乌拉尔图小麦(Triticum urartu)1Ay高分子量麦谷蛋白亚基基因编码区的克隆与鉴定

应用简并性引物和基因组PCR反应从乌拉尔图小麦(Triticum urartu)不同种质材料中获得并测定了表达型和沉默型1Ay高分子量麦谷蛋白亚基基因全长编码区的基因组DNA序列.表达型1Ay基因编码区的序列与前人已发表的y型高分子量麦谷蛋白亚基基因编码区的序列高度同源,由其推导的1Ay亚基的一级结构与已知的高分子量麦谷蛋白亚基相似.在细菌细胞中,表达型1Ay基因编码区的克隆序列可经诱导而产生1Ay蛋白,该蛋白与种子中1Ay亚基在电泳迁移率和抗原性上类似,表明所克隆的序列真实地代表了表达型1Ay基因的全长编码区.但是,本研究所克隆的沉默型1Av基因的编码区序列因含有3个提前终止子而不能翻译成完整的1Ay蛋白.讨论了表达型1Ay基因在小麦籽粒加工品质改良中的潜在利用价值以及lAy基因沉默的机制.     

乌拉尔图小麦（Triticumurartu）lAy高分子量麦谷蛋白亚基基因编码区的克隆与鉴定

应用简并性引物和基因组PCR反应从乌拉尔图小麦(Triticumurartu)不同种质材料中获得并测定了表达型和沉默型lAy高分子量麦谷蛋白亚基基因全长编码区的基因组DNA序列。表达型lAy基因编码区的序列与前人已发表的y型高分子量麦谷蛋白亚基基因编码区的序列高度同源,由其推导的lAy亚基的一级结构与已知的高分子量麦谷蛋白亚基相似。在细菌细胞中,表达型lAy基因编码区的克隆序列可经诱导而产生lAy蛋白,该蛋白与种子中lAy亚基在电泳迁移率和抗原性上类似,表明所克隆的序列真实地代表了表达型lAy基因的全长编码区。但是,本研究所克隆的沉默型lAy基因的编码区序列因含有3个提前终止子而不能翻译成完整的lAy蛋白。讨论了表达型lAy基因在小麦籽粒加工品质改良中的潜在利用价值以及lAy基因沉默的机制。     

高冰草中高分子量麦谷蛋白亚基的编码基因

通过SDS-PAGE法分析了高冰草(Agropyron elongatum (Host) Nevski)种子麦谷蛋白亚基,发现高冰草的麦谷蛋白亚基种类比普通小麦更加丰富。通过基因组PCR法用高分子量麦谷蛋白亚基基因的特异引物从高冰草核基因组中分离出了7条麦谷蛋白亚基的全编码序列,分别命名为AgeloG1~AgeloG7。其中的5条已进行全序列测定,对AgeloG1和AgeloG4进行了末端测序。尽管其中的4条基因的编码序列(AgeloG4, AgeloG5, AgeloG6和AgeloG7)小于1.8 kb,但是对从克隆到的序列推导出的氨基酸序列与已经发表的小麦高分子量麦谷蛋白亚基序列进行对比分析发现,这些亚基与来自小麦的高分子量麦谷蛋白亚基具有很高的同源性。并且对信号肽、N-、C-末端的氨基酸序列分析显示,这7条序列编码的亚基皆为y-型亚基。用5条全部测序的编码序列与普通小麦的A、B、D、粗山羊草的D、圆柱山羊草的C、伞穗山羊草的U、黑麦的R染色体的编码高分子量麦谷蛋白的序列进行了聚类分析。表明,AgeloG2与小麦1Dy, AgeloG3与小麦1By, AgeloG5、AgeloG6和AgeloG7与小麦1Ay在起源和进化上有较高的相似性。     

高冰草中高分子量麦谷蛋白亚基的编码基因

通过SDS-PAGE法分析了高冰草(Agropyron elongatum(Host)Nevski)种子麦谷蛋白亚基,发现高冰草的麦谷蛋白亚基种类比普通小麦更加丰富.通过基因组PCR法用高分子量麦谷蛋白亚基基因的特异引物从高冰草核基因组中分离出了7条麦谷蛋白亚基的全编码序列,分别命名为AgeloGl～AgeloG7.其中的5条已进行全序列测定,对AgeloGl和AgeloG4进行了末端测序.尽管其中的4条基因的编码序列(AgeloG4,AgeloG5,AgeloG6和AgeloG7)小于1.8kb,但是对从克隆到的序列推导出的氨基酸序列与已经发表的小麦高分子量麦谷蛋白亚基序列进行对比分析发现,这些亚基与来自小麦的高分子量麦谷蛋白亚基具有很高的同源性.并且对信号肽、N-、C-末端的氨基酸序列分析显示,这7条序列编码的亚基皆为y-型亚基.用5条全部测序的编码序列与普通小麦的A、B、D、粗山羊草的D、圆柱山羊草的C、伞穗山羊草的U、黑麦的R染色体的编码高分子量麦谷蛋白的序列进行了聚类分析.表明,AgeloG2与小麦lDy,AgeloG3与小麦1By,AgeloG5、AgeloG6和AgeloG7与小麦1Ay在起源和进化上有较高的相似性.     

