miR156靶基因SPL在植物中的系统分布和进化模式分析

Squamosa promoterbinding proteinlike genes （SPLs）在植物发育过程中具有重要作用。很多SPLs被miR156调节,然而,对于它们在植物中的系统分布和进化模式还知之甚少。本文对9个测序物种（藻类,苔藓,石松,单子叶和双子叶植物）的183个SPLs进行了生物信息学分析。结果表明miR156应答元件（MREs）仅在陆生植物SPLs中发现,藻类中不存在。系统进化分析显示陆生植物SPLs分为两大分支：group I和group II。 MiR156靶基因仅分布于group II,表明它们有着共同的祖先。Group II进一步分为7个亚支（IIaIIg）,miR156靶基因分布在除IId外的其余6个亚支的特定SPLs。系统分类与基因结构的相关性反映了SPL靶基因结构上的变化。在进化过程中,它们可能发生外显子的丢失且伴随MRE的丢失。另外,基因重复对SPL靶基因的丰度变化影响很大,尤其是被子植物与低等植物分歧后它们数量明显增加。以拟南芥为模式植物分析发现串联重复和片段重复是SPL靶基因扩张的主要机制。     

三裂叶薯SPL基因家族鉴定、表达及miR156的调控分析

SQUAMOSA promoter binding protein-like(SPL)是一类广泛存在于植物中的转录因子,均含有一个高度保守的SBP结构域(SQUAMOSA-PROMOTER BINDING PROTEIN)。本研究通过SBP结构域的隐马尔可夫模型、Blastp、CDD和SMART等程序从栽培甘薯的二倍体近缘野生种三裂叶薯(Ipomoea triloba L.)全基因组中鉴定出26个SPL基因家族成员。它们不均匀分布于三裂叶薯的12条染色体上。利用系统进化分析将新鉴定的26个三裂叶薯ItbSPL基因和来源于苔藓植物、单子叶植物、双子叶植物的116个SPL基因构建进化树,并根据拟南芥AtSPL基因家族的分类标准将26个ItbSPL基因家族分为7组。GSDS 2.0基因结构和MEME 4.12.0保守基序分析表明,不同进化分支中的ItbSPL基因的外显子/内含子数目及其蛋白基序组成差异明显。利用拟南芥中已知功能的SPL对ItbSPL基因的功能进行预测,发现三裂叶薯ItbSPL家族基因成员可能与植物开花、逆境胁迫、次生代谢产物等生物学过程相关。通过预测microRNA156(miR156)的作用位点发现,在26个ItbSPL基因中14个含有miR156的作用位点,其中13个ItbSPL基因具有PCR扩增产物。利用qRT-PCR检测13个候选靶基因及miR156在三裂叶薯叶、茎、根中的表达量,发现13个ItbSPL均在茎中的表达量最低,显著低于叶与根中的表达,而miR156则在茎中的表达量最高,在根中的表达量最低,初步推测这13个ItbSPL是miR156的靶基因。以上研究结果为六倍体栽培甘薯SPL基因家族成员的鉴定、进化分析及功能研究提供了方法和基础。     

小麦tae-MIR156前体基因的克隆及其靶基因TaSPL17多态性分析

Squamosa-promoter binding protein (SBP)-box基因是植物特有的一类转录因子, 广泛参与植物生长发育, 其部分成员受miR156调控。文章克隆了小麦(Triticum aestivum) tae-MIR156前体基因, 转录后能够形成茎环结构。小麦10个SBP-box基因中, 仅TaSPL3和TaSPL17在编码区存在tae-miR156识别位点。SPL17在普通小麦的A基因组供体种乌拉尔图小麦(Triticum urartu, AA) UR209和B基因组供体种拟斯卑尔脱山羊草(Aegilops speltoides, BB) Y2001中均为多拷贝(SPL17-A1、SPL17-A2和SPL17-A3; SPL17-B1、SPL17-B2和SPL17-B3), 在D基因组供体种粗山羊草(Aegilops tauschii, DD) Ae38中仅检测到一种序列(SPL17-D); SPL17-A2与SPL17-B2, SPL17-A3与SPL17-B3、SPL17-D两两之间序列的一致性程度均大于99%, 且与普通小麦(中国春、衡观35和双丰收)的TaSPL17序列具有较高的一致性, 提示它们可能来源于共同的祖先基因, 并且在进化过程中高度保守。靶基因TaSPL17中的tae-miR156识别位点非常保守, 在根据单株穗数和基因型多样性挑选的SubP1和SubP2群体中均未检测到tae-miR156识别位点存在变异碱基。     

