中国地方品种香猪的肌肉特异组织表达序列标签(ESTs)的

通过构建香猪肌肉组织cDNA文库,并在文库中随机挑选克隆进行测序的方法,获得了131个香猪肌肉EST序列.在这131个EST序列所代表的109个单一克隆中,有99个为人类及其他物种的同源序列,3个为已知的猪的ESTs,7个为未知ESTs.对这10个已知、未知ESTs进行开放阅读框预测并进行B1ast分析,没有找到高度同源的氨基酸序列.对上述EST所对应的基因功能分析结果表明,除去27.27%的EST未能分类外,克隆到的EST大多来自与基因/蛋白的表达调控相关的基因(占45.46%).来自具有其他功能的基因的EST依次是细胞代谢占10.10%、细胞结构/迁移占10.10%、细胞/机体防御占5.05%和细胞信号/传导占2.02%.没有发现和细胞分裂相关的已知功能基因.本研究结果为中国地方品种香猪提供了第一个骨骼肌的基因表达谱,为今后寻找猪肌肉生长和肉用品质的候选基因奠定了基础.     

处于性腺不同发育阶段斜带石斑鱼垂体的EST表达差异分析

斜带石斑鱼是重要的海产经济鱼类,在其个体发育过程中存在先雌后雄的天然性反转现象。垂体是调节生长和生殖等生理过程的重要内分泌器官。构建了斜带石斑鱼分别处于卵巢发育起始和性反转后期的垂体SMARTcDNA的质粒文库,并通过测序分别筛选到232个和258个表达序列标签(expressed sequence tags,EST)。将所得EST与GenBank数据库中的序列进行比对,结果表明,处于卵巢发育起始和性反转后期斜带石斑鱼垂体EST中,激素所占比例均为最高,分别为40.5%和34.9%。进一步比较分析了这两个性腺发育时期斜带石斑鱼垂体EST中各种激素相对表达丰度,表明生长/催乳激素家族(GH、PRL和SL)和阿黑皮素原(POMC)表达水平下降;促性腺激素α亚基(GTHα)表达水平急剧上升,促滤泡激素β亚基(FSHβ)、促黄体激素β亚基(LHβ)表达水平上升。     

中国地方品种香猪的肌肉特异组织表达序列标签（ESTs）的分析

通过构建香猪肌肉组织cDNA文库,并在文库中随机挑选克隆进行测序的方法,获得了131个香猪肌肉EST序列。在这131个EST序列所代表的109个单一克隆中,有99个为人类及其他物种的同源序列,3个为已知的猪的ESTs,7个为未知ESTs。对这10个已知、未知ESTs进行开放阅读框预测并进行BlastX分析,没有找到高度同源的氨基酸序列。对上述EST所对应的基因功能分析结果表明,除去27．27％的EST未能分类外,克隆到的EST大多来自与基因／蛋白的表达调控相关的基因（占45．46％）。来自具有其他功能的基因的EST依次是细胞代谢占10．10％、细胞结构／迁移占10．10％、细胞／机体防御占5．05％和细胞信号／传导占2．02％。没有发现和细胞分裂相关的已知功能基因。本研究结果为中国地方品种香猪提供了第一个骨骼肌的基因表达谱,为今后寻找猪肌肉生长和肉用品质的候选基因奠定了基础。     

处于性腺不同发育阶段斜带石斑鱼垂体的EST表达差异分析

斜带石斑鱼是重要的海产经济鱼类，在其个体发育过程中存在先雌后雄的天然性反转现象。垂体是调节生长和生殖等生理过程的重要内分泌器官。构建了斜带石斑鱼分别处于卵巢发育起始和性反转后期的垂体SMART cDNA的质粒文库，并通过测序分别筛选到232个和258个表达序列标签(expressed sequence tags, EST)。将所得EST与GenBank数据库中的序列进行比对，结果表明，处于卵巢发育起始和性反转后期斜带石斑鱼垂体EST中，激素所占比例均为最高，分别为40.5%和34.9%。进一步比较分析了这两个性腺发育时期斜带石斑鱼垂体EST中各种激素相对表达丰度，表明生长/催乳激素家族（GH、PRL和SL）和阿黑皮素原（POMC）表达水平下降；促性腺激素α亚基（GTHα）表达水平急剧上升，促滤泡激素β亚基（FSHβ）、促黄体激素β亚基（LHβ）表达水平上升。     

