拟南芥F-box基因At3g16740的表达分析

拟南芥At3g16740基因为F-box基因家族成员,其功能尚不清楚.通过连续和瞬时光照处理分析,发现蓝光、红光和远红光都诱导At3g16740基因的表达,其中远红光的诱导作用最明显.蓝光受体cry1、cry2,红光受体phyB或远红光受体phyA突变导致At3g16740基因表达的光诱导作用减弱或者消失,表明该基因为光信号通路相关基因.通过实时荧光定量PCR分析At3g16740基因在拟南芥不同组织器官中的表达,发现其在拟南芥根、茎、叶、花和果荚中都有表达,花和果荚中的表达量最高,推测该基因可能参与植物花和/或果荚的发育.酵母双杂交分析发现,At3g16740蛋白通过F-box结构域与拟南芥ASK(arabidopsis-SKP1-like)家族成员ASK1、ASK2和ASK11相互作用,表明At3g16740是SCF(Skp、Cullin、F-box)复合物的成员.     

花粉特异F-box基因及其表达产物可能参与的SCF途径

泛素蛋白体目标性降解蛋白途径是许多细胞学过程的重要调节体系,底物蛋白泛素化涉及3个酶激反应,其中,作为E3连接酶的SCF复合体对底物的识别是通过亚体F-box蛋白C末端的特异性结构实现的.利用染色体步移等方法,最近在一些配子体型自交不亲和植物S-RNase基因近旁相继发现了一类花粉特异性表达的F-box基因,从而预示泛素介导的SCF蛋白降解途径可能参与配子体自交不亲和反应.     

植物F-box基因家族的研究进展

F-box基因家族是植物中最大的基因家族之一,由于其数量巨多,根据其蛋白C末端结构域的不同被分为不同的亚家族。F-box基因编码的蛋白能够调节多种多样的生命活动,如延缓植物衰老、调控植物开花以及响应生物胁迫、干旱和盐等逆境胁迫。近年来,随着全基因组测序的不断完善,越来越多物种的F-box基因被分析鉴定出来。已经鉴定出功能的F-box基因编码的蛋白大多能够和结合蛋白Skp1、骨架蛋白Cullin 1及Rbx1形成SCF复合体,进而参与泛素-蛋白酶途径(UPP)而发挥作用;少部分F-box蛋白以非SCF复合体形式发挥作用。泛素-蛋白酶途径(UPP)是机体重要的调节机制之一,大多数细胞内蛋白都是经过这一途径降解。主要对其蛋白结构,作用途径以及生物学功能进行概述,探讨F-box基因参与的生命活动,旨为F-box的深入研究奠定基础。     

拟南芥磷酸酶基因亚细胞定位与组织表达

通过克隆拟南芥磷酸酶PP2C家族基因At3g51370,构建了绿色荧光蛋白融合表达载体,用基因枪将构建好的载体轰击洋葱表皮细胞进行瞬时表达分析,发现该At3g51370基因表达蛋白定位在细胞核中;用实时定量PCR方法分析At3g51370基因的组织表达特性,发现该基因在花器官中的表达量明显高于其它组织.进一步构建了含At3g51370基因的启动子和GUS报告基因的植物表达载体,经农杆菌介导转化拟南芥,对转基因拟南芥进行GUS组织化学染色,分析该启动子在不同生长时期与不同组织中的转录活性,结果发现,在幼苗期At3g51370基因主要集中在根尖分生组织和顶端分生组织表达,在成年植株中则集中在生殖器官如花和果荚柄等部位表达,在光照和黑暗条件下,At3g51370基因的表达特性没有明显差异.研究表明,At3g51370可能与其它核定位的PP2C磷酸酶一样参与了基因表达的调控,可能在拟南芥早期发育阶段的细胞增值分裂相关信号转导途径中发挥功能,并在花器官的发育过程中行使功能,且不参与光信号转导.     

