Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.

Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.

Here, we present a highly sensitive method to study protein-protein interactions and subcellular location selectively for active multicomponent enzymes. We apply the method on γ-secretase, the enzyme complex that catalyzes the cleavage of the amyloid precursor protein (APP) to generate amyloid β-pep...

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Main Authors: Sophia Schedin-Weiss, Mitsuhiro Inoue, Yasuhiro Teranishi, Natsuko Goto Yamamoto, Helena Karlström, Bengt Winblad, Lars O Tjernberg
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23717518/pdf/?tool=EBI
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spelling doaj-b9e640dc4365438a8b633674be6a50c62021-03-03T20:22:57ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-0185e6396210.1371/journal.pone.0063962Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.Sophia Schedin-WeissMitsuhiro InoueYasuhiro TeranishiNatsuko Goto YamamotoHelena KarlströmBengt WinbladLars O TjernbergHere, we present a highly sensitive method to study protein-protein interactions and subcellular location selectively for active multicomponent enzymes. We apply the method on γ-secretase, the enzyme complex that catalyzes the cleavage of the amyloid precursor protein (APP) to generate amyloid β-peptide (Aβ), the major causative agent in Alzheimer disease (AD). The novel assay is based on proximity ligation, which can be used to study protein interactions in situ with very high sensitivity. In traditional proximity ligation assay (PLA), primary antibody recognition is typically accompanied by oligonucleotide-conjugated secondary antibodies as detection probes. Here, we first performed PLA experiments using antibodies against the γ-secretase components presenilin 1 (PS1), containing the catalytic site residues, and nicastrin, suggested to be involved in substrate recognition. To selectively study the interactions of active γ-secretase, we replaced one of the primary antibodies with a photoreactive γ-secretase inhibitor containing a PEG linker and a biotin group (GTB), and used oligonucleotide-conjugated streptavidin as a probe. Interestingly, significantly fewer interactions were detected with the latter, novel, assay, which is a reasonable finding considering that a substantial portion of PS1 is inactive. In addition, the PLA signals were located more peripherally when GTB was used instead of a PS1 antibody, suggesting that γ-secretase matures distal from the perinuclear ER region. This novel technique thus enables highly sensitive protein interaction studies, determines the subcellular location of the interactions, and differentiates between active and inactive γ-secretase in intact cells. We suggest that similar PLA assays using enzyme inhibitors could be useful also for other enzyme interaction studies.https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23717518/pdf/?tool=EBI
collection DOAJ
language English
format Article
sources DOAJ
author Sophia Schedin-Weiss
Mitsuhiro Inoue
Yasuhiro Teranishi
Natsuko Goto Yamamoto
Helena Karlström
Bengt Winblad
Lars O Tjernberg
spellingShingle Sophia Schedin-Weiss
Mitsuhiro Inoue
Yasuhiro Teranishi
Natsuko Goto Yamamoto
Helena Karlström
Bengt Winblad
Lars O Tjernberg
Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
PLoS ONE
author_facet Sophia Schedin-Weiss
Mitsuhiro Inoue
Yasuhiro Teranishi
Natsuko Goto Yamamoto
Helena Karlström
Bengt Winblad
Lars O Tjernberg
author_sort Sophia Schedin-Weiss
title Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
title_short Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
title_full Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
title_fullStr Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
title_full_unstemmed Visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
title_sort visualizing active enzyme complexes using a photoreactive inhibitor for proximity ligation--application on γ-secretase.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description Here, we present a highly sensitive method to study protein-protein interactions and subcellular location selectively for active multicomponent enzymes. We apply the method on γ-secretase, the enzyme complex that catalyzes the cleavage of the amyloid precursor protein (APP) to generate amyloid β-peptide (Aβ), the major causative agent in Alzheimer disease (AD). The novel assay is based on proximity ligation, which can be used to study protein interactions in situ with very high sensitivity. In traditional proximity ligation assay (PLA), primary antibody recognition is typically accompanied by oligonucleotide-conjugated secondary antibodies as detection probes. Here, we first performed PLA experiments using antibodies against the γ-secretase components presenilin 1 (PS1), containing the catalytic site residues, and nicastrin, suggested to be involved in substrate recognition. To selectively study the interactions of active γ-secretase, we replaced one of the primary antibodies with a photoreactive γ-secretase inhibitor containing a PEG linker and a biotin group (GTB), and used oligonucleotide-conjugated streptavidin as a probe. Interestingly, significantly fewer interactions were detected with the latter, novel, assay, which is a reasonable finding considering that a substantial portion of PS1 is inactive. In addition, the PLA signals were located more peripherally when GTB was used instead of a PS1 antibody, suggesting that γ-secretase matures distal from the perinuclear ER region. This novel technique thus enables highly sensitive protein interaction studies, determines the subcellular location of the interactions, and differentiates between active and inactive γ-secretase in intact cells. We suggest that similar PLA assays using enzyme inhibitors could be useful also for other enzyme interaction studies.
url https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23717518/pdf/?tool=EBI
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