日本三角涡虫热休克蛋白70(DjHSP70)C-端多肽表达及其抗血清制备

首先运用在线生物学软件对日本三角涡虫(Degusia japonica)热休克蛋白70(DjHSP70)氨基酸序列进行亲水区分析,发现该蛋白C-端含有较多亲水性氨基酸,然后以该段多肽序列为基础构建原核表达载体.采用PCR方法扩增450 bp cDNA片段,编码DjHSP70 C-端150个氨基酸多肽.将双酶切的cDNA...     

东亚三角涡虫cDNA文库的构建及EST初步分析

为了快速高效地分离鉴定东亚三角涡虫的发育和再生相关基因,以总RNA为模板,借助CreatorTM SMARTTM cDNA Library Construction Kit和Advantage 2 PCR Kit成功构建了东亚三角涡虫的cDNA文库.经测定,cDNA文库原始库容为1.22×105个独立克隆,重组率超过98 %,插入片段平均大小为900 bp.从文库中随机挑选重组克隆测序,并在NCBI数据库中比对,结果获得208个rRNA基因,148个编码蛋白基因,78个染色体片段基因.该研究为我国涡虫发育和再生的深入研究奠定了坚实的分子基础.     

草鱼RBM cDNA克隆及序列分析

目的:克隆草鱼RNA剪切蛋白(RNA binding motif protein-RBM)基因.方法:采用RT -PCR技术从草鱼性腺总RNA中克隆RBM基因,将其插入pBS-T载体上,经菌液PCR鉴定后进行 测序并对测序结果进行生物信息分析.结果:获得草鱼RBM cDNA部分序列 ,大小为384bp,预 测编码127个氨基酸残基;RBM基因进化与物种形态进化类似;不同物种间RBM基因一级结构 保守性不高,但氨基酸序列保守性较高,且存在高度保守的氨基酸位点.结论: 成功地克隆了草鱼RBM cDNA部分序列,为获RBM cDNA全长序列及后续研究提供理论基础.     

文昌鱼AmphiRab23b基因的克隆、进化分析及表达模式

Hedgehog信号通路在胚胎发育过程中发挥着重要作用, 同时与多种肿瘤的发生密切相关。Rab23蛋白在Hedgehog信号通路中扮演着十分重要的角色。目前关于文昌鱼Rab23同源基因的研究仅局限于佛罗里达文昌鱼(Branchiostoma floridae)基因组中的注释。文章首次克隆了中国文昌鱼(Branchiostoma belcheri) Rab23b基因 (AmphiRab23b)cDNA全序列 , 对其演译的蛋白序列进行了序列比对、进化树分析以及基因时空表达分析。研究结果显示, 文昌鱼AmphiRab23b基因的 cDNA总长为2 062 bp (包括UTR区), 其中开放阅读框 (Open reading frame, ORF) 714 bp, 编码237个氨基酸; 虽然在进化树中不属于脊椎动物Rab23进化支, 但是AmphiRab23具有保守的Rab23_lke结构域, 暗示该基因在进化过程中可能在功能上是保守的。时空表达的研究结果进一步显示, AmphiRab23b基因在胚胎发育中的神经板和消化道中表达, 与其脊椎动物同源基因的表达模式相似, 这说明该基因可能对文昌鱼神经系统和消化道的发育有重要作用。     

苦荞谷胱甘肽转移酶(FtGST)基因的克隆与序列分析

采用RACE技术,从苦荞(Fagopyrum tatarium)中克隆得到一个谷胱甘肽转移酶(Glutathione S-transferase protein,FtGST)基因。序列分析表明,FtGST基因全长DNA序列和cDNA序列编码区分别为746 bp和666 bp,DNA序列含有一个长度为80 bp(342-421 bp)的内含子;开放阅读框(ORF)长666 bp,编码221个氨基酸。生物信息学分析表明,FtGST基因推导的蛋白质含有Tau家族典型的底物结合口袋、谷胱甘肽结合位点(G-site)和疏水性底物结合位点(H-site)氨基酸残基,表明FtGST为Tau家族蛋白。     

