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通过修饰近失 cis-acting 元件激活天然 PHYTOENE SYNTHASE 1 启动子诱导胚性水稻愈伤组织中的类胡萝卜素生物合成。

Activation of the native PHYTOENE SYNTHASE 1 promoter by modifying near-miss cis-acting elements induces carotenoid biosynthesis in embryogenic rice callus.

机构信息

Applied Plant Biotechnology Group, Department of Agricultural and Forest Sciences and Engineering, University of Lleida-Agrotecnio CERCA Center, Lleida, Spain.

Division of Biological and Environmental Sciences and Engineering, Center for Desert Agriculture, BioActives Lab, King Abdullah University of Science and Technology (KAUST), Thuwal, Saudi Arabia.

出版信息

Plant Cell Rep. 2024 Apr 17;43(5):118. doi: 10.1007/s00299-024-03199-7.

Abstract

Modification of silent latent endosperm-enabled promoters (SLEEPERs) allows the ectopic activation of non-expressed metabolic genes in rice callus Metabolic engineering in plants typically involves transgene expression or the mutation of endogenous genes. An alternative is promoter modification, where small changes in the promoter sequence allow genes to be switched on or off in particular tissues. To activate silent genes in rice endosperm, we screened native promoters for near-miss cis-acting elements that can be converted to endosperm-active regulatory motifs. We chose rice PHYTOENE SYNTHASE 1 (PSY1), encoding the enzyme responsible for the first committed step in the carotenoid biosynthesis pathway, because it is not expressed in rice endosperm. We identified six motifs within a 120-bp region, upstream of the transcriptional start site, which differed from endosperm-active elements by up to four nucleotides. We mutated four motifs to match functional elements in the endosperm-active BCH2 promoter, and this promoter was able to drive GFP expression in callus and in seeds of regenerated plants. The 4 M promoter was not sufficient to drive PSY1 expression, so we mutated the remaining two elements and used the resulting 6 M promoter to drive PSY1 expression in combination with a PDS transgene. This resulted in deep orange callus tissue indicating the accumulation of carotenoids, which was subsequently confirmed by targeted metabolomics analysis. PSY1 expression driven by the uncorrected or 4 M variants of the promoter plus a PDS transgene produced callus that lacked carotenoids. These results confirm that the adjustment of promoter elements can facilitate the ectopic activation of endogenous plant promoters in rice callus and endosperm and most likely in other tissues and plant species.

摘要

沉默潜势胚乳启动子(SLEEPERs)的修饰可使水稻愈伤组织中未表达的代谢基因异位激活 植物代谢工程通常涉及转基因表达或内源性基因的突变。另一种方法是启动子修饰,其中启动子序列的微小变化可以使基因在特定组织中开启或关闭。为了激活水稻胚乳中的沉默基因,我们筛选了天然启动子,以寻找可以转化为胚乳活性调控元件的近顺式作用元件。我们选择编码负责类胡萝卜素生物合成途径第一步的酶的水稻质体烯醇化酶 1(PSY1),因为它在水稻胚乳中不表达。我们在转录起始位点上游的 120bp 区域内鉴定了六个与胚乳活性元件相差多达四个核苷酸的元件。我们将四个元件突变为与胚乳活性 BCH2 启动子中的功能元件匹配,并使该启动子能够在愈伤组织和再生植物的种子中驱动 GFP 表达。4M 启动子不足以驱动 PSY1 表达,因此我们突变了另外两个元件,并使用所得的 6M 启动子与 PDS 转基因一起驱动 PSY1 表达。这导致深橙色的愈伤组织表明类胡萝卜素的积累,随后通过靶向代谢组学分析得到证实。由未校正或 4M 变体的启动子加上 PDS 转基因驱动的 PSY1 表达产生的愈伤组织缺乏类胡萝卜素。这些结果证实,启动子元件的调整可以促进内源植物启动子在水稻愈伤组织和胚乳中的异位激活,很可能在其他组织和植物物种中也是如此。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4764/11024007/3264e2ebbb80/299_2024_3199_Fig1_HTML.jpg

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