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1.
刘志华  杨谦 《生物信息学》2005,3(3):108-111
构建了球毛壳菌菌丝的cDNA文库,并获得了1410条ESTs序列,用里氏木霉(Hypocrea jecorina,AAM76068)和粗糙脉胞菌(Neurospora crassa,CAA25761)的组蛋白H3基因(Histone H3)蛋白序列对球毛壳菌(Chaetomium globosum)ESTs序列本地数据库进行tBlastn检索,获得了球毛壳菌组蛋白H3cDNA序列。cDNA序列全长739bp,开放阅读框411bp,编码136个氨基酸组成的多肽,蛋白分子量为15.4kD。BlastP同源性分析表明该基因与里氏木霉同源性最高为100%;与地钱(Marchantia polymorpha)同源性最低为95%。三级结构预测表明,该蛋白C端为球状结构域,而N端结构对其发挥调控作用起重要作用。该基因的cDNA序列及推测的氨基酸序列在GenBank登录(登录号分别为AY669068,AAT74576)。  相似文献   

2.
以球毛壳菌cDNA文库中获得过氧化物膜蛋白(pero)基因片段(GenBank Accn:BP099709)为基础,用RACE 技术获得该基因的全长cDNA序列。序列长747bp,由412bp的3′RACE产物和508bp的5′RACE产物拼接而成。开放阅读框501bp,编码166个氨基酸,蛋白分子量为17.5kD,理论等电点为5.75。利用cDNA两侧非编码区序列作引物克隆出该基因的DNA序列,序列分析表明该基因由2个内含子和3个外显子组成。ClustalX多序列比对表明:该基因与粗糙脉孢菌(Neurospora crassa)的过氧化物膜蛋白过敏原同源性最高(83%)。将pero基因编码区克隆到原核表达载体pET28a中,构建成表达质粒pET28a-pero并转化大肠杆菌BL21,IPTG诱导后SDS-PAGE检测表达情况,结果发现在21kD处有一特异性融合蛋白带,大小与预期相符,说明该基因已经在大肠杆菌中表达。克隆的cDNA序列、DNA序列及推测的氨基酸序列在GenBank登录(登录号分别为AY555771,AY584753,AAS66898)。  相似文献   

3.
球毛壳菌60S核糖体蛋白L10a基因克隆与特性分析   总被引:6,自引:0,他引:6  
用粗糙脉孢菌(Neurospora crassa)XP_322380和赤霉菌(Gibberella zeag)PH-1(EAA76971)的60S核糖体蛋白L10a基因(60S ribosomal protein L10a,RPL10a)蛋白序列对球毛壳菌(Chaetomium globosum)ESTs序列数据库进行tBlastn检索,获得了球毛壳菌RPL10a cDNA序列。cDNA序列长765bp,开放阅读框654bp,编码217个氨基酸组成的多肽,蛋白分了量为23.9kD。BlastP分析表明该基因氨基酸序列与粗糙脉胞菌相似最高为89%;与玉蜀黍黑粉菌(Ustilago maydis)相似性最低为78%。cDNA序列及推测的氨基酸序列在GenBank登录(登录号分别为AY669070,AAT74578)。  相似文献   

4.
运用RT-PCR和RACE技术,以粘虫(Mythimna separata(Walker))cDNA为模板,对甘油醛-3-磷酸脱氢酶(glyceraldehyde-3-phosphate dehydrogenase,GAPDH)基因进行克隆获得全长cDNA序列,并利用生物信息学方法,对GAPDH全长cDNA序列及推测得到的GAPDH蛋白序列进行分析.结果表明,获得的粘虫GAPDH基因cDNA序列长度为1 317 bp,其中包括80 bp的5′非编码区、238 bp的3′非编码区和999 bp的开放阅读框(Open Reading Frame,ORF),编码一个332个氨基酸蛋白,具有GAPDH蛋白家族的两个功能结构域.该GAPDH蛋白理论相对分子质量为35.498 6 kDa,等电点为7.63,富含6种类型的特定功能位点.该蛋白序列与其他动物GAPDH蛋白序列具有77.4%~92.9%高度同源性.GAPDH基因表达量检测结果显示GAPDH在粘虫6种不同组织间表达量无显著差异(P0.05),表明GAPDH可作为研究粘虫功能基因表达量分析的可靠内参基因.该基因的cDNA序列已经递交GenBank并获得登录号为HM055756.  相似文献   

