蒺藜苜蓿全基因组中WRKY转录因子的鉴定与分析

WRKY基因家族是植物基因组内一类重要的转录因子, 参与植物许多生理生化过程, 如植物发育、代谢以及生物和非生物胁迫。目前, 已在多种植物中鉴定出WRKY基因家族, 但是关于蒺藜苜蓿(Medicago truncatula L.) WRKY基因家族的系统分析鲜有报道。文章利用生物信息学方法, 从蒺藜苜蓿全基因组中共鉴定出93个WRKY基因, 包括81个标准的WRKY基因(19个Ⅰ型基因, 49个Ⅱ型基因以及13个Ⅲ型基因)和12个非标准类型的WRKY基因。对这些WRKY基因进行了基因重复、染色体定位、基因结构、保守基序和系统进化等方面的分析。蒺藜苜蓿WRKY基因家族中最近共发生了11次基因重复事件, 共涉及24个基因, 占全部WRKY基因的26%。染色体物理定位分析表明, 蒺藜苜蓿WRKY基因在染色体上呈不均匀分布, 存在6个基因簇。对WRKY Ⅲ型基因的进化分析表明, 它们在长期的进化过程中受纯化选择压力。     

Genome-wide identification of Brassica napus microRNAs and their targets in response to cadmium

MicroRNAs (miRNAs) are a distinct class of small RNAs in plants that not only regulate biological processes but also regulate response to environmental stresses. The toxic heavy metal cadmium (Cd) induces expression of several miRNAs in rapeseed (Brassica napus), but it is not known on a genome-wide scale how the expression of miRNAs and their target genes, is regulated by Cd. In this study, four small RNA libraries and four degradome libraries were constructed from Cd-treated and non-Cd-treated roots and shoots of B. napus seedlings. Using high-throughput sequencing, the study identified 84 conserved and non-conserved miRNAs (belonging to 37 miRNA families) from Cd-treated and non-treated B. napus, including 19 miRNA members that were not identified before. Some of the miRNAs were validated by RNA gel blotting. Most of the identified miRNAs were found to be differentially expressed in roots/shoots or regulated by Cd exposure. The study simultaneously identified 802 targets for the 37 (24 conserved and 13 non-conserved) miRNA families, from which there are 200, 537, and 65 targets, belonging to categories I, II, and III, respectively. In category I alone, many novel targets for miRNAs were identified and shown to be involved in plant response to Cd.     

Genome-wide identification and characterization of the aquaporin gene family in Medicago truncatula

Journal of Plant Biochemistry and Biotechnology - Aquaporins (AQPs), or major intrinsic proteins (MIPs), constitute a large and diverse family of protein channel transporter in plants. However, the...     

蒺藜苜蓿多聚半乳糖醛酸酶基因家族的全基因组分析

多聚半乳糖醛酸酶(Polygalacturonases,PGs)是一种果胶水解酶,参与果实成熟、器官脱落、花粉成熟等多个植物发育过程。采用相似性比对和结构域搜索方法,从蒺藜苜蓿基因组中共鉴定出74个MtPG基因。根据系统进化关系将其分为6个亚家族,分别包含9、7、4、11,18和25个MtPG基因家族成员。染色体定位分析发现,MtPG基因在蒺藜苜蓿的8条染色体上呈现不均匀分布,每条染色体上分布有2-16个MtPG基因;同时,基因组复制分析结果显示,蒺藜苜蓿的PG基因家族成员之间存在大量的基因复制。最后,通过蒺藜苜蓿的高通量测序数据分析发现,MtPG基因家族广泛地在根部、结瘤、叶片、芽,心皮和花等组织中表达。根据它们在不同组织中表达水平,将31个MtPG基因聚类为4组,分别探讨了四组基因在蒺藜苜蓿组织器官分化中表达模式,重点解析了它们在花器官发育以及根部组织分化中可能的调控机制,这将为进一步研究蒺藜苜蓿MtPG基因家族成员的基因功能提供了理论基础。     

Identification of aluminum-responsive microRNAs in Medicago truncatula by genome-wide high-throughput sequencing

MicroRNAs (miRNAs) play important roles in response of plants to biotic and abiotic stresses. Aluminum (Al) toxicity is a major factor limiting plant growth in acidic soils. However, there has been limited report on the involvement of miRNAs in response of plants to toxic Al³⁺. To identify Al³⁺-responsive miRNAs at whole-genome level, high-throughput sequencing technology was used to sequence libraries constructed from root apices of the model legume plant Medicago truncatula treated with and without Al³⁺. High-throughput sequencing of the control and two Al³⁺-treated libraries led to generation of 17.1, 14.1 and 17.4 M primary reads, respectively. We identified 326 known miRNAs and 21 new miRNAs. Among the miRNAs, expression of 23 miRNAs was responsive to Al³⁺, and the majority of Al³⁺-responsive mRNAs was down-regulated. We further classified the Al³⁺-responsive miRNAs into three groups based on their expression patterns: rapid-responsive, late-responsive and sustained-responsive miRNAs. The majority of Al³⁺-responsive miRNAs belonged to the ‘rapid-responsive’ category, i.e. they were responsive to short-term, but not long-term Al³⁺ treatment. The Al³⁺-responsive miRNAs were also verified by quantitative real-time PCR. The potential targets of the 21 new miRNAs were predicted to be involved in diverse cellular processes in plants, and their potential roles in Al³⁺-induced inhibition of root growth were discussed. These findings provide valuable information for functional characterization of miRNAs in Al³⁺ toxicity and tolerance.     

Post-translational regulation of cytosolic glutamine synthetase of Medicago truncatula

It was reported recently that the plastid-located glutamine synthetase (GS2) from Medicago truncatula is regulated by phosphorylation catalysed by a calcium-dependent protein kinase and 14-3-3 interaction. Here it is shown that the two cytosolic GS isoenzymes, GS1a and GS1b, are also regulated by phosphorylation but, in contrast to GS2, GS1 phosphorylation is catalysed by calcium-independent kinase(s) and the phosphorylated enzymes fail to interact with 14-3-3s. Phosphorylation of GS1a occurs at more than one residue and was found to increase the affinity of the enzyme for the substrate glutamate. In vitro phosphorylation assays were used to compare the activity of GS kinase, present in different plant organs, against the three M. truncatula GS isoenzymes. All three GS proteins were phosphorylated by kinases present in leaves, roots, and nodules, but to different extents, suggesting a differential regulation under different metabolic contexts. Cytosolic GS phosphorylation was found to be affected by light in leaves and by active nitrogen fixation in root nodules, whereas GS2 phosphorylation was unaffected by these conditions. Some putative GS-binding phosphoproteins were identified showing both isoenzyme and organ specificity. Two phosphoproteins of 70 and 72 kDa were specifically bound to the cytosolic GS isoenzymes. Interestingly, phosphorylation of these proteins was also influenced by the nitrogen-fixing status of the nodule, suggesting that their phosphorylation and/or binding to GS are related to nitrogen fixation. Taken together, the results presented indicate that GS phosphorylation is modulated by nitrogen fixation in root nodules; these findings open up new possibilities to explore the involvement of this post-translational mechanism in nodule functioning.