Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.

Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.

Proteolytic processing of mutant huntingtin (mHtt), the protein that causes Huntington's disease (HD), is critical for mHtt toxicity and disease progression. mHtt contains several caspase and calpain cleavage sites that generate N-terminal fragments that are more toxic than full-length mHtt. Fu...

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Main Authors: Amber L Southwell, Charles W Bugg, Linda S Kaltenbach, Denise Dunn, Stefanie Butland, Andreas Weiss, Paolo Paganetti, Donald C Lo, Paul H Patterson
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2011-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3031625?pdf=render
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spelling doaj-83d61df88355459e91c3326b3f7f65cd2020-11-25T02:46:54ZengPublic Library of Science (PLoS)PLoS ONE1932-62032011-01-0161e1667610.1371/journal.pone.0016676Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.Amber L SouthwellCharles W BuggLinda S KaltenbachDenise DunnStefanie ButlandAndreas WeissPaolo PaganettiDonald C LoPaul H PattersonProteolytic processing of mutant huntingtin (mHtt), the protein that causes Huntington's disease (HD), is critical for mHtt toxicity and disease progression. mHtt contains several caspase and calpain cleavage sites that generate N-terminal fragments that are more toxic than full-length mHtt. Further processing is then required for the degradation of these fragments, which in turn, reduces toxicity. This unknown, secondary degradative process represents a promising therapeutic target for HD.We have used intrabodies, intracellularly expressed antibody fragments, to gain insight into the mechanism of mutant huntingtin exon 1 (mHDx-1) clearance. Happ1, an intrabody recognizing the proline-rich region of mHDx-1, reduces the level of soluble mHDx-1 by increasing clearance. While proteasome and macroautophagy inhibitors reduce turnover of mHDx-1, Happ1 is still able to reduce mHDx-1 under these conditions, indicating Happ1-accelerated mHDx-1 clearance does not rely on these processes. In contrast, a calpain inhibitor or an inhibitor of lysosomal pH block Happ1-mediated acceleration of mHDx-1 clearance. These results suggest that mHDx-1 is cleaved by calpain, likely followed by lysosomal degradation and this process regulates the turnover rate of mHDx-1. Sequence analysis identifies amino acid (AA) 15 as a potential calpain cleavage site. Calpain cleavage of recombinant mHDx-1 in vitro yields fragments of sizes corresponding to this prediction. Moreover, when the site is blocked by binding of another intrabody, V(L)12.3, turnover of soluble mHDx-1 in living cells is blocked.These results indicate that calpain-mediated removal of the 15 N-terminal AAs is required for the degradation of mHDx-1, a finding that may have therapeutic implications.http://europepmc.org/articles/PMC3031625?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Amber L Southwell
Charles W Bugg
Linda S Kaltenbach
Denise Dunn
Stefanie Butland
Andreas Weiss
Paolo Paganetti
Donald C Lo
Paul H Patterson
spellingShingle Amber L Southwell
Charles W Bugg
Linda S Kaltenbach
Denise Dunn
Stefanie Butland
Andreas Weiss
Paolo Paganetti
Donald C Lo
Paul H Patterson
Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
PLoS ONE
author_facet Amber L Southwell
Charles W Bugg
Linda S Kaltenbach
Denise Dunn
Stefanie Butland
Andreas Weiss
Paolo Paganetti
Donald C Lo
Paul H Patterson
author_sort Amber L Southwell
title Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
title_short Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
title_full Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
title_fullStr Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
title_full_unstemmed Perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
title_sort perturbation with intrabodies reveals that calpain cleavage is required for degradation of huntingtin exon 1.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2011-01-01
description Proteolytic processing of mutant huntingtin (mHtt), the protein that causes Huntington's disease (HD), is critical for mHtt toxicity and disease progression. mHtt contains several caspase and calpain cleavage sites that generate N-terminal fragments that are more toxic than full-length mHtt. Further processing is then required for the degradation of these fragments, which in turn, reduces toxicity. This unknown, secondary degradative process represents a promising therapeutic target for HD.We have used intrabodies, intracellularly expressed antibody fragments, to gain insight into the mechanism of mutant huntingtin exon 1 (mHDx-1) clearance. Happ1, an intrabody recognizing the proline-rich region of mHDx-1, reduces the level of soluble mHDx-1 by increasing clearance. While proteasome and macroautophagy inhibitors reduce turnover of mHDx-1, Happ1 is still able to reduce mHDx-1 under these conditions, indicating Happ1-accelerated mHDx-1 clearance does not rely on these processes. In contrast, a calpain inhibitor or an inhibitor of lysosomal pH block Happ1-mediated acceleration of mHDx-1 clearance. These results suggest that mHDx-1 is cleaved by calpain, likely followed by lysosomal degradation and this process regulates the turnover rate of mHDx-1. Sequence analysis identifies amino acid (AA) 15 as a potential calpain cleavage site. Calpain cleavage of recombinant mHDx-1 in vitro yields fragments of sizes corresponding to this prediction. Moreover, when the site is blocked by binding of another intrabody, V(L)12.3, turnover of soluble mHDx-1 in living cells is blocked.These results indicate that calpain-mediated removal of the 15 N-terminal AAs is required for the degradation of mHDx-1, a finding that may have therapeutic implications.
url http://europepmc.org/articles/PMC3031625?pdf=render
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