日本通草蛉cDNA文库构建及部分ESTs分析

本研究以日本通草蛉Chrysoperla nipponensis (Okamoto)为材料,采用Oligo(dT)引物定向克隆构建cDNA文库并进行EST序列测定,旨在以基因库的形式进行种质资源的保存,为其遗传改良奠定基础,并为探讨其分类地位提供分子依据。对该文库质量分析表明：库容量为1.0×10⁶,重组率为80.0％,平均插入片段为512 bp。测序后最终成功得到323条表达序列标签（expressed sequence tags,ESTs）序列,经Phrap程序聚类拼接后得到236条单基因簇（unigene）,包括86个重叠群（congtigs）和150个单拷贝（singlets）。使用NCBI中的BlastN和BlastX程序对236条ESTs进行本地化搜索,BlastN的结果表明：180条ESTs（76.3%）没有注解,56条ESTs（23.7%）与GenBank上公布的序列有较高的同源性,其中一条序列被确定为该种的16S rRNA基因,利用MEGA软件构建了基于该16S rRNA序列草蛉科的系统发育树,结果显示通草蛉属Chrysoperla与叉草蛉属Dichochrysa、玛草蛉属Mallada、草蛉属Chrysopa的亲缘关系比较近,这与传统分类相吻合。BlastX的比对结果为197条ESTs（83.5%）有功能注解,39条ESTs（16.5%）无注解或score值小于100。使用GO(gene ontology)数据库对236条ESTs序列进行功能注释,结果表明：142条ESTs（59.7％）有注解,并表达出40多种基因产物。     

T-DNA标签在转基因水稻基因组中的整合特点

利用热不对称交错PCR (TAIL-PCR),对200个含T-DNA插入的转基因水稻株系进行分析,获得了159个T-DNA右边界侧翼序列. 其中,92个序列含有T-DNA右边界和侧邻的水稻基因组序列,78个序列与已公布的水稻BAC/PAC克隆有97%～100%的同源性,从而可作为T-DNA标签定位在水稻的12条染色体上. 结合先前定位的169个T-DNA标签,对T-DNA在水稻基因组中的整合特点进行了分析. 结果发现,在T-DNA右边界和侧邻的水稻基因组序列的连接处,14.6%的T-DNA标签含有3～74bp的填充序列. 在不含填充序列的连接处,21.3%的T-DNA标签,在整合后的T-DNA右边界与侧翼的水稻基因组序列之间显示出3～5 bp的微同源性. 填充序列和微同源性的存在,揭示了T-DNA在水稻基因组中的整合既存在双链断裂修补机制,又存在单链裂缝修补机制. T-DNA倾向于整合到富含A/T核苷酸的基因组区域,即主要在基因的5′和3′端调控区以及内含子中.     

毛竹基因组大小和序列构成的比较分析

毛竹(P. pubescens)是世界重要的竹类植物之一, 是中国分布范围最广、种植面积最大(占全国竹林总面积的2/3以上)、经济价值最高的竹种. 毛竹属于禾本科, 为四倍体(4x = 48), 是该科中特殊的草本植物. 禾本科中多个基因组已被或正在被测序, 但竹类植物基因组研究还未见报 道. 本研究以被测序的玉米(B73)和水稻(日本晴) 基因组作为内参, 利用流式细胞仪(FCM)获得大小约为2034 Mb毛竹基因组, 其与玉米基因组大小相仿, 远大于水稻基因组. 为了明确毛竹基因组是否与玉米基因组一样由大量重复序列组成, 进行了毛竹基因组随机测序, 获得近1000条基因组调查序列(GSS). 序列分析表明, 毛竹基因组的重复序列组成比例23.3%, 明显低于玉米(65.7%); 其重复序列主要由Ty1/Copia和Gypsy/DIRS1 2类LTR逆转座子(14.7%)构成, DNA转座子和其他重复序列比例均较低. 但由于测序数量等原因,该结果还有待今后更大规模的基因组测序分析. 本研究对毛竹和其他竹种的基因组学研究提供了一些有价值的基础数据, 同时该研究是第一次对竹类植物基因组的序列构成进行了初步描述.     

