The in Vivo TRPV6 Protein Starts at a Non-AUG Triplet, Decoded as Methionine, Upstream of Canonical Initiation at AUG

TRPV6 channels function as epithelial Ca2+ entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein relies on predicted gene coding regions and is only known to a certain level of approximation. We show that in vivo the TRPV6 protein has an exte...

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Published inThe Journal of biological chemistry Vol. 288; no. 23; pp. 16629 - 16644
Main Authors Fecher-Trost, Claudia, Wissenbach, Ulrich, Beck, Andreas, Schalkowsky, Pascal, Stoerger, Christof, Doerr, Janka, Dembek, Anna, Simon-Thomas, Martin, Weber, Armin, Wollenberg, Peter, Ruppert, Thomas, Middendorff, Ralf, Maurer, Hans H., Flockerzi, Veit
Format Journal Article
LanguageEnglish
Published United States Elsevier Inc 07.06.2013
American Society for Biochemistry and Molecular Biology
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Abstract TRPV6 channels function as epithelial Ca2+ entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein relies on predicted gene coding regions and is only known to a certain level of approximation. We show that in vivo the TRPV6 protein has an extended N terminus. Translation initiates at a non-AUG codon, at ACG, which is decoded by methionine and which is upstream of the annotated AUG, which is not used for initiation. The in vitro properties of channels formed by the extended full-length TRPV6 proteins and the so-far annotated and smaller TRPV6 are similar, but the extended N terminus increases trafficking to the plasma membrane and represents an additional scaffold for channel assembly. The increased translation of the smaller TRPV6 cDNA version may overestimate the in vivo situation where translation efficiency may represent an additional mechanism to tightly control the TRPV6-mediated Ca2+ entry to prevent deleterious Ca2+ overload. Background: The TRPV6 amino acid sequence is predicted from its cDNA. Results: The TRPV6 protein purified from human tissues has an extended N terminus not present in the predicted protein. Conclusion: Full-length TRPV6 is trafficked to the plasma membrane, and its translation efficiency tightly controls TRPV6-mediated Ca2+ entry. Significance: This study provides mechanistic insights into the function of the full-length TRPV6.
AbstractList Background: The TRPV6 amino acid sequence is predicted from its cDNA. Results: The TRPV6 protein purified from human tissues has an extended N terminus not present in the predicted protein. Conclusion: Full-length TRPV6 is trafficked to the plasma membrane, and its translation efficiency tightly controls TRPV6-mediated Ca 2+ entry. Significance: This study provides mechanistic insights into the function of the full-length TRPV6. TRPV6 channels function as epithelial Ca 2+ entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein relies on predicted gene coding regions and is only known to a certain level of approximation. We show that in vivo the TRPV6 protein has an extended N terminus. Translation initiates at a non-AUG codon, at ACG, which is decoded by methionine and which is upstream of the annotated AUG, which is not used for initiation. The in vitro properties of channels formed by the extended full-length TRPV6 proteins and the so-far annotated and smaller TRPV6 are similar, but the extended N terminus increases trafficking to the plasma membrane and represents an additional scaffold for channel assembly. The increased translation of the smaller TRPV6 cDNA version may overestimate the in vivo situation where translation efficiency may represent an additional mechanism to tightly control the TRPV6-mediated Ca 2+ entry to prevent deleterious Ca 2+ overload.
