拟南芥AST基因的精细作图

拟南芥(Arabidopsis thaliana(L.)Heynh.)ast(anthocyanin spottedtesta)突变体是由碳离子辐射诱导产生的与花青苷生物合成有关的基因突变体,受单隐性核基因控制.根据拟南芥数据库中的SNPs(single nucleotide polv-mophisms)序列和插入/缺失多态性(insertion/deletion polymorphisms)序列,设计了一系列分子标记.采用图位克隆策略,应用这些分子标记完成了对拟南芥AST基因的精细作图,成功地将AST基因定位到BAC克隆T13M11上,初步认为该BAC克隆中的基因T13M11.8可能是AST基因.该基因的DNA序列长1432bp,含有6个外显子和5个内含子,编码的蛋白与花青苷生物合成途径中的二氢黄酮醇-4-还原酶有较高的同源性.将进一步通过功能互补实验验证图位克隆的结果.     

拟南芥细胞死亡突变体mod1突变座位的精细物理图谱构建

拟南芥细胞死亡突变体mod1突变位点位于第2染色体分子标记IGS1和mi421之间. 以这一区域YAC重叠群中的YAC克隆末端DNA片段CIC9A3R, CIC11C7L, CIC2G5R及RFLP分子标记克隆CDs3为探针筛选TAMU BAC文库, 获得31个阳性BAC克隆. 用BAC克隆的末端DNA片段杂交所有阳性BAC克隆, 确立了由T6P5, T7M23, T12A21, T8L6及T18A18等克隆组成的MOD1基因所在区域的BAC重叠群. 同时在这一区域发展出11个CAPS分子标记和12个STS序标, 为MOD1基因的图位克隆与鉴定分析及这一区域的全序列测定奠定了基础.     

拟南芥DNA去甲基化基因RLL4的定位与功能分析

该研究以携带2×35S:LUC报告基因的转基因拟南芥Col-LUC为亲本系,将其种子进行甲基磺酸乙酯(EMS)诱变,在M2代筛选出1株低荧光的候选突变体,命名为rll4(reduced LUC luminescence 4)。遗传学分析表明,rll4突变位点包含1个核基因隐性突变。图位克隆技术定位结果显示,突变基因的位点位于4号染色体2个分子标记CL417-B10M1和CL418-B2M2之间,这2个分子标记分别位于F20D10和F20M13BAC(bacterial artificial chromosome)克隆。酶切PCR(Chop-PCR)结果显示,rll4突变体中基因组DNA的部分位点甲基化显著升高。反转录PCR(RT-PCR)结果显示,rll4突变体中ROS1(REPRESSOR OF SILENCING 1)的表达量并没有明显变化,而一些RNA介导的DNA甲基化(RdDM)过程靶位点的基因表达量有明显下降。研究表明,RLL4位点很可能参与了拟南芥DNA去甲基化过程。     

拟南芥网状突变体E-210基因精细定位

通过甲基磺酸乙酯(EMS)诱变与遗传分析,从拟南芥(Arabidopsis thaliana)中筛选到一株隐性单基因控制的网状突变体E-210。该突变体植株生长缓慢,叶脉呈绿色,叶肉呈黄色。通过透射电镜观察,发现野生型植株和突变植株在叶绿体结构上差异不大,猜测该突变体E-210基因与叶绿体的发育可能没有直接关系,而很可能同叶绿素或叶绿体的生物合成有关。通过图位克隆的方法,将该突变体的突变基因定位在第5条染色体上的MRB17和MBG8-5的分子标记之间,精确到87.130kb。对MRB17和MBG8-5的分子标记之间的22个基因进行了分析,预测突变体E-210基因可能是At5g54770,编码THI1,即噻唑合成酶。     