水稻Xa21基因在水稻和玉米中的比较物理定位

比较基因组分析证明,禾本科不同种基因组间存在广泛的同线性和共线性。对水稻（ＯｒｙｚａｓａｔｉｖａＬ．）这一模式植物与其它禾本科植物基因的原位杂交比较定位可以揭示禾本科植物基因组结构的共同特点和进化规律。利用含Ｘａ２１基因的ｐＢ８２２作探针筛选水稻的细菌人工染色体（ＢＡＣ）文库,建立了一个包含３个ＢＡＣ克隆的重叠群。用生物素标记其中一个ＢＡＣ克隆,对水稻“广陆矮４号”和玉米自交系黄早四进行了染色体荧光原位杂交。同时,用ｐＢ８２２也作了原位杂交检测。在水稻第１１染色体长臂中间检出了杂交信号,信号与着丝粒的百分距离约为２４。在玉米的第１、３和第８染色体长臂观察到杂交信号,表明玉米基因组中具有三个Ｘａ２１的同源序列座位。ＢＡＣＦＩＳＨ的信号检出率达在４０％以上,大大高于质粒探针ｐＢ８２２的检出率（１５％）,而且可在同源染色体和姊妹染色单体上同时检出杂交信号的比例较高,证明了利用ＢＡＣ克隆荧光原位杂交进行比较物理定位的可行性和优越性。在ＢＡＣＦＩＳＨ中必须用相应基因组的ＣｏｔⅠＤＮＡ封阻,以排除重复序列的干扰。     

黄瓜抗黑星病相关基因的差异表达分析

以抗黑星病黄瓜材料HX1为试材,接种黑星病菌（Cladosporium cucumerinum）2h、8h、20h、32h和72h的叶片作为试验方（Tester）,相应的未接种叶片作为对照方（Driver）,利用SSH技术,构建了黑星病菌侵染初期的正向和反向cDNA-SSH文库。用巢式引物PCR检测插入片段,获得了200个阳性克隆,通过测序,除去重复序列,共得到105个Unique ESTs。与非冗余蛋白数据库进行BLASTx比对,结果显示,17条ESTs未找到同源序列,88条非重复序列和已知基因的同源性较高,占全部ESTs序列的83.8%,其中86条ESTs与非冗余蛋白数据库已知功能的蛋白具有高度的相似性。结合高密度点阵膜杂交差异筛选,阳性率为75.0%。经初步分析这些序列的功能,差异表达的ESTs功能涉及能量和基础代谢、信号转导、蛋白和核酸代谢、光合作用及逆境中特异表达的基因等方面。为研究黄瓜抗黑星病基因提供了依据。     

成都平原水稻-油菜轮作系统氧化亚氮排放

2005年6月—2006年6月利用静态箱/气相色谱法对成都平原水稻 油菜轮作系统氧化亚氮（N₂O）排放进行定位观测, 研究了该系统N₂O排放特征及土壤水热状况、氮肥施用、作物参与对N₂O排放的影响. 结果表明: 成都平原水稻-油菜轮作系统N₂O排放总量为（8.3±2.8）kg·hm^-2·a^-1, 水稻季、油菜季和休闲期对整个轮作周期N₂O排放总量的贡献分别为30%、65%和5%. 水稻季N₂O平均排放速率表现为排灌交替期最大, 持续淹水期和排水晒田期相当;氮肥施用是N₂O排放高峰出现的主要驱动力;土壤表层含水量偏低是旱季出现土壤N₂O吸收现象的主要原因. 土壤水分、土壤温度、施用氮肥和作物参与均在不同程度上影响N₂O排放, 土壤水分是影响N₂O排放的关键因子, 避免水稻季土壤频繁干湿交替或控制旱季土壤水分(表层土壤含水孔隙率介于50%～70%)可有效抑制N₂O排放.     

