Faculty of Agriculture, Kyushu University, Fukuoka, Japan.
PLoS One. 2013;8(3):e57286. doi: 10.1371/journal.pone.0057286. Epub 2013 Mar 5.
Pentatricopeptide repeat (PPR) proteins are eukaryotic RNA-binding proteins that are commonly found in plants. Organelle transcript processing and stability are mediated by PPR proteins in a gene-specific manner through recognition by tandem arrays of degenerate 35-amino-acid repeating units, the PPR motifs. However, the sequence-specific RNA recognition mechanism of the PPR protein remains largely unknown. Here, we show the principle underlying RNA recognition for PPR proteins involved in RNA editing. The distance between the PPR-RNA alignment and the editable C was shown to be conserved. Amino acid variation at 3 particular positions within the motif determined recognition of a specific RNA in a programmable manner, with a 1-motif to 1-nucleotide correspondence, with no gap sequence. Data from the decoded nucleotide frequencies for these 3 amino acids were used to assign accurate interacting sites to several PPR proteins for RNA editing and to predict the target site for an uncharacterized PPR protein.
五肽重复(PPR)蛋白是真核生物 RNA 结合蛋白,普遍存在于植物中。通过串联排列的 35 个氨基酸重复单元(PPR 基序)的简并识别,PPR 蛋白以基因特异性的方式介导细胞器转录的加工和稳定性。然而,PPR 蛋白的序列特异性 RNA 识别机制在很大程度上仍是未知的。在这里,我们展示了参与 RNA 编辑的 PPR 蛋白的 RNA 识别的基本原理。PPR-RNA 比对与可编辑 C 之间的距离被证明是保守的。基序内 3 个特定位置的氨基酸变异以可编程的方式决定了对特定 RNA 的识别,具有 1 个基序对应 1 个核苷酸,没有间隔序列。这 3 个氨基酸的解码核苷酸频率数据被用于将准确的相互作用位点分配给几个参与 RNA 编辑的 PPR 蛋白,并预测一个未表征的 PPR 蛋白的靶标位点。
Zotero 插件