小伞山羊草高分子量麦谷蛋白亚基及其基因的鉴定

运用SDS_PAGE和分子克隆技术 ,对小伞山羊草 (Aegilopsumbellulata ,UU ,2n =2x =14)的高分子量麦谷蛋白亚基 (1Ux ,1Uy)及其编码基因进行了鉴定。SDS_PAGE分析表明小伞山羊草不同基因型中的 1Ux的电泳迁移率接近或慢于普通小麦 1Dx2 .2亚基的电泳迁移率 ,1Uy亚基的电泳迁移率一般接近或慢于普通小麦的 1Dy类亚基。采用PCR扩增技术获得了 1Ux和 1Uy亚基编码基因的全长编码区 ,并对一个 1Uy基因的全长编码区进行了全序列测定。对推导的氨基酸序列进行比较发现 1Ux和 1Uy亚基具有与来自于其他物种的高分子量麦谷蛋白亚基一致的一级结构 ,聚类分析显示 1Ux和 1Uy亚基与D基因组编码的高分子量麦谷蛋白亚基在起源和进化上具有较高的相似性。     

小偃麦异附加系TAI-13中来自中间偃麦草的低分子量麦谷蛋白亚基基因的分子克隆

通过分析小麦(Triticum aestivum L.)-中间偃麦草(Agropyron intermedium(Host)Beav)异附加系TA1-Ⅰ系列的麦谷蛋白SDS-PAGE电泳图谱和基因组DNA的PCR扩增产物,发现在异附加系TAI-13中附加的中间偃麦草染色体上具有编码高分子量和低分子量麦谷蛋白亚基基因的位点,属于第一同源群.随后,采用RT-PCR方法,从TAI-13的未成熟子粒中克隆了4个来自中间偃麦草的低分子量麦谷蛋白亚基基因.序列分析表明,13003、13006和13054是包括信号肽编码序列的全长基因,而13514没有信号肽编码序列.根据由核苷酸序列推导的蛋白质分子的N-末端氨基酸序列,这4个基因编码的麦谷蛋白亚基可分为3种类型,即Ai-M型(由基因13514编码,命名为LAi1)、Ai-Q型(由基因13006和13045编码,分别命名为LAi2和LAi3)和Ai-Ⅰ型(由基因13003编码,命名为LAi4).通过与小麦的低分子量麦谷蛋白亚基分子比较,发现Ai-M和Ai-Q是两种未见报道的新的低分子量麦谷蛋白亚基类型,而Ai-Ⅰ型与小麦的Ⅰ型亚基相似.氨基酸序列分析发现,基因13514编码的蛋白质亚基分子LAi1有较长的重复区(26个重复模块)和较多的半胱氨酸残基(9个),推测其可形成3个分子间二硫键,可能对增强面团的强度和粘弹性有正面效应.     

小偃麦异附加系TAI-13中来自中间偃麦草的低分子量麦谷蛋白亚基基因的分子克隆

通过分析小麦(TriticumaestivumL.)-中间偃麦草(Agropyronintermedium(Host)Beav)异附加系TAI-Ⅰ系列的麦谷蛋白SDS-PAGE电泳图谱和基因组DNA的PCR扩增产物,发现在异附加系TAI-13中附加的中间偃麦草染色体上具有编码高分子量和低分子量麦谷蛋白亚基基因的位点,属于第一同源群。随后,采用RT-PCR方法,从TAI-13的未成熟子粒中克隆了4个来自中间偃麦草的低分子量麦谷蛋白亚基基因。序列分析表明,13003、13006和13054是包括信号肽编码序列的全长基因,而13514没有信号肽编码序列。根据由核苷酸序列推导的蛋白质分子的N-末端氨基酸序列,这4个基因编码的麦谷蛋白亚基可分为3种类型,即Ai-M型(由基因13514编码,命名为LAi1)、Ai-Q型(由基因13006和13045编码,分别命名为LAi2和LAi3)和Ai-I型(由基因13003编码,命名为LAi4)。通过与小麦的低分子量麦谷蛋白亚基分子比较,发现Ai-M和Ai-Q是两种未见报道的新的低分子量麦谷蛋白亚基类型,而Ai-I型与小麦的I型亚基相似。氨基酸序列分析发现,基因13514编码的蛋白质亚基分子LAi1有较长的重复区(26个重复模块)和较多的半胱氨酸残基(9个),推测其可形成3个分子间二硫键,可能对增强面团的强度和粘弹性有正面效应。     

