De novo Short Read Assembly and Functional Annotation of Eleocharis vivipara , a C 3 /C 4 Interconvertible Sedge Plant

Q3 Agricultural and Biological Sciences Environmental Control in Biology Pub Date : 2018-01-01 DOI:10.2525/ECB.56.81
Daijiro Harada, K. Yamato, K. Izui, M. Akita
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引用次数: 2

Abstract

More than 90% of terrestrial plant species possess the C3 photosynthetic system, while only about 3% undergo C4 photosynthesis. Nevertheless, C4 plants are responsible for 25% of the annual total terrestrial plant biomass production (Langdale, 2011; Sage and Zhu, 2011). Compared with C3 plants, C4 plants generally exhibit higher CO2 assimilation abilities (about 1.5 2-fold higher in individual blades), higher yields per growing area (approximately 2 3-fold) and higher water and nitrogen use efficiencies (Black, 1979). The productivity of major C3 crops, such as rice, wheat and soybean, could be greatly increased if the CO2 concentrating mechanism of C4 photosynthesis could be introduced into these C3 plants through genetic engineering. Such attempts have been made by various investigators (Häusler et al., 2002; Miyao et al., 2011), but no promising results have been obtained thus far. For example, several genes encoding C4 photosynthesis-related enzymes were successfully overexpressed individually or in combination in mesophyll cells of rice plants, but the transgenic plants did not perform C4-like photosynthesis and their growth rate was not accelerated appreciably (Taniguchi et al., 2008). These observations imply the introduction of genes for CO2-concentrating proteins is not sufficient to confer the C4 photosynthetic framework to C3 plants. In fact, two functionally differentiated cell types mesophyll cells and bundle-sheath cells and their structural arrangement called Kranz anatomy are required to concentrate CO2 and deliver it to ribulose-1,5-bisphosphate carboxylase/oxygenase. This CO2 concentration system has been thought to be essential for C4 photosynthesis. To convert C3 plants into C4 ones, all genes that are related to cellular and functional C4 differentiation, including those associated with C4 metabolism, transport of C4-related compounds and development of Kranz anatomy, must be identified and introduced into C3 plants (Covshoff and Hibberd, 2012). To identify the genes required for C4 photosynthesis, a straightforward approach was comparative analysis of C4 and C3 plants. However, identification of the key C4 photosynthetic genes is difficult because many of them are species-specific even among C4 model plants (e.g., Zea mays and Sorghum bicolor). Although the genera Flaveria and Cleome include both C3 and C4 species and have attracted much attention as alternative systems (Brown et al., 2005; Külahoglu et al., 2014), there are still speciesspecific genes, which makes it difficult to identify the core functional set of C4 photosynthetic genes (Gowik et al., 2011). Eleocharis vivipara (Cyperaceae), first investigated by Ueno et al. (1988) is an amphibious leafless sedge. This plant develops Kranz anatomy and shows C4 biochemical traits under terrestrial conditions, and performs NADdependent malic enzyme (NAD-ME)-type C4 photosynthesis. Interestingly, under submerged conditions, it grows without Kranz anatomy and exhibits C3 biochemical traits. When the submerged plants are exposed to air, they develop new shoots with C4 traits within about a week. This species is thus suitable for screening genes indispensable to the biochemical, cellular and structural transition from the C3 to the C4 photosynthetic system; however, its relevant genomic and transcriptomic information is currently lim-
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一种c3 / c4可转换莎草植物Eleocharis vivipara的重新短读汇编和功能注释
90%以上的陆生植物具有C3光合系统,而只有约3%的陆生植物具有C4光合作用。然而,C4植物占陆地植物年总生物量产量的25% (Langdale, 2011;Sage and Zhu, 2011)。与C3植物相比,C4植物通常具有更高的CO2同化能力(单个叶片约高1.5倍),每种植面积产量更高(约23倍),水和氮利用效率更高(Black, 1979)。通过基因工程将C4光合作用的CO2浓缩机制引入到水稻、小麦和大豆等主要C3作物中,可以大大提高这些C3作物的产量。各种调查人员都进行了这种尝试(Häusler等人,2002年;Miyao et al., 2011),但到目前为止还没有得到有希望的结果。例如,几个编码C4光合作用相关酶的基因在水稻叶肉细胞中成功地单独或联合过表达,但转基因植株不进行类似C4的光合作用,其生长速度没有明显加快(Taniguchi et al., 2008)。这些观察结果表明,二氧化碳浓缩蛋白基因的引入不足以将C4光合框架赋予C3植物。事实上,叶肉细胞和束鞘细胞两种功能分化的细胞类型及其结构安排(称为Kranz解剖)需要将CO2浓缩并将其传递给核酮糖-1,5-二磷酸羧化酶/加氧酶。这种二氧化碳浓度系统被认为对C4光合作用至关重要。要将C3植物转化为C4植物,必须确定所有与细胞和功能C4分化相关的基因,包括与C4代谢、C4相关化合物的运输和克兰兹解剖发育相关的基因,并将其引入C3植物中(Covshoff和Hibberd, 2012)。为了确定C4光合作用所需的基因,比较分析C4和C3植物是一种简单的方法。然而,鉴定关键的C4光合作用基因是困难的,因为许多基因甚至在C4模式植物(如玉米和高粱双色)中也是种特异性的。尽管黄草属和克莱梅属同时包括C3和C4种,并且作为替代系统引起了广泛关注(Brown et al., 2005;k lahoglu et al., 2014),但仍存在物种特异性基因,这使得C4光合作用基因的核心功能集难以识别(Gowik et al., 2011)。Eleocharis vivipara(苏柏科)是一种两栖无叶莎草,最早由Ueno等人(1988)研究。该植物在陆生条件下具有克兰兹解剖和C4生化性状,并进行NADdependent malic enzyme (nade - me)型C4光合作用。有趣的是,在水下条件下,它生长没有克兰兹解剖结构,并表现出C3生化特征。当被淹没的植物暴露在空气中,它们在大约一周内长出具有C4特征的新芽。因此,该物种适合筛选从C3光合系统到C4光合系统的生化、细胞和结构转变所必需的基因;然而,其相关的基因组和转录组学信息目前还很少
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来源期刊
Environmental Control in Biology
Environmental Control in Biology Agricultural and Biological Sciences-Agronomy and Crop Science
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2.00
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发文量
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