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.     

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。     

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。     

白粉病菌诱导的小麦表达序列标签(EST)研究(英)

白粉病是我国小麦的主要病害之一。尝试用表达序列标签 (expressedsequencetags,EST)技术 ,研究了经白粉病菌诱导后的小麦基因表达。从构建的普通cDNA文库中随机挑取约 15 0 0个阳性克隆并进行测序 ,获不重复ESTs序列 387条。不重复序列均获GenBank的存储号。其中 4 9.4 %的序列与已知基因同源 ,196条序列功能未知 ,84条序列为新ESTs。将不重复序列制备成高密度点阵膜 ,用差示杂交法筛选到几个抗病相关序列。     

白粉病菌诱导的小麦表达序列标签（EST）研究

白粉病是我国小麦的主要病害之一,尝试用表达序列标签（expressed sequence tage,EST）技术,研究了经白粉病菌诱导后的小麦基因表达。从构建的普通cDNA库中随机挑取约1500个阳性克隆并进行测序,获不重复ESTs序列387条,不重复序列均获GenBank的存储号,其中49.4%的序列与已知基因同源,196条序列功能未知,84条序列为新ESTs。将不重复序列制备成高密度点阵膜,用差示杂交法筛选到几个抗病相关序列。     

白粉病菌诱导的小麦表达序列标签(EST)研究

白粉病是我国小麦的主要病害之一.尝试用表达序列标签(expressed sequence tags, EST)技术,研究了经白粉病菌诱导后的小麦基因表达.从构建的普通cDNA文库中随机挑取约1 500个阳性克隆并进行测序, 获不重复ESTs序列387条.不重复序列均获GenBank的存储号.其中49.4%的序列与已知基因同源,196条序列功能未知, 84条序列为新ESTs.将不重复序列制备成高密度点阵膜,用差示杂交法筛选到几个抗病相关序列.     

基于比较基因组学的玉米ESTs定位方法

描述了以水稻基因组数据和玉米与水稻的比较遗传图谱为桥梁,基于水稻和玉米间存在的标记和序列水平上的广泛的共线性,对大量的玉米ESTs初步定位于玉米连锁群上新方法,为对ESTs开展进一步的基因组学研究和基因克隆提供参考信息。对139条玉米ESTs的定位发现,96条玉米ESTs（69%）可在水稻基因组中找到同源序列,77条ESTs（55%）可使用该策略进行定位,证实了该方法的可行性和有效性。      

小麦抗白粉病侵染初期的表达序列标签分析

以抗白粉病品系“百农 32 17×Mardler”　BC5F4为材料 ,构建了一个白粉病菌接种初期的抑制消减杂交cDNA文库 ,测序获得 76 0条ESTs。与GenBank序列进行BLASTx分析 ,获功能已知ESTs 2 71条。通过分析抗病相关基因 ,推测G蛋白介导的信号传导途径、SA信号传递系统、MAP相关信号传递系统等参与了小麦抗白粉病过程。SAR基因在抗病相关ESTs中的种类与数量最多。数据显示苯丙烷代谢途径、细胞壁结构修饰作用、细胞保卫机制参与了抗病过程。未知功能ESTs与GenBank序列进行BLASTn分析 ,其中许多与病原菌、非病原菌诱导cDNA文库来源的ESTs同源 ;新ESTs占全部ESTs的 16 6 %。     

抗口蹄疫病毒相关基因的筛选及分析

口蹄疫是一种烈性传染病,其广泛流行给社会造成了巨大经济损失。为了研究口蹄疫灭活疫苗免疫的分子机制,同时也为抗口蹄疫病毒药物的研制奠定基础,本研究应用mRNA差异显示技术,以PK-15细胞为材料,系统比较了口蹄疫疫苗刺激组（A组）和正常的PK-15细胞（B组）的基因表达情况,回收差异片段,经二次扩增并纯化后,得到30条ESTs。将30条ESTs采用以地高辛标记的反向Northern点杂交鉴定,将阳性条带克隆测序,筛选出8条ESTs,编号E1~E8,应用BLASTn工具将8条ESTs对核酸数据库nr和dbEST中所有序列进行了同源性分析,其中E1,E2分别与猪的热休克蛋白基因、猪的MHCⅠ类基因同源,序列相似性都达到100%。E3,E4,E5,E7分别与已有核酸数据库中的基因克隆或EST具有较高同源性,为已知的EST,但功能未知;E6,E8在数据库中没有发现与其相似性较高的序列,为新的EST。应用数据库资源将E5、E7进行电子延伸后,将延伸序列进行开放阅读框分析,又经TBLASTx分析发现E7蛋白质序列与猪的精氨酸酶Ⅰ类蛋白序列有很高同源性。将E1、E2、E4、E5序列进行了基因表达谱分析,对E6、E8用BLASTx工具对非冗余蛋白质数据库nr进行了相似性搜索,在其他物种中找到了相似的基因序列。本研究筛选出的热休克蛋白基因、MHCⅠ类基因、精氨酸酶Ⅰ类基因和其他未知功能基因可以作为抗口蹄疫病毒研究中的侯选基因,其具体的功能有待今后进一步研究。     

黄瓜芽黄突变体抑制消减杂交文库的构建及初步分析

利用抑制消减杂交技术(suppression subtractive hybridization,SSH)分离了黄瓜芽黄突变体及其野生型之间差异表达的cDNA片段.以突变体和野生型分别作检测子和驱赶子,建立正向和反向两个消减杂交cDNA文库;经阳性克隆鉴定,在正向文库中获得特异表达的阳性克隆有133个,在反向文库中得到的阳性克隆有73个.测序后将所得到的159条非重复且非黄瓜的ESTs(登录号:GH270133～GH270291)进行序列同源性比对分析,发现这些ESTs分别与叶绿素合成、光合系统、信号转导、转录因子、氨基酸代谢、糖类代谢、脂类代谢等相关酶及蛋白基因高度同源.     

