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Abstract
Replication protein A (RPA), the eukaryotic single-stranded DNA (ssDNA) binding protein, is essential for all pathways of DNA metabolism. To study the function of RPA in living cells the second largest RPA subunit and an N-terminal deletion mutant thereof were fused to green fluorescent protein (GFP; GFP-RPA2 and GFP-RPA2deltaN, respectively) in a controlled, molecular biological way. These proteins were expressed in HeLa cells under the control of the inducible tetracycline expression system. GFP-RPA2 and GFP-RPA2deltaN are predominately nuclear proteins as determined by confocal laser scanning microscopy. Low basal expression of GFP-R-PA2deltaN allowed the measurement of kinetic parameters of RPA. Using fluorescence correlation spectroscopy (FCS) two populations - a fast and a slow moving species - were detected in the nucleus and the cytosol of human cells. The translational diffusion rates of these two RPA populations were approximately 15 mu m(2) S and 1.8 mu m(2) S. This new finding reveals the existence of different multiprotein and ssDNA-protein complexes of RPA in both cellular compartments and opens the possibility for their analyses. (C) 2007 Elsevier Inc. All rights reserved.
| Original language | English (Ireland) |
|---|---|
| Pages (from-to) | 156-162 |
| Number of pages | 7 |
| Journal | EXPERIMENTAL AND MOLECULAR PATHOLOGY |
| Volume | 82 |
| Issue number | 2 |
| DOIs | |
| Publication status | Published - 1 Apr 2007 |
Keywords
- DNA repair
- DNA replication
- Fluorescence correlation spectroscopy (FCS)
- Genome stability
- Green fluorescent protein
- Laser scanning microscopy (LSM)
- Replication protein A
Authors (Note for portal: view the doc link for the full list of authors)
- Authors
- Braet, C,Stephan, H,Dobbie, IM,Togashi, DM,Ryder, AG,Foldes-Papp, Z,Lowndes, N,Nasheuer, HP
- Braet, C;Stephan, H;Dobbie, IM;Togashi, DM;Ryder, AG;Foldes-Papp, Z;Lowndes, N;Nasheuer, HP
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