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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Main Authors: Maryam Ostadsharif, Kamran Ghaedi, Mohammad Hossein Nasr Esfahani, Somayeh Tanhaie, Khadijeh Karbalaii, Kazem Parivar, Hossein Baharvand
Format: Article
Language:English
Published: Royan Institute (ACECR), Tehran 2009-01-01
Series:Cell Journal
Subjects:
Online Access:http://celljournal.org/library/upload/article/Article7.pdf
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spelling 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
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