石刁柏雄性偏向核质体DNA的克隆与分析

该研究以雌雄异株植物石刁柏为材料,利用基因组消减杂交技术对石刁柏雌雄核基因组中的性别差异核质体DNA（nuclear plastid DNA,NUPTs）进行了分离和分析。结果表明：（1）通过构建消减杂交文库共获得了52个雄性偏向序列,序列长度分布在63~297 bp之间,其中有19个差异序列属于叶绿体来源序列（命名为Ao1~Ao19）,且这些序列与石刁柏叶绿体基因组的相似性均大于84%,Ao19与石刁柏叶绿体基因组相似性为100%。（2）利用基因组半定量PCR对19个NUPTs序列的性别差异分析表明,有4条序列为稳定的雄性偏向NUPTs序列,分别为Ao1、Ao3、Ao10和Ao18。（3）序列比对表明,转移到核基因组的NUPTs主要来源于叶绿体基因组的反向重复区（包含IRa和IRb区）,说明石刁柏叶绿体基因组重复区序列更容易向核基因组进行转移形成雄性偏向的NUPTs序列。     

西方蜜蜂表皮蛋白基因apd-like转录起始位点的定位及cDNA序列的分析

Apidermin蛋白家族是根据蜜蜂表皮蛋白apidermin 1-3（APD 1-3）而命名的一个新型的昆虫结构性表皮蛋白家族。为了鉴定西方蜜蜂Apis mellifera基因组序列上毗邻基因簇apd 1-3的一个预测基因座LOC727145是否为一个新的apd基因,本研究在用5′LongSAGE标签定位该基因的转录起始位点（TSS）的基础上,利用其中的3条5′LongSAGE标签序列作为上游引物,通过RT-PCR方法克隆了该基因的cDNA序列（GenBank登录号： GU358197, GU358199, GU358198）。生物信息学分析发现,基因座LOC727145含有2个外显子和1个“GT-AG”型内含子,其cDNA序列富含GC（70％）,可编码一条长152 aa残基的高度疏水性多肽。此多肽序列的氨基酸组成与蜜蜂APD 1-3表皮蛋白类似, 富含Ala, Gly, Pro, Leu 和Val 5种氨基酸（占77％）, 其中Ala残基含量最高（29％）。该多肽序列与蜜蜂APD-1表皮蛋白序列的相似性为50％, 且其N末端的预测信号肽序列与APD 蛋白的信号肽序列类似。5′LongSAGE标签的基因组定位结果显示,基因座LOC727145在雄蜂头部中表达丰度很高,RNA PolⅡ可从6个不同的TSS上以不同效率起始转录,其中由一个优势TSS上起始了90％的转录。本研究为apidermin表皮蛋白家族增添了一个新成员, 命名为apidermin-like (apd-like)。     

程序性细胞死亡抑制基因Dad-1在水稻和玉米中的FISH定位(英文)

Dad-1是一种在动物和植物中都非常保守的细胞程序性死亡 (PCD) 抑制基因。作者利用 FISH (荧光原位杂交)首次把单拷贝水稻Dad-1基因物理定位在水稻第2号染色体短臂的端部(Fig.2 A,B&C)。我们还分析了它在玉米基因组中的同源序列。Southern 杂交结果显示在玉米基因组中确实存在水稻Dad-1 的同源序列(Fig.1)。FISH进一步展示了三个杂交信号分别在玉米4、5号染色体长臂和9号染色体短臂上(Fig.2 D,E&F),其信号距着丝粒的百分距离(FL值)分别为 91、98和96。其杂交位点的位置与水稻Dad-1所处的相对位置是相似的,它们都处于染色体臂的端部。这表明在一定的程度上,Dad-1基因不仅在序列同源性上而且在所处的染色体位置上具有保守性。 水稻Dad-1基因在水稻中的杂交信号检出率 (38%) 高于玉米中的。这表明与玉米相比,水稻Dad-1 基因的编码序列更容易与水稻染色体杂交;它与玉米中的相应序列可能只是部分同源。     

Genetic mapping of expressed sequences in onion and in silico comparisons with rice show scant colinearity

