46 resultados para 5 UTR
em Chinese Academy of Sciences Institutional Repositories Grid Portal
Resumo:
稻属Oryza隶属禾本科Poaceae,包括20多个野生种和2个栽培种(亚洲栽培稻O. sativa L和非洲栽培稻O. glaberrima Steud) ,广泛分布于全球热带和亚热带。稻属物种可划分为10个基因组(又称染色体组)类型:A, B, C, BC, CD, E, F, G, HJ 和 HK。栽培稻所属的A基因组是稻属中物种数目最多、地理分布最广的基因组类型,由8个种组成。由于栽培稻属于A基因组,故A基因组物种是栽培稻遗传改良的巨大基因源。数十年来,国际上许多学者对A基因组类群开展了大量涉及形态、细胞、同工酶和分子标记方面的研究,但由于A基因组物种间遗传关系十分接近,形态上差异小且地理分布重叠,使得A基因组物种的系统发育、物种起源和生物地理学等方面存在诸多悬而未决的问题,是稻属中分类和鉴定困难较多的类群。本文利用核基因内含子序列,结合转座子插入分析,重建了A基因组的系统发育,估测了各类群的分化时间;与此同时,基于多克隆测序和基因谱系分析,探讨了O. rufipogon和O. nivara遗传关系以及亚洲栽培稻起源。主要研究结果如下: 1. A基因组的系统发育 在水稻全基因组数据库搜索的基础上,测定了4个单拷贝核基因(Adh1 及3个未注释基因)的内含子序列,构建了稻属A基因组8个种的系统发育关系。基于最大简约法和贝叶斯法的系统发育分析表明:1)澳大利亚的O. meridionalis为A基因组的基部类群;2)亚洲栽培稻两个亚种O. sativa ssp. japonica 和 O. sativa ssp. indica分别和不同的野生类群聚为独立的两个分支,支持japonica 和 indica为多次起源;3)O. rufipogon和O. nivara在系统发育树上完全混在一起,显示出二者间不存在遗传分化;4)非洲一年生野生种O. barthii是非洲栽培稻O. glaberrima的祖先,而非洲多年生野生种O. longistaminata与O. glaberrima/O. barthii.亲缘关系较远;5)分子钟方法估测A基因组类群约在2百万年前(2.0MYA)开始分化,亚洲栽培稻和非洲栽培稻,以及亚洲栽培稻的两个亚种则分别在0.7和 0.4 MYA左右开始分化。此外,通过核基因内含子序列与其它常用片段如ITS,matK等对比分析表明,进化速率相对较快的核基因内含子序列可以有效地用于近缘类群的系统发育研究。 2. Oryza rufipogon 和O. nivara群体遗传研究及亚洲栽培稻起源 对于亚洲野生类群O. rufipogon和O. nivara是合并为一个种还是处理为两个独立的种一直存在争议。在系统发育研究基础上,我们选取4个核基因内含子或5’-UTR区(Waxy, LHS,CatA和1个未注释基因),对采自整个分布区的群体样品进行了多克隆测序,结果表明:1)检测到O. rufipogon和O. nivara均有较高的核苷酸多态性,4个位点上π值和θw值平均分别为0.011和0.014;2)且二者在遗传上没有明显分化,两个类群在4个核基因位点上均检测到大量共享多态(shared polymorphism),未发现固有差异(fixed difference),表明它们历史上可能属于一个大群体,支持将二者作为种内不同生态型或亚种处理;3)基因谱系树表明亚洲栽培稻的两个亚种indica和japonica分别和不同的O. rufipogon (包括O. nivara)群体聚在一起,进一步从基因谱系角度支持亚洲栽培稻多次起源假说。 