Differential Use of Myristoyl Groups on Neuronal Calcium Sensor Proteins as a Determinant of Spatio-temporal Aspects of Ca2+ Signal Transduction

Differential Use of Myristoyl Groups on Neuronal Calcium Sensor Proteins as a Determinant of Spatio-temporal Aspects of Ca2+ Signal Transduction

The localizations of three members of the neuronal calcium sensor (NCS) family were studied in HeLa cells. Using hippocalcin-EYFP and NCS-1-ECFP, it was found that their localization differed dramatically in resting cells. NCS-1 had a distinct predominantly perinuclear localization (similar to trans...

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Veröffentlicht in:The Journal of biological chemistry 2002-04, Vol.277 (16), p.14227-14237
Hauptverfasser: O'Callaghan, Dermott W., Ivings, Lenka, Weiss, Jamie L., Ashby, Michael C., Tepikin, Alexei V., Burgoyne, Robert D.
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Adaptor Protein Complex gamma Subunits
Blotting, Western
Calcium - metabolism
Calcium-Binding Proteins - metabolism
Cytosol - metabolism
Digitonin - pharmacology
Electrophoresis, Polyacrylamide Gel
HeLa Cells
Hippocalcin
Humans
Ionomycin - pharmacology
Ionophores - pharmacology
Kinetics
Membrane Proteins - metabolism
Microscopy, Fluorescence
Myristic Acid - metabolism
Nerve Tissue Proteins
Neurons - metabolism
Plasmids - metabolism
Protein Transport
Receptors, Transferrin - metabolism
Recombinant Fusion Proteins - metabolism
Signal Transduction
Time Factors
Transfection
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container_end_page 14237
container_issue 16
container_start_page 14227
container_title The Journal of biological chemistry
container_volume 277
creator O'Callaghan, Dermott W.
Ivings, Lenka
Weiss, Jamie L.
Ashby, Michael C.
Tepikin, Alexei V.
Burgoyne, Robert D.
description The localizations of three members of the neuronal calcium sensor (NCS) family were studied in HeLa cells. Using hippocalcin-EYFP and NCS-1-ECFP, it was found that their localization differed dramatically in resting cells. NCS-1 had a distinct predominantly perinuclear localization (similar to trans-Golgi markers), whereas hippocalcin was present diffusely throughout the cell. Upon the elevation of intracellular Ca2+, hippocalcin rapidly translocated to the same perinuclear compartment as NCS-1. Another member of the family, neurocalcin δ, also translocated to this region after a rise in Ca2+ concentration. Permeabilization of transfected cells using digitonin caused loss of hippocalcin and neurocalcin δ in the absence of calcium, but in the presence of 10 μm Ca2+, both proteins translocated to and were retained in the perinuclear region. NCS-1 localization was unchanged in permeabilized cells regardless of calcium concentration. The localization of NCS-1 was unaffected by mutations in all functional EF hands, indicating that its localization was independent of Ca2+. A minimal myristoylation motif (hippocalcin-(1–14)) fused to EGFP resulted in similar perinuclear targeting, showing that localization of these proteins is because of the exposure of the myristoyl group. This was confirmed by mutation of the myristoyl motif of NCS-1 and hippocalcin that resulted in both proteins remaining cytosolic, even at elevated Ca2+concentration. Dual imaging of hippocalcin-EYFP and cytosolic Ca2+ concentration in Fura Red-loaded cells demonstrated the kinetics of the Ca2+/myristoyl switch in living cells and showed that hippocalcin rapidly translocated with a half-time of ∼12 s after a short lag period when Ca2+ was elevated. These results demonstrate that closely related Ca2+sensor proteins use their myristoyl groups in distinct ways in vivo in a manner that will determine the time course of Ca2+ signal transduction.
doi_str_mv 10.1074/jbc.M111750200
