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Third-Generation Sequencing Indicated that LncRNA Could RegulateeIF2Dto Enhance Protein Translation Under Heat Stress inPopulus simonii

机译:第三代测序表明,LNCRNA可以调节IIF2DTO增强热应激Inpopulus Simonii的蛋白质翻译

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摘要

As global temperatures rise, plants are being increasingly exposed to high-temperature stress. Although long non-coding RNAs (lncRNAs) are regulatory elements of gene expression under heat stress in trees, the limitation of sequencing technology and methods in identifying lncRNAs has hindered the exploration of their roles. To explore the role of lncRNAs in response to heat stress, we treatedPopulus simoniiseedlings at 40 degrees C for 1 h and performed third-generation sequencing (Iso-Seq) and high-throughput RNA sequencing (RNA-seq). A total of 239,142,803 short reads were used to correct 101,791 long reads (average length 2400 bp) resulting in 101,791 full-length transcripts and representing 45,217 genes. Then, 829 lncRNAs were identified, including 757 sense lncRNAs (91.31%), 25 long intergenic non-coding RNAs (3.02%), seven antisense lncRNAs (0.84%), and 40 sense intronic lncRNAs (4.83%). Using the criteria |log(2)Fold Change| >= 1 and q-value < 0.05, 2787 genes and 21 lncRNAs were observed to be differentially expressed under heat stress. Functional annotation showed that these genes were associated with "response to stress", "response to stimulus", and "unfolded protein binding". Furthermore, 149 genes were predicted as targets of 17 significantly differentially expressed lncRNAs. A total of 11 genes in significantly enriched gene ontology (GO) terms were annotated, including four genes encoding disease resistance proteins targeted by lncPs2 and seven eukaryotic translation initiation factor 2D (eIF2D) genes targeted by lncPs3. Expression and functional analysis revealed that lncPs3 and fiveeIF2Dswere synergistically upregulated, indicating that lncPs3 may enhance protein translation by regulatingeIF2Din response to heat stress.
机译:随着全球气温上升,植物越来越多地暴露在高温胁迫下。尽管长非编码RNA(long non-coding RNAs,lncRNAs)是树木在热胁迫下基因表达的调控元件,但由于测序技术和鉴定lncRNAs方法的局限性,阻碍了对其作用的探索。为了探索lncRNAs在热应激反应中的作用,我们在40℃下处理西杨1h,并进行第三代测序(Iso-Seq)和高通量RNA测序(RNA-Seq)。共使用239142803个短读来纠正101791个长读(平均长度2400bp),得到101791个全长转录本,代表45217个基因。共鉴定出829个lncRNAs,包括757个义lncRNAs(91.31%)、25个长基因间非编码RNA(3.02%)、7个反义lncRNAs(0.84%)和40个义内含子lncRNAs(4.83%)。使用标准| log(2)Fold Change |>=1和q值<0.05,观察到2787个基因和21个lncRNAs在热应激下差异表达。功能注释显示,这些基因与“应激反应”、“刺激反应”和“未折叠蛋白结合”有关。此外,有149个基因被预测为17个显著差异表达的lncRNAs的靶基因。共注释了11个显著丰富基因本体(GO)术语的基因,包括编码lncPs2靶向的抗病蛋白的4个基因和lncPs3靶向的7个真核翻译起始因子2D(eIF2D)基因。表达和功能分析显示,LNCP3和FIVEEIF2协同上调,表明LNCP3可能通过调节热应激反应增强蛋白质翻译。

著录项

  • 来源
    《Plant molecular biology reporter》 |2021年第1期|共11页
  • 作者单位

    Hainan Univ Key Lab Genet &

    Germplasm Innovat Trop Special Fo Minist Educ Coll Forestry Engn Res Ctr Rare &

    Precious Tree S Haikou 570228 Hainan Peoples R China;

    Hainan Univ Key Lab Genet &

    Germplasm Innovat Trop Special Fo Minist Educ Coll Forestry Engn Res Ctr Rare &

    Precious Tree S Haikou 570228 Hainan Peoples R China;

    Hainan Univ Key Lab Genet &

    Germplasm Innovat Trop Special Fo Minist Educ Coll Forestry Engn Res Ctr Rare &

    Precious Tree S Haikou 570228 Hainan Peoples R China;

    Hainan Univ Key Lab Genet &

    Germplasm Innovat Trop Special Fo Minist Educ Coll Forestry Engn Res Ctr Rare &

    Precious Tree S Haikou 570228 Hainan Peoples R China;

    Hainan Univ Key Lab Genet &

    Germplasm Innovat Trop Special Fo Minist Educ Coll Forestry Engn Res Ctr Rare &

    Precious Tree S Haikou 570228 Hainan Peoples R China;

    Hainan Univ Key Lab Genet &

    Germplasm Innovat Trop Special Fo Minist Educ Coll Forestry Engn Res Ctr Rare &

    Precious Tree S Haikou 570228 Hainan Peoples R China;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 植物学;分子生物学;
  • 关键词

    Populus simonii; Heat stress; Full-length transcriptome sequencing; High-throughput sequencing; Long non-coding RNAs;

    机译:Populus Simonii;热应力;全长转录组测序;高通量测序;长编码RNA;
  • 入库时间 2022-08-20 19:02:55

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