5.
根据NaHCO3胁迫下西伯利亚蓼茎部消减库中甘油醛-3-磷酸脱氢酶基因(GAPDH)表达序列标签序列设计引物,采用cDNA末端快速扩增技术,从西伯利亚蓼茎中扩增出GAPDH的全长cDNA序列。该cDNA序列全长1331bp,完整阅读框1014bp,编码337个氨基酸。属于稳定蛋白,具有GAPDH保守功能域。氨基酸组成与其他已知高等植物来自细胞质中的GAPDH基因cDNA序列具有很高的同源性,最高可以达到96%。通过转酿酒酵母INVSC1的NaHCO3和NaCl胁迫试验表明,转基因INVSC1(pYES2-GAPDH)有明显的抗盐胁迫特性。在10%NaHCO3和4mol·L-1 NaCl胁迫下,转基因INVSC1(pYES2-GAPDH)菌株存活率明显比INVSC1(pYES2)高,可以推测GAPDH基因赋予INVSC1(pYES2-GAPDH)抗NaHCO3和NaCl的能力。该基因的cDNA序列在GenBank中登录号为DQ922680。  相似文献   

6.
用粗糙脉孢菌(Neurospora crassa)XP_322380和赤霉菌(G ibberella zeae)PH-1(EAA76971)的60S核糖体蛋白L10 a基因(60S ribosom al prote in L10 a,RPL10 a)蛋白序列对球毛壳菌(Chaetom ium globosum)ESTs序列数据库进行tB lastn检索,获得了球毛壳菌RPL10 a cDNA序列。cDNA序列长765 bp,开放阅读框654 bp,编码217个氨基  相似文献   

7.
根据禾谷镰孢菌参考菌株NRRL310 84 (PH 1)的α- 微管蛋白基因核苷酸序列设计 4对引物 ,采用PCR方法克隆并测序了禾谷镰孢菌 (Fusariumgraminearum)对多菌灵 (MBC)不同敏感性表型的 6个中国菌株的α 微管蛋白基因全序列。DNA序列对照表明中国的 3个敏感菌株和 3个抗药菌株的α- 微管蛋白基因核苷酸序列同源性没有差异 ,多菌灵抗药性与α- 微管蛋白无关。该基因全长 1718bp ,含有 6个内元 ,编码 4 4 9aa ;与NRRL310 84的α- 微管蛋白基因核苷酸序列同源性为 99% ,存在 5个差异核苷酸 ,与其所编码的氨基酸序列同源性为 99 78% ;与其他 6种真菌α- 微管蛋白基因所编码的氨基酸序列同源性为 37%~ 86 %。  相似文献   

8.
以高羊茅茎基部与叶基部的mRNA为模板,引用基于多年生黑麦草GAPDH基因序列设计的引物,进行RT-PCR分析,同时结合3'RACE和5'RACE方法从高羊茅中扩增出两个GAPDH基因,命名为Fa-GAPDH1(GQ480772)与FaGAPDH2(GQ480773)。两序列cDNA全长分别为1281bp和1348bp,具有完整的开放阅读框(ORF,FaGAPDH1:74~1087bp;FaGAPDH2:106~1119bp),编码蛋白都为337个氨基酸。保守结构域功能分析表明两基因编码的蛋白质都具有典型的Rossman-NAD连接折叠和C-末端结构域。FaGAPDH1和FaGAPDH2蛋白与禾本科植物的该基因蛋白产物比较发现氨基酸序列的同源性都在90%以上,说明两基因具有高度的保守性。  相似文献   

9.
在分析一株球孢白僵菌TDNA插入突变体T12的Tagging序列的基础上,根据与其具有高度同源性的一条金龟子绿僵菌EST序列(编号为AJ273226)设计简并引物,用YADE法从球孢白僵菌中扩增出该EST的同源序列及其延伸序列。序列分析表明,该片段与粗糙脉孢霉的羧基转运蛋白JEN1具有高度同源性,由此确定该序列为球孢白僵菌羧基转运蛋白JEN1基因的部分序列。然后利用YADE法延伸扩增该序列的上、下游序列,获得球孢白僵菌羧基转运蛋白JEN1的全长DNA序列,命名为GBbJEN1。利用3′RACE扩增出球孢白僵菌羧基转运蛋白JEN1的cDNA序列,命名为BbJEN1。BbJEN1全长1656bp,编码514个氨基酸的蛋白。推测蛋白分子量为55975.37Da,等电点9.32。氨基酸序列与金龟子绿僵菌、粗糙脉孢霉和酿酒酵母羧基转运蛋白JEN1的同源性分别为77%、66%和30%。序列分析表明,GBbJEN1含有2个内含子。Southern杂交表明,GBbJEN1基因在球孢白僵菌基因组中为单拷贝。利用RTPCR法对BbJEN1的表达特性进行了分析,结果发现BbJEN1基因的转录受蟑螂壳、蝉蜕等昆虫体壁的诱导,受葡萄糖的抑制。进一步利用YADE法获得了长为977bp的GBbJEN1上游序列,其中含有可能的葡萄糖抑制调控序列和压力反应元件。  相似文献   