The Poales (which include the grasses) and Asparagales [which include onion (Allium cepa L.) and other Allium species] are the two most economically important monocot orders. Enormous genomic resources have been developed for the grasses; however, their applicability to other major monocot groups, such as the Asparagales, is unclear. Expressed sequence tags (ESTs) from onion that showed significant similarities (80% similarity over at least 70% of the sequence) to single positions in the rice genome were selected. One hundred new genetic markers developed from these ESTs were added to the intraspecific map derived from the BYG15-23×AC43 segregating family, producing 14 linkage groups encompassing 1,907 cM at LOD 4. Onion linkage groups were assigned to chromosomes using alien addition lines of Allium fistulosum L. carrying single onion chromosomes. Visual comparisons of genetic linkage in onion with physical linkage in rice revealed scant colinearity; however, short regions of colinearity could be identified. Our results demonstrate that the grasses may not be appropriate genomic models for other major monocot groups such as the Asparagales; this will make it necessary to develop genomic resources for these important plants. Electronic Supplementary Material Supplementary material is available for this article at     

白菜EST-SSR标记的通用性

EST-SSR是从表达序列标签(expressedsequencetag,EST)中开发的新型简单序列重复(simplesequencerepeat,SSR)标记。根据白菜EST设计了15对SSR引物,对白菜、油菜、玉米、高粱、水稻和茶树等进行了PCR,研究了白菜的EST-SSR标记在不同物种间的通用性。所设计的引物对不同白菜品种、近缘种油菜和远缘种玉米、高粱、水稻和茶树的扩增成功率分别为100%、93.3%、80%、93.3%、93.3%和86.7%。在15对引物中,有11对在远缘种中都有扩增产物,而且一些引物可显示多态性,多态性引物分别占了可扩增引物的33.3%、28.6%、28.6%和61.5%。这些结果表明,白菜EST-SSR引物具有较高的通用性,这对于比较基因组学研究有重要意义。     

Inferences on the genome structure of progenitor maize through comparative analysis of rice, maize and the domesticated panicoids.

Corn and rice genetic linkage map alignments were extended and refined by the addition of 262 new, reciprocally mapped maize cDNA loci. Twenty chromosomal rearrangements were identified in maize relative to rice and these included telomeric fusions between rice linkage groups, nested insertion of rice linkage groups, intrachromosomal inversions, and a nonreciprocal translocation. Maize genome evolution was inferred relative to other species within the Panicoideae and a progenitor maize genome with eight linkage groups was proposed. Conservation of composite linkage groups indicates that the tetrasomic state arose during maize evolution either from duplication of one progenitor corn genome (autoploidy) or from a cross between species that shared the composite linkages observed in modern maize (alloploidy). New evidence of a quadruplicated homeologous segment on maize chromosomes 2 and 10, and 3 and 4, corresponded to the internally duplicated region on rice chromosomes 11 and 12 and suggested that this duplication in the rice genome predated the divergence of the Panicoideae and Oryzoideae subfamilies. Charting of the macroevolutionary steps leading to the modern maize genome clarifies the interpretation of intercladal comparative maps and facilitates alignments and genomic cross-referencing of genes and phenotypes among grass family members.     

New in silico insight into the synteny between rice (Oryza sativa L.) and maize (Zea mays L.) highlights reshuffling and identifies new duplications in the rice genome

A unigene set of 1411 contigs was constructed from 2629 redundant maize expressed sequence tags (ESTs) mapped on the maizeDB genetic map. Rice orthologous sequences were identified by blast alignment against the rice genomic sequence. A total of 1046 (74%) maize contigs were associated with their corresponding homologues in the rice genome and 656 (47%) defined as potential orthologous relationships. One hundred and seventeen (8%) maize EST contigs mapped to two distinct loci on the maize genetic map, reflecting the tetraploid nature of the maize genome. Among 492 mono-locus contigs, 344 (484 redundant ESTs) identify collinear blocks between maize chromosomes 2 and 4 and a single rice chromosome, defining six new collinear regions. Fine-scale analysis of collinearity between rice chromosomes 1 and 5 with maize chromosomes 3, 6 and 8 shows the presence of internal rearrangements within collinear regions. Mapping of maize contigs to two distinct loci on the rice sequence identifies five new duplication events in rice. Detailed analysis of a duplication between rice chromosomes 1 and 5 shows that 11% of the annotated genes from the chromosome 1 locus are found duplicated on the chromosome 5 paralogous counterpart, indicating a high degree of re-organisations. The implications of these findings for map-based cloning in collinear regions are discussed.     

