Priyadarshani S V G N, Hu Bingyan, Li Weimin, Ali Hina, Jia Haifeng, Zhao Lihua, Ojolo Simon Peter, Azam Syed Muhammad, Xiong Junjie, Yan Maokai, Ur Rahman Zia, Wu Qingsong, Qin Yuan
1State Key Laboratory of Ecological Pest Control for Fujian and Taiwan Crops, Key Lab of Genetics, Breeding and Multiple Utilization of Crops, Ministry of Education, Fujian Provincial Key Laboratory of Haixia Applied Plant Systems Biology, Center for Genomics and Biotechnology, College of Crop Sciences, College of Resources and Environment, Fujian Agriculture and Forestry University, Fuzhou, 350002 Fujian Province China.
2College of Life Sciences, Fujian Agriculture and Forestry University, Fuzhou, 350002 Fujian Province China.
Plant Methods. 2018 Oct 29;14:95. doi: 10.1186/s13007-018-0365-9. eCollection 2018.
An efficient transformation protocol is a primary requisite to study and utilize the genetic potential of any plant species. A quick transformation system is also crucial for the functional analysis of genes along with the study of proteins and their interactions in vivo. Presently, however, quick and effective transformation systems are still lacking for many plant species including pineapple. This has limited the full exploration of the genetic repository of pineapple as well as the study of its genes, protein localization and protein interactions.
To address the above limitations, we have developed an efficient system for protoplast isolation and subcellular localization of desired proteins using pineapple plants derived from tissue culture. A cocktail of 1.5% (W/V) Cellulase R-10 and 0.5% (W/V) Macerozyme R-10 resulted in 51% viable protoplasts with 3 h digestion. Compared to previously reported protocols, our protoplast isolation method is markedly faster (saving 4.5 h), requires only a small quantity of tissue sample (1 g of leaves) and has high yield (6.5 × 10). The quality of the isolated protoplasts was verified using organelle localization in protoplasts with different organelle markers. Additionally, colocalization analysis of two pineapple Mg transporter genes in pineapple protoplasts was consistent with the results in a tobacco transient expression system, confirming that the protoplast isolation method can be used to study subcellular localization. Further findings showed that the system is also suitable for protein-protein interaction studies.
Based on our findings, the presently described method is an efficient and effective strategy for pineapple protoplast isolation and transformation; it is convenient and time saving and provides a greater platform for transformation studies.
高效的转化方案是研究和利用任何植物物种遗传潜力的首要条件。快速转化系统对于基因的功能分析以及体内蛋白质及其相互作用的研究也至关重要。然而,目前包括菠萝在内的许多植物物种仍缺乏快速有效的转化系统。这限制了对菠萝遗传库的全面探索以及对其基因、蛋白质定位和蛋白质相互作用的研究。
为解决上述局限性,我们利用组织培养获得的菠萝植株开发了一种高效的原生质体分离和所需蛋白质亚细胞定位系统。1.5%(W/V)纤维素酶R-10和0.5%(W/V)离析酶R-10的混合酶液在消化3小时后可产生51%的活原生质体。与先前报道的方案相比,我们的原生质体分离方法明显更快(节省4.5小时),仅需少量组织样本(1克叶片)且产量高(6.5×10)。使用不同细胞器标记物在原生质体中进行细胞器定位验证了分离的原生质体的质量。此外,对菠萝原生质体中两个菠萝镁转运蛋白基因的共定位分析与烟草瞬时表达系统中的结果一致,证实该原生质体分离方法可用于研究亚细胞定位。进一步的研究结果表明该系统也适用于蛋白质-蛋白质相互作用研究。
基于我们的研究结果,目前所描述的方法是一种高效有效的菠萝原生质体分离和转化策略;它方便省时,为转化研究提供了一个更好的平台。
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