Ribosome binding of phasiRNA precursors accelerates the 24-nt phasiRNA burst in meiotic maize anthers

Yingjia Han, Siqi Jiang, Xiaomei Dong, Xing Dai, Shunxi Wang, Ying Zheng, Ge Yan, Shengben Li, Liuji Wu, Virginia Walbot, Blake C Meyers, Mei Zhang
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Abstract

Reproductive phasiRNAs (phased, small interfering RNAs), produced from numerous PHAS loci, are essential for plant anther development. PHAS transcripts are enriched on endoplasmic reticulum-bound ribosomes in maize (Zea mays), but the impact of ribosome binding on phasiRNA biogenesis remains elusive. Through ribosome profiling of maize anthers at 10 developmental stages, we demonstrated that 24-PHAS transcripts are bound by ribosomes, with patterns corresponding to the timing and abundance of 24-PHAS transcripts. Ribosome binding to 24-PHAS transcripts is conserved among different maize inbred lines, with ribosomes enriched upstream of miR2275 target sites. We detected short open reading frames (sORFs) in the ribosome-binding regions of some 24-PHAS transcripts and observed a 3-nt periodicity in most sORFs, but mass spectrometry failed to detect peptides corresponding to the sORFs. Deletion of the entire ribosome-binding region of 24PHAS_NO296 locus eliminated ribosome binding and decreased 24-nt phasiRNA production, without affecting 24PHAS_NO296 transcript levels. In contrast, disrupting only the sORFs in 24PHAS_NO296 did not substantially affect the generation of 24-nt phasiRNAs. A newly formed sORF in these mutants may have re-directed ribosome binding to its transcripts. Overall, these findings demonstrate that sORFs facilitate ribosome binding to 24-PHAS transcripts, thereby promoting phasiRNA biogenesis in meiotic anthers.
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核糖体与 phasiRNA 前体的结合加速了减数分裂期玉米花药中 24-nt phasiRNA 的迸发
由许多 PHAS 基因座产生的生殖性 phasiRNA(分阶段小干扰 RNA)对植物花药的发育至关重要。在玉米(Zea mays)中,PHAS 转录本富集在内质网结合的核糖体上,但核糖体结合对 phasiRNA 生物发生的影响仍然难以捉摸。通过对玉米花药 10 个发育阶段的核糖体分析,我们证明 24-PHAS 转录本与核糖体结合,其模式与 24-PHAS 转录本的时间和丰度相对应。核糖体与 24-PHAS 转录本的结合在不同的玉米近交系中是一致的,核糖体富集在 miR2275 目标位点的上游。我们在一些 24-PHAS 转录本的核糖体结合区检测到了短开放阅读框(sORFs),并观察到大多数 sORFs 具有 3-nt 周期性,但质谱分析未能检测到与 sORFs 相对应的肽段。删除 24PHAS_NO296 基因座的整个核糖体结合区可消除核糖体结合,减少 24-nt phasiRNA 的产生,但不影响 24PHAS_NO296 转录本的水平。相比之下,只破坏 24PHAS_NO296 中的 sORF 并不会对 24-nt phasiRNA 的产生产生实质性影响。这些突变体中新形成的 sORF 可能重新引导了核糖体与其转录本的结合。总之,这些研究结果表明,sORFs 促进了核糖体与 24-PHAS 转录本的结合,从而促进了减数分裂花药中 phasiRNA 的生物发生。
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