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在甘蔗(一种高度多倍体作物)中,与已知功能启动子相连的报告转基因的有效沉默。

Efficient silencing of reporter transgenes coupled to known functional promoters in sugarcane, a highly polyploid crop species.

作者信息

Mudge Stephen R, Osabe Kenji, Casu Rosanne E, Bonnett Graham D, Manners John M, Birch Robert G

机构信息

Botany Department, School of Integrative Biology, The University of Queensland, Brisbane, 4072, Australia.

出版信息

Planta. 2009 Feb;229(3):549-58. doi: 10.1007/s00425-008-0852-8. Epub 2008 Nov 15.

Abstract

Sugarcane is a crop of great interest for engineering of sustainable biomaterials and biofuel production. Isolated sugarcane promoters have generally not maintained the expected patterns of reporter transgene expression. This could arise from defective promoters on redundant alleles in the highly polyploid genome, or from efficient transgene silencing. To resolve this question we undertook detailed analysis of a sugarcane gene that combines a simple pattern in genomic Southern hybridization analysis with potentially useful, sink-specific, expression. Sequence analysis indicates that this gene encodes a member of the SHAQYF subfamily of MYB transcription factors. At least eight alleles were revealed by PCR analysis in sugarcane cultivar Q117 and a similar level of heterozygosity was seen in BAC clones from cultivar Q200. Eight distinct promoter sequences were isolated from Q117, of which at least three are associated with expressed alleles. All of the isolated promoter variants were tested for ability to drive reporter gene expression in sugarcane. Most were functional soon after transfer, but none drove reporter activity in mature stems of regenerated plants. These results show that the ineffectiveness of previously tested sugarcane promoters is not simply due to the isolation of non-functional promoter copies from the polyploid genome. If the unpredictable onset of silencing observed in most other plant species is associated with developmental polyploidy, approaches that avoid efficient transgene silencing in polyploid sugarcane are likely to have much wider utility in molecular improvement.

摘要

甘蔗是可持续生物材料工程和生物燃料生产中备受关注的作物。分离得到的甘蔗启动子通常无法维持报告基因转基因表达的预期模式。这可能是由于高度多倍体基因组中冗余等位基因上的启动子缺陷,或者是由于有效的转基因沉默。为了解决这个问题,我们对一个甘蔗基因进行了详细分析,该基因在基因组Southern杂交分析中具有简单模式,并具有潜在有用的、库特异性的表达。序列分析表明,该基因编码MYB转录因子SHAQYF亚家族的一个成员。通过PCR分析在甘蔗品种Q117中揭示了至少八个等位基因,并且在品种Q200的BAC克隆中也观察到了类似水平的杂合性。从Q117中分离出八个不同的启动子序列,其中至少三个与表达的等位基因相关。对所有分离的启动子变体进行了在甘蔗中驱动报告基因表达能力的测试。大多数在转移后很快就具有功能,但没有一个能在再生植株的成熟茎中驱动报告基因活性。这些结果表明,先前测试的甘蔗启动子无效并非仅仅是由于从多倍体基因组中分离出无功能的启动子拷贝。如果在大多数其他植物物种中观察到的不可预测的沉默起始与发育多倍体相关,那么避免多倍体甘蔗中有效转基因沉默的方法可能在分子改良中具有更广泛的用途。

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