Exploiting rice–sorghum synteny for targeted development of EST-SSRs to enrich the sorghum genetic linkage map

The sequencing and detailed comparative functional analysis of genomes of a number of select botanical models open new doors into comparative genomics among the angiosperms, with potential benefits for improvement of many orphan crops that feed large populations. In this study, a set of simple sequence repeat (SSR) markers was developed by mining the expressed sequence tag (EST) database of sorghum. Among the SSR-containing sequences, only those sharing considerable homology with rice genomic sequences across the lengths of the 12 rice chromosomes were selected. Thus, 600 SSR-containing sorghum EST sequences (50 homologous sequences on each of the 12 rice chromosomes) were selected, with the intention of providing coverage for corresponding homologous regions of the sorghum genome. Primer pairs were designed and polymorphism detection ability was assessed using parental pairs of two existing sorghum mapping populations. About 28% of these new markers detected polymorphism in this 4-entry panel. A subset of 55 polymorphic EST-derived SSR markers were mapped onto the existing skeleton map of a recombinant inbred population derived from cross N13 × E 36-1, which is segregating for Striga resistance and the stay-green component of terminal drought tolerance. These new EST-derived SSR markers mapped across all 10 sorghum linkage groups, mostly to regions expected based on prior knowledge of rice–sorghum synteny. The ESTs from which these markers were derived were then mapped in silico onto the aligned sorghum genome sequence, and 88% of the best hits corresponded to linkage-based positions. This study demonstrates the utility of comparative genomic information in targeted development of markers to fill gaps in linkage maps of related crop species for which sufficient genomic tools are not available.     

The Ph2 pairing homoeologous locus of wheat (Triticum aestivum): identification of candidate meiotic genes using a comparative genetics approach

Colinearity in gene content and order between rice and closely related grass species has emerged as a powerful tool for gene identification. Using a comparative genetics approach, we have identified the rice genomic region syntenous to the region deleted in the wheat chromosome pairing mutant ph2a, with a view to identifying genes at the Ph2 locus that control meiotic processes. Utilising markers known to reside within the region deleted in ph2a, and data from wheat, barley and rice genetic maps, markers delimiting the region deleted on wheat chromosome 3DS in the ph2a mutant were used to locate the syntenous region on the short arm of rice chromosome 1. A contig of rice genomic sequence was identified from publicly available sequence information and used in blast searches to identify wheat expressed sequence tags (ESTs) exhibiting significant similarity. Southern analysis using a subset of identified wheat ESTs confirmed a syntenous relationship between the rice and wheat genomic regions and defined precisely the extent of the deleted segment in the ph2a mutant. A 6.58-Mb rice contig generated from 60 overlapping rice chromosome 1 P1 artificial chromosome (PAC) clones spanning the syntenous rice region has enabled identification of 218 wheat ESTs putatively located in the region deleted in ph2a. What seems to be a terminal deletion on chromosome 3DS is estimated to be 80 Mb in length. Putative candidate genes that may contribute to the altered meiotic phenotype of ph2a are discussed.     

Targeted molecular mapping of a major wheat QTL for Fusarium head blight resistance using wheat ESTs and synteny with rice.

