Regulation of DNA transposition by CpG methylation and chromatin structure in human cells

被引:21
|
作者
Jursch, Tobias [1 ]
Miskey, Csaba [2 ]
Izsvak, Zsuzsanna [1 ]
Ivics, Zoltan [1 ,2 ]
机构
[1] Max Delbruck Ctr Mol Med, D-13125 Berlin, Germany
[2] Paul Ehrlich Inst, Div Med Biotechnol, D-63225 Langen, Germany
来源
MOBILE DNA | 2013年 / 4卷
关键词
SLEEPING-BEAUTY TRANSPOSITION; DROSOPHILA MOBILE ELEMENT; TRANSPOSABLE ELEMENT; GERM-LINE; MUTAGENESIS; EXPRESSION; PROTEIN; REPAIR; DNMT1; MINOS;
D O I
10.1186/1759-8753-4-15
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
Background: The activity of transposable elements can be regulated by different means. DNA CpG methylation is known to decrease or inhibit transpositional activity of diverse transposons. However, very surprisingly, it was previously shown that CpG methylation of the Sleeping Beauty (SB) transposon significantly enhanced transposition in mouse embryonic stem cells. Results: In order to investigate the unexpected response of SB transposition to CpG methylation, related transposons from the Tc1/mariner superfamily, that is, Tc1, Himar1, Hsmar1, Frog Prince (FP) and Minos were tested to see how transposition was affected by CpG methylation. A significant increase of >20-fold in transposition of SB, FP and Minos was seen, whereas Tc1, Himar1 and Hsmar1 showed no difference in transposition upon CpG-methylation. The terminal inverted repeats (TIRs) of the SB, FP and Minos elements share a common structure, in which each TIR contains two functionally important binding sites for the transposase (termed the IR/DR structure). The group of IR/DR elements showed increased excision after CpG methylation compared to untreated transposon donor plasmids. We found that de novo CpG methylation is not required for transposition. A mutated FP donor plasmid with depleted CpG sites in both TIRs was as efficient in transposition as the wild-type transposon, indicating that CpG sites inside the TIRs are not responsible for altered binding of factors potentially modulating transposition. By using an in vivo one-hybrid DNA-binding assay in cultured human cells we found that CpG methylation had no appreciable effect on the affinity of SB transposase to its binding sites. However, chromatin immunoprecipitation indicated that CpG-methylated transposon donor plasmids are associated with a condensed chromatin structure characterized by trimethylated histone H3K9. Finally, DNA compaction by protamine was found to enhance SB transposition. Conclusions: We have shown that DNA CpG methylation upregulates transposition of IR/DR elements in the Tc1/mariner superfamily. CpG methylation provokes the formation of a tight chromatin structure at the transposon DNA, likely aiding the formation of a catalytically active complex by facilitating synapsis of sites bound by the transposase.
引用
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页数:11
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