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内含肽介导的 Cre 蛋白组装用于转基因拟南芥杂交后代中转基因的切除。

Intein-mediated Cre protein assembly for transgene excision in hybrid progeny of transgenic Arabidopsis.

机构信息

Institute of Resources Botany, School of Life Sciences, Southwest University, Chongqing, 400715, China.

出版信息

Plant Cell Rep. 2016 Oct;35(10):2045-53. doi: 10.1007/s00299-016-2015-x. Epub 2016 Jun 20.

Abstract

An approach for restoring recombination activity of complementation split-Cre was developed to excise the transgene in hybrid progeny of GM crops. Growing concerns about the biosafety of genetically modified (GM) crops has currently become a limited factor affecting the public acceptance. Several approaches have been developed to generate selectable-marker-gene-free GM crops. However, no strategy was reported to be broadly applicable to hybrid crops. Previous studies have demonstrated that complementation split-Cre recombinase restored recombination activity in transgenic plants. In this study, we found that split-Cre mediated by split-intein Synechocystis sp. DnaE had high recombination efficiency when Cre recombinase was split at Asp232/Asp233 (866 bp). Furthermore, we constructed two plant expression vectors, pCA-NCre-In and pCA-Ic-CCre, containing NCre866-In and Ic-CCre866 fragments, respectively. After transformation, parent lines of transgenic Arabidopsis with one single copy were generated and used for hybridization. The results of GUS staining demonstrated that the recombination activity of split-Cre could be reassembled in these hybrid progeny of transgenic plants through hybridization and the foreign genes flanked by two loxP sites were efficiently excised. Our strategy may provide an effective approach for generating the next generation of GM hybrid crops without biosafety concerns.

摘要

开发了一种恢复互补分裂 Cre 重组活性的方法,以切除转基因作物杂种后代中的转基因。对转基因生物(GM)作物的生物安全性的日益关注目前已成为影响公众接受度的一个限制因素。已经开发了几种方法来生成无选择标记基因的 GM 作物。然而,据报道,没有一种策略可广泛适用于杂交作物。先前的研究表明,互补分裂 Cre 重组酶可恢复转基因植物中的重组活性。在本研究中,我们发现当 Cre 重组酶在 Asp232/Asp233(866bp)处分裂时,来自集胞藻 sp. DnaE 的分裂整合酶介导的分裂 Cre 具有很高的重组效率。此外,我们构建了两个植物表达载体,pCA-NCre-In 和 pCA-Ic-CCre,分别含有 NCre866-In 和 Ic-CCre866 片段。转化后,生成了具有一个拷贝的转基因拟南芥亲本系,并用于杂交。GUS 染色的结果表明,通过杂交,两个loxP 位点侧翼的外源基因可在这些转基因植物的杂种后代中重新组装分裂 Cre 的重组活性,并有效地切除。我们的策略可能为生成下一代无生物安全问题的 GM 杂交作物提供一种有效方法。

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