifications with 5380-fold less antibody compared to traditional protein immunoblotting. Additionally, this microfluidic device interfaces with commonly available immunoblotting equipment, has the ability to multiplex, and is compatible with several protein detection methodologies. We anticipate that this microfluidic device will complement existing techniques and is well suited for life science applications.http://europepmc.org/articles/PMC3842271?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Huai-Ning Chang
Pascale R Leroueil
Katherine Selwa
C J Gasper
Ryan E Tsuchida
Jason J Wang
Walker M McHugh
Timothy T Cornell
James R Baker
Sascha N Goonewardena
spellingShingle Huai-Ning Chang
Pascale R Leroueil
Katherine Selwa
C J Gasper
Ryan E Tsuchida
Jason J Wang
Walker M McHugh
Timothy T Cornell
James R Baker
Sascha N Goonewardena
Profiling inflammatory responses with microfluidic immunoblotting.
PLoS ONE
author_facet Huai-Ning Chang
Pascale R Leroueil
Katherine Selwa
C J Gasper
Ryan E Tsuchida
Jason J Wang
Walker M McHugh
Timothy T Cornell
James R Baker
Sascha N Goonewardena
author_sort Huai-Ning Chang
title Profiling inflammatory responses with microfluidic immunoblotting.
title_short Profiling inflammatory responses with microfluidic immunoblotting.
title_full Profiling inflammatory responses with microfluidic immunoblotting.
title_fullStr Profiling inflammatory responses with microfluidic immunoblotting.
title_full_unstemmed Profiling inflammatory responses with microfluidic immunoblotting.
title_sort profiling inflammatory responses with microfluidic immunoblotting.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description Rapid profiling of signaling pathways has been a long sought after goal in biological sciences and clinical medicine. To understand these signaling pathways, their protein components must be profiled. The protein components of signaling pathways are typically profiled with protein immunoblotting. Protein immunoblotting is a powerful technique but has several limitations including the large sample requirements, high amounts of antibody, and limitations in assay throughput. To overcome some of these limitations, we have designed a microfluidic protein immunoblotting device to profile multiple signaling pathways simultaneously. We show the utility of this approach by profiling inflammatory signaling pathways (NFκB, JAK-STAT, and MAPK) in cell models and human samples. The microfluidic immunoblotting device can profile proteins and protein modifications with 5380-fold less antibody compared to traditional protein immunoblotting. Additionally, this microfluidic device interfaces with commonly available immunoblotting equipment, has the ability to multiplex, and is compatible with several protein detection methodologies. We anticipate that this microfluidic device will complement existing techniques and is well suited for life science applications.
url http://europepmc.org/articles/PMC3842271?pdf=render
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