3.转座子在群体遗传与系统发育研究中的应用 鉴于目前植物谱系地理学研究中缺乏具有足够信息量的分子标记用于检测种内遗传变异,我们选取3个核基因中的转座子,通过对取自O. rufipogon和O. nivara整个分布区的37份样品的克隆测序,探讨了进化速率快、信息含量丰富的转座子序列在群体遗传上的应用。结果表明:1)无论在物种水平还是群体水平,转座子能检测到比包括内含子在内的其它DNA区域高得多的遗传变异;2)在物种水平上,异交多年生的O. rufipogon和自交一年生的O. nivara多样性均较高,且2个种间相差很小,二者在3个位点上平均核苷酸多样性π值均为0.013,差别主要表现在O. rufipogon杂合位点比例(46.1%)明显高于O. nivara(9.1%),说明交配系统不同并不一定和物种多样性水平相关;3)是否发生转座子序列插入是有价值的系统发育信息,发生在不同染色体上3个基因中的转座子插入进一步证实A基因组基部类群是O. meridionalis;通过叶绿体中3个转座子的插入现象推断了稻族一些四倍体物种,如稻属BC基因组的一些类群的母本来源。
Resumo:
水母雪莲(Saussurea medusa Maxim)为名贵珍稀中药材,其主要药用成分为类黄酮,尤其是3-脱氧类黄酮。目前关于雪莲的研究主要集中在采用细胞培养生产类黄酮等方面,但对于雪莲类黄酮生物合成的分子机制了解甚少,极大限制了这一珍贵资源的利用。本研究采用水母雪莲红色系愈伤组织及悬浮细胞为材料,构建cDNA文库,从中克隆水母雪莲类黄酮次生代谢中的相关基因并对这些基因进行了深入的生物信息学分析、转基因研究初步确定其功能,以期了解雪莲类黄酮次生代谢的分子机制,为提高类黄酮的合成奠定基础。主要结果如下: 1. 成功地构建了水母雪莲红色系愈伤组织与悬浮细胞cDNA文库,原始文库滴度达到4×106pfu/ml,扩增文库滴度接近1011 pfu/ml,重组率达98%。PCR检测插入片段,均在0.5kb到3kb之间,1kb以上占62%。从文库中检测到了chs、dfr及Myb转录因子SmP,文库覆盖度达到要求且为PCR筛选文库提供了可能。 2. 采用部分简并引物,通过RT-PCR克隆了水母雪莲查尔酮异构酶基因Smchi特异探针,并根据这一探针序列设计特异引物,采用TD-PCR法筛选cDNA文库,获得Smchi cDNA序列,全长831bp,编码一个232氨基酸残基的蛋白。根据cDNA序列克隆了Smchi DNA序列,结果表明Smchi基因无内含子。Smchi cDNA序列与翠菊chi基因高度同源,ORF区域同源性高达84%,但推测氨基酸序列则只有79.3%。Smchi mRNA具有复杂的二级结构。SmCHI具有典型的Chalcone结构域,其二级结构与苜蓿CHI蛋白十分相似,7个α-螺旋与8个延伸链由随机结构联系起来。但其活性中心的第三个关键氨基酸残基N115为M115所取代,这一取代可能导致该蛋白无生物活性,也可能使它具有一般CHI不同的功能。构建Smchi正义、反义真核表达载体,通过农杆菌介导导入烟草,获得转正义、反义Smchi基因的烟草。转基因烟草花色未改变,但叶片总黄酮发生了显著的变化,50%转正义基因烟草总黄酮含量显著提高,最高比对照提高6倍,70%转反义基因烟草总黄酮含量显著下降,最多达85.1%,初步证明Smchi具有功能,并能有效调控烟草类黄酮次生代谢。因此,SmCHI可能是不同于已知CHI的一类新的CHI蛋白,它催化的反应可能与花色素合成无关,其反应机制也可能有所不同。 3. 伴随Smchi的克隆获得了一个黄烷酮3-羟化酶类似基因Smf3h的cDNA,全长1334bp,编码一个343aa的蛋白。