Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells
Objective: Amino acid alignment analysis of deduced amino acid residues revealed a tripeptide(SKI) at the carboxy terminus of peroxisomal protein cDNA. In order to see the importanceof the above sorting signal, we have performed a site-directed mutagenesis to deleteSKI tripeptide and its transfectio...
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Royan Institute (ACECR), Tehran
2009-01-01
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doaj-780228a4946e4587a0e2b812129b95cb2020-11-25T01:37:47ZengRoyan Institute (ACECR), TehranCell Journal2228-58062228-58142009-01-01112154159Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 CellsMaryam OstadsharifKamran GhaediMohammad Hossein Nasr EsfahaniSomayeh TanhaieKhadijeh KarbalaiiKazem ParivarHossein BaharvandObjective: Amino acid alignment analysis of deduced amino acid residues revealed a tripeptide(SKI) at the carboxy terminus of peroxisomal protein cDNA. In order to see the importanceof the above sorting signal, we have performed a site-directed mutagenesis to deleteSKI tripeptide and its transfection into CHO-K1 and P19 cells.Materials and Methods: In order to create the appropriate site-directed mutant, PCR wasdone with specific primers. Amplified PeP cDNAs either containing SKI or deleted ones wereconstructed downstream of EGFP cDNA under regulation of the cytomegalovirus (CMV)promoter in a pEGFP-C1 vector. Transfection of P19 and CHO cells was done with lipofectamine2000.Results: Gradient PCR showed that the best annealing temperature was 71.6 ºC. Transfectionof plasmids containing chimera of EGFP-PEP cDNAs into the CHO-K1 and P19 cellsshowed several punctuate structures, presumably peroxisomes, while SKI deletion showeda cytosolic mislocalization of the EGFP pattern.Conclusion: Taken together, these data strongly suggest that SKI, which is located at theC- terminus of the protein, is required for sorting this protein.http://celljournal.org/library/upload/article/Article7.pdfPeroxisomal ProteinPeroxisome TargetingSignal Peptide |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Maryam Ostadsharif Kamran Ghaedi Mohammad Hossein Nasr Esfahani Somayeh Tanhaie Khadijeh Karbalaii Kazem Parivar Hossein Baharvand |
spellingShingle |
Maryam Ostadsharif Kamran Ghaedi Mohammad Hossein Nasr Esfahani Somayeh Tanhaie Khadijeh Karbalaii Kazem Parivar Hossein Baharvand Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells Cell Journal Peroxisomal Protein Peroxisome Targeting Signal Peptide |
author_facet |
Maryam Ostadsharif Kamran Ghaedi Mohammad Hossein Nasr Esfahani Somayeh Tanhaie Khadijeh Karbalaii Kazem Parivar Hossein Baharvand |
author_sort |
Maryam Ostadsharif |
title |
Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells |
title_short |
Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells |
title_full |
Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells |
title_fullStr |
Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells |
title_full_unstemmed |
Cytosolic Localization of Mouse Peroxisomal Protein/ΔSKI Fused with Enhanced Green Fluorescent Protein into Chinese Hamster Ovary-K1 and P19 Cells |
title_sort |
cytosolic localization of mouse peroxisomal protein/δski fused with enhanced green fluorescent protein into chinese hamster ovary-k1 and p19 cells |
publisher |
Royan Institute (ACECR), Tehran |
series |
Cell Journal |
issn |
2228-5806 2228-5814 |
publishDate |
2009-01-01 |
description |
Objective: Amino acid alignment analysis of deduced amino acid residues revealed a tripeptide(SKI) at the carboxy terminus of peroxisomal protein cDNA. In order to see the importanceof the above sorting signal, we have performed a site-directed mutagenesis to deleteSKI tripeptide and its transfection into CHO-K1 and P19 cells.Materials and Methods: In order to create the appropriate site-directed mutant, PCR wasdone with specific primers. Amplified PeP cDNAs either containing SKI or deleted ones wereconstructed downstream of EGFP cDNA under regulation of the cytomegalovirus (CMV)promoter in a pEGFP-C1 vector. Transfection of P19 and CHO cells was done with lipofectamine2000.Results: Gradient PCR showed that the best annealing temperature was 71.6 ºC. Transfectionof plasmids containing chimera of EGFP-PEP cDNAs into the CHO-K1 and P19 cellsshowed several punctuate structures, presumably peroxisomes, while SKI deletion showeda cytosolic mislocalization of the EGFP pattern.Conclusion: Taken together, these data strongly suggest that SKI, which is located at theC- terminus of the protein, is required for sorting this protein. |
topic |
Peroxisomal Protein Peroxisome Targeting Signal Peptide |
url |
http://celljournal.org/library/upload/article/Article7.pdf |
work_keys_str_mv |
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