杜氏盐藻泛素基因cDNA的克隆及系统进化分析

根据玉米,水稻等物种泛素序列设计一对简并引物.提取杜氏盐藻细胞的总RNA,利用RT-PCR方法扩增盐藻泛素基因的cDNA片断,回收两个长度不同的片断ubi-1和ubi-2,将其克隆到pMDl8-T载体上,测序后进行序列分析,为克隆杜氏盐藻泛素基因的cDNA序列并进行进化分析.结果 ubi-1经测序后得到一个完整拷贝(228 bp)和一个不完整的泛素cDNA序列(191 bp).Ubi-2经测序后得到两个拷贝(556 bp)和一个不完整的泛素cDNA序列(191 bp).盐藻3个不同拷贝泛素cDNA序列之间存在差异,但所编码氨基酸序列相同.盐藻泛素cDNA序列与其他物种的泛素cDNA序列具有高的同源(70%～85%),所推导的氨基酸序列与其他物种仅存在1～2个氨基酸的差异.进化分析显示,所分离的盐藻泛素基因与两个模式生物果蝇和衣藻的泛素基因共处一个进化支,彼此亲缘关系最近.盐藻泛素基因与其他物种的泛素基因可能来自共同的"祖先"基因.在进化中高度保守.     

日本三角涡虫hsp70 cDNA克隆及原核表达

热休克蛋白70 是热休克蛋白家族中的重要成员, 它在保护生物体免受各种胁迫中发挥重要作用。由于其惊人的再生能力, 淡水涡虫作为研究再生和发育的模式动物受到研究者关注。但是, 有关涡虫抗逆性的分子机制却少有报道。研究采用 RACE (Rapid amplification of cDNA end) 技术首次从日本三角涡虫中克隆出hsp70 (Djhsp70)全长cDNA 序列。Djhsp70 cDNA 全长2066 bp, 含有1947 bp 的开放阅读框, 编码648 个氨基酸, 分子量71.18 kD, GenBank 登录号EU380241。DjHSP70 的氨基酸含有真核生物HSP70 家族蛋白的三个标签序列(9–16 位的IDLGTTYS、199—206 位的 DLGGGTFD、334–339 位的IVLVGG)和末端高度保守序列EEVD。经BLAST 检索分析, Djhsp70 的核苷酸序列和推定的氨基酸序列与目前已知HSP70 家族成员高度同源。有趣的是, HSP70 亲缘关系分析表明: 涡虫更靠近脊椎动物, 而与无脊椎动物果蝇和线虫相距较远。为了制备抗体研究DjHSP70 的组织学定位, 实验还成功构建了DjHSP70 表达载体, 在IPTG 诱导下表达出约76 kD 的融合蛋白。Djhsp70 cDNA 的克隆与表达载体的构建为下一步工作奠定了基础。       

盐藻小G蛋白基因(DsRab)的克隆及在高盐胁迫下的表达分析

采用RT-PCR和RACE技术扩增了杜氏盐藻小G蛋白基因cDNA全长序列(GenBank Accession No.JN989548),命名为DsRab,对其进行生物信息学分析,并通过实时荧光定量PCR方法检测盐胁迫下该基因的表达情况。结果表明,DsRab基因的cDNA全长为1 299 bp,开放阅读框(ORF)为612 bp,编码203个氨基酸,5’非编码区78 bp,3’非编码区609 bp;保守性结构域分析可知编码的小G蛋白有4个GTP/GDP保守结构域,1个效应区、1个羧基端的半胱氨酸结构域和5个Rab亚家族共有的结构域;二级结构预测表明该蛋白有32.02%的α-螺旋,23.65%的伸展片段,44.33%的自由卷曲,三维建模成功;比对分析发现DsRab蛋白与多种生物的Ypt/Rab的氨基酸序列具有较高的同源性。荧光定量PCR结果表明,盐藻在高盐(3.0 mol/L)胁迫下,DsRab基因表达量显著上调,1 h后表达量达到最大值,为正常培养下对照组(0 h)的4.9倍,差异极显著(P<0.01)。     