ABA信号通路对葡萄果皮花青苷生物合成的调控机制研究

以‘红巴拉多’葡萄为试验材料,在转色前期(约花后6周)用300 mg/L的ABA对果穗进行处理,以清水处理为对照;测定不同发育时期葡萄果实的单果重、可滴定酸、可溶性固性物等生理指标,同时测定果皮中总花青苷及ABA含量;检测不同发育时期果皮中ABA信号通路和花青苷生物合成相关基因表达量,克隆6个与花青苷生物合成相关基因的启动子,并预测启动子中的顺式作用元件,在转录调控水平上探讨ABA信号通路对葡萄果皮花青苷生物合成的调控作用。结果表明:(1)ABA处理的葡萄果实可溶性固形物含量明显提高、可滴定酸含量下降。(2)ABA处理显著提高了‘红巴拉多’葡萄果皮的着色水平以及总花青苷和ABA含量。(3)ABA处理后,9个ABA信号通路基因以及6个花青苷生物合成相关基因表达水平明显提高。(4)6个花青苷生物合成相关基因的启动子序列中均含有多个与ABA响应相关的ABRE作用元件。研究发现,9个ABA信号通路基因可能在葡萄果皮着色中发挥着重要作用,其中2个VvABFs转录因子可能直接作用于含有ABRE元件的花青苷生物合成相关基因的启动子序列,推测可通过调控这些基因的转录水平来调控葡萄果皮花青苷的积累。     

拟南芥网状突变体E-210基因精细定位

通过甲基磺酸乙酯(EMS)诱变与遗传分析,从拟南芥(Arabidopsis thaliana)中筛选到一株隐性单基因控制的网状突变体E-210.该突变体植株生长缓慢,叶脉呈绿色,叶肉呈黄色.通过透射电镜观察,发现野生型植株和突变植株在叶绿体结构上差异不大,猜测该突变体E-210基因与叶绿体的发育可能没有直接关系,而很可能同叶绿素或叶绿体的生物合成有关.通过图位克隆的方法,将该突变体的突变基因定位在第5条染色体上的MRBl7和MBG8-5的分子标记之间,精确到87.130 kb.对MRB17和MBG8-5的分子标记之间的22个基因进行了分析,预测突变体E-210基因可能是At5g54770,编码THI1,即噻唑合成酶.     

拟南芥白化突变体心口的基因定位与分析

EMS30是拟南芥经甲基磺酸乙酯（EMS）诱变得到的白化突变体。该突变体的叶绿体结构存在严重缺陷,同时伴随叶绿素缺失。遗传分析显示EMS30突变体的突变表型受隐性单基因控制。采用图位克隆的方法对EMS30突变基因进行定位的结果显示,该基因位于拟南芥第一条染色体的分子标记F21M12和F14N23之间的96kb区间内,该区间包含25个基因。通过生物信息学分析发现,该区间内有3个基因定位在叶绿体或与叶绿体发育相关。这些结果有助于该基因的克隆,为阐释叶绿体发育提供线索。     

水稻抗白叶枯病基因Xa4位点跨叠BAC克隆群的构建

水稻白叶枯病抗性基因Xa4已被定位于第11染色体长臂末端的分子标记VG181和L1044之间,并与抗性基因同源序列片段RS13共分离。利用这3个标记筛选IRBB56的BAC文库,共得到128个阳性BAC克隆,其中RS13获得18个阳性克隆,这18个克隆中有4个和6个我隆分别同时为G181和L1044的阳性克隆,选其中的12克隆进行分析,构建了一个从G181到L1044区间的BAC跨叠克隆,全长420kb,并且56M22、106P13和104B153个BAC克隆可覆盖整个跨叠克隆群。这一研究结果为进一步分离Xa4基因打下基础。     

一个控制拟南芥小孢子发育基因的定位

通过EMS诱变、背景纯化与遗传分析,从拟南芥突变群体中分离到一株单隐性核位点控制的雄性部分不育突变体pms15-16-2-3.细胞学观察表明,突变体在花药发育的过程中,中层细胞延迟降解,绒毡层细胞形态分化异常,出现异常的四分体,导致最终只能形成少量的花粉.利用图位克隆的方法对该基因进行了定位,结果表明PMSl5-16-2.3基因位于拟南芥第3条染色体BAC克隆T24C20 上的28 kb区间内.目前该区间内尚未见到控制小孢子发育基因的报道,因此该基因是一个控制小孢子发育的新基因.本研究结果对同的基因的克隆及其在化粉发育中的功能研究奠定了基础.     

