R2 retrotransposons are site-specific eukaryotic non-long terminal repeat retrotransposons that copy and paste into gene loci encoding ribosomal RNAs. Recently, we demonstrated that avian A-clade R2 proteins achieve efficient and precise insertion of transgenes into their native safe-harbor loci in human cells. The features of A-clade R2 proteins that support gene insertion are not well characterized. Here, we report high-resolution cryo-electron microscopy structures of two vertebrate A-clade R2 proteins at the initiation of target-primed reverse transcription and after cDNA synthesis and second-strand nicking. Using biochemical and cellular assays, we illuminate the basis for high selectivity of template use and unique roles for each of the three zinc-finger domains in nucleic acid recognition. Reverse transcriptase active site architecture is reinforced by an unanticipated insertion motif specific to vertebrate A-clade R2 proteins. Our work provides the first insights into A-clade R2 protein structure during gene insertion and may enable future improvement and adaptation of R2-based systems for precise transgene insertion.
Structures of vertebrate R2 retrotransposon complexes during target-primed reverse transcription and after second-strand nicking.
脊椎动物 R2 逆转录转座子复合物在靶标引发逆转录过程中以及第二链切口后的结构
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作者:Thawani Akanksha, RodrÃguez-Vargas Anthony, Van Treeck Briana, Hassan Nozhat T, Adelson David L, Nogales Eva, Collins Kathleen
| 期刊: | Science Advances | 影响因子: | 12.500 |
| 时间: | 2025 | 起止号: | 2025 Jun 20; 11(25):eadu5533 |
| doi: | 10.1126/sciadv.adu5533 | 研究方向: | 其它 |
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