草鱼cadm2b基因的克隆及在成体组织中的表达分析

为研究CADMs（Cell adhesion molecules）在草鱼构建抵御病害感染的第一道防线中发挥的作用,用RT-PCR和RACE方法结合测序分析,在草鱼脑组织中检测到了该基因家族成员cadm2b基因的4条不同的cDNA全长序列。序列比对结果表明这4条全长cDNA在5'端的序列完全相同,在3'端的3个局部区域有不同片段的缺失。因此,可以确定这4条不同的mRNA是cadm2b的不同剪接体。这4条不同的剪接体被分别命名为cadm2b、cadm2bX2、cadm2bX3和cadm2bX6。cadm2b的cDNA序列全长1669 bp,开放阅读框（ORF）1203 bp,编码400个氨基酸。cadm2bX2的cDNA序列全长2783 bp,开放阅读框长1323 bp,编码440个氨基酸;cadm2bX3的cDNA序列全长2755 bp,开放阅读框1296 bp,编码431个氨基酸;cadm2bX6基因的cDNA序列全长2649 bp,开放阅读框1161 bp,编码386个氨基酸。根据碱基序列所进行的氨基酸序列和蛋白结构预测显示这4个CADM2b蛋白亚型都具有CADM家族保守的4个功能区,但其C端的蛋白结合位点存在差异。CADM2b具有近膜4.1蛋白结合位点和Ⅱ型PDZ蛋白结合位点,CADM2bX2、X3缺失了PDZ蛋白结合位点,而CADM2bX6则同时缺失4.1蛋白和PDZ蛋白的结合位点。实时定量RT-PCR检测结果显示cadm2b剪接突变体是该基因mRNA的主要形式。半定量RT-PCR和套式PCR实验检测结果表明cadm2b基因在草鱼成体脑中高水平表达,在肝、肾、心脏和肌肉组织中有微量表达。这种表达模式提示草鱼中CADM2b主要是由非免疫细胞,而不是由免疫肥大细胞合成分泌的细胞黏附因子,可能通过介导免疫肥大细胞与病原靶细胞的黏附而起非特异性抵御病害感染的作用。     

疣粒野生稻金属硫蛋白基因的获得及序列分析

对SMARTTM技术构建的疣粒野生稻叶片cDNA文库克隆进行随机测序,获得了疣粒野生稻金属硫蛋白基因的cDNA序列.该序列全长412 bp,开放阅读框长186 bp,编码62个氨基酸,10个半胱氨酸集中分布在肽链的N端和C端,该蛋白的分子量为6.4 kD,理论等电点(pI)为5.14.Blastp同源性分析表明其属于金属硫蛋白基因家族.     

Molecular cloning of cDNA encoding human Rab3D whose expression is upregulated with myeloid differentiation

To identify genes expressed in myeloid differentiation, we isolated a cDNA fragment by differential display using RNA prepared from HT93A cells, a human cell line capable of differentiating into neutrophil and eosinophil lineages in response to retinoic acid (RA). Evaluation of the full-length clone isolated from an HT93A cDNA library showed that it encoded a 24 kDa protein comprised of several domains conserved in the Ras superfamily. Comparison of the deduced amino acid sequence of this clone with Rab proteins revealed that it had highest homology to a small GTP-binding protein, murine Rab3D. The mRNA expression of human Rab3D was upregulated in the course of myeloid differentiation, and it was preferentially expressed in granulocytes. These results suggest that human Rab3D may play a specific role in granulocytes, for example in exocytosis of neutrophil-specific granules or in degranulation of both eosinophils and basophils.     

Analysis of the transcriptional response to Rice Yellow Mottle Virus infection in<Emphasis Type="Italic"> Oryza sativa indica</Emphasis> and<Emphasis Type="Italic"> japonica</Emphasis> cultivars

Several cDNA libraries were constructed using mRNA isolated from roots, panicles, cell suspensions and leaves of non-stressed Oryza sativa indica (IR64) and japonica (Azucena) plants, from wounded leaves, and from leaves of both cultivars inoculated with Rice Yellow Mottle Virus (RYMV). A total of 5549 cleaned expressed sequence tags (ESTs) were generated from these libraries. They were classified into functional categories on the basis of homology, and analyzed for redundancy within each library. The expression profiles represented by each library revealed great differences between indica and japonica backgrounds. EST frequencies during the early stages of RYMV infection indicated that changes in the expression of genes involved in energy metabolism and photosynthesis are differentially accentuated in susceptible and partially resistant cultivars. Mapping of these ESTs revealed that several co-localize with previously described resistance gene analogs and QTLs (quantitative trait loci).     

