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Position-Dependent Methylation and Transcriptional Silencing of Transgenes in Inverted T-DNA Repeats: Implications for Posttranscriptional Silencing of Homologous Host Genes in Plants

机译:反向T-DNA重复序列中转基因的位置依赖性甲基化和转录沉默:植物中同源宿主基因的转录后沉默的含义。

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摘要

Posttranscriptional silencing of chalcone synthase (Chs) genes in petunia transformants occurs by introducing T-DNAs that contain a promoter-driven or promoterless Chs transgene. With the constructs we used, silencing occurs only by T-DNA loci which are composed of two or more T-DNA copies that are arranged as inverted repeats (IRs). Since we are interested in the mechanism by which these IR loci induce silencing, we have analyzed different IR loci and nonsilencing single-copy (S) T-DNA loci with respect to the expression and methylation of the transgenes residing in these loci. We show that in an IR locus, the transgenes located proximal to the IR center are much more highly methylated than are the distal genes. A strong silencing locus composed of three inverted T-DNAs bearing promoterless Chs transgenes was methylated across the entire locus. The host Chs genes in untransformed plants were moderately methylated, and no change in methylation was detected when the genes were silenced. Run-on transcription assays showed that promoter-driven transgenes located proximal to the center of a particular IR are transcriptionally more repressed than are the distal genes of the same IR locus. Transcription of the promoterless Chs transgenes could not be detected. In the primary transformant, some of the IR loci were detected together with an unlinked S locus. We observed that the methylation and expression characteristics of the transgenes of these S loci were comparable to those of the partner IR loci, suggesting that there has been cross talk between the two types of loci. Despite the similar features, S loci are unable to induce silencing, indicating that the palindromic arrangement of the Chs transgenes in the IR loci is critical for silencing. Since transcriptionally silenced transgenes in IRs can trigger posttranscriptional silencing of the host genes, our data are most consistent with a model of silencing in which the transgenes physically interact with the homologous host gene(s). The interaction may alter epigenetic features other than methylation, thereby impairing the regular production of mRNA.
机译:矮牵牛转化子中查尔酮合酶(Chs)基因的转录后沉默是通过引入含有启动子驱动或无启动子Chs转基因的T-DNA来实现的。使用我们使用的构建体,沉默仅由T-DNA位点发生,T-DNA位点由两个或多个以反向重复(IR)排列的T-DNA拷贝组成。由于我们对这些IR基因座诱导沉默的机制感兴趣,因此我们就驻留在这些基因座中的转基因的表达和甲基化分析了不同的IR基因座和非沉默单拷贝(S)T-DNA基因座。我们表明,在一个红外基因座中,位于远红外中心的转基因比远侧基因的甲基化程度高得多。在整个基因座上甲基化了一个由三个带有无启动子Chs转基因的反向T-DNA组成的强沉默基因座。未转化植物中的宿主Chs基因被中等程度地甲基化,而沉默这些基因时未检测到甲基化的变化。连续转录测定法显示,与特定IR基因座的远端基因相比,位于特定IR中心附近的启动子驱动的转基因在转录上受到更大的抑制。不能检测到无启动子Chs转基因的转录。在初级转化体中,检测到一些IR基因座以及一个未连接的S基因座。我们观察到,这些S基因座的转基因的甲基化和表达特征与伴侣IR基因座的转基因相当,表明这两种基因座之间存在串扰。尽管具有相似的特征,S基因座仍不能诱导沉默,表明IR基因座中Chs转基因的回文排列对于沉默至关重要。由于IR中转录沉默的转基因可以触发宿主基因的转录后沉默,因此我们的数据与沉默模型最一致,在该模型中,转基因与同源宿主基因发生物理相互作用。相互作用可能会改变除甲基化以外的表观遗传学特征,从而损害mRNA的正常产生。

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