Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.

Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.

In eukaryotic cells, surface expression of most type I transmembrane proteins requires translation and simultaneous insertion of the precursor protein into the endoplasmic reticulum (ER) membrane for subsequent routing to the cell surface. This co-translational translocation pathway is initiated whe...

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Main Authors: Kurt Vermeire, Thomas W Bell, Victor Van Puyenbroeck, Anne Giraut, Sam Noppen, Sandra Liekens, Dominique Schols, Enno Hartmann, Kai-Uwe Kalies, Mark Marsh
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2014-12-01
Series:PLoS Biology
Online Access:https://doi.org/10.1371/journal.pbio.1002011
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spelling doaj-a6149d961e614163a9b26be9fb51962d2021-07-02T17:19:52ZengPublic Library of Science (PLoS)PLoS Biology1544-91731545-78852014-12-011212e100201110.1371/journal.pbio.1002011Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.Kurt VermeireThomas W BellVictor Van PuyenbroeckAnne GirautSam NoppenSandra LiekensDominique ScholsEnno HartmannKai-Uwe KaliesMark MarshIn eukaryotic cells, surface expression of most type I transmembrane proteins requires translation and simultaneous insertion of the precursor protein into the endoplasmic reticulum (ER) membrane for subsequent routing to the cell surface. This co-translational translocation pathway is initiated when a hydrophobic N-terminal signal peptide (SP) on the nascent protein emerges from the ribosome, binds the cytosolic signal recognition particle (SRP), and targets the ribosome-nascent chain complex to the Sec61 translocon, a universally conserved protein-conducting channel in the ER-membrane. Despite their common function in Sec61 targeting and ER translocation, SPs have diverse but unique primary sequences. Thus, drugs that recognise SPs could be exploited to inhibit translocation of specific proteins into the ER. Here, through flow cytometric analysis the small-molecule macrocycle cyclotriazadisulfonamide (CADA) is identified as a highly selective human CD4 (hCD4) down-modulator. We show that CADA inhibits CD4 biogenesis and that this is due to its ability to inhibit co-translational translocation of CD4 into the lumen of the ER, both in cells as in a cell-free in vitro translation/translocation system. The activity of CADA maps to the cleavable N-terminal SP of hCD4. Moreover, through surface plasmon resonance analysis we were able to show direct binding of CADA to the SP of hCD4 and identify this SP as the target of our drug. Furthermore, CADA locks the SP in the translocon during a post-targeting step, possibly in a folded state, and prevents the translocation of the associated protein into the ER lumen. Instead, the precursor protein is routed to the cytosol for degradation. These findings demonstrate that a synthetic, cell-permeable small-molecule can be developed as a SP-binding drug to selectively inhibit protein translocation and to reversibly regulate the expression of specific target proteins.https://doi.org/10.1371/journal.pbio.1002011
collection DOAJ
language English
format Article
sources DOAJ
author Kurt Vermeire
Thomas W Bell
Victor Van Puyenbroeck
Anne Giraut
Sam Noppen
Sandra Liekens
Dominique Schols
Enno Hartmann
Kai-Uwe Kalies
Mark Marsh
spellingShingle Kurt Vermeire
Thomas W Bell
Victor Van Puyenbroeck
Anne Giraut
Sam Noppen
Sandra Liekens
Dominique Schols
Enno Hartmann
Kai-Uwe Kalies
Mark Marsh
Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
PLoS Biology
author_facet Kurt Vermeire
Thomas W Bell
Victor Van Puyenbroeck
Anne Giraut
Sam Noppen
Sandra Liekens
Dominique Schols
Enno Hartmann
Kai-Uwe Kalies
Mark Marsh
author_sort Kurt Vermeire
title Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
title_short Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
title_full Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
title_fullStr Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
title_full_unstemmed Signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
title_sort signal peptide-binding drug as a selective inhibitor of co-translational protein translocation.
publisher Public Library of Science (PLoS)
series PLoS Biology
issn 1544-9173
1545-7885
publishDate 2014-12-01
description In eukaryotic cells, surface expression of most type I transmembrane proteins requires translation and simultaneous insertion of the precursor protein into the endoplasmic reticulum (ER) membrane for subsequent routing to the cell surface. This co-translational translocation pathway is initiated when a hydrophobic N-terminal signal peptide (SP) on the nascent protein emerges from the ribosome, binds the cytosolic signal recognition particle (SRP), and targets the ribosome-nascent chain complex to the Sec61 translocon, a universally conserved protein-conducting channel in the ER-membrane. Despite their common function in Sec61 targeting and ER translocation, SPs have diverse but unique primary sequences. Thus, drugs that recognise SPs could be exploited to inhibit translocation of specific proteins into the ER. Here, through flow cytometric analysis the small-molecule macrocycle cyclotriazadisulfonamide (CADA) is identified as a highly selective human CD4 (hCD4) down-modulator. We show that CADA inhibits CD4 biogenesis and that this is due to its ability to inhibit co-translational translocation of CD4 into the lumen of the ER, both in cells as in a cell-free in vitro translation/translocation system. The activity of CADA maps to the cleavable N-terminal SP of hCD4. Moreover, through surface plasmon resonance analysis we were able to show direct binding of CADA to the SP of hCD4 and identify this SP as the target of our drug. Furthermore, CADA locks the SP in the translocon during a post-targeting step, possibly in a folded state, and prevents the translocation of the associated protein into the ER lumen. Instead, the precursor protein is routed to the cytosol for degradation. These findings demonstrate that a synthetic, cell-permeable small-molecule can be developed as a SP-binding drug to selectively inhibit protein translocation and to reversibly regulate the expression of specific target proteins.
url https://doi.org/10.1371/journal.pbio.1002011
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