10.
杜氏盐藻RuBisCO小亚基基因的克隆和分析   总被引:1,自引:0,他引:1  
根据莱菌衣藻(Chlamydomonas reinhardtii)、团藻(Volvox carteri)、伞藻(Acetabularia cliftonii)等生物的1,5-二磷酸核酮糖羧化酶/加氧酶(RuBisCO)的小亚基rbcS基因氨基酸的高度保守序列,设计一对简并引物,进行RT-PCR.209 bp的PCR产物经测序分析及进行氨基酸序列同源性比对,表明克隆的序列为盐藻rbcS基因的cDNA片段.根据该序列信息,采用RACE(rapid amplification of cDNA ends) 方法扩增其5'上游未知区和3'下游未知区.5'RACE得到的cDNA长度为约300 bp,3'RACE得到的长度约380 bp.三段序列拼接后cDNA全长为878bp,其中开放读码框包括190个氨基酸.此cDNA序列,推导成氨基酸序列与已知物种的rbcS基因相比对,同源性分别为V.carteri 78%,C.reinhardtii 75%,A.cliftonii 67%,据此可推断所克隆的序列为盐藻RuBisCO的小亚基cDNA序列,GenBank收录号为AY739272.  相似文献   

11.
根据从柽柳cDNA文库克隆获得的脂质转运蛋白(LTP)的部分序列,用RACE技术克隆出其全长cDNA序列.基因的5'非翻译区96bp,3'非翻译区222bp,开放阅读框285bp,编码94个氨基酸,预计蛋白的分子量为9.9 kD,等电点为8.02.此基因有8个位置保守的Cys残基及26个氨基酸的信号肽,为典型的植物脂质转运蛋白基因.其基因序列数据库(GenBank)登录号为AY574218(基因)和AAS79106(蛋白).  相似文献   

12.
The cDNA clone encoding human prechymotrypsinogen was isolated from a human pancreas cDNA library and its nucleotide sequence was determined. The sequence consists of a 16 bp 5' non-coding region, a 789 bp amino acid coding region and a 60 bp 3' non-coding region. The predicted product consists of 263 amino acids, including 18 amino acids for a signal peptide and 15 amino acids possible for an activation peptide. Southern blot analyses using the cloned cDNA as a probe revealed that human genomic DNA carries at least two genes that are related to chymotrypsinogen.  相似文献   

13.
根据中性海藻糖酶NTL基因的同源序列设计引物,PCR扩增出杀蝗专一菌株———金龟子绿僵菌CQMa102NTL基因片段,利用5′_RACE和3′_RACE扩增出NTLcDNA的5′和3′端序列,经拼接得到CQMa102NTL基因cDNA全长。根据其全长cDNA序列,设计引物PCR扩增出CQMa102NTL的完整基因。为了解该基因的上游调控信息,采用PanhandlePolymeraseChainReactionAmplification方法扩增其上游序列。序列分析表明,CQMa102NTL全长DNA3484bp,cDNA全长2385bp,编码737个氨基酸的蛋白,推测蛋白分子量为83.1kD;含有3个内含子,包含一个依赖于cAMP的磷酸化作用位点(RRGS)和一个钙附着位点(DTDGNMQITIED);上游序列含有一个压力反应元件(CCCCT);与金龟子绿僵菌广谱性菌株ME1NTL的核苷酸序列和氨基酸序列分别具有93%和99%同源性,由此确定该序列为金龟子绿僵菌中性海藻糖酶基因序列。Southern杂交表明,NTL基因在CQMa102基因组中为单拷贝。Northern杂交表明,NTL基因转录出约2.5kb的mRNA单带,在液体培养条件下,对数生长前期表达水平最高,对数生长后期降到最低,进入稳定生长期后表达水平又有所提高。金龟子绿僵菌CQMa102中性海藻糖酶基因DNA全长和cDNA全长登录GenBank,登录号分别为:AY557613,AY557612。  相似文献   