小伞山羊草高分子量麦谷蛋白亚基及其基因的鉴定

运用SDS-PAGE和分子克隆技术,对小伞山羊草(Aegilops umbellulata,UU, 2n = 2x = 14)的高分子量麦谷蛋白亚基(1Ux, 1Uy)及其编码基因进行了鉴定.SDS-PAGE分析表明小伞山羊草不同基因型中的1Ux的电泳迁移率接近或慢于普通小麦1Dx2.2亚基的电泳迁移率,1Uy亚基的电泳迁移率一般接近或慢于普通小麦的1Dy类亚基.采用PCR扩增技术获得了1Ux和1Uy亚基编码基因的全长编码区,并对一个1Uy基因的全长编码区进行了全序列测定.对推导的氨基酸序列进行比较发现1Ux和1Uy亚基具有与来自于其他物种的高分子量麦谷蛋白亚基一致的一级结构,聚类分析显示1Ux和1Uy亚基与D基因组编码的高分子量麦谷蛋白亚基在起源和进化上具有较高的相似性.     

高冰草中一种新型高分子量麦谷蛋白亚基编码序列的研究

高冰草(Agropyron elongatun)是普通小麦(Triticum aestivum)的近缘禾草,SDS-PAGE显示其所编码的麦谷蛋白亚基的类型较普通小麦更加丰富,是普通小麦品质改良的重要亲本之一。利用基因组PCR的方法从高冰草中克隆到一个新的高分子量麦谷蛋白亚基(HMW-GS)基因(AgeloG2)全编码序列,同源性分析表明：与普通小麦的1Dy12基因比较在少数位点发生了碱基替换和一处6碱基序列的缺失,同源性为99％;与普通小麦的1Dy10基因比较,该基因亦只有少数碱基的替换和两处18碱基序列的增加及一处6碱基序列的缺失,同源性为98％。从推导的编码序列分析,AgeloG2编码y型HMW—GS。综上分析,AgeloG2是一个新的高分子量麦谷蛋白y-型亚基基因。聚类分析结果显示,无论在基因序列还是推导的氨基酸序列上,小麦1Dy亚基与AgeloG2的同源性都高于与粗山羊来源的y型亚基的同源性。     

小麦HMW-GS 12基因克隆及植物表达载体构建

目的:为了利用基因遗传转化改良小麦品质,采用聚合酶链式反应(PCR)技术。方法:从小麦品种东农7742基因组DNA中扩增并克隆了小麦高分子量谷蛋白12亚基基因(HMW-GS 12)。结果:序列分析结果表明,该基因全长1 980bp,其核苷酸顺序和推导的氨基酸顺序与已发表的序列相比,同源性分别为99.5%和99.7%。经过基因拼接,分别构建了胚乳特异性表达和组成型表达的高分子量谷蛋白12亚基基因的两个植物表达载体pDNPPBIHG和pUbPBIHG。     

Molecular cloning and comparative analysis of a y-type inactive HMW glutenin subunit gene from cultivated emmer wheat (Triticum dicoccum L.)

Cultivated emmer (Triticum dicoccum, 2n = 4x = 28, AABB) is closely related to bread wheat and possesses extensive allelic variations in high molecular weight glutenin subunit (HMW-GS) composition. These alleles may be an important genetic resource for wheat quality improvement. To isolate and clone HMW-GS genes from cultivated emmer, two pairs of allele-specific (AS) PCR primers were designed to amplify the coding sequence of y-type HMW-GS genes and their upstream sequences, respectively. The results showed that single bands of strong amplification were obtained through AS-PCR of genomic DNA from emmer. After cloning and sequencing the complete sequence of coding and 5'-flanking regions of a y-type subunit gene at Glu-A1 locus was obtained. Nucleotide and deduced amino acid sequences analysis showed that this gene possessed a similar structure as the previously reported Ay gene from common wheat, and is hence designated as Ay1d. The distinct feature of the Ay1d gene is that its coding region contains four stop codons and its upstream region has a 85-bp deletion in the same position of the Ay gene, which are probably responsible for the silencing of y-type subunit genes at Glu-A1 locus. Phylogenetic analysis of HMW glutenin subunit genes from different Triticum species and genomes were also carried out.     

