| Literature DB >> 21175898 |
Akira Kanazawa1, Jun-Ichi Inaba1, Hanako Shimura1, Shungo Otagaki1, Sayuri Tsukahara1, Akihiko Matsuzawa1, Bo Min Kim1, Kazunori Goto1, Chikara Masuta1.
Abstract
Gene silencing through transcriptional repression can be induced by targeting double-stranded RNA (dsRNA) to a gene promoter. It has been reported that a transgene was silenced by targeting dsRNA to the promoter, and the silenced state was inherited to the progeny plant even after removal of the silencing inducer from cells. In contrast, no plant has been produced that harbors silenced endogenous gene after removal of promoter-targeting dsRNA. Here, we show that heritable gene silencing can be induced by targeting dsRNA to the endogenous gene promoters in petunia and tomato plants, using the Cucumber mosaic virus (CMV)-based vector. We found that efficient silencing of endogenous genes depends on the function of the 2b protein encoded in the vector virus, which has the ability to facilitate epigenetic modifications through the transport of short interfering RNA to nucleus. Bisulfite sequencing analyses on the targeted promoter in the virus-infected and its progeny plants revealed that cytosine methylation was found not only at CG or CNG but also at CNN sites. The observed inheritance of asymmetric DNA methylation is quite unique, suggesting that plants have a mechanism to maintain even asymmetric methylation. This CMV-based gene silencing system provides a useful tool to artificially modify DNA methylation in plant genomes and elucidate the mechanism for epigenetic controls.Entities:
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Year: 2010 PMID: 21175898 DOI: 10.1111/j.1365-313X.2010.04401.x
Source DB: PubMed Journal: Plant J ISSN: 0960-7412 Impact factor: 6.417