小鼠睾丸特异表达基因TSEG-1的克隆及序列分析

从表达序列标签(expressed sequence tags, ESTs)数据库ZooDDD中获得小鼠正常睾丸表达的EST, 通过dbEST数据库检索出与其高度同源的EST序列, 构建EST叠加群(contigs), Biolign软件拼接, GeneScan软件预测contigs对应的基因组序列中的外显子、内含子; 针对开放阅读框设计引物序列, 采用RT-PCR从小鼠睾丸组织中克隆新基因的cDNA, 分析该基因在小鼠各脏器中的mRNA表达, 并对测序结果进行生物信息学分析。结果表明: 在小鼠X染色体的1 668~2 011 kb间克隆出一新基因TSEG-1, 全长为510 bp, 开放阅读框为336 bp, 编码111氨基酸, 分子量12.84258 kDa, 等电点11.4000。RT-PCR证实该基因开放阅读框正确, 在小鼠睾丸组织中特异性表达, 且与小鼠其他cDNA 无同源性, 获得GenBank 登录号EU079024。功能区分析发现TSEG-1蛋白可能为一种跨膜蛋白, 跨膜区位于第41~61氨基酸残基。TSEG-1基因与人类睾丸特异性组蛋白2a变异体基因有较高同源性, 在TSEG-1基因5′-端非编码侧翼预测发现存在1个启动子区域, 范围为680 bp。 TSEG-1蛋白可能有4个抗原性位点, 2个特异性蛋白激酶的磷酸化位点, 其亚细胞定位可能位于线粒体。小鼠睾丸特异性基因TSEG-1的克隆为进一步研究其生物学功能和表达调控奠定了基础。     

橡胶树甲基化过滤文库的构建

为高通量富集橡胶树基因编码序列,文章首次利用大肠杆菌McrBC限制修饰系统构建了巴西橡胶树基因组甲基化过滤文库.该文库未扩增和扩增后的滴度分别为2.6×106pfu/mL和9×109pfu/mL,阳性克隆率为86.4%,插入片段大小为1～2.5 kb,平均长度为1.2 kb.随机挑选100个克隆进行测序,共拼接出81个非冗余序列,其中包括6个重叠群(Contigs)和75个单一序列(Singlets),冗余度为17.35%.Blast分析发现,39.5%非冗余序列与Nr库中功能基因同源,14.81%与EST数据库中序列同源,32.1%序列为未知序列,且部分序列为开花调控、抗虫和抗病等功能相关的同源基因.橡胶树甲基化文库的建立为橡胶树重要功能基因发现和克隆提供一条重要途径.     

中华鲟促性腺激素释放激素受体基因cDNA序列的克隆及表达分析

为了研究中华鲟(Acipenser sinensis)促性腺激素释放激素受体(Gonadotropin-releasing hormone receptor, GnRH-R)基因在中华鲟中的组织表达特征, 为中华鲟生长发育调控研究提供基础数据, 通过构建中华鲟(Acipenser sinensis)垂体的SMART cDNA质粒文库, 采用cDNA末端快速扩增(RACE), 克隆得到了中华鲟GnRH-R基因的cDNA全长序列。该序列全长1530 bp, 有478 bp的5′非翻译区, 579 bp的开放阅读框和473 bp的3′非翻译区, 共编码192个氨基酸, 其成熟多肽含有5个Ｎ连糖基化位点。通过和已知其他鱼类的GnRH-R基因进行氨基酸序列多重比对, 发现其与真鲷(Pagrus major)的同源性最高, 为76%, 与米氏叶吻银鲛(Callorhinchus milii)的同源性最低, 为39%。采用实时荧光定量PCR (Real time PCR)方法, 检测了GnRH-R的mRNA在中华鲟心、肝、脾、肾、肠道、精巢、肌肉及脑组织中的表达状况, 发现其在精巢中大量转录, 而在其他组织中则表达微弱。以上结果表明中华鲟GnRH-R基因在性腺发育特别是精子发生过程中可能起重要作用。     

