Lin Chien-Yuan, Jakes Joseph E, Donohoe Bryon S, Ciesielski Peter N, Yang Haibing, Gleber Sophie-Charlotte, Vogt Stefan, Ding Shi-You, Peer Wendy A, Murphy Angus S, McCann Maureen C, Himmel Michael E, Tucker Melvin P, Wei Hui
Biosciences Center, National Renewable Energy Laboratory, Golden, CO 80401 USA.
Forest Biopolymer Science and Engineering, USDA Forest Service, Forest Products Laboratory, Madison, WI 53726 USA.
Biotechnol Biofuels. 2016 Oct 21;9:225. doi: 10.1186/s13068-016-0639-2. eCollection 2016.
Plant lignocellulosic biomass is an abundant, renewable feedstock for the production of biobased fuels and chemicals. Previously, we showed that iron can act as a co-catalyst to improve the deconstruction of lignocellulosic biomass. However, directly adding iron catalysts into biomass prior to pretreatment is diffusion limited, and increases the cost of biorefinery operations. Recently, we developed a new strategy for expressing iron-storage protein ferritin intracellularly to accumulate iron as a catalyst for the downstream deconstruction of lignocellulosic biomass. In this study, we extend this approach by fusing the heterologous ferritin gene with a signal peptide for secretion into cell walls (referred to here as FerEX).
The transgenic plants. FerEX. accumulated iron under both normal and iron-fertilized growth conditions; under the latter (iron-fertilized) condition, FerEX transgenic plants showed an increase in plant height and dry weight by 12 and 18 %, respectively, compared with the empty vector control plants. The SDS- and native-PAGE separation of cell-wall protein extracts followed by Western blot analyses confirmed the extracellular expression of ferritin in FerEX plants. Meanwhile, Perls' Prussian blue staining and X-ray fluorescence microscopy (XFM) maps revealed iron depositions in both the secondary and compound middle lamellae cell-wall layers, as well as in some of the corner compound middle lamella in FerEX. Remarkably, their harvested biomasses showed enhanced pretreatability and digestibility, releasing, respectively, 21 % more glucose and 34 % more xylose than the empty vector control plants. These values are significantly higher than those of our recently obtained ferritin intracellularly expressed plants.
This study demonstrated that extracellular expression of ferritin in can produce plants with increased growth and iron accumulation, and reduced thermal and enzymatic recalcitrance. The results are attributed to the intimate colocation of the iron co-catalyst and the cellulose and hemicellulose within the plant cell-wall region, supporting the genetic modification strategy for incorporating conversion catalysts into energy crops prior to harvesting or processing at the biorefinery.
植物木质纤维素生物质是生产生物基燃料和化学品的丰富可再生原料。此前,我们表明铁可以作为助催化剂来改善木质纤维素生物质的解构。然而,在预处理之前直接将铁催化剂添加到生物质中存在扩散限制,并增加了生物精炼操作的成本。最近,我们开发了一种新策略,即在细胞内表达铁储存蛋白铁蛋白以积累铁,作为木质纤维素生物质下游解构的催化剂。在本研究中,我们通过将异源铁蛋白基因与信号肽融合以分泌到细胞壁中(此处称为FerEX)来扩展此方法。
转基因植物FerEX在正常和铁施肥生长条件下均积累铁;在后者(铁施肥)条件下,与空载体对照植物相比,FerEX转基因植物的株高和干重分别增加了12%和18%。对细胞壁蛋白提取物进行SDS和天然PAGE分离,随后进行蛋白质印迹分析,证实了FerEX植物中铁蛋白的细胞外表达。同时,Perls普鲁士蓝染色和X射线荧光显微镜(XFM)图谱显示,在FerEX的次生和复合中层细胞壁层以及一些角部复合中层中都有铁沉积。值得注意的是,它们收获的生物质显示出增强的预处理性和消化性,分别比空载体对照植物释放出多21%的葡萄糖和多34%的木糖。这些值明显高于我们最近获得的细胞内表达铁蛋白的植物的值。
本研究表明,在植物中细胞外表达铁蛋白可以产生生长增加、铁积累增加且热抗性和酶抗性降低的植物。结果归因于铁助催化剂与植物细胞壁区域内的纤维素和半纤维素紧密共定位,支持了在收获或生物精炼厂加工之前将转化催化剂纳入能源作物的基因改造策略。
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