拟南芥ASK基因研究进展拟南芥ASK基因研究进展拟南芥ASK基因研究进展拟南芥ASK基因研究进展拟南芥ASK基因研究进展

泛素-蛋白酶体系统（ubiquitin-proteasome system, UPS）是广泛存在于真核生物中的一种重要的蛋白降解系统。拟南芥ASK （Arabidopsis SKP1-LIKE）基因编码拟南芥E3连接酶SCF复合物的一个亚蛋白, 在拟南芥SCF复合物中起到连接器的作用。近年来, 人们对ASK基因及其同源基因进行了很多表达规律、基因功能方面的研究。本文从ASK基因表达方式、对生理发育过程的调节、与F-box相互作用及ASK基因的进化方式4个方面对这些进展进行总结。已有的研究结果表明, ASK基因在拟南芥中广泛地表达并表现出各自不同的表达水平和表达方式, 它们在很多发育和生理过程中起到重要作用。     

拟南芥ASK基因研究进展

泛素-蛋白酶体系统(ubiquitin-proteasome system,UPS)是广泛存在于真核生物中的一种重要的蛋白降解系统。拟南芥ASK(Arabidopsis SKP1-LIKE)基因编码拟南芥E3连接酶SCF复合物的一个亚蛋白,在拟南芥SCF复合物中起到连接器的作用。近年来,人们对ASK基因及其同源基因进行了很多表达规律、基因功能方面的研究。本文从ASK基因表达方式、对生理发育过程的调节、与F-box相互作用及ASK基因的进化方式4个方面对这些进展进行总结。已有的研究结果表明,ASK基因在拟南芥中广泛地表达并表现出各自不同的表达水平和表达方式,它们在很多发育和生理过程中起到重要作用。     

F-box蛋白质在植物生长发育中的功能

在真核生物中, 泛素介导的蛋白降解途径参与了许多生物学过程。SCF复合体是一种非常重要的E3泛素连接酶, 在植物中研究的最为深入。F-box蛋白包含一个F-box 基序, 是SCF复合体的一个亚基, 它决定了底物识别的特异性。目前, 从各种植物中已鉴定出大量的F-box蛋白质, 它们参与了植物激素(乙烯, 生长素, GA, JA)的信号传导以及自交不亲和、花器官发育等生物学过程, F-box蛋白还参与了植物的胁迫反应。最新研究结果显示, 一个F-box蛋白TIR1是生长素的受体。因此, F-box蛋白质介导的泛素化蛋白质降解途径可能是植物基因表达调控的重要机制。     

WRKY25过量表达导致拟南芥在长光照下开花提前

WRKY基因家族是主要存在于植物中的一大类转录调控因子,拥有很多家族成员.拟南芥WRKY25属于第Ⅰ类WRKY蛋白,参与植物生物和非生物胁迫反应.通过GUS染色和qRT-PCR发现WRKY25基因主要在根,叶和茎生叶中表达.过量表达WRKY25的转基因植株在长光照下比野生型拟南芥提前开花.通过RT-PCR检测与开花时间相关基因发现,AP1基因的表达量在培养21 d和27d的WRKY25过量表达植株中上调,由此推测WRKY25很可能通过增强AP1的表达来影响开花.     

人工microRNAs对拟南芥At1g13770和At2g23470基因的特异沉默

DUF647 (Domain of unknown function 647) 蛋白家族是在真核生物中广泛存在的、高度保守的蛋白家族。拟南芥中该基因家族共有6个成员, 迄今为止拟南芥DUF647家族中4个成员的功能尚不清楚。文章以拟南芥内源MIR319a前体为骨架, 构建了敲减DUF647家族中2个基因At1g13770和At2g23470表达的人工microRNAs(Artifical microRNAs, amiRNAs)。利用WMD(Web microRNA designer)平台设计分别靶向At1g13770和At2g23470基因的amiRNAs序列, 通过重叠PCR置换拟南芥MIR319a前体序列。构建融合amiRNAs前体的植物表达载体pCHF3-amiRNAs, 在农杆菌介导下转化拟南芥。RT-PCR分析表明, amiRNAs能够显著抑制At1g13770和At2g23470基因的表达, 获得了抑制效果明显的转基因株系。At2g23470-amiRNA转基因植株At2g23470转录水平的下调导致育性严重下降。文章为进一步研究这两个基因的功能奠定了良好的基础。     