14.
Authentic cDNAs encoding the activator protein for acid beta-glucosidase (EC3.2.1.45), co-beta-glucosidase, were cloned from the pCD and lambda gt11 human cDNA libraries. Initial screening with oligonucleotide mixtures encoding amino acid sequences of co-beta-glucosidase identified partial cDNAs which were used to obtain a potentially full-length cDNA from the lambda gt11 library. This clone (2767 bp), EGTISI, contained 5' (38 bp) and 3' (1157 bp) noncoding sequences, a translation initiation site, and an open reading frame encoding 524 amino acids which included a typical hydrophobic signal sequence (16 amino acids). Computer analyses identified three regions of high similarity to co-beta-glucosidase encoded by tandem sequences in EGTISI. Searches revealed that two of these regions encoded peptides of known function; SAP1 (sphingolipid activator protein 1) and protein C (a new sphingolipid activator protein) were encoded by EGTISI sequences 5' and 3', respectively, to those for co-beta-glucosidase. The third region of similarity, encoding a theoretical peptide (undefined function), was located most 5' in the cDNA. EGTISI and its encoded polypeptide had high similarity (77% nucleotide identity and about 80% amino acid similarity) to a rat Sertoli cell cDNA and its encoded sulfated glycoprotein-1. These results indicate that a single highly conserved gene encodes the precursor for four potential sphingolipid activator proteins in rat and man.  相似文献   

15.
A 2112-bp cDNA clone (lambda CT29) encoding the entire sequence of the human lysosomal acid phosphatase (EC 3.1.3.2) was isolated from a lambda gt11 human placenta cDNA library. The cDNA hybridized with a 2.3-kb mRNA from human liver and HL-60 promyelocytes. The gene for lysosomal acid phosphatase was localized to human chromosome 11. The cDNA includes a 12-bp 5' non-coding region, an open reading frame of 1269 bp and an 831-bp 3' non-coding region with a putative polyadenylation signal 25 bp upstream of a 3' poly(A) tract. The deduced amino acid sequence reveals a putative signal sequence of 30 amino acids followed by a sequence of 393 amino acids that contains eight potential glycosylation sites and a hydrophobic region, which could function as a transmembrane domain. A 60% homology between the known 23 N-terminal amino acid residues of human prostatic acid phosphatase and the N-terminal sequence of lysosomal acid phosphatase suggests an evolutionary link between these two phosphatases. Insertion of the cDNA into the expression vector pSVL yielded a construct that encoded enzymatically active acid phosphatase in transfected monkey COS cells.  相似文献   

16.
柽柳金属硫蛋白基因的克隆及序列分析   总被引:2,自引:0,他引:2  
张艳  杨传平  王玉成 《植物研究》2007,27(3):293-296
用木麻黄(Casuarina glauca)的金属硫蛋白基因(metallothionein 1)氨基酸序列对柽柳ESTs序列本地数据库进行tBlastn检索,获得了柽柳金属硫蛋白基因全长cDNA序列,去除polyA后该基因全长366 bp,其中5′非翻译区97 bp,3′非翻译区59 bp,开放读码框(ORF)长210 bp,编码70 个氨基酸组成的多肽,蛋白分子量为6.793 kD,理论等电点为4.99,含10个Cys,集中分布在肽链的N端和C端。BlastP同源性分析表明该基因与花生同源性最高,与小豆同源性最低。该基因的EST序列在GenBank登录(登录号:CV792539)。  相似文献   

17.
cDNA encoding the bound type trehalase of the European honeybee was cloned. The cDNA (3,001 bp) contained the long 5' untranslated region (UTR) of 869 bp, and the 3' UTR of 251 bp including a poly(A) tail, and the open reading frame of 1,881 bp consisting of 626 amino acid residues. The Mr of the mature enzyme comprised of 591 amino acids, excluded a signal sequence of 35 amino acid residues, was 69,177. Six peptide sequences analyzed were all found in the deduced amino acid sequence. The amino acid sequence exhibited high identity with trehalases belonging to glycoside hydrolase family 37. A putative transmembrane region similar to trehalase-2 of the silkworm was found in the C-terminal amino acid sequence. Recombinant enzyme of the trehalase was expressed in the methylotrophic yeast Pichia pastoris as host, and displayed properties identical to those of the native enzyme except for higher sugar chain contents. This is the first report of heterologous expression of insect trehalase.  相似文献   

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