根据这一cDNA序列克隆了Smf3h DNA序列,全长1630bp,结果表明该基因由4个外显子和3个内含子组成。Smf3h mRNA具有十分复杂的二级结构。 推测蛋白氨基酸同源性分析表明,SmF3H属于2OG-FeII_Oxy家族,与同一家族的的颠茄H6H的同源性为45%,与拟南芥F3H的同源性为40%,但对SmF3H、典型F3H及典型H6H推测蛋白二级结构、活性中心关键氨基酸残基的位置与相对距离、软件进行功能预测分析,发现SmF3H与F3H更相似。构建Smf3h的正义与反义真核表达载体,通过农杆菌介导导入烟草,但只获得一批转正义基因的烟草,反义基因导致烟草不能再生而未获得转反义基因烟草。转基因烟草花色未改变,叶片总黄酮也与对照相似,初步确认Smf3h与烟草类黄酮生物合成无关,而是一个既不属于f3h也不属于h6h的功能未确定的新基因。 4. 采用与克隆Smchi基因相似的方法,从cDNA文库中克隆了SmP基因cDNA,全长969bp,编码一个256 aa的蛋白质。根据cDNA序列克隆了SmP基因的DNA序列,结果表明,SmP基因无内含子。SmP基因cDNA 一级结构及mRNA二级结构预测分析表明,该基因A+T含量很高(63%),所形成二级结构以A-T配对为主,其稳定性可能较差。SmP推测蛋白序列具有R2R3-Myb转录因子的典型特征,在N-端具有两个Myb DNA-binding Domain,其二级结构与鸡Myb转录因子1A5J十分相似,与其他基因如水稻OsMYB、番茄ThMYB的同源区域主要集中在这一结构域,分别为71.3%和70.8%;C-端富含丝氨酸,与烟草NtMYB、葡萄VlMYB等类黄酮调控因子相似,都呈寡聚体分布,并具有相同的保守磷酸化位点S170与S206。构建SmP基因真核表达载体,通过农杆菌介导导入烟草,获得大量转基因烟草。转基因烟草花色未发生改变,但51%的转基因烟草叶片总黄酮含量都显著提高(0.5-6倍),表明SmP具有促进烟草类黄酮生物合成的功能,但所调控的支路与花色素合成无关。初步试验结果表明,转SmP基因烟草对蚜虫具有很高的抗性,可有效地抑制蚜虫在烟草上的生长,抑制率最高可达92%-100%。这一抗性与烟草中类黄酮的积累可能具有直接的联系,但还需要进一步的试验证明。 5. 与美国俄亥俄州立大学Erich Grotewold 博士实验室合作,完成了微型EST库50个克隆的测序并进行了分析,从中获得了水母雪莲花色素合酶基因SmANS及醛脱氢酶基因SmALDH的特异探针。根据SmANS特异探针设计引物,采用PCR从这50个克隆中筛选获得了SmANS的cDNA序列,全长1229bp,编码一个356aa的蛋白质。SmANS在cDNA水平上与同属的翠菊ANS基因高度同源,但同源区域集中在ORF区域,达到80%,mRNA 预测二级结构十分复杂;推测氨基酸序列与翠菊ANS同源性达到82.9%。SmANS属于2OG-FeII_Oxy家族,在2OG-FeII_Oxy结构域高度保守,与翠菊、甜橙ANS保守结构域同源性达到94%。预测蛋白二级结构以α-螺旋-β-折叠为主,由7个主螺旋和11个主β-折叠及随机结构连接而成,并具有2OG-FeII_Oxy家族活性中心的三个保守的组氨酸残基(His84、His235、His291)和一个天冬氨酸残基(Asp237)。 6. 根据微型EST库中获得的SmALDH特异探针设计引物,采用PCR从这50个克隆中筛选获得了SmALDH基因cDNA 序列,全长1664bp,编码一个491aa的蛋白质。