Complete mtDNA of Meretrix lusoria (Bivalvia: Veneridae) reveals the presence of an atp8 gene, length variation and heteroplasmy in the control region

The complete nucleotide sequence of the mitochondrial genome of the clam Meretrix lusoria (Bivalvia: Veneridae) was determined. It comprises 20,268 base pairs (bp) and contains 13 protein-coding genes, including ATPase subunit 8 (atp8), two ribosomal RNAs, 22 transfer RNAs, and a non-coding control region. The atp8 encodes a protein of 39 amino acids. All genes are encoded on the same strand. A putative control region (CR or D-loop) was identified in the major non-coding region (NCR) between the tRNA^Gly and tRNA^Gln. A 1087 bp tandem repeat fragment was identified that comprises nearly 11 copies of a 101 bp motif and accounts for approximately 41% of the NCR. The 101 bp tandem repeat motif of the NCR can be folded into a stem–loop secondary structure. Samples of eight individuals from Hainan and Fujian provinces were collected and their NCR regions were successfully amplified and sequenced. The data revealed a highly polymorphic VNTR (variable number of tandem repeats) associated with high levels of heteroplasmy in the D-loop region. The size of the CR ranged from 1942 to 3354 bp depending upon the copy number of the repeat sequence.     

Cloning,characterization and expression of a cDNA encoding a granulin-like polypeptide in Ciona savignyi

Previous study in our laboratory confirmed that a novel polypeptide, CS5931 derived from Ciona savignyi possesses potent antitumor activity. In the present study, the full length cDNA of CS5931 precursor, termed Cs-pgrn-1 was cloned. The complete cDNA sequence of this gene consists of 685 bp containing an open reading frame (ORF) of 522 bp (173 amino acid residues). In silico analysis revealed that the polypeptide consists of two identical domains, similar with granulin (GRN) found in other species, and each of the domain encodes a polypeptide identical with CS5931. Phylogenetic analysis confirmed that CS5931 shares high homology with Ciona intestinalis GRN and is conserved during evolution. The polypeptide also shows high similarity with human GRN A, B, and C. Prediction of 3D protein structure revealed the 3D structure of CS5931 is very similar with human GRN A. The CS5931 was expressed using a prokaryotic expression system and the purified polypeptide inhibited the growth of several tumor cell lines in vitro via apoptotic pathway. Our study revealed that CS5931 has the potential to be developed as a novel antitumor agent.     

Molecular cloning and functional expression of a fibrinolytic protease gene from the polychaeta, Periserrula leucophryna

Full-length cDNA encoding a fibrinolytic protease (PLFP) from the cDNA library of the polychaete, Periserrula leucophryna was cloned, sequenced and expressed in Escherichia coli. The entire cDNA of the PLFP clone was 921 bp (CDS: 41-837), including a coding nucleotide sequence of 798 bp, a 5′-untranslaed region of 40 bp, and a 3′-noncoding region of 83 bp. The ORF encoded a 265-amino acid polypeptide precursor consisting of a 36-residue signal sequence and a 229-residue mature polypeptide. The sequence alignment results of PLFP revealed sequence similarity with several fibrinolytic enzymes. Sequence analysis revealed a conserved catalytic triad of His78, Asp126 and Ser219 residues, suggesting that PLFP is a serine protease. Mature PLFP had an apparent molecular weight of approximately 25 kDa and was produced in inclusion bodies when expressed in E. coli. Substrate specificity results that recombinant PLFP was active towards Arg-X or Lys-X and did not hydrolyze substrates with nonpolar amino acids at the P1 site. Recombinant PLFP was strongly inhibited by typical serine protease inhibitors, further indicating that PLFP is a member of the serine protease family. PLFP was able to dissolve artificial plasminogenfree fibrin, and its fibrinolytic behavior was similar to that of plasmin. Taken these results together, PLFP is a new member of the fibrinolytic enzyme family with selective specificity on fibrin, and the availability of PLFP offers an attractive alternative approach for thrombolysis therapy because rPLFP is believed to have advantages over currently used plasminogen activators, that is, lower price and lower side effect.     

Molecular cloning, characterization and expression analysis of cathepsin A gene in Chinese mitten crab, Eriocheir sinensis

Cathepsins, a superfamily of hydrolytic enzymes produced and enclosed within lysosomes, function in immune response in vertebrates; however, their function within the innate immune system of invertebrates remains largely unknown. Therefore, we investigated the immune functionality of cathepsin A (catA) in Chinese mitten crab (Eriocheir sinensis), a commercially important and disease vulnerable aquaculture species. The full length catA cDNA (2200 bp) was cloned via PCR based upon an initial expressed sequence tag (EST) isolated from a hepatopancreatic cDNA library. The catA cDNA contained a 1398 bp open reading frame (ORF) that encoded a putative 465 amino acid (aa) protein. Comparisons with other reported vertebrate cathepsins sequences revealed percent identity range from 48 to 51%. CatA mRNA expression in E. sinensis was (a) tissue-specific, with the highest expression observed in gill and (b) responsive in hemocytes to a Vibrio anguillarum challenge, with peak exposure observed 12 h post-injection. Collectively, data demonstrate the successful isolation of catA from the Chinese mitten crab, and its involvement in the innate immune system of an invertebrate.     