人工microRNAs对拟南芥At1g13770和At2g23470基因的特异沉默

DUF647(Domain of unknown function 647)蛋白家族是在真核生物中广泛存在的、高度保守的蛋白家族。拟南芥中该基因家族共有6个成员,迄今为止拟南芥DUF647家族中4个成员的功能尚不清楚。文章以拟南芥内源MIR319a前体为骨架,构建了敲减DUF647家族中2个基因At1g13770和At2g23470表达的人工microRNAs(Artifical microRNAs,amiRNAs)。利用WMD(Web microRNA designer)平台设计分别靶向At1g13770和At2g23470基因的amiRNAs序列,通过重叠PCR置换拟南芥MIR319a前体序列。构建融合amiRNAs前体的植物表达载体pCHF3-amiRNAs,在农杆菌介导下转化拟南芥。RT-PCR分析表明,amiRNAs能够显著抑制At1g13770和At2g23470基因的表达,获得了抑制效果明显的转基因株系。At2g23470-amiRNA转基因植株At2g23470转录水平的下调导致育性严重下降。文章为进一步研究这两个基因的功能奠定了良好的基础。     

Wheat F-box protein recruits proteins and regulates their abundance during wheat spike development

F-box proteins, components of the Skp1-Cullin1-F-box (SCF) protein E3 ubiquitin ligase complex, serve as the variable component responsible for substrate recognition and recruitment in SCF-mediated proteolysis. F-box proteins interact with Skp1 through the F-box motif and with ubiquitination substrates through C-terminal protein interaction domains. F-box proteins regulate plant development, various hormonal signal transduction processes, circadian rhythm, and cell cycle control. We isolated an F-box protein gene from wheat spikes at the onset of flowering. The Triticum aestivum cyclin F-box domain (TaCFBD) gene showed elevated expression levels during early inflorescence development and under cold stress treatment. TaCFBD green fluorescent protein signals were localized in the cytoplasm and plasma membrane. We used yeast two-hybrid screening to identify proteins that potentially interact with TaCFBD. Fructose bisphosphate aldolase, aspartic protease, VHS, glycine-rich RNA-binding protein, and the 26S proteasome non-ATPase regulatory subunit were positive candidate proteins. The bimolecular fluorescence complementation assay revealed the interaction of TaCFBD with partner proteins in the plasma membranes of tobacco cells. Our results suggest that the TaCFBD protein acts as an adaptor between target substrates and the SCF complex and provides substrate specificity to the SCF of ubiquitin ligase complexes.     

The COP9 signalosome interacts with SCF UFO and participates in Arabidopsis flower development

The COP9 signalosome (CSN) is involved in multiple developmental processes. It interacts with SCF ubiquitin ligases and deconjugates Nedd8/Rub1 from cullins (deneddylation). CSN is highly expressed in Arabidopsis floral tissues. To investigate the role of CSN in flower development, we examined the expression pattern of CSN in developing flowers. We report here that two csn1 partially deficient Arabidopsis strains exhibit aberrant development of floral organs, decline of APETALA3 (AP3) expression, and low fertility in addition to defects in shoot and inflorescence meristems. We show that UNUSUAL FLORAL ORGANS (UFO) forms a SCF(UFO) complex, which is associated with CSN in vivo. Genetic interaction analysis indicates that CSN is necessary for the gain-of-function activity of the F-box protein UFO in AP3 activation and in floral organ transformation. Compared with the previously reported csn5 antisense and csn1 null mutants, partial deficiency of CSN1 causes a reduction in the level of CUL1 in the mutant flowers without an obvious defect in CUL1 deneddylation. We conclude that CSN is an essential regulator of Arabidopsis flower development and suggest that CSN regulates Arabidopsis flower development in part by modulating SCF(UFO)-mediated AP3 activation.     

高表达miR396小分子导致拟南芥花柱头弯曲

MicroRNAs（miRNAs）是大小约21个碱基、内源、非编码的小分子RNA。以拟南芥（Arabidopsis thaliana）miR396小分子为研究对象,分别克隆到了miR396小分子的两个前体（MIR396a,MIR396b）,得到了转基因植株。通过转基因植株的遗传学研究发现,高表达miR396小分子导致转基因拟南芥的花柱头弯曲。花柱头的弯曲影响了角果的正常发育。另外,Northern杂交结果表明转基因拟南芥花部位的miR396及其前体的表达量与对照相比显著增加。这些结果表明高表达miR396小分子可以导致拟南芥花柱头弯曲。     