SmALDH基因cDNA具有独特的碱基组成,3/-UTR富含A+T,占该区域碱基总量的80%,5/-UTR的A+T和G+C各占50%,比ORF区域(52%)还低,因此其mRNA二级结构中5/-UTR可以单独形成自身二级结构并且十分稳定,这可能影响基因的表达。这一现象在水稻、玉米等植物中也存在。SmALDH在cDNA水平上在ORF区域与拟南芥、藏红花、水稻等具有较高同源性,分别为64.03%、63.89%、63.72%,但在推测蛋白氨基酸序列水平上同源性反而较低,分别为54.9%、54.3%、54.0%。SmALDH缺少线粒体定位信号,为胞质醛脱氢酶,具有一个Aldedh 保守结构域,还具有与1OF7-H相似的以α-螺旋-β-折叠为主的二级结构,由10个主螺旋和15个主β-折叠及随机结构连接而成。由于ALDH在植物细胞乙醇发酵中具有解除醛类物质毒害的功能,因此SmALDH基因的克隆为改造细胞自身以适应发酵培养条件,解决水母雪莲细胞大规模培养中需氧问题提供了可能。
Resumo:
第一部分 水稻E类MADS-box 基因在花发育中的功能分析 MADS-box 基因是一个大的转录因子家族,在花发育过程中起重要作用。根据对双子叶模式植物拟南芥、金鱼草和矮牵牛遗传突变体的研究,提出了花发育的ABCDE模型。该模型认为:A、B、C、D、E代表了5类功能不同的花器官特征基因,单独或联合控制花器官的发育。A类基因控制萼片的发育;A、B和E类基因控制花瓣的发育;B、C和E类基因控制雄蕊的发育;C和E类基因控制心皮的发育;D类基因控制胚珠的发育;A和C类基因相互抑制。在这5类基因中,E类基因的功能较为复杂,它不仅是花器官特征基因,而且具有花分生组织决定性(Floral meristem determinency)。在单子叶植物中,E类基因的功能发生了很大的分化。水稻是单子叶植物的模式植物,水稻中至少有5个E类基因,分别是OsMADS1、OsMADS5、OsMADS7、OsMADS8和OsMADS34,在这5个E类基因中,除了对OsMADS1基因有较深入的研究外,对其它几个E类基因的功能了解甚少。我们在现有的研究基础上,根据对双子叶植物中E类基因的研究结果,以OsMADS8基因为出发点,利用组织原位杂交,RNAi技术对水稻中的E类基因进行了深入的研究。结果表明:OsMADS8/7基因早在花序枝梗分生组织原基就有转录,随着小穗的生长发育,逐渐集中在小穗分生组织原基,小花分生组织原基,浆片、雄蕊和心皮中表达;在胚珠形成时,内外珠被有很强的杂交信号,而且在幼胚和胚乳中也有表达。OsMADS5在幼花时期,四轮花器官均有表达,在小穗发育后期及受精后的表达方式与OsMADS8/7基因相同。OsMADS8基因被抑制后,转基因植株没有任何表型变化,说明很可能有其它E类基因弥补了OsMADS8基因的功能缺失;当同时抑制其它E类基因的表达时,转基因植株抽穗期明显延长,四轮花器官的发育均受到影响:稃片类似叶片状;浆片转变为稃片类的结构;雄蕊没有花粉;心皮具有了稃片的特点;没有胚珠结构的形成,同时失去了花分生组织决定性,在心皮的部位产生了新的花器官或花分生组织逆转为花序分生组织。说明水稻四轮花器官及胚珠的正常发育需要E类基因的参与,但其功能与双子叶植物如拟南芥,西红柿、矮牵牛等直系同源基因相比已经发生变化;水稻中的E类基因在维持花分生组织特征性方面起重要作用;另外对抽穗期有影响。 第二部分 玉米MADS-box基因ZAG2转录调控区的研究 基因的时空表达受基因中的顺式作用元件及其反式作用因子调控。顺式作用元件由位于基因编码区上游的启动子区域和位置不确定的增强子区域组成。顺式作用元件对基因表达的开启至关重要。MADS-box 基因编码一类控制花器官发育的转录因子,在花的发育过程中顺序表达。MADS-box 基因突变,花器官发生同源异型转换。