| Literature DB >> 23456296 |
Rikno Harmoko1, Wahyu Indra Duwi Fanata, Jae Yong Yoo, Ki Seong Ko, Yeong Gil Rim, Mohammad Nazim Uddin, Tri Agus Siswoyo, Seung Sik Lee, Dool Yi Kim, Sang Yeol Lee, Kyun Oh Lee.
Abstract
In plants, transgenes with inverted repeats are used to induce efficient RNA silencing, which is also frequently induced by highly transcribed sense transgenes. RNA silencing induced by sense transgenes is dependent on RNA-dependent RNA polymerase 6 (RDR6), which converts single-stranded (ss) RNA into double-stranded (ds) RNA. By contrast, it has been proposed that RNA silencing induced by self-complementary hairpin RNA (hpRNA) does not require RDR6, because the hpRNA can directly fold back on itself to form dsRNA. However, it is unclear whether RDR6 plays a role in hpRNA-induced RNA silencing by amplifying dsRNA to spread RNA silencing within the plant. To address the efficiency of hpRNA-induced RNA silencing in the presence or absence of RDR6, Wild type (WT, Col-0) and rdr6-11 Arabidopsis thaliana lines expressing green fluorescent protein (GFP) were generated and transformed with a GFP-RNA interference (RNAi) construct. Whereas most GFP-RNAi-transformed WT lines exhibited almost complete silencing of GFP expression in the T1 generation, various levels of GFP expression remained among the GFP-RNAi-transformed rdr6-11 lines. Homozygous expression of GFP-RNAi in the T3 generation was not sufficient to induce complete GFP silencing in several rdr6-11 lines. Our results indicate that RDR6 is required for efficient hpRNA-induced RNA silencing in plants.Entities:
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Year: 2013 PMID: 23456296 PMCID: PMC3887914 DOI: 10.1007/s10059-013-2203-2
Source DB: PubMed Journal: Mol Cells ISSN: 1016-8478 Impact factor: 5.034