Structure and expression of the gene encoding mouse F-box protein, Fwd2

A novel class of ubiquitin ligases, termed the SCF complex, consists of invariable components, Skp1 and Cullin, and variable components called F-box proteins, which have a primary role in determining substrate specificity. We have isolated a cDNA encoding the mouse F-box protein Fwd2 (also known as MD6) as a possible constituent of an SCF-type ubiquitin ligase. Fwd2 cDNA contains 1890 bp with a 1362-bp open reading frame and encodes an approximately 51.5-kDa protein. Fwd2 is expressed predominantly in liver and, to a lesser extent, in the testis, lung, heart, and skeletal muscle. Immunofluorescence staining for Fwd2 protein shows a pattern with the cytoplasm. A coimmunoprecipitation assay has revealed the in vivo interaction between Skp1 and Fwd2 through the F-box domain. Fwd2 also interacts with Cul1 through Skp1, suggesting that Skp1, Cul1, and the F-box protein Fwd2 form an SCF complex (SCF(Fwd2)). We have also isolated and determined the nucleotide sequence and genomic organization of the gene that encodes mouse Fwd2. This gene spans approximately 17 kb and consists of six exons and five introns. Our results suggest that Fwd2 is an F-box protein that constitutes an SCF ubiquitin ligase complex and that it plays a critical role in the ubiquitin-dependent degradation of proteins expressed in the liver.     

The abundance of Met30p limits SCF(Met30p) complex activity and is regulated by methionine availability

Ubiquitin-mediated degradation plays a crucial role in many fundamental biological pathways, including the mediation of cellular responses to changes in environmental conditions. A family of ubiquitin ligase complexes, called SCF complexes, found throughout eukaryotes, is involved in a variety of biological pathways. In Saccharomyces cerevisiae, an SCF complex contains a common set of components, namely, Cdc53p, Skp1p, and Hrt1p. Substrate specificity is defined by a variable component called an F-box protein. The F- box is a approximately 40-amino-acid motif that allows the F-box protein to bind Skp1p. Each SCF complex recognizes different substrates according to which F-box protein is associated with the complex. In yeasts, three SCF complexes have been demonstrated to associate with the ubiquitin-conjugating enzyme Cdc34p and have ubiquitin ligase activity. F-box proteins are not abundant and are unstable. As part of the SCF(Met30p) complex, the F-box protein Met30p represses methionine biosynthetic gene expression when availability of L-methionine is high. Here we demonstrate that in vivo SCF(Met30p) complex activity can be regulated by the abundance of Met30p. Furthermore, we provide evidence that Met30p abundance is regulated by the availability of L-methionine. We propose that the cellular responses mediated by an SCF complex are directly regulated by environmental conditions through the control of F-box protein stability.     

Occurrence of a putative SCF ubiquitin ligase complex in Drosophila

Many proteins are targeted to proteasome degradation by a family of E3 ubiquitin ligases, termed SCF complexes, that link substrate proteins to an E2 ubiquitin-conjugating enzyme. SCFs are composed of three core proteins-Skp1, Cdc53/Cull, Rbx1/Hrt1-and a substrate specific F-box protein. We have identified in Drosophila melanogaster the closest homologues to the human components of the SCF(betaTrCP) complex and the E2 ubiquitin-conjugating enzyme UbcH5. We show that putative Drosophila SCF core subunits dSkpA and dRbx1 both interact directly with dCu11 and the F-box protein Slmb. We also describe the direct interaction of the UbcH5 related protein UbcD1 with dCul1 and Slmb. In addition, a functional complementation test performed on a Saccharomyces cerevisiae Hrt1p-deficient mutant showed that Drosophila Rbx1 is able to restore the yeast cells viability. Our results suggest that dRbx1, dSkpA, dCullin1, and Slimb proteins are components of a Drosophila SCF complex that functions in combination with the ubiquitin conjugating enzyme UbcD1.     

The F-box protein family

The F-box is a protein motif of approximately 50 amino acids that functions as a site of protein-protein interaction. F-box proteins were first characterized as components of SCF ubiquitin-ligase complexes (named after their main components, Skp I, Cullin, and an F-box protein), in which they bind substrates for ubiquitin-mediated proteolysis. The F-box motif links the F-box protein to other components of the SCF complex by binding the core SCF component Skp I. F-box proteins have more recently been discovered to function in non-SCF protein complexes in a variety of cellular functions. There are 11 F-box proteins in budding yeast, 326 predicted in Caenorhabditis elegans, 22 in Drosophila, and at least 38 in humans. F-box proteins often include additional carboxy-terminal motifs capable of protein-protein interaction; the most common secondary motifs in yeast and human F-box proteins are WD repeats and leucine-rich repeats, both of which have been found to bind phosphorylated substrates to the SCF complex. The majority of F-box proteins have other associated motifs, and the functions of most of these proteins have not yet been defined.