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在Physcomitrella patens 中采用基因内诱变策略来保留内含子剪接。

An intragenic mutagenesis strategy in Physcomitrella patens to preserve intron splicing.

机构信息

Inland Norway University of Applied Sciences, Holsetgata 31, N-2318, Hamar, Norway.

Philipps University Marburg, Plant Cell Biology II, Karl-von-Frisch-Str. 8, 35043, Marburg, Germany.

出版信息

Sci Rep. 2017 Jul 11;7(1):5111. doi: 10.1038/s41598-017-05309-w.

Abstract

Gene targeting is a powerful reverse genetics technique for site-specific genome modification. Intrinsic homologous recombination in the moss Physcomitrella patens permits highly effective gene targeting, a characteristic that makes this organism a valuable model for functional genetics. Functional characterization of domains located within a multi-domain protein depends on the ability to generate mutants harboring genetic modifications at internal gene positions while maintaining the reading-frames of the flanking exons. In this study, we designed and evaluated different gene targeting constructs for targeted gene manipulation of sequences corresponding to internal domains of the DEFECTIVE KERNEL1 protein in Physcomitrella patens. Our results show that gene targeting-associated mutagenesis of introns can have adverse effects on splicing, corrupting the normal reading frame of the transcript. We show that successful genetic modification of internal sequences of multi-exon genes depends on gene-targeting strategies which insert the selection marker cassette into the 5' end of the intron and preserve the nucleotide sequence of the targeted intron.

摘要

基因打靶是一种用于特定基因组修饰的强大反向遗传学技术。藓类植物Physcomitrella patens 中的内源性同源重组允许高效的基因靶向,这一特性使该生物成为功能遗传学的有价值模型。位于多域蛋白内的结构域的功能特征取决于在保持侧翼外显子阅读框的同时,在内部基因位置产生携带基因修饰的突变体的能力。在这项研究中,我们设计并评估了不同的基因靶向构建体,用于靶向操纵 Physcomitrella patens 中 DEFECTIVE KERNEL1 蛋白内部结构域的序列。我们的结果表明,与基因靶向相关的内含子诱变可能对剪接产生不利影响,使转录本的正常阅读框发生错误。我们表明,多外显子基因内部序列的成功遗传修饰取决于基因靶向策略,该策略将选择标记盒插入内含子的 5'端,并保留靶内含子的核苷酸序列。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5536/5505980/27f079617720/41598_2017_5309_Fig1_HTML.jpg

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