桃中两个MADS box基因的克隆与表达分析

为研究李属(Prunus sp．)果树生殖调控的相关基因,对国际公共数据库中的李属植物的EST(expressed sequence tags)序列进行了电子拼接,获得了8个MADS box基因的cDNA序列,并利用PCR技术从桃中克隆出其中的两个cDNA,分别命名为PpMDS4和PpMADS6,在GenBank中的登录号为AY705972和AY705973。PpMADS4基因长850bp,包含一个732bp的开放阅读框,编码243个氨基酸。PpMADS6基因长1190bp,包含1个768bp的开放阅读框,编码256个氨基酸。PpMADS4和PpMADS6在序列上分别与拟南芥中的AGAMOUS基因和矮牵牛中的PFG基因高度同源。RT-PCR分析表明,PpMADS4基因在桃的花瓣、心皮、果实及果仁中表达,应属于控制花器官发育的C类MADS box基因。PpMADS6基因在桃的叶、萼片、花瓣、心皮及果实中表达,应属于调控植物由营养生长向生殖生长过渡的A类MADSbox基因。     

分析EST寻找小鼠胸腺基质细胞表达基因

网上生物信息量的膨胀导致新基因寻找手段的改变,借助mRNA差异显示技术获得的17个表达序列标签（EST）,通过对美国国家生物技术信息中心（NCBI）的非冗余序列库（NT）和小鼠EST库的BLAST同源检索,发现有4个序列与已知基因高度同源,其中的HDPs和Eps8两个基因是首次在小鼠胸腺基质细胞中发现,它们可能与T细胞在胸腺内的发育分化有关,其它EST则为新基因,本结果也为下一步新基因的克隆及功能研究提供了有益的线索。     

Gene Expression Profiling of Coccolith-Bearing Cells and Naked Cells in Haptophyte <Emphasis Type="Italic">Pleurochrysis haptonemofera</Emphasis> with a cDNA Macroarray System

Pleurochrysis haptonemofera is a unicellular marine coccolithophorid that has calcified scales, coccoliths, on the cell surface. Some coccolithophorids including P. haptonemofera have a coccolith-bearing stage and a naked stage in their life cycles. To characterize genes involved in the coccolithogenesis, we generated a total of 9550 expressed sequence tags (EST) from a normalized cDNA library that was prepared using both coccolith-bearing cells (C-cells) and naked cells (N-cells), constructed a cDNA macroarray using the EST clones, and then analyzed the gene expression specificity in C-cells and N-cells. When cDNA clones whose expression ratio exceeded 3-fold were selected, as many as 180 clones were identified as C-cell-specific ones, while only 12 were found to be N-cell-specific ones. These clones were sequenced, assembled, and homology-searched against a public nonredundant protein database. As a result, they were grouped into 54 C-cell-specific and 6 N-cell-specific genes, and 59% and 50% of these genes exhibited significant similarity to those of other known proteins, respectively. To assess mRNA expression further, Northern hybridization was performed for 12 of the C-cell-specific genes and one of the N-cell-specific ones. These clones, together with the new cDNA macroarray, will provide a powerful tool for the future genome-wide functional analysis of uncharacterized genes related to the regulation of the calcification and life cycle of coccolithophorids. Shoko Fujiwara and Yasutaka Hirokawa contributed equally to this work.     

Genes expressed in Blue Fin Tuna (Thunnus thynnus) liver and gonads

Blue Fin Tuna (BFT), Thunnus thynnus, has been seriously endangered by global massive overfishing and by the pollution of marine environment. Feeding and fattening of caught tuna in marine cages is a recent resource, but the development of a self-sustained aquaculture activity, being independent from the supply of wild fish, is required from both industrial and conservation perspectives. At this scope, several technical problems have to be solved and the control of reproduction is the cardinal one. Beside the technological developments of farming facilities and protocols, a molecular approach seems promising for the studies of appropriate nutritional strategies, reproduction physiology and animal welfare, as well as lifestyle and response to endocrine disruptor pollutants. In this context, we have started an EST project on this species sequencing 2743, 2907, and 3014 clones from expression libraries of ovary, testis and liver, respectively, and 1499 clones from an ovary normalized library. Thanks to this project, we have identified several sequences with known function in other organisms, but not previously described in this species. Among the new genes, 712 were found only in the expression library of the ovary, 613 in that of the testis and 318 in that of the liver, while 324 additional genes were shared by two or more expression libraries; other 127 genes not found in the expression libraries were obtained from the ovary normalized library. This represents a contribution to the knowledge of the molecular basis of BFT and a necessary step for facilitating further molecular studies on this species. Accession numbers: EC 091633 to EC 093160; EG 629962 to EG 631176; EC 917676 to EC 919417; EG 999340 to EG 999999; EH 000001 to EH 000505; EH 667253 to EH 668984; EL 610526 to EL 611807; EC 42144 to EC 422414; and EH 379568 to EH 380065.     