Molecular and expression characterization of a nanos1 homologue in Chinese sturgeon, Acipenser sinensis

The nanos gene family was essential for germ line development in diverse organisms. In the present study, the full-length cDNA of a nanos1 homologue in A. sinensis, Asnanos1, was isolated and characterized. The cDNA sequence of Asnanos1 was 1489 base pairs (bp) in length and encoded a peptide of 228 amino acid residues. Multiple sequence alignment showed that the zinc-finger motifs of Nanos1 were highly conserved in vertebrates. By RT-PCR analysis, Asnanos1 mRNAs were ubiquitously detected in all tissues examined except for the fat, including liver, spleen, heart, ovary, kidney, muscle, intestines, pituitary, hypothalamus, telencephalon, midbrain, cerebellum, and medulla oblongata. Moreover, a specific polyclonal antibody was prepared from the in vitro expressed partial AsNanos1 protein. Western blot analysis revealed that the tissue expression pattern of AsNanos1 was not completely coincided with that of its mRNAs, which was not found in fat, muscle and intestines. Additionally, by immunofluoresence localization, it was observed that AsNanos1 protein was in the cytoplasm of primary oocytes and spermatocytes. The presented results indicated that the expression pattern of Asnanos1 was differential conservation and divergence among diverse species.     

巴西橡胶树HbHEV3基因的克隆和表达分析

根据EST序列信息,通过RT-PCR获得了一个编码橡胶素前体的基因,命名为HbHEV3。HbHEV3编码区cDNA长度为630bp,编码209个氨基酸。预测的HbHEV3蛋白包含1个信号肽,1个具有几丁质结合特性的Hevein结构域和1个Barwinn结构域,HbHEV3与橡胶树及其他植物中类似蛋白具有很高的同源性。分离获得了HbHEV3起始密码子上游1 050bp的启动子序列,该序列含有众多应答激素和胁迫信号元件。实时荧光定量PCR分析结果表明,HbHEV3在所检测的组织中均有表达,其中在胶乳中的表达量最高,乙烯诱导能显著上调胶乳中HbHEV3的表达。研究表明,HbHEV3可能参与了橡胶树乙烯介导的防御反应,并在橡胶凝集过程中具有重要功能。     

沙田柚无机焦磷酸酶基因的cDNA克隆及序列分析

植物自交不亲和性是植物生殖过程中普遍存在的一种现象,是植物特异性识别并拒绝自身花粉或亲缘关系很相近的花粉的一种遗传机制。无机焦磷酸酶(inorganic pyrophosphatase,IPPase)在植物生长发育方面起重要作用。该研究根据沙田柚花柱消减文库中EST序列(无机焦磷酸酶基因内部片段),设计了2对特异引物5'-GSP1,5'-n GSP1,3'-GSP2 and 3'-n GSP2,通过SMART-RACE PCR技术从所构建的沙田柚花柱抑制性消减文库中克隆了沙田柚无机焦磷酸酶基因的c DNA全长序列,利用Blastn、DNAman和Expasy软件对所克隆的基因进行同源性分析,以及基因编码的氨基酸的分子量、等电点、疏水性等理化性质分析。结果表明:IPPase基因c DNA全长为1 136 bp(Gen Bank登录号为KF990474),开放阅读框(ORF)全长为654 bp,共编码217个氨基酸,包括170 bp 5'UTR和312 bp的3'UTR;编码的蛋白质的分子量为24.4 k Da,等电点为5.96;蛋白结构域分析显示沙田柚IPPase与焦磷酸酶具有相同的保守结构域;对沙田柚IPPase蛋白质序列进行疏水性分析,结果表明沙田柚IPPase基因编码的肽链中疏水性最大值约为3.21,最小值约为-2.98,属于亲水性蛋白,无跨膜区域;Blastn搜索的结果显示,沙田柚IPPase基因序列与多种植物的IPP基因高度同源;序列分析表明,沙田柚IPPase基因核苷酸的同源性与毛果杨(Populus trichocarpa)和橡胶树(Hevea brasiliensis)IPPase基因均为87%;氨基酸序列与克莱门柚(Citrus clementina)无机焦磷酸酶完全一致。该研究结果可为深入研究无机焦磷酸酶在沙田柚自交不亲和中的作用机理提供基础。     

奥利亚罗非鱼髓样分化因子(MyD88)的克隆及其在组织中的表达

髓样分化因子（myeloid differentiation factor 88,MyD88）是TLR（toll-like receptor）信号通路的关键接头蛋白,在先天性免疫中具有重要作用。通过RACE-RCR技术克隆了奥利亚罗非鱼（Oreochromis aureus）MyD88基因cDNA全长序列（GenBank登录号：JN032017）。序列分析表明,奥利亚罗非鱼MyD88 基因全长为1 611 bp,其中包括155 bp的5’非编码区,589 bp的3’非编码区和867 bp的编码区,编码288个氨基酸残基。MyD88蛋白N端具有死亡结构域,C端具有TIR结构域。同源性分析表明,奥利亚罗非鱼MyD88氨基酸序列与鳜鱼（Siniperca chuats）相似性最高,为85.8%,与其他鱼类相似性为70%~82%,与哺乳动物相似性为63%~66%;系统进化树分析表明,奥利亚罗非鱼MyD88与同属鲈形目的鳜鱼、大黄鱼（Larimichthys crocea）聚在一起。采用实时定量PCR方法检测MyD88在奥利亚罗非鱼各组织中的表达情况。结果显示,MyD88在所有被测组织中都有表达,其中表达量最高的是卵巢,其次在小肠、脾、肝、肾、鳃和血液中有较高的表达量,肌肉、精巢组织中表达量最低。本研究可为进一步探讨MyD88在奥利亚罗非鱼TLR信号通路中的作用奠定一定的基础。