TRPV6 channels function as epithelial Ca2+ entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein relies on predicted gene coding regions and is only known to a certain level of approximation. We show that in vivo the TRPV6 protein has an extended N terminus. Translation initiates at a non-AUG codon, at ACG, which is decoded by methionine and which is upstream of the annotated AUG, which is not used for initiation. The in vitro properties of channels formed by the extended full-length TRPV6 proteins and the so-far annotated and smaller TRPV6 are similar, but the extended N terminus increases trafficking to the plasma membrane and represents an additional scaffold for channel assembly. The increased translation of the smaller TRPV6 cDNA version may overestimate the in vivo situation where translation efficiency may represent an additional mechanism to tightly control the TRPV6-mediated Ca2+ entry to prevent deleterious Ca2+ overload. Background: The TRPV6 amino acid sequence is predicted from its cDNA. Results: The TRPV6 protein purified from human tissues has an extended N terminus not present in the predicted protein. Conclusion: Full-length TRPV6 is trafficked to the plasma membrane, and its translation efficiency tightly controls TRPV6-mediated Ca2+ entry. Significance: This study provides mechanistic insights into the function of the full-length TRPV6.
TRPV6 channels function as epithelial Ca(2+) entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein relies on predicted gene coding regions and is only known to a certain level of approximation. We show that in vivo the TRPV6 protein has an extended N terminus. Translation initiates at a non-AUG codon, at ACG, which is decoded by methionine and which is upstream of the annotated AUG, which is not used for initiation. The in vitro properties of channels formed by the extended full-length TRPV6 proteins and the so-far annotated and smaller TRPV6 are similar, but the extended N terminus increases trafficking to the plasma membrane and represents an additional scaffold for channel assembly. The increased translation of the smaller TRPV6 cDNA version may overestimate the in vivo situation where translation efficiency may represent an additional mechanism to tightly control the TRPV6-mediated Ca(2+) entry to prevent deleterious Ca(2+) overload.
Author Flockerzi, Veit
Wollenberg, Peter
Wissenbach, Ulrich
Stoerger, Christof
Simon-Thomas, Martin
Maurer, Hans H.
Beck, Andreas
Schalkowsky, Pascal
Dembek, Anna
Middendorff, Ralf
Ruppert, Thomas
Fecher-Trost, Claudia
Doerr, Janka
Weber, Armin
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  givenname: Peter
  surname: Wollenberg
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  organization: Institut für Experimentelle und Klinische Pharmakologie und Toxikologie, Universität des Saarlandes, 66421 Homburg, Germany
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  givenname: Thomas
  surname: Ruppert
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  organization: Institut für Anatomie und Zellbiologie, Justus Liebig Universität Gieβen, Aulweg 123, 35385 Giessen, Germany
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2013 by The American Society for Biochemistry and Molecular Biology, Inc. 2013
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DocumentTitleAlternate Extended TRPV6 Channel Proteins in Vivo
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Keywords Translation
Calcium Channels
TRPV6
TRP Channels
Antibodies
Mass Spectrometry (MS)
Translation Initiation at Non-AUG
Language English
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Snippet TRPV6 channels function as epithelial Ca2+ entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein...
TRPV6 channels function as epithelial Ca(2+) entry pathways in the epididymis, prostate, and placenta. However, the identity of the endogenous TRPV6 protein...
Background: The TRPV6 amino acid sequence is predicted from its cDNA. Results: The TRPV6 protein purified from human tissues has an extended N terminus not...
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SubjectTerms Antibodies
Calcium Channels
Calcium Channels - biosynthesis
Calcium Channels - genetics
Cell Membrane - genetics
Cell Membrane - metabolism
Codon, Initiator - genetics
Codon, Initiator - metabolism
HEK293 Cells
Humans
Mass Spectrometry (MS)
Methionine
Protein Biosynthesis - physiology
Protein Transport - physiology
Signal Transduction
Translation
Translation Initiation at Non-AUG
TRP Channels
TRPV Cation Channels - biosynthesis
TRPV Cation Channels - genetics
TRPV6
Title The in Vivo TRPV6 Protein Starts at a Non-AUG Triplet, Decoded as Methionine, Upstream of Canonical Initiation at AUG
URI https://dx.doi.org/10.1074/jbc.M113.469726
https://www.ncbi.nlm.nih.gov/pubmed/23612980
https://search.proquest.com/docview/1366578712
https://pubmed.ncbi.nlm.nih.gov/PMC3675598
Volume 288
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