研究MADS-box 基因的调控序列可以进一步揭示影响基因时空表达的内外因素。ZAG2是玉米MADS-box 基因中的D类基因,控制胚珠的发育,在胚珠和心皮的内表面特异表达。ZAG2基因有7个外显子和6个内含子。我们从玉米基因组分离到了ZAG2基因翻译起始点上游3040bp的序列,并利用5’-RACE方法鉴定出了转录起始点的位置。序列比较发现,在 5’-UTR内有一个1299bp的内含子,这个内含子可能对基因的表达有调控作用,因此构建了两个与GUS基因融合的表达载体:一个是pZAG2-1::GUS,包括翻译起始点以上所有的调控序列;另一个是pZAG2-2::GUS,去掉了5’-UTR中的内含子序列,转化水稻。结果这两个构建都没有使GUS基因在正确的位置表达。pZAG2-1::GUS构建在心皮基部类似花托的部位及稃片顶端着色,pZAG2-2::GUS构建在内外稃片沿稃脉的部位有很强的着色,说明翻译起始点上游的调控序列不足以使基因正常表达。两个构建着色方式不同,可能pZAG2-1::GUS构建在5’-UTR部分含有抑制ZAG2基因在稃片表达的顺式元件,或者启用了在5’-UTR中的转录起始点,因为在5’-UTR的内含子中也有一个很典型的TATA-box。我们推测,在ZAG2基因编码区的第一内含子可能存在另外一些使基因正常表达的增强元件,需要进一步的序列缺失实验加以验证。
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非编码区序列在基因表达调控中起着重要作用, 但其在进化过程中是否受到选择作用一直较难检 测。最近有一些研究使用平均的核苷酸替换速率与中性序列的核苷酸替换速率的比值(ω) 作为检测非编码区 总体受选择作用的指标; 但是对于非编码区而言, 了解具体哪些核苷酸受到选择作用更具有意义。我们借鉴 Nielsen & Yang (1998) 检测单个氨基酸位点是否受选择作用的思路, 在最大似然法的模型下, 提出一种在核苷 酸位点水平上对自然选择作用检测的方法。本方法能够检测在进化过程中对功能分化有重要贡献的核苷酸位 点, 包括编码和非编码区。将此方法应用于熟知的受到正选择作用的蛋白编码基因序列( HIV21 包装蛋白基因 编码区) , 均能够检测到那些已知的受到正选择的核苷酸(密码子) 位点, 说明此方法可以有效地在核苷酸位 点水平检测选择作用; 又将此方法应用于非编码区( CTGF 基因5′UTR) , 也得到了良好的结果。
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为了比较不同地域萤火虫荧光素酶基因的进化关系,通过GenBank中已知的荧光素酶基因保守区段设计引物,利用5'-RACE(rapid-amplification of cDNA ends)和3'-RACE技术克隆了来自云南省文山州和西双版纳州的同种卵黄萤荧光素酶基因cDNA和全基因序列.来自不同地域的2种卵黄萤荧光素酶在基因序列上存在3个不同碱基位点,但是它们编码的荧光素酶只存在1个不同的氨基酸.卵黄萤荧光素酶基因全长(从起始密码子到终止密码子)1998 bp,包含7个外显子,6个内含子,其cDNA序列共1976 bp,包含102 bp 5'UTR(untranslated region)、1635 bp的荧光素酶基因开放阅读框和239 bp的3'UTR序列.卵黄萤荧光素酶基因的开放阅读框编码1个544个氨基酸的蛋白质,比同属的其它几种荧光素酶少4个氨基酸.来自2个不同地域的卵黄萤荧光素酶在进化上是比较保守的,它们与北美萤火虫Photinus pyralis荧光素酶在碱基序列上分别有62.9%和63%相似性.
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对酵母中高效转录和低效转录基因内含子序列寡核苷酸使用情况的对照分析,显示两类内含子的序列结构有差异,并且高效转录基因内含子序列含有较多潜在的转录因子结合位点,由此推测内含子可能参与基因转录的调控。这个结论有待更多的数据证实。对内含子和外显子在两组基因序列中的分布(长度、位置等)进行详细比较分析后显示,高效转录基因内含子和低效转录基因内含子的长度有比较明显的界限。两组基因中外显子长度的均值虽然有些差异,却没有明显的界限。基因序列长度与外显子长度的情况相似。虽然内含子的相对位置在两类基因中都很靠近5^端,但是从实际位置看,高效转录基因中比较多的内含子很靠近基因的5^端,有些则位于5^-UTR区域。这些结果提示,基因的转录效率与内含子的长度有关,与外显子及基因序列的长度无关,内含子的位置也可能影响转录效率,内含子对基因转录的调控可能与基因上游的转录调控有关联,或者是上游调控的延续。
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A comparative analysis on the intron sequence oligonucleotide usages in two sets of yeast genes with higher and lower transcription frequencies, respectively, has shown that the intron sequence structures of the two sets of genes are different. There are more potential binding sites for transcription factors in the introns of the genes with high transcription frequencies. So it is speculated that introns regulate the transcription of genes. But more evidences are needed to favor this speculation. The detailed comparative analyses on the distribution ( length and position) of introns and exons in the two sets of gene sequences also show that there is an obvious boundary between the lengths of the two sets of introns. There is no boundary between the lengths of the two sets of exons, although the means of their lengths are of discrepancy. The situation of the gene lengths ( length of intron and exon) is similar to exon lengths. As far as the relative position, the introns in two sets of genes all have a bias toward the 5' ends of genes. But as the actual position is considered, more introns in high transcription genes have a tendency to be located toward the 5' ends of genes, some even located at 5'-UTR. These results suggest that the gene transcription rates are related to the length of intron, but not to the lengths of exons and genes sequences. The positions of introns may also influence the transcription rates. The transcriptional regulation of introns may be correlative with the transcriptional regulation of the upstream of genes, or be its continuous action.
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SIMP (source of immunodominant MHC-associated peptides) plays a key rote in N-linked glycosylation with the active site of oligosaccharyltransferase, being the source of MHC-peptides in the MHC I presentation pathway. In the present study, the SIMP gene has been cloned from grass carp Ctenopharyngodon idella by rapid amplification of cDNA ends (RACE). The full length of the cDNA sequence is 4384 bp, including a 1117 bp 5' UTR (untranslated region), a 2418 bp open reading frame, and a 849 bp 3' UTR. The deduced amino acids of the grass carp SIMP (gcSIMP) are a highly conserved protein with a STT3 domain and 11 transmembrane regions. The gcSIMP spans over more than 24,212 bp in length, containing 16 exons and 15 introns. Most encoding exons, except the first and the 15th, have the same length as those in human and mouse. The gcSIMP promoter contains many putative transcription factor binding sites, such as Oct-1, GCN4, YY1, Sp1, Palpha, TBP, GATA-1, C/EBP beta, and five C/EBP alpha binding sites. The mRNA expression of gcSIMP in different organs was examined by real-time PCR. The gcSIMP was distributed in all the organs examined, with the highest level in brain, followed by the level in the heart, liver, gill, trunk kidney, muscle, head kidney, thymus, and the lowest level in spleen. Furthermore, the recombinant gcSIMP has been constructed successfully and expressed in Escherichia coli by using pQE-40 vector, and the polyclonal antibody for rabbit has been successfully obtained, which was verified to be specific. Identification of gcSIMP will help to explore the function in fish innate immunity. (c) 2007 Elsevier Ltd. All rights reserved.
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Three interferon regulatory factor (IRF) genes, CaIRF-1, CaIRF-2 and CaIRF-7, and their promoters of snakehead (Channa argus) were cloned and characterized. The CaIRF-1 gene consists of ten exons, spans 4.3 kb and encodes a putative peptide of 299 aa. The CaIRF-2 gene consists of nine exons, spans 8 kb and encodes a putative peptide of 328 aa. The gene organizations of CaIRF-1 and CaIRF-2 are very similar to that of human IRF-1 and IRF-2 except more compact. Comparison of exon-intron organization of the two genes indicated a common evolutionary structure, notably within the exons encoding the DNA binding domain (DBD) of the two factors. The CaIRF-7 gene spans 4.1 kb and encodes a putative peptide of 437 aa. However, the gene organization of CaIRF-7 consisting of ten exons is different to human IRF-7a gene which has an intron in 5' UTR. Three CaIRFs share homology in N-terminal encompassing the DBD that contains a characteristic repeat of tryptophan residues. The promoters of CaIRF-1 and CaIRF-2 genes contain the conserved sites for NF-kappa B and Sp1. The gamma-IFN activation sites (GAS) were found in the promoters of CaIRF-1 and CaIRF-7. The promoter of CaIRF-7 contains conserved interferon stimulating response element (ISRE) which is characteristic of IFN-induced gene promoter, and suggests that there also exist intracellular amplifier circuit in fish IFN signal pathway. Moreover, the element GAAANN oriented in both directions is repeated in CaIRF promoter regions, which confers to further inducibility by IFN. The constitutive expression of CaIRF genes were found to increase obviously in response to induction by the known IFN-inducer poly I:C. (c) 2008 Published by Elsevier Ltd.