中华鲟阿黑皮素原cDNA 序列克隆及其序列分析

通过构建中华鲟(Acipenser sinensis)垂体的SMART cDNA 质粒文库, 首次从文库中筛选得到阿黑皮素原(Proopiomelanocortin, POMC) cDNA 全长序列, 分别为阿黑皮素原A 型基因 (Proopiomelanocortin I,AsPOMC-A, EV824935) 和阿黑皮素原B 型基因(Proopiomelanocortin II, AsPOMC-B, EV825368)。 其中,AsPOMC-A 和AsPOMC-B 分别在文库中出现128 次和19 次。AsPOMC-A 全长1122 bp, 有792 bp 的开放阅读框, 共编码264 个氨基酸。 AsPOMC-B 全长1216 bp, 有792 bp 的开放阅读框, 共编码264 个氨基酸。以其氨基酸序列为分子标记, 比较了3 种鲟鱼的共6 种POMC 的氨基酸同源性, 并利用已报道的鱼类的POMC氨基酸序列构建了系统发育树, 可识别2 个大的单系类群, 即类群I: 非新鳍亚纲类群(仅包含辐鳍亚纲的长吻雀鳝), 类群II: 新鳍亚纲类群。AsPOMC 可能是一种进化上更原始的基因。       

Discovery of 342 putative new genes from the analysis of 5'-end-sequenced full-length-enriched cDNA human transcripts

In this work we describe the process that, starting with the production of human full-length-enriched cDNA libraries using the CAP-Trapper method, led us to the discovery of 342 putative new human genes. Twenty-three thousand full-length-enriched clones, obtained from various cell lines and tissues in different developmental stages, were 5'-end sequenced, allowing the identification of a pool of 5300 unique cDNAs. By comparing these sequences to various human and vertebrate nucleotide databases we found that about 40% of our clones extended previously annotated 5' ends, 662 clones were likely to represent splice variants of known genes, and finally 342 clones remained unknown, with no or poor functional annotation. cDNA-microarray gene expression analysis showed that 260 of 342 unknown clones are expressed in at least one cell line and/or tissue. Further analysis of their sequences and the corresponding genomic locations allowed us to conclude that most of them represent potential novel genes, with only a small fraction having protein-coding potential.     

Generation of 919 expressed sequence tags from immature flower buds and gene expression analysis using expressed sequence tags in the model plant Lotus japonicus

Lotus japonicus has received increased attention as a potential model legume plant. In order to study gene expression in reproductive organs and to identify genes that play a crucial function in sexual reproduction, we constructed a cDNA library from immature flower buds containing anthers at the stage of developing tapetum cells in L. japonicus, and characterized 919 expressed sequence tags (ESTs) randomly selected from a cDNA library of the immature flower buds. The 919 ESTs analyzed were clustered into 821 non-redundant EST groups. As a result of a database search, 436 groups (53%) out of the 821 groups showed sequence similarity to genes registered in the public database. Out of these 436 groups, 109 groups showed similarity to genes encoding hypothetical proteins whose function had not yet been estimated. Three hundred eighty five groups (47%) showed no significant homology to known sequences and were classified as novel sequences. A comparison of 821 non-redundant EST sequences and EST sequences derived from the whole plant L. japonicus revealed that 474 EST sequences derived from immature flower buds were not found in the EST sequences of the whole plant. In order to confirm the expression pattern of potential reproductive-organ specific EST clones, nine clones, which were not matched to ESTs derived from the whole plant, were selected, and RT-PCR analysis was performed on these clones. As a result of RT-PCR, we found two novel anther specific clones. One clone was homologous to a gene encoding human cleft lip and palate associated transmembrane protein (CLPTM1) like protein, and the other clone did not show a significant similarity to any genes deposited in the public database. These results indicate that ESTs analyzed here represent a valuable resource for finding reproductive-organ specific genes in Lotus japonicus.