Molecular cloning and functional characterization of a RabGTPase in large yellow croaker (Pseudosciaena crocea)

The molecular mechanisms of the immune system against pathogens in large yellow croaker (Pseudosciaena crocea) are not well known, despite its economic importance as an aquaculture species. In this investigation, a Rab gene (named as LycRab gene) was obtained from this fish, which exhibited high homology with Rab8 of other species. It was expressed in Escherichia coli, and the specific antibody was raised using the purified fusion protein (GST-LycRab). The LycRab protein, containing characteristic signatures of Rab proteins with 5 GTP-binding domains, had GTP-binding activity. The LycRab gene was ubiquitously expressed in all analyzed tissues as revealed by Western blot, although expression levels varied from tissue to tissue. Real-time PCR revealed that the LycRab gene was up-regulated after immunization with poