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茶树组织去分化和再分化过程中差异表达基因的分析。

Analysis of Differentially Expressed Genes in Tissues of Camellia sinensis during Dedifferentiation and Root Redifferentiation.

机构信息

Zhejiang University Tea Research Institute, Hangzhou, 310058, P.R. China.

The World Vegetable Centre, Guwahati, Assam, India.

出版信息

Sci Rep. 2019 Feb 27;9(1):2935. doi: 10.1038/s41598-019-39264-5.

Abstract

Tissue culture is very important for identifying the gene function of Camellia sinensis (L.) and exploiting novel germplasm through transgenic technology. Regeneration system of tea plant has been explored but not been well established since the molecular mechanism of tea plant regeneration is not clear yet. In this study, transcriptomic analysis was performed in the initial explants of tea plant and their dedifferentiated and redifferentiated tissues. A total of 93,607 unigenes were obtained through de novo assembly, and 7,193 differentially expressed genes (DEGs) were screened out from the 42,417 annotated unigenes. Much more DEGs were observed during phase transition rather than at growth stages of callus. Our KOG and KEGG analysis, and qPCR results confirmed that phase transition of tea plant was closely related to the mechanism that regulate expression of genes encoding the auxin- and cytokinin-responsive proteins, transcription factor MYB15 and ethylene-responsive transcription factor ERF RAP2-12. These findings provide a reliable foundation for elucidating the mechanism of the phase transition and may help to optimize the regeneration system by regulating the gene expression pattern.

摘要

组织培养对于鉴定茶树(Camellia sinensis (L.))的基因功能以及通过转基因技术开发新的种质资源非常重要。尽管茶树的再生系统已经被探索过,但由于茶树再生的分子机制尚不清楚,因此尚未得到很好的建立。在这项研究中,对茶树的初始外植体及其去分化和再分化组织进行了转录组分析。通过从头组装获得了 93607 条 unigenes,从 42417 个注释的 unigenes中筛选出 7193 个差异表达基因(DEGs)。在愈伤组织的生长阶段,而非在转变阶段,观察到更多的 DEGs。我们的 KOG 和 KEGG 分析以及 qPCR 结果证实,茶树的转变与调节生长素和细胞分裂素响应蛋白、转录因子 MYB15 和乙烯响应转录因子 ERF RAP2-12 基因表达的机制密切相关。这些发现为阐明转变机制提供了可靠的基础,并可能有助于通过调节基因表达模式来优化再生系统。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/52ab/6393419/5ed9e5c175c3/41598_2019_39264_Fig1_HTML.jpg

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