用于拟南芥染色体着陆的一套InDel标记的设计与应用

在拟南芥图位克隆中SSLP(simple sequence length polymorphism)是首选分子标记,当无可用SSLP时才会考虑CAPS(cleaved amplified polymorphic sequence)、d CAPS(designed CAPS)及SNAP(single nucleotide amplified polymorphism)等标记。图位克隆的第1步就是染色体着陆,需逐个检测覆盖全基因组的标记,工作繁琐,更加依赖操作相对简单的SSLP标记。但是,SSLP标记在染色体上分布不均,有些标记缺乏物理位置记录,而且很多标记的PCR反应体系和扩增条件不同,这些瑕疵增加了染色体着陆乃至图位克隆其他步骤的工作量,有碍图位克隆的顺利开展。针对上述不足,以InDel多态性位点为基础设计一组标记,专门用于染色体着陆,以弥补现有SSLP标记的不足。这套标记有确切的物理位置,每个标记所控制的染色体区间小于30 cM,而且这套标记可采用相同的PCR反应体系和反应程序。随即用这套标记成功地实现了6个Ler背景的隐性突变体的染色体着陆,显示这组标记能够满足实验要求,使得拟南芥图位克隆得到简化。     

Mapping and Analysis of a Yellow Mutant chlm-4 of Arabidopsis thaliana (Cruciferae)

Chlorophylls are essential for photosynthesis. Chlorophyll biosynthesis is catalyzed by a series of enzyme complexes, such as Mg protoporphyrin IX methyltransferase. A yellow mutant of Arabidopsis was isolated using an enthyl methane sulfonate (EMS) mutagenesis strategy. Chlorophyll content dramatically reduced and grana stacking was absent in the mutant. Genetic analysis indicated that the mutant was controlled by a single recessive gene. Using map based cloning strategy, the gene responsible for the mutant phenotype was mapped to a region of 114 kb between the molecular markers F13M23 and T30C3 on chromosome 4, in which the CHLM gene encoding Mg protoporphyrin IX methyltransferase was included. The mutant was proved to be an allelic mutant of CHLM gene by sequencing and allelism test and then was designated as chlm 4. Gly59 of CHLM was replaced by Glu59 in chlm 4, which indicated that Gly59 was essential for the function of Mg protoporphyrin IX methyltransferase.     

拟南芥黄化突变体chlm-4的基因定位与分析

叶绿素是光合作用必需的重要色素,其合成需要Mg-原卟啉Ⅸ甲基转移酶等一系列酶的催化。我们通过筛选拟南芥EMS（乙基磺酸甲酯,ethyl-methane sulphonate）突变体库,分离到一个黄化突变体。该突变体叶绿素含量显著减少,叶绿体内垛叠的基粒缺失。遗传学分析表明,该突变体的黄化表型是由单基因控制的隐性性状。利用图位克隆的方法最终将基因定位在第IV条染色体分子标记F13M23和T30C3之间114kb的区间内,其中包含编码Mg-原卟啉Ⅸ甲基转移酶的CHLM基因。通过测序及等位分析表明该突变体是chlm的等位突变体,命名为chlm-4。在chlm-4中,CHLM蛋白的Gly59突变成Glu59,说明Gly59对于Mg-原卟啉Ⅸ甲基转移酶功能的行使是必需的。     

Cloning and expression analysis of a gene that shows developmental regulation upon tuberization in potato

An Arabidopsis cDNA clone encoding a DNA-binding protein, RAP-1, was isolated by southwestern screening of an Escherichia coli cDNA expression library. The protein contains a bHLH DNA-binding domain and is homologous to R proteins, regulating anthocyanin biosynthesis. RAP-1 binds to the sequence CACNTG. It is encoded by a single gene, which is expressed to high levels in root and stem and to low levels in leaf and flower. No expression could be detected in siliques. Rap-1 does not correspond to one of the known loci involved in anthocyanin biosynthesis, since it is located at a different map position. In contrast to the maize R protein Lc, RAP-1 did not induce anthocyanin biosynthesis in pea cotyledons. Thus, RAP-1 is a novel member of the bHLH class of DNA-binding proteins.     

Transparent Testa Glabra 1 (TTG1) and TTG1-like genes in Matthiola incana R. Br. and related Brassicaceae and mutation in the WD-40 motif