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A minimal myristoylation motif (hippocalcin-(1–14)) fused to EGFP resulted in similar perinuclear targeting, showing that localization of these proteins is because of the exposure of the myristoyl group. This was confirmed by mutation of the myristoyl motif of NCS-1 and hippocalcin that resulted in both proteins remaining cytosolic, even at elevated Ca2+concentration. Dual imaging of hippocalcin-EYFP and cytosolic Ca2+ concentration in Fura Red-loaded cells demonstrated the kinetics of the Ca2+/myristoyl switch in living cells and showed that hippocalcin rapidly translocated with a half-time of ∼12 s after a short lag period when Ca2+ was elevated. 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A minimal myristoylation motif (hippocalcin-(1–14)) fused to EGFP resulted in similar perinuclear targeting, showing that localization of these proteins is because of the exposure of the myristoyl group. This was confirmed by mutation of the myristoyl motif of NCS-1 and hippocalcin that resulted in both proteins remaining cytosolic, even at elevated Ca2+concentration. Dual imaging of hippocalcin-EYFP and cytosolic Ca2+ concentration in Fura Red-loaded cells demonstrated the kinetics of the Ca2+/myristoyl switch in living cells and showed that hippocalcin rapidly translocated with a half-time of ∼12 s after a short lag period when Ca2+ was elevated. 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Using hippocalcin-EYFP and NCS-1-ECFP, it was found that their localization differed dramatically in resting cells. NCS-1 had a distinct predominantly perinuclear localization (similar to trans-Golgi markers), whereas hippocalcin was present diffusely throughout the cell. Upon the elevation of intracellular Ca2+, hippocalcin rapidly translocated to the same perinuclear compartment as NCS-1. Another member of the family, neurocalcin δ, also translocated to this region after a rise in Ca2+ concentration. Permeabilization of transfected cells using digitonin caused loss of hippocalcin and neurocalcin δ in the absence of calcium, but in the presence of 10 μm Ca2+, both proteins translocated to and were retained in the perinuclear region. NCS-1 localization was unchanged in permeabilized cells regardless of calcium concentration. The localization of NCS-1 was unaffected by mutations in all functional EF hands, indicating that its localization was independent of Ca2+. A minimal myristoylation motif (hippocalcin-(1–14)) fused to EGFP resulted in similar perinuclear targeting, showing that localization of these proteins is because of the exposure of the myristoyl group. This was confirmed by mutation of the myristoyl motif of NCS-1 and hippocalcin that resulted in both proteins remaining cytosolic, even at elevated Ca2+concentration. Dual imaging of hippocalcin-EYFP and cytosolic Ca2+ concentration in Fura Red-loaded cells demonstrated the kinetics of the Ca2+/myristoyl switch in living cells and showed that hippocalcin rapidly translocated with a half-time of ∼12 s after a short lag period when Ca2+ was elevated. 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ispartof The Journal of biological chemistry, 2002-04, Vol.277 (16), p.14227-14237
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source MEDLINE; Elektronische Zeitschriftenbibliothek - Frei zugängliche E-Journals; Alma/SFX Local Collection
subjects Adaptor Protein Complex gamma Subunits
Blotting, Western
Calcium - metabolism
Calcium-Binding Proteins - metabolism
Cytosol - metabolism
Digitonin - pharmacology
Electrophoresis, Polyacrylamide Gel
HeLa Cells
Hippocalcin
Humans
Ionomycin - pharmacology
Ionophores - pharmacology
Kinetics
Membrane Proteins - metabolism
Microscopy, Fluorescence
Myristic Acid - metabolism
Nerve Tissue Proteins
Neurons - metabolism
Plasmids - metabolism
Protein Transport
Receptors, Transferrin - metabolism
Recombinant Fusion Proteins - metabolism
Signal Transduction
Time Factors
Transfection
title Differential Use of Myristoyl Groups on Neuronal Calcium Sensor Proteins as a Determinant of Spatio-temporal Aspects of Ca2+ Signal Transduction
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