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Cyclophosphamide Perturbs Cytosine Methylation in Jurkat-T Cells through LSD1-Mediated Stabilization of DNMT1 Protein.

Authors :
Jing Zhang
Bifeng Yuan
Fan Zhang
Lei Xiong
Jiang Wu
Pradhan, Sriharsa
Yinsheng Wang
Source :
Chemical Research in Toxicology. Nov2011, Vol. 24 Issue 11, p2040-2043. 3p.
Publication Year :
2011

Abstract

Aberrant cytosine methylation is known to be associated with cancer development Here, we assessed how common cancer chemotherapeutic agents perturb cytosine methylation in Jurkat-T acute lymphoblastic leukemia cells. We tested six antitumor agents and found that cyclophosphamide induced the most pronounced increase in global DNA cytosine methylation after a 24-h treatment Long-term treatment with cyclophosphamide led to a time-dependent increase in cytosine methylation level with up to 4 days of treatment, and the 1 extent of cytosine methylation returned to normal level after 8 days. The trend of 5 change in DNA methylation level paralleled that of the expression level of DNMT1 protein, whereas no significant increase in DNMT1 mRNA level was observed. Previous studies showed that the stability of endogenous DNMT1 protein is regulated by lysine methylation through histone lysine memyltransferase Set7 and lysine-specific demethylase 1 (LSD 1), with the methylated DNMT1 being the target for proteasomal degradation. We observed that the elevated expression of DNMT1 protein at 4 days of treatment was correlated with die increased expression of LSD1 protein and with the decreased frequency of K142 methylation in DNMT1. Taken together, our results showed that cyclophosphamide perturbed temporarily global cytosine methylation in Jurkat-T cells via regulation of the lysine mediation level in DNMT1. [ABSTRACT FROM AUTHOR]

Details

Language :
English
ISSN :
0893228X
Volume :
24
Issue :
11
Database :
Academic Search Index
Journal :
Chemical Research in Toxicology
Publication Type :
Academic Journal
Accession number :
97951981
Full Text :
https://doi.org/10.1021/tx2003849