MIR166基因家族在陆生植物中的进化模式分析

MicroRNA（miRNA）是一类广泛存在于真核生物中的具有转录后水平调控功能的内源非编码小分子RNA。在植物中．miRNA通过对靶基因的剪切或沉默来实现对植物生命活动的调控,它是基因表达调控网络的重要组成部分。miR165／166（miR166）是陆生植物中最为古老的MIRNA家族之一,它通过对3型同源异域型-亮氨酸拉链（1id—ZIPⅢ）等靶标的调控,在植物的众多发育时期起着关键的调控作用。本文分析了MIR166基因在陆生植物中的进化关系,并对MIR166在基部陆生植物小立碗藓（Physcomitrella patens）中的复制及进化进行了研究。此外,HD—ZIPⅢ蛋白是植物中重要的一类转录因子,miR166对HD-ZIP Ⅲ基因的调控作用在陆地植物保守的存在,本文对HD—ZIP Ⅲ基因和miR166在进化中的相互作用进行了初步的探讨。     

植物SPL转录因子研究进展

SPL(SQUAMOSA promoter-binding protein-like)是一类植物特有的转录因子, 在调控植物胚胎发育、间隔期长度、叶片发育、发育阶段转变、花和果实发育、育性、顶端优势、花青素积累、赤霉素响应、光信号转导及体内铜离子稳态平衡等方面发挥重要作用。SPL含有一个由80个氨基酸残基组成的高度保守的SBP结构域, 以此同下游靶基因启动子区域结合, 调控靶基因的表达。大多数SPL均具有miR156/157识别位点, miR156/157可以通过mRNA剪切或翻译抑制来调控SPL的表达。该文重点综述了植物SPL基因的结构、表达调控及生物学功能, 并对其研究前景进行了展望。     

植物调控枢纽miR156及其靶基因SPL家族研究进展

SPL(SQUAMOSA promoter binding like)家族蛋白是植物特有的一类具有多功能的转录因子家族。在拟南芥中,SPL家族的11个基因受miR156的调控。该家族成员蛋白质都含有十分保守的SBP结构域,该结构域包含2个Zn2+结合位点和1个核定位信号序列。近年来,已从多种植物中分离出miR156及SPL基因。越来越多的研究表明,miR156及SPL家族参与了植物的生长发育、代谢调节及非生物胁迫等多种生物过程,成为植物生长发育的调控枢纽。本文综述了miR156及SPL家族在阶段转变、叶片发育、次生代谢及非生物胁迫等过程中的分子机制,并对其研究前景提出展望。     

植物miR159家族成员分子特性及其进化规律研究

为了解植物miR159家族成员的分子特性及其进化规律,该研究对miRBase数据库中登录的miR159家族成员进行分类统计、进化树构建、科间比较、二级结构预测及靶基因分析。结果表明:miR159家族在植物界分布非常广泛,蕨类植物可能是miR159家族的进化祖先;系统发育进化树分析显示,植物miR159家族成员间存在多个进化分支,且进化关系与植物属性有关,即植物亲缘关系越近的成员更易成枝,且具有相同进化方向的成员序列高度同源;Mfold预测显示,pre-miR159均会自发形成典型、稳定的茎环二级结构,并包含19~21个碱基为单位的功能片段,每个单位均有可能形成miR159成熟体;靶基因分析发现,miR159家族成员主要作用于MYB转录因子、转座因子和假定蛋白等,但在不同物种间及相同物种的不同成员间作用的靶标种类与靶基因ID数量均存在差异,尤其是miR159-3p与miR159-5p间的差异最为显著。     