A major QTL for resistance to Fusarium head blight (FHB) in wheat, Qfhs.ndsu-3BS, has been identified and verified by several research groups. The objective of this study was to increase the marker density in this QTL region using STS (sequence-tagged site) markers developed from wheat expressed sequence tags (ESTs) near Qfhs.ndsu-3BS. Because wheat chromosome 3BS and rice chromosome 1S are syntenous, the sequences of P1-derived artificial chromosome (PAC) and (or) bacterial artificial chromosome (BAC) clones covering the sub-distal portion of rice chromosome 1S were used as queries for a BLASTn search to identify wheat ESTs most likely near Qfhs.ndsu-3BS. Sixty-eight out of 79 STS primer pairs designed from wheat ESTs amplified PCR products from the genomic DNA of Triticum aestivum 'Chinese Spring'. Twenty-eight STS markers were localized on chromosome 3BS by aneuploid analysis. Six out of the nine STS markers that could be mapped in the T. aestivum 'Sumai 3'/T. aestivum 'Stoa' population had higher R2 and LOD values for this QTL than the most significant marker reported previously. Therefore, leveraging genome sequence information available in rice for wheat genetics is an effective strategy to develop DNA markers for Qfhs.ndsu-3BS, and this strategy may have broad applications for targeted mapping of other traits in cereal crops.     

Large-scale identification of expressed sequence tags involved in rice and rice blast fungus interaction

To better understand the molecular basis of the defense response against the rice blast fungus (Magnaporthe grisea), a large-scale expressed sequence tag (EST) sequencing approach was used to identify genes involved in the early infection stages in rice (Oryza sativa). Six cDNA libraries were constructed using infected leaf tissues harvested from 6 conditions: resistant, partially resistant, and susceptible reactions at both 6 and 24 h after inoculation. Two additional libraries were constructed using uninoculated leaves and leaves from the lesion mimic mutant spl11. A total of 68,920 ESTs were generated from 8 libraries. Clustering and assembly analyses resulted in 13,570 unique sequences from 10,934 contigs and 2,636 singletons. Gene function classification showed that 42% of the ESTs were predicted to have putative gene function. Comparison of the pathogen-challenged libraries with the uninoculated control library revealed an increase in the percentage of genes in the functional categories of defense and signal transduction mechanisms and cell cycle control, cell division, and chromosome partitioning. In addition, hierarchical clustering analysis grouped the eight libraries based on their disease reactions. A total of 7,748 new and unique ESTs were identified from our collection compared with the KOME full-length cDNA collection. Interestingly, we found that rice ESTs are more closely related to sorghum (Sorghum bicolor) ESTs than to barley (Hordeum vulgare), wheat (Triticum aestivum), and maize (Zea mays) ESTs. The large cataloged collection of rice ESTs in this study provides a solid foundation for further characterization of the rice defense response and is a useful public genomic resource for rice functional genomics studies.     

Development and mapping of EST-derived simple sequence repeat markers for hexaploid wheat.

Expressed sequence tags (ESTs) are a valuable source of molecular markers. To enhance the resolution of an existing linkage map and to identify putative functional polymorphic gene loci in hexaploid wheat (Triticum aestivum L.), over 260,000 ESTs from 5 different grass species were analyzed and 5418 SSR-containing sequences were identified. Using sequence similarity analysis, 156 cross-species superclusters and 138 singletons were used to develop primer pairs, which were then tested on the genomic DNA of barley (Hordeum vulgare), maize (Zea mays), rice (Oryza sativa), and wheat. Three-hundred sixty-eight primer pairs produced PCR amplicons from at least one species and 227 primer pairs amplified DNA from two or more species. EST-SSR sequences containing dinucleotide motifs were significantly more polymorphic (74%) than those containing trinucleotides (56%), and polymorphism was similar for markers in both coding and 5' untranslated (UTR) regions. Out of 112 EST-SSR markers, 90 identified 149 loci that were integrated into a reference wheat genetic map. These loci were distributed on 19 of the 21 wheat chromosomes and were clustered in the distal chromosomal regions. Multiple-loci were detected by 39% of the primer pairs. Of the 90 mapped ESTs, putative functions for 22 were identified using BLASTX queries. In addition, 80 EST-SSR markers (104 loci) were located to chromosomes using nullisomic-tetrasomic lines. The enhanced map from this study provides a basis for comparative mapping using orthologous and PCR-based markers and for identification of expressed genes possibly affecting important traits in wheat.