TTG1 (Transparent Testa Glabra 1), a WD-40 repeat protein, is involved in regulation of flavonoid/anthocyanin biosynthesis, seed coat (mucilage) development/pigmentation and trichome formation in leaves. Here, we characterized the TTG1 gene of Matthiola incana wild type ( e locus), showing 85.3% similarity to TTG1 of A. thaliana on the nucleotide level and 96.2% on the protein level. A white-flowered and glabrous mutant, line 17, of M. incana exhibits one nucleotide change, leading to an amino acid substitution directly in the WD motif (W158R). Correspondingly, the DFR (dihydroflavonol 4-reductase) gene, in which the expression is known to be dependent on TTG1, is not expressed in Matthiola mutant lines 17 (and 19). Comparison of the GC content of the Matthiola TTG1 (54.1%) and Arabidopsis TTG1 (46.1%) genes revealed a strong difference, mostly obtained by neutral substitutions (C to T transitions). To examine whether this is an ecologically influenced trend, a fragment of TTG1 was characterized from another Matthiola species ( M. tricuspidata ) and from Malcolmia flexuosa subsp. naxensis from the eastern Mediterranean, near a beach with sandy and salty soils. Both Matthiola species have a higher GC content in the TTG1 gene than Arabidopsis and the closer-related Malcolmia , indicating that the GC content is rather an evolutionary than an ecological signal. A similar WD-40 repeat protein gene (containing no intron in the 3' untranslated region) with high similarity to the Arabidopsis TTG1 -like ( AtAN11 ) gene was found in Matthiola .     

The COI1 and DFR Genes are Essential for Regulation of Jasmonate-Induced Anthocyanin Accumulation in Arabidopsis

Jasmonates(JAs)are a class of plant hormones that play important roles in the regulation of plant development and plantdefense.It has been shown that Arabidopsis plants produce much higher levels of anthocyanins when treated exogenouslywith methyl jasmonate(MeJA).However,a molecular link between the JA response and anthocyanin production hasnot been determined.The CORONATINE INSENTITIVE1(COI1)gene is a key player in the regulation of many JA-relatedresponses.In the present study,we demonstrate that the COI1 gene is also required for the JA-induced accumulation ofanthocyanins in Arabidopsis.Furthermore,the MeJA-inducible expression of DIHYDROFLAVONOL REDUCTASE(DFR),anessential component in the anthocyanin biosynthesis pathway,was completely eliminated in the coil mutant.Jasmonate-induced anthocyanin accumulation was found to be independent of auxin signaling.The present results indicate that theexpression of both COI1 and DFR genes is required for the regulation of JA-induced anthocyanin accumulation and thatDFR may be a key downstream regulator for this process.     

The COI1 and DFR Genes are Essential for Regulation of Jasmonate-Induced Anthocyanin Accumulation in Arabidopsis

Jasmonates （JAs） are a class of plant hormones that play important roles in the regulation of plant development and plant defense. It has been shown that Arabidopsis plants produce much higher levels of anthocyanins when treated exogenously with methyl jasmonate （MeJA）. However, a molecular link between the JA response and anthocyanin production has not been determined. The CORONATINE INSENTITIVE1 （COI1） gene is a key player in the regulation of many JA-related responses. In the present study, we demonstrate that the COI1 gene is also required for the JA-induced accumulation of anthocyanins in Arabidopsis. Furthermore, the MeJA-inducible expression of DIHYDROFLAVONOL REDUCTASE （DFR）, an essential component in the anthocyanin biosynthesis pathway, was completely eliminated in the coil mutant. Jasmonateinduced anthocyanin accumulation was found to be independent of auxin signaling. The present results indicate that the expression of both COI1 and DFR genes is required for the regulation of JA-induced anthocyanin accumulation and that DFR may be a key downstream regulator for this process.     

Analysis of flavanone 3-hydroxylase in Arabidopsis seedlings. Coordinate regulation with chalcone synthase and chalcone isomerase.

A genomic clone encoding flavanone 3-hydroxylase (F3H) was isolated from Arabidopsis thaliana. The deduced amino acid sequence is 72 to 94% identical to all previously reported F3H proteins. Low-stringency DNA blot analysis indicated that F3H is encoded by a single gene in Arabidopsis. The F3H locus was mapped to the bottom of chromosome 3 and therefore does not correspond to any of the 13 flavonoid-deficient transparent testa mutants for which a map position is known. Analysis of gene expression in etiolated seedlings exposed to white light and in two putative regulatory mutants, ttg and tt8, demonstrated that the Arabidopsis F3H gene is coordinately expressed with chalcone synthase and chalcone isomerases is seedlings, whereas dihydroflavonol reductase expression is controlled by distinct regulatory mechanisms. The F3H gene may represent a pivotal point in the regulation of flavonoid biosynthesis because its expression is coordinated with different subsets of genes in different plant species.