芥蓝miR156a家族进化特性及表达分析

miRNA广泛参与植物的发育过程。芥蓝形态多样,叶片发育因品种而异。为了解miR156a家族的进化特性及其在芥蓝叶片发育中的表达模式。该研究对芥蓝miR156a成员及其前体pre miR156a成员进行生物信息学分析,比较不同品种芥蓝叶形的差异,并采用qRT PCR方法分析芥蓝不同组织部位中pre miR156a的表达水平、以及叶形相似的芥蓝品种‘翠宝’和‘改良香菇’中不同类型叶片的pre miR156a成员及其靶基因的表达水平。结果表明：(1)多序列比对和进化树分析发现芥蓝miR156a家族成员和pre miR156a 3p_1在进化过程中高度保守;二级结构预测发现pre miR156a每个成员均能形成茎环结构并包含2～3个miR156a成员序列;靶基因预测显示miR156a 5p和miR156a主要靶向SPL,而miR156a 3p_1则靶向CTPS等不同的基因。(2)‘翠宝’和‘改良香菇’芥蓝的叶形最为相似,qRT PCR分析显示,pre miR156a在‘翠宝’营养生长期的叶片中高度表达。(3)pre miR156a成员在‘翠宝’和‘改良香菇’不同类型叶片中差异表达,pre miR156a主要在成熟叶和菇叶中表达,而pre miR156a 3p_1和pre miR156a 5p在第一片真叶中表达量更高。(4)靶基因分析的结果在不同品种中呈现不同趋势,‘翠宝’成熟叶中SPL10/15高表达,SPL2表达量降低;‘改良香菇’中SPL10在成熟叶和菇叶中表达降低,SPL15在菇叶中高表达,SPL2在不同类型叶片中表达无差异。研究认为,miR156a成员及其靶基因SPL2/10/15可能参与调控芥蓝叶片发育,不同品种中作用的靶基因可能存在差异,从而导致了各品种芥蓝叶片发育的差异。     

大豆KNOX基因家族的结构和表达分析

KNOX基因家族编码同源异型盒蛋白, 在植物生长发育过程中起重要调控作用。利用生物信息学手段在全基因组水平上对大豆(Glycine max)KNOX家族基因进行鉴定和分类, 并分析其基因结构、蛋白同源结构域特征以及基因表达方式。研究结果表明: 大豆中的27个GmKNOX基因可以分为GmKNOX I和GmKNOX II两个亚类, 其中GmKNOX I类可分为3个主要的进化支, GmKNOX II类分为2个主要的进化支; 26个GmKNOX基因不均匀地分布在16条染色体上, GmKNOX27尚无法定位。不同组织表达谱的分析表明: GmKNOX I类基因表达部位比较集中, 以茎顶端分生组织中表达量最高; 而GmKNOX II类基因的表达特异性较GmKNOX I类低, 表达部位更广泛。     

植物颗粒结合淀粉合酶GBSS基因家族的进化

为全面理解植物颗粒结合淀粉合酶(GBSS)基因在植物中的进化模式并重建其进化历史, 利用20种陆生植物和2种藻类植物的基因组数据, 通过生物信息学手段, 深入挖掘和分析植物类群基因组中GBSS基因家族的构成和基因特点, 推测其可能的扩增和丢失规律。结果共识别42条同源序列。系统发育和进化分析表明, GBSS基因起源古老, 可能在所有绿色植物的祖先中就已经出现, 之后在进化过程中不断发生谱系的特异扩张和拷贝丢失, 并最终通过功能分化的形式在植物类群中被固定。     

Unraveling the Distribution and Evolution of miR156 targeted SPLs in Plants by Phylogenetic Analysis

Squamosa promoter binding protein like genes (SPLs) are critical during plant development and mostly regulated by miR156. However, little is known about phylogenetic distribution and evolutionary patterns of miR156 targeted SPLs. In this study, 183 SPLs from nine genome sequenced species representing algae, bryophytes, lycophyte, monocots, and eudicots were computationally analyzed. Our results showed that miR156 responsive elements (MREs) on SPLs were present in land plants but absent from unicellular green algae. Phylogenetic analysis revealed that miR156 targeted SPLs only distributed in group II not group I of land plants, suggesting they originated from a common ancestor. In addition, group II were further divided into seven subgroups (IIa IIg) and miR156 targeted SPLs distributed in some specific members of SPLs from six subgroups except subgroup IId. Such distribution pattern was well elucidated by gene structure evolution of miR156 targeted SPLs based on the correlation of phylogenetic classification and gene structure. They could suffer from the exon loss events combined with MREs loss during evolution. Moreover, gene duplication contributed to the abundance of miR156 targeted SPLs, which had significantly increased after angiosperms and lower plants split. With Arabidopsis as the model species, we found segmental and tandem gene duplications predominated during miR156 targeted SPLs expansion. Taken together, these results provide better insights in understanding the function diversity and evolution of miR156 targeted SPLs in plants.     

