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Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells
Objective(s) : Stem cell differentiation into different cell lineages depends upon several factors, cell cycle control elements and intracellular signaling elements, including P15INK4b and P16INK4a genes. Epigenetics may be regarded as a control mechanism which is affected by these factors with resp...
Autores principales: | , , , , , , , , , , , |
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Formato: | Online Artículo Texto |
Lenguaje: | English |
Publicado: |
Mashhad University of Medical Sciences
2013
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Materias: | |
Acceso en línea: | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3758052/ https://www.ncbi.nlm.nih.gov/pubmed/23997911 |
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author | Azad, Mehdi Kaviani, Saeid Noruzinia, Mehrdad Mortazavi, Yousef Mobarra, Naser Alizadeh, Shaban Shahjahani, Mohammad Skandari, Fatemeh Ahmadi, Mohammad Hosein Atashi, Amir Abroun, Saeid Zonoubi, Zahra |
author_facet | Azad, Mehdi Kaviani, Saeid Noruzinia, Mehrdad Mortazavi, Yousef Mobarra, Naser Alizadeh, Shaban Shahjahani, Mohammad Skandari, Fatemeh Ahmadi, Mohammad Hosein Atashi, Amir Abroun, Saeid Zonoubi, Zahra |
author_sort | Azad, Mehdi |
collection | PubMed |
description | Objective(s) : Stem cell differentiation into different cell lineages depends upon several factors, cell cycle control elements and intracellular signaling elements, including P15INK4b and P16INK4a genes. Epigenetics may be regarded as a control mechanism which is affected by these factors with respect to their promoter structure. Materials and Methods : The CD34 + cord blood stem cells were purified, isolated and then expanded. The undifferentiated day genome was isolated from part of the cultured cells, and the seventh day differentiated genome was isolated from the other part after differentiation to erythroid lineage. The procedure was followed by a separate Real-Time PCR for the two genes using the obtained cDNA. The processed DNA of the former stages was used for MSP (Methylation Specific PCR) reaction. Finally, pre- and post differentiation results were compared. Results : After performing MSP for each gene, it became clear that P15INK4b gene has undergone methylation and expression in predifferentiation stage. In addition, its status has not been changed after differentiation. P15INK4b gene expression was reduced after the differentiation. The other gene, P16INK4a, showed no predifferentiation methylation. Itwas completely expressed methylated and underwent reduced expression after differentiation. Conclusion : Specific predifferentiation expression of P15INK4b and P16INK4a genes along with reduction in their expression after erythroid differentiation indicated animportant role for these two genes in biology of CD34+ cells in primary stages and before differentiation. In addition, both genes are capable of epigenetic modifications due to the structure of their promoters. |
format | Online Article Text |
id | pubmed-3758052 |
institution | National Center for Biotechnology Information |
language | English |
publishDate | 2013 |
publisher | Mashhad University of Medical Sciences |
record_format | MEDLINE/PubMed |
spelling | pubmed-37580522013-08-30 Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells Azad, Mehdi Kaviani, Saeid Noruzinia, Mehrdad Mortazavi, Yousef Mobarra, Naser Alizadeh, Shaban Shahjahani, Mohammad Skandari, Fatemeh Ahmadi, Mohammad Hosein Atashi, Amir Abroun, Saeid Zonoubi, Zahra Iran J Basic Med Sci Original Article Objective(s) : Stem cell differentiation into different cell lineages depends upon several factors, cell cycle control elements and intracellular signaling elements, including P15INK4b and P16INK4a genes. Epigenetics may be regarded as a control mechanism which is affected by these factors with respect to their promoter structure. Materials and Methods : The CD34 + cord blood stem cells were purified, isolated and then expanded. The undifferentiated day genome was isolated from part of the cultured cells, and the seventh day differentiated genome was isolated from the other part after differentiation to erythroid lineage. The procedure was followed by a separate Real-Time PCR for the two genes using the obtained cDNA. The processed DNA of the former stages was used for MSP (Methylation Specific PCR) reaction. Finally, pre- and post differentiation results were compared. Results : After performing MSP for each gene, it became clear that P15INK4b gene has undergone methylation and expression in predifferentiation stage. In addition, its status has not been changed after differentiation. P15INK4b gene expression was reduced after the differentiation. The other gene, P16INK4a, showed no predifferentiation methylation. Itwas completely expressed methylated and underwent reduced expression after differentiation. Conclusion : Specific predifferentiation expression of P15INK4b and P16INK4a genes along with reduction in their expression after erythroid differentiation indicated animportant role for these two genes in biology of CD34+ cells in primary stages and before differentiation. In addition, both genes are capable of epigenetic modifications due to the structure of their promoters. Mashhad University of Medical Sciences 2013-07 /pmc/articles/PMC3758052/ /pubmed/23997911 Text en © 2013: Iranian Journal of Basic Medical Sciences This is an Open Access article distributed under the terms of the Creative Commons Attribution License, (http://creativecommons.org/licenses/by/3.0/) which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. |
spellingShingle | Original Article Azad, Mehdi Kaviani, Saeid Noruzinia, Mehrdad Mortazavi, Yousef Mobarra, Naser Alizadeh, Shaban Shahjahani, Mohammad Skandari, Fatemeh Ahmadi, Mohammad Hosein Atashi, Amir Abroun, Saeid Zonoubi, Zahra Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells |
title | Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells |
title_full | Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells |
title_fullStr | Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells |
title_full_unstemmed | Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells |
title_short | Gene Expression Status and Methylation Pattern in Promoter of P15INK4b and P16INK4a in Cord Blood CD34(+) Stem Cells |
title_sort | gene expression status and methylation pattern in promoter of p15ink4b and p16ink4a in cord blood cd34(+) stem cells |
topic | Original Article |
url | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3758052/ https://www.ncbi.nlm.nih.gov/pubmed/23997911 |
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