Li Huixiang, Liang Ruiting, Turner Douglas H, Rothberg Lewis J, Duan Shenghua
Department of Chemistry, University of Rochester, Rochester, NY 14627-0216, USA.
RNA. 2007 Nov;13(11):2034-41. doi: 10.1261/rna.138807. Epub 2007 Sep 25.
Binding of small oligonucleotides to the periphery of folded RNA can provide insight into the secondary structure of complex RNA in solution. To discriminate between bound and unbound fluorescein-labeled 2'-O-methyl RNA probes, we use ionically coated gold nanoparticles to selectively adsorb unbound probes and quench their fluorescence. The target is the 3' untranslated region of Bombyx mori R2 RNA. Fluorescence indicates that R2 sequences complementary to some of the probes are accessible for binding in the three-dimensional structure. Hybridization occurs under homogeneous conditions in the absence of the gold nanoparticles so that steric issues associated with chip-based assays are avoided. The assay is compatible with well plate formats, takes less than 5 min, and requires only 2 pmol or less of unlabeled target RNA per probe sequence tested.
小寡核苷酸与折叠RNA的外围结合可以为溶液中复杂RNA的二级结构提供见解。为了区分结合和未结合的荧光素标记的2'-O-甲基RNA探针,我们使用离子包覆的金纳米颗粒选择性吸附未结合的探针并淬灭其荧光。靶标是家蚕R2 RNA的3'非翻译区。荧光表明与某些探针互补的R2序列在三维结构中可用于结合。杂交在没有金纳米颗粒的均匀条件下发生,从而避免了与芯片检测相关的空间问题。该检测与微孔板形式兼容,耗时不到5分钟,每个测试的探针序列仅需要2 pmol或更少的未标记靶RNA。