miRNA control of vegetative phase change in trees

After germination, plants enter juvenile vegetative phase and then transition to an adult vegetative phase before producing reproductive structures. The character and timing of the juvenile-to-adult transition vary widely between species. In annual plants, this transition occurs soon after germination and usually involves relatively minor morphological changes, whereas in trees and other perennial woody plants it occurs after months or years and can involve major changes in shoot architecture. Whether this transition is controlled by the same mechanism in annual and perennial plants is unknown. In the annual forb Arabidopsis thaliana and in maize (Zea mays), vegetative phase change is controlled by the sequential activity of microRNAs miR156 and miR172. miR156 is highly abundant in seedlings and decreases during the juvenile-to-adult transition, while miR172 has an opposite expression pattern. We observed similar changes in the expression of these genes in woody species with highly differentiated, well-characterized juvenile and adult phases (Acacia confusa, Acacia colei, Eucalyptus globulus, Hedera helix, Quercus acutissima), as well as in the tree Populus x canadensis, where vegetative phase change is marked by relatively minor changes in leaf morphology and internode length. Overexpression of miR156 in transgenic P. x canadensis reduced the expression of miR156-targeted SPL genes and miR172, and it drastically prolonged the juvenile phase. Our results indicate that miR156 is an evolutionarily conserved regulator of vegetative phase change in both annual herbaceous plants and perennial trees.     

Evolutionary Comparison of Two Combinatorial Regulators of SBP-Box Genes,MiR156 and MiR529, in Plants

A complete picture of the evolution of miRNA combinatorial regulation requires the synthesis of information on all miRNAs and their targets. MiR156 and miR529 are two combinatorial regulators of squamosa promoter binding protein-like (SBP-box) genes. Previous studies have clarified the evolutionary dynamics of their targets; however, there have been no reports on the evolutionary patterns of two miRNA regulators themselves to date. In this study, we investigated the evolutionary differences between these two miRNA families in extant land plants. Our work found that miR529 precursor, especially of its mature miRNA sequence, has a higher evolutionary rate. Such accelerating evolution of miR529 has significantly effects on its structural stability, and sequence conservation against existence of itself. By contrast, miR156 evolves more rapidly in loop region of the stable secondary structure, which may contribute to its functional diversity. Moreover, miR156 and miR529 genes have distinct rates of loss after identical duplication events. MiR529 genes have a higher average loss rate and asymmetric loss rate in duplicated gene pairs, indicating preferred miR529 gene losses become another predominant mode of inactivation, that are implicated in the contraction of this family. On the contrary, duplicated miR156 genes have a low loss rate, and could serve as another new source for functional diversity. Taken together, these results provide better insight into understanding the evolutionary divergence of miR156 and miR529 family in miRNA combinational regulation network.     

Distribution of introns in the mitochondrial gene nad1 in land plants: phylogenetic and molecular evolutionary implications

Forty-six species of diverse land plants were investigated by sequencing for their intron content in the mitochondrial gene nad1. A total of seven introns, all belonging to group II, were found, and two were newly discovered in this study. All 13 liverworts examined contain no intron, the same condition as in green algae. Mosses and hornworts, however, share one intron by themselves and another one with vascular plants. These intron distribution patterns are consistent with the hypothesis that liverworts represent the basal-most land plants and that the two introns were gained in the common ancestor of mosses-hornworts-vascular plants after liverworts had diverged. Hornworts also possess a unique intron of their own. A fourth intron was found only in Equisetum L., Marattiaceae, Ophioglossum L., Osmunda L., Asplenium L., and Adiantum L., and was likely acquired in their common ancestor, which supports the monophyly of moniliformopses. Three introns that were previously characterized in angiosperms and a few pteridophytes are now all extended to lycopods, and were likely gained in the common ancestor of vascular plants. Phylogenetic analyses of the intron sequences recovered topologies mirroring those of the plants, suggesting that the introns have all been vertically inherited. All seven nad1 group II introns show broad phylogenetic distribution patterns, with the narrowest being in moniliformopses and hornworts, lineages that date back to at least the Devonian (345 million years ago) and Silurian (435 million years ago), respectively. Hence, these introns must have invaded the genes via ancient transpositional events during the early stage of land plant evolution. Potentially heavy RNA editing was observed in nad1 of Haplomitrium Dedecek, Takakia Hatt. & Inoue, hornworts, Isoetes L., Ophioglossum, and Asplenium. A new nomenclature is proposed for group II introns.