Characterization of HMW prolamines and their coding sequences from Crithopsis delileana

The high-molecular-weight (HMW) prolamines subunits and their coding sequences from wheat-related diploid species Crithopsis delileana were investigated. Only one HMW prolamine subunit with the similar electrophoresis mobility to the y-type HMW glutenin subunit of hexaploid wheat was observed in two accessions of C. delileana by SDS-PAGE analyses of the total storage protein fractions. It was confirmed by sequencing and expression analysis that this prolamine subunit was an x-type subunit. The amino acid sequence of this subunit had the similar typical structure to those of x-type HMW glutenin genes previously described in wheat. An in-frame stop codon was found in the coding sequences of y-type prolamine subunits. It was found by specifically extraction of HMW prolamines and sequence analysis that the coding regions of Ky prolamine subunit gene is very likely to be not expressed as a full-length protein. Phylogenetic analysis indicated that the Kx subunit could be clustered together with 1Ax1 subunit by an interior paralleled branch, and Ky subunit (inactive) was most closely related to the 1Ay subunit. The coding sequences of Kx subunit could successfully be expressed in bacterial expression system, and the expressed protein had the same electrophoresis mobility as the Kx subunit from the seed of C. delileana. It was the first time that the HMW prolamines subunits encoded by K genome of C. delileana were characterized.     

Isolation and characterization of five novel high molecular weight subunit of glutenin genes from Triticum timopheevi and Aegilops cylindrica

Analysis by SDS-PAGE of total protein fractions from single seeds of Aegilops cylindrica (genomes C and D) and Triticum timopheevi (genomes A and G) showed the presence of three bands corresponding to high molecular weight subunits of glutenin (HMW subunits) in the former and two major bands and a minor band corresponding to HMW subunits in the latter. Three Ae. cylindrica and two T. timopheevi HMW subunit gene sequences, each comprising the entire coding region, were amplified by polymerase chain reaction (PCR) and their complete nucleotide sequences determined. A combination of N-terminal amino acid sequencing of the proteins identified by SDS-PAGE and alignments of the derived amino acid sequences of the proteins encoded by the PCR products identified the Ae. cylindrica HMW subunits as 1Cx, 1Cy and 1Dy, and the T. timopheevi HMW subunits as 1Gx, 1Ax and 1Ay. It was not clear whether or not a 1Gy HMW subunit was present in T. timopheevi. The PCR products from Ae. cyclindrica were derived from 1Cy and 1Dy genes and a silent 1Dx gene containing an in-frame internal stop codon, while those from T. timopheevi were derived from 1Ax and 1Ay genes. The 1Cx, 1Gx and 1Gy sequences were not amplified successfully. The proteins encoded by the five novel genes had similar structures to previously characterized HMW subunits of bread wheat (Triticum aestivum). Differences and similarities in sequence and structure, and in the distribution of cysteine residues (relevant to the ability of HMW subunits to form high M_r polymers) distinguished the HMW subunits of x- and y-type and of each genome rather than those of the different species. There was no evidence of a change in HMW subunit expression or structure resulting from selective breeding of bread wheat. The novel 1Ax, 1Ay, 1Cy and 1Dy HMW subunits were expressed in Escherichia coli, and the expressed proteins were shown to have very similar mobilities to the endogenous HMW subunits on SDS-PAGE. The truncated 1Dx gene from Ae. cylindrica failed to express in E. coli, and no HMW subunit-related protein of the size predicted for the truncated 1Dx subunit could be identified by immunodetection in seed extracts.     

Characterization of the HMW glutenin subunits from Aegilops searsii and identification of a novel variant HMW glutenin subunit

High molecular weight (HMW) glutenin subunits are conserved seed storage proteins in wheat and related species. Here we describe a more detailed characterization of the HMW glutenin subunits from Aegilops searsii, which is diploid and contains the S^s genome related to the S genome of Aegilops speltoides and the A, B and D genomes of hexaploid wheat. SDS-PAGE experiments revealed two subunits (one x and one y) for each of the nine Ae. searsii accessions analyzed, indicating that the HMW glutenin subunit gene locus of Ae. searsii is similar to the Glu-1 locus found in wheat in containing both x and y genes. The primary structure of the four molecularly cloned subunits (from two Ae. searsii accessions) was highly similar to that of the previously reported x and y subunits. However, in one accession (IG49077), the last 159 residues of the x subunit (1S^sx49077), which contained the sequence element GHCPTSPQQ, were identical to those of the y subunit (1S^sy49077) from the same accession. Consequently, 1S^sx49077 contains an extra cysteine residue located at the C-terminal part of its repetitive domain, which is novel compared to the x-type subunits reported so far. Based on this and previous studies, the structure and expression of the Glu-1 locus in Ae. searsii is discussed. A hypothesis on the genetic mechanism generating the coding sequence for the novel 1S^sx49077 subunit is presented.     