Analysis of Expressed Sequence Tags from Skeletal Muscle-specific cDNA Library of Chinese Native Xiang Pig

A Longissimus Dorsi muscle cDNA library of Xiang Pig was constructed, and 131 randomly isolated clones were sequenced in this study. The results of bioinformatics analysis showed that 131 ESTs represented 109 unique clones sequences, of which 99 showed homology to previously identified genes in humans or other mammals, 3 matched other uncharacterized expressed sequence tags (ESTs), and 7 showed no significant matches to sequences already present in DNA databases. No protein matches were found for 10 ESTs. Functional analysis of the ESTs showed that a considerable proportion of them encoded proteins involved in gene/protein expression (45.46%). Other classes included genes involved in metabolism (10.10%), cell structure/motility (10.10%), cell/organism defense (5.05%), cell signaling/communication (2.02%), and cell division (0.0%). Unclassified genes constituted the remaining 27.27%. This study reported the results of the first gene expression profile analysis of Chinese native Xiang Pig skeletal muscle cells, thereby greatly facilitating the functional study of candidate genes involved in muscle growth as well as in the improvement of meat quality in domestic pigs.     

A rapid assay of the sialidase activity in species of the Bacteroides fragilis group by using peanut lectin hemagglutination

In this study, a novel, simple and rapid hemagglutination assay by using a peanut lectin to detect a neuraminidase activity in strains of the Bacteroides fragilis group was developed. One hundred and fourteen species of the B. fragilis group isolated from children with and without diarrhea and 15 reference strains were evaluated. Neuraminidase production was determined by using the method above described and its inhibition was observed by using galactose. The neuraminidase production was observed in 54 (84.37%) diarrhea and in 43 (86%) non-diarrhea strains. HA titers were ranged from 2 to 32. This neuraminidase assays based on PNA hemagglutination is highly sensitive, reproducible and could be used as a tool to detect the sialidase activity in anaerobic bacteria, particularly, in species of the B. fragilis group.     

Analysis of expressed sequence tags (ESTs) from Lentinula edodes

The 1,031 expressed sequence tags (ESTs) from the basidiomycete Lentinula edodes were generated as a pilot experiment to see distribution of genes expressed in L. edodes. Among them, genes for hydrophobin, which are specifically found in filamentous fungi, were the most frequently obtained ESTs (33 times), suggesting that they are highly expressed in L. edodes. In addition to known hydrophobin 1 and 2 types, our analysis revealed the existence of novel types of hydrophobin, which we named hydrophobin 3, 4, and 5. The second and the third most highly obtained ESTs were phosphatidylserine decarboxylase and formate dehydrogenase, which were obtained eight and seven times, respectively. It should be noted that two important genes (argonaute and RNA-dependent RNA polymerase) involved in the RNAi pathway were found, suggesting a future application for gene knock-down by RNA interference. The 53 ESTs were identical with the sequences already reported in L. edodes. The 433 ESTs were found to show significant sequence similarity (E value <1 x 10(-5)) with the proteins reported (or predicted) in other species. In total, 387,952 bp were sequenced and registered in DDBJ/GenBank (accession number BJ998097-BJ999127).     

DNA sequence-based "bar codes" for tracking the origins of expressed sequence tags from a maize cDNA library constructed using multiple mRNA sources

To enhance gene discovery, expressed sequence tag (EST) projects often make use of cDNA libraries produced using diverse mixtures of mRNAs. As such, expression data are lost because the origins of the resulting ESTs cannot be determined. Alternatively, multiple libraries can be prepared, each from a more restricted source of mRNAs. Although this approach allows the origins of ESTs to be determined, it requires the production of multiple libraries. A hybrid approach is reported here. A cDNA library was prepared using 21 different pools of maize (Zea mays) mRNAs. DNA sequence "bar codes" were added during first-strand cDNA synthesis to uniquely identify the mRNA source pool from which individual cDNAs were derived. Using a decoding algorithm that included error correction, it was possible to identify the source mRNA pool of more than 97% of the ESTs. The frequency at which a bar code is represented in an EST contig should be proportional to the abundance of the corresponding mRNA in the source pool. Consistent with this, all ESTs derived from several genes (zein and adh1) that are known to be exclusively expressed in kernels or preferentially expressed under anaerobic conditions, respectively, were exclusively tagged with bar codes associated with mRNA pools prepared from kernel and anaerobically treated seedlings, respectively. Hence, by allowing for the retention of expression data, the bar coding of cDNA libraries can enhance the value of EST projects.