Molecular and biochemical analyses of OsRab7, a rice Rab7 homolog

Rab7 is a small GTP-binding protein important in early to late endosome/lysosome vesicular transport in mammalian cells. We have isolated a Rab7 cDNA clone, OsRab7, from a cold-treated rice cDNA library by the subtraction screening method. The cDNA encodes a polypeptide of 206 amino acids with a calculated molecular mass of about 23 kDa. Its predicted amino acid sequence shows significantly high identity with the sequences of other Rab7 proteins. His-tagged OsRab7 bound to radiolabeled GTPgammaS in a specific and stoichiometric manner. Biochemical and structural properties of the Rab7 wild type (WT) protein were compared to those of Q67L and T22N mutants. The detergent 3-([3-cholamidopropyl]dimethylammonio)-1-propane sulfonate (CHAPS) increased the guanine nucleotide binding and hydrolysis activities of Rab7WT. The OsRab7Q67L mutant showed much lower GTPase activity compared to the WT protein untreated with CHAPS, and the T22N mutant showed no GTP binding activity at all. The OsRab7Q67L mutant was constitutively active for guanine nucleotide binding while the T22N mutant (dominant negative) showed no guanine nucleotide binding activity. When bound to GTP, the Rab7WT and the Q67L mutants were protected from tryptic proteolysis. The cleavage pattern of the Rab7T22N mutant, however, was not affected by GTP addition. Northern and Western blot analyses suggested that OsRab7 is distributed in various tissues of rice. Furthermore, expression of a rice Rab7 gene was differentially regulated by various environmental stimuli such as cold, NaCl, dehydration, and ABA. In addition, subcellular localization of OsRab7 was investigated in the Arabidopsis protoplasts by a double-labeling experiment using GFP-fused OsRab7 and FM4-64. GFP-OsRab7 is localized to the vacuolar membrane, suggesting that OsRab7 is implicated in a vesicular transport to the vacuole in plant cells.     

Expression of Rab small GTPases in epithelial Caco-2 cells: Rab21 is an apically located GTP-binding protein in polarised intestinal epithelial cells

Rab proteins belong to a subfamily of small GTP-binding protein genes of the Ras superfamily and play an important role in intracellular vesicular targeting. The presence of members of this protein family was examined in Caco-2 cells by a PCR-based strategy. Twenty-five different partial cDNA sequences were isolated, including 18 Rab protein family members. Seven novel human sequences, representing Rab2B, Rab6A', Rab6B, Rab10, Rab19B, Rab21 and Rab22A, were identified. For one clone, encoding Rab21, full-length cDNA was isolated from a Caco-2 cDNA library. Northern blot analysis showed a ubiquitous expression pattern of Rab21. To study Rab21 protein expression in Caco-2 cells, polyclonal antibodies were raised against GST-Rab21 fusion protein and characterised. The antibodies recognised Rab21 as a protein of approximately 25 kDa. Interestingly, the protein shows a general ER-like staining in nonpolarised Caco-2 cells in contrast to an apically located vesicle-like staining in polarised Caco-2 cells. Furthermore, immunohistochemical staining on human jejunal tissue showed a predominant expression of Rab21 in the epithelial cell layer with high expression levels in the apical region, whereas stem cells in the crypts were negative. We therefore suggest an alternative role for Rab21 in the regulation of vesicular transport in polarised intestinal epithelial cells.     

Molecular characterization of an Arabidopsis thaliana cDNA encoding a small GTP-binding protein, Rha1.

We have isolated a cDNA encoding a small GTP-binding protein from an Arabidopsis thaliana cDNA library using an oligonucleotide probe derived from the most conserved domain of the ras superfamily. The cDNA encodes a 21.8 kDa protein, designated Rha1, which shows high homology to members of the ras superfamily in the regions involved in GTP binding, GTPase activity, and membrane attachment. The amino acid sequence is 60% identical to the sequence of the mammalian Rab5 protein, a small GTP-binding protein which is believed to be involved in endocytosis. Several regions, including the putative effector domain are completely conserved. This high percentage of amino acid identity suggests that the Rha1 protein is the functional plant counterpart of the Rab5 protein. When expressed in E. coli, the Rha1 protein was shown to bind GTP. The rha1 gene is most highly expressed in root and callus tissue, weakly expressed in stems and inflorescences and virtually not expressed in leaves and seed pods. Genomic Southern analysis revealed that rha 1 is part of a small multigene family.     