High-Molecular-Weight Glutenin Subunit Genesin in Decaploid Agropyron elongatum

Seven genes encoding glutenin subunits that present in Agropyron elongatum (Host) Nevski were cloned by PCR analysis and named AgeloG1 to AgeloG7. The complete open reading frames (ORFs) of the seven genes were amplified with primers special for high-molecular-weight (HMW) glutenin subunit genes and subsequently cloned and sequenced. Five of them were completely sequenced, and the other two (AgeloG1 and AgeloG4) were sequenced at the two ends only. Comparison of amino acid sequences suggested that the primary structure of the subunits encoded by the seven genes was very similar to that of y-type HMW glutenin subunits published from wheat, though four of them (AgeloG4, AgeloG5, AgeloG6 and AgeloG7) were shorter than 1.8 kb. Phylogenetic analysis of the five completely sequenced genes and those subunit genes of Triticum aestivum L. (AABBDD), Aegilops tauschii Coss. (DD), Aegilops caudata L. (CC), Secale cereale L. (RR) and Aegilops umbellulata Zhuk. (UU) indicated that the AgeloG2 was most closely related to 1Dy; the AgeloG3 was to 1By; the AgeloG5, AgeloG6 and AgeloG7 were to 1Ay.     

类大麦属高分子量谷蛋白基因Kx的序列测定及表达

利用SDS-PAGE检测了2份类大麦属(Crithopsis delileana)材料的高分子量谷蛋白亚基组成,并对其中1份材料的x型亚基进行了克隆和测序。结果表明,2份材料具有完全相同的蛋白电泳图谱。在小麦的高分子量区域仅检测到一条蛋白质带,与小麦y型亚基的迁移率接近,但克隆测序表明其为x型高分子量谷蛋白亚基,其编码基因命名为Kx。Kx基因编码区序列长度为2052bp．编码长度为661个氨基酸残基的蛋白质,其序列具有典型的x型高分子量谷蛋白亚基的特征。Kx基因能在原核表达系统内正确表达,其表达蛋白与来源于种子中的Kx亚基的迁移率完全一致。Kx亚基与小麦属A、B和D,山羊草属C和U以及黑麦属R染色体组编码的高分子量谷蛋白亚基氨基酸序列非常相似,但在N和C保守区的氨基酸组成以及重复区长度上与它们存在明显差异。聚类分析可将Kx与Ax1聚类为平行的分支。由此可见,来源于C．delileana的Kx基因为一新的x型高分子量谷蛋白亚基基因。     

Characterization of two HMW glutenin subunit genes from Taenitherum Nevski

The compositions of high molecular weight (HMW) glutenin subunits from three species of Taenitherum Nevski (TaTa, 2n = 2x = 14), Ta. caput-medusae, Ta. crinitum and Ta. asperum, were investigated by SDS-PAGE analysis. The electrophoresis mobility of the x-type HMW glutenin subunits were slower or equal to that of wheat HMW glutenin subunit Dx2, and the electrophoresis mobility of the y-type subunits were faster than that of wheat HMW glutenin subunit Dy12. Two HMW glutenin genes, designated as Tax and Tay, were isolated from Ta. crinitum, and their complete nucleotide coding sequences were determined. Sequencing and multiple sequences alignment suggested that the HMW glutenin subunits derived from Ta. crinitum had the similar structures to the HMW glutenin subunits from wheat and related species with a signal peptide, and N- and C-conservative domains flanking by a repetitive domain consisted of the repeated short peptide motifs. However, the encoding sequences of Tax and Tay had some novel modification compared with the HMW glutenin genes reported so far: (1) A short peptide with the consensus sequences of KGGSFYP, which was observed in the N-terminal of all known HMW glutenin genes, was absent in Tax; (2) There is a specified short peptide tandem of tripeptide, hexapeptide and nonapeptide and three tandem of tripeptide in the repetitive domain of Tax; (3) The amino acid residues number is 105 (an extra Q presented) but not 104 in the N-terminal of Tay, which was similar to most of y-type HMW glutenin genes from Elytrigia elongata and Crithopsis delileana. Phylogenetic analysis indicated that Tax subunit was mostly related to Ax1, Cx, Ux and Dx5, and Tay was more related to Ay, Cy and Ry.