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TNF receptor associated factor 1 (TRAF1) plays an important role in regulating the TNF signaling and protecting cells from apoptosis. In the present study, a TRAF1 gene has been cloned from grass carp (Ctenopharyngodon idella) by reverse transcription (RT)-PCR and rapid amplification of cDNA ends (RACE). The full-length cDNA is 2235 bp, including a 250 bp 5' UTR (untranslated region), a 1659 bp open reading frame, and a 326 bp 3'UTR. The polyadenylation signal (AATAAA, AATAA) and one mRNA instability motif (AUUUA) were found followed by a poly (A) tail in the 3'UTR. No signal peptide or transmembrane region has been found in the putative amino acids of grass carp TRAF1 (gcTRAF1). The putative amino acids of gcTRAF1 share 72% identity with the homologue in zebrafish. It is characterized by a zinc finger at the N-terminus and a TRAF domain (contains one TRAF-C and one TRAF-N) at the C-terminus. The identity of the TRAF domain among all the TRAF1 homologues in vertebrates varies from 52% to 58%, while the identities of TRAF-C were almost the same as 70%. The recombinant gcTRAF1 has been constructed successfully and expressed in Escherichia coli by using pET-32a expression vector. The polyclonal antibody for rabbit has been successfully obtained. The expression of gcTRAF1 in different organs was examined by real-time quantitative PCR and Western blotting, respectively. It was widely distributed in heart, head kidney, thymus, brain, gill, liver, spleen, and trunk kidney. This is the first report of TRAF1 homologue molecule found in fish. (c) 2007 Elsevier B.V. All rights reserved.
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Previous studies have demonstrated that germinal vesicle of amphibian oocyte contains small nuclear ribonucleoprotein polypeptide C (SNRPC). In this study, a putative member of SNRPC was identified from Carassius auratus gibelio oocyte cDNA library. Its full-length cDNA has an open reading frame of 201 nt for encoding a peptide of 66 an, a short 5'-UTR of 19 nt and a long 3'-UTR of 347 nt including a polyadenylation signal and poly- (A) tail, and the deduced amino acid sequence has 47% identity with the C-terminal of the zebrafish small nuclear ribonucleoprotein polypeptide C. Western blot analysis revealed its oocyte-specific expression. Immunofluorescence localization indicated that its gene product localized to numerous nucleoli within the oocytes and showed dynamic changes with the nucleoli during oocyte maturation. RT-PCR and Western blot analysis further revealed its constant presence in the oocytes and in the embryos until hatching. The data suggested that the newly identified CagOSNRPC might be a nucleolar protein. (c) 2006 Elsevier Inc. All rights reserved.
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A novel fish chemokine receptor gene, chemokine (C-X-C motif) receptor 3 (CXCR3)-like was isolated from the grass carp Ctenopharyngodon idella , with its full-length genomic sequence. The cDNA of grass carp CXCR3-like (gcCXCR3-like) consists of 1261 bp with a 49bp 5'-UTR and a 189 bp 3'-UTR. An open reading frame of 1023 bp encodes a 341-amino acid peptide, with seven transmembrane helices. The deduced amino acid sequence showed the same sequence identities (37.8%) with its counterparts in goat and human. The gcCXCR3-like gene consists of two exons, with one intervening intron, spaced over approximately 2 kb of genomic sequence. Phylogenetic analyses clearly demonstrated that the gcCXCR3-like resembles the CXCR3s of other vertebrates. Real-time PCR analysis showed that gcCXCR3-like was expressed in all tested organs except heart and the expression level of gcCXCR3-like was highest in brain. Flow cytometric analyses showed the positive rate of labelled leukocytes from the healthy grass carp was 17.3%, and the labelled leukocytes were divided into three types by cell sorting. Immunohistochemical localization revealed that gcCXCR3-like expressed in whole brain regions including cerebel, diencephalon, medulla oblongata, optic lobe, and rhinencephalon, and that the labelled leukocytes are actually populations of monocyte and/or phagocyte, lymphocyte and the granulocyte. It is considered that fish CXCR expression and their function may need to be investigated in both nervous and immune systems. (c) 2006 Elsevier Ltd. All rights reserved.