Cloning of cDNA for UDP-glucose pyrophosphorylase and the expression of mRNA in rice endosperm

Rice endosperm UDP-glucose pyrophosphorylase (UGPase) cDNA clones were isolated by screening a lambda ZAP II library prepared from poly (A(+)) RNA of japonica rice (cv Sasanishiki) endosperm with a probe of potato UGPase cDNA. One cDNA clone, possessing about 1,700 nucleotides, contained the complete open reading frame of rice UGPase. At the nucleotide-sequence level, the UGPase cDNA of rice endosperm had high homology with the UGPase cDNA of barley endosperm (84%) and potato tuber (71%). The calculated molecular weight (50 kDa) agrees with the value determined by SDS-PAGE (51 kDa). At the amino-acid sequence level, rice UGPase has high homology with the UGPase of barley (92%) and potato (85%). The enzyme contained conserved sequence elements which are thought to be involved in substrate binding and catalytic activity. A Southern-blot analysis indicated that the gene existed as a single copy. Expression of the enzyme in rice endosperm examined by Northern-blot analysis was high at 10-15 days after heading.     

A small GTP-binding protein from Arabidopsis thaliana functionally complements the yeast YPT6 null mutant.

A clone designated A.t.RAB6 encoding a small GTP-binding protein was isolated from a cDNA library of Arabidopsis thaliana leaf tissue. The predicted amino acid sequence was highly homologous to the mammalian and yeast counterparts, H.Rab6 and Ryh1/Ypt6, respectively. Lesser homology was found between the predicted Arabidopsis protein sequence and two small GTP-binding proteins isolated from plant species (44% homology to Zea mays Ypt1 and 43% homology to Nicotiana tabacum Rab5). Conserved stretches in the deduced amino acid sequence of A.t.Rab6 include four regions involved in GTP-binding, an effector region, and C-terminal cysteine residues required for prenylation and subsequent membrane attachment. Northern blot analysis demonstrated that A.t.Rab6 mRNA was expressed in root, leaf, stem, and flower tissues from A. thaliana with the highest levels present in roots. Escherichia coli produced histidine-tagged A.t.Rab6 protein-bound GTP, whereas a mutation in one of the guanine nucleotide-binding sites (asparagine122 to isoleucine) rendered it incapable of binding GTP. Functionally, the A.t.RAB6 gene was able to complement the temperature-sensitive phenotype of the YPT6 null mutant in yeast. The isolation of this gene will aid in the dissection of the machinery involved in soluble protein sorting at the trans-Golgi network of plants.     

G蛋白Rab3a cDNA的克隆与表达

利用PCR法 ,从人胎盘总cDNA中扩增得到Rab3acDNA的全编码区 .序列分析表明 ,扩增得到的Rab3acDNA有 5个核苷酸发生了变异 ,但翻译的氨基酸与发表的完全一致 .将扩增得到的Rab3acDNA克隆于原核融合表达载体pGEX 4T 1中 ,在E .coliBL2 1中经IPTG诱导表达 .为了进一步鉴定表达产物 ,对纯化后的Rab3a蛋白进行了SDS PAGE、N端氨基酸测序、质谱分子量测定及氨基酸组成分析鉴定 .结果显示 ,表达蛋白的分子量约 2 5kD ,N端氨基酸序列为MASATDSR ,氨基酸组成分析表明 ,Rab3a蛋白获得了正确表达     

Rabconnectin-3, a novel protein that binds both GDP/GTP exchange protein and GTPase-activating protein for Rab3 small G protein family.

Rab3A, a member of the Rab3 small G protein family, regulates Ca(2+)-dependent exocytosis of neurotransmitter. The cyclical activation and inactivation of Rab3A are essential for the Rab3A action in exocytosis. GDP-Rab3A is activated to GTP-Rab3A by Rab3 GDP/GTP exchange protein (Rab3 GEP), and GTP-Rab3A is inactivated to GDP-Rab3A by Rab3 GTPase-activating protein (Rab3 GAP). It remains unknown how or in which step of the multiple exocytosis steps these regulators are activated and inactivated. We isolated here a novel protein that was co-immunoprecipitated with Rab3 GEP and GAP by their respective antibodies from the crude synaptic vesicle fraction of rat brain. The protein, named rabconnectin-3, bound both Rab3 GEP and GAP. The cDNA of rabconnectin-3 was cloned from a human cDNA library and its primary structure was determined. Human rabconnectin-3 consisted of 3,036 amino acids and showed a calculated M(r) of 339,753. It had 12 WD domains. Tissue and subcellular distribution analyses in rat indicated that rabconnectin-3 was abundantly expressed in the brain where it was enriched in the synaptic vesicle fraction. Immunofluorescence and immunoelectron microscopy revealed that rabconnectin-3 was concentrated on synaptic vesicles at synapses. These results indicate that rabconnectin-3 serves as a scaffold molecule for both Rab3 GEP and GAP on synaptic vesicles.