The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells

The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells

<p>Abstract</p> <p>Background</p> <p>Two-photon-excitation fluorescence lifetime imaging (2P-FLIM) was used to investigate the association of protein kinase C alpha (PKCα) with caveolin in CHO cells. PKCα is found widely in the cytoplasm and nucleus in most cells. Upon...

Full description

Bibliographic Details
Main Authors: Slater Simon J, Botchway Stanley W, Stubbs Christopher D, Parker Anthony W
Format: Article
Language:English
Published: BMC 2005-04-01
Series:BMC Cell Biology
Online Access:http://www.biomedcentral.com/1471-2121/6/22
id doaj-ca8a5dd2ae3a4e2a99cb333d9bb29de0
record_format Article
spelling doaj-ca8a5dd2ae3a4e2a99cb333d9bb29de02020-11-24T21:40:39ZengBMCBMC Cell Biology1471-21212005-04-01612210.1186/1471-2121-6-22The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cellsSlater Simon JBotchway Stanley WStubbs Christopher DParker Anthony W<p>Abstract</p> <p>Background</p> <p>Two-photon-excitation fluorescence lifetime imaging (2P-FLIM) was used to investigate the association of protein kinase C alpha (PKCα) with caveolin in CHO cells. PKCα is found widely in the cytoplasm and nucleus in most cells. Upon activation, as a result of increased intracellular Ca<sup>2+ </sup>and production of DAG, through G-protein coupled-phospholipase C signalling, PKC translocates to a variety of regions in the cell where it phosphorylates and interacts with many signalling pathways. Due to its wide distribution, discerning a particular interaction from others within the cell is extremely difficult</p> <p>Results</p> <p>Fluorescence energy transfer (FRET), between GFP-PKCα and DsRed-caveolin, was used to investigate the interaction between caveolin and PKC, an aspect of signalling that is poorly understood. Using 2P-FLIM measurements, the lifetime of GFP was found to decrease (quench) in certain regions of the cell from ~2.2 ns to ~1.5 ns when the GFP and DsRed were sufficiently close for FRET to occur. This only occurred when intracellular Ca<sup>2+ </sup>increased or in the presence of phorbol ester, and was an indication of PKC and caveolin co-localisation under these conditions. In the case of phorbol ester stimulated PKC translocation, as commonly used to model PKC activation, three PKC areas could be delineated. These included PKCα that was not associated with caveolin in the nucleus and cytoplasm, PKCα associated with caveolin in the cytoplasm/perinuclear regions and probably in endosomes, and PKC in the peripheral regions of the cell, possibly indirectly interacting with caveolin.</p> <p>Conclusion</p> <p>Based on the extent of lifetime quenching observed, the results are consistent with a direct interaction between PKCα and caveolin in the endosomes, and possibly an indirect interaction in the peripheral regions of the cell. The results show that 2P-FLIM-FRET imaging offers an approach that can provide information not only confirming the occurrence of specific protein-protein interactions but where they occur within the cell.</p> http://www.biomedcentral.com/1471-2121/6/22
collection DOAJ
language English
format Article
sources DOAJ
author Slater Simon J
Botchway Stanley W
Stubbs Christopher D
Parker Anthony W
spellingShingle Slater Simon J
Botchway Stanley W
Stubbs Christopher D
Parker Anthony W
The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells
BMC Cell Biology
author_facet Slater Simon J
Botchway Stanley W
Stubbs Christopher D
Parker Anthony W
author_sort Slater Simon J
title The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells
title_short The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells
title_full The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells
title_fullStr The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells
title_full_unstemmed The use of time-resolved fluorescence imaging in the study of protein kinase C localisation in cells
title_sort use of time-resolved fluorescence imaging in the study of protein kinase c localisation in cells
publisher BMC
series BMC Cell Biology
issn 1471-2121
publishDate 2005-04-01
description <p>Abstract</p> <p>Background</p> <p>Two-photon-excitation fluorescence lifetime imaging (2P-FLIM) was used to investigate the association of protein kinase C alpha (PKCα) with caveolin in CHO cells. PKCα is found widely in the cytoplasm and nucleus in most cells. Upon activation, as a result of increased intracellular Ca<sup>2+ </sup>and production of DAG, through G-protein coupled-phospholipase C signalling, PKC translocates to a variety of regions in the cell where it phosphorylates and interacts with many signalling pathways. Due to its wide distribution, discerning a particular interaction from others within the cell is extremely difficult</p> <p>Results</p> <p>Fluorescence energy transfer (FRET), between GFP-PKCα and DsRed-caveolin, was used to investigate the interaction between caveolin and PKC, an aspect of signalling that is poorly understood. Using 2P-FLIM measurements, the lifetime of GFP was found to decrease (quench) in certain regions of the cell from ~2.2 ns to ~1.5 ns when the GFP and DsRed were sufficiently close for FRET to occur. This only occurred when intracellular Ca<sup>2+ </sup>increased or in the presence of phorbol ester, and was an indication of PKC and caveolin co-localisation under these conditions. In the case of phorbol ester stimulated PKC translocation, as commonly used to model PKC activation, three PKC areas could be delineated. These included PKCα that was not associated with caveolin in the nucleus and cytoplasm, PKCα associated with caveolin in the cytoplasm/perinuclear regions and probably in endosomes, and PKC in the peripheral regions of the cell, possibly indirectly interacting with caveolin.</p> <p>Conclusion</p> <p>Based on the extent of lifetime quenching observed, the results are consistent with a direct interaction between PKCα and caveolin in the endosomes, and possibly an indirect interaction in the peripheral regions of the cell. The results show that 2P-FLIM-FRET imaging offers an approach that can provide information not only confirming the occurrence of specific protein-protein interactions but where they occur within the cell.</p>
url http://www.biomedcentral.com/1471-2121/6/22
work_keys_str_mv AT slatersimonj theuseoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT botchwaystanleyw theuseoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT stubbschristopherd theuseoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT parkeranthonyw theuseoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT slatersimonj useoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT botchwaystanleyw useoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT stubbschristopherd useoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
AT parkeranthonyw useoftimeresolvedfluorescenceimaginginthestudyofproteinkinaseclocalisationincells
_version_ 1725925355597856768

Similar Items