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Interferon (IFN) can induce an antiviral state via interferon-regulatory transcription factors (IRFs), which bind to and control genes directed by the interferon-stimulated response element (ISRE). Here we describe a fish IRF, termed CaIRF7, cloned from a subtractive cDNA library which is constructed with mRNAs obtained from crucian carp (Carassius auratus L.) blastulae embryonic (CAB) cells infected by UV-inactivated GCHV and mock-infected cells. CaIRF7 cDNA was found to be 1816 bp in length, with a 42 bp 5' UTR and a 508 bp 3' UTR. The open reading frame translates into 421 amino acids in which a DNA-binding domain (DBD) containing the repeated tryptophan motif and IRFs association domain have been identified. Like chicken GgIRF3, CaIRF7 was most similar to mammalian IRF7 with 27 to 30% identity overall and some 37% identity in their DBDs. A single transcript of 1.9 kb was detected in virally induced CAB cells by virtual Northern blotting. RT-PCR analysis revealed a wide tissue distribution of CaIRF7 constitutive expression, with detectable transcript in non-infected CAB cells and various tissues of healthy crucian carp. In addition, CaIRF7 expression was differentially increased by stimulation of the CAB cells with active GCHV, UV-inactivated GCHV or CAB IFN, indicating that the activation of CaIRF7 was directly regulated by IFN. (C) 2003 Published by Elsevier Ltd.
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To understand the molecular events governing fish oogenesis, a multiple technique was used to identify the genes differentially expressed at different phases during fish oogenesis. This technique is a combination of suppression subtractive hybridization, SMART cDNA synthesis and RACE-PCR. Here we report the cDNA cloning and expression characterization of a novel SNX gene based on its differential transcription between previtellogenic and fully mature oocytes in naturally gynogenetic gibel carp. First, a cDNA fragment selectively expressed in previtellogenic oocytes was identified and used to screen a SMART cDNA library prepared from the same mRNA sample by RACE-PCR for cloning fully length cDNA. The full length cDNA was 1392-bp long and coded for a novel SNX protein with 225 amino acids. The 5' UTR had 72 bp and 3' UTR had 642 bp. Unlike most of maternal genes that are transcribed after vitellogenesis and stored in oocytes, this gene is expressed at a higher level in the previtellogenic oocytes and at a much lower level in fully matured oocytes. However, RT-PCR analysis of tissues showed it was ubiquitous transcription. The novel gene is named fish sorting nexin (fSNX), because it contains a conserved PX domain. The fact which major expression of the gene occurs in the previtellogenic oocytes suggests that it might have an important function in the oogenesis. (C) 2003 Elsevier Inc. All rights reserved.
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To gain information on the integration pattern of pMThGH-transgene, 50 transgenes were recovered from F-4 generation of pMThGH transgenic common carp (Cyprinus carpio L,) and 33 recovered genes were analyzed. The restriction maps of these recovered genes were constructed by digestion with five kinds of enzymes. These transgenes can be classified into 4 types according to their restriction maps. Only one type of transgenes maintains its original molecular form, whereas the other three types are very different from the original one and vary each other on both molecular weight and restriction maps. This implies that the sequences of most transgenes have been deleted and/or rearranged during integration and inheritance. The results of PCR amplification and Southern blot hybridization indicate that MThGH in Type I transgene keeps intact but most of its sequence has been deleted in other three types. All these results suggest that transgenes in F-4 generation of transgenic carp are highly polymorphic. Two DNA fragments concerning integration site of transgenes were cloned from recovered transgenes, and found to be homologous to the 5'UTR of beta -actin gene of common carp and mouse mRNA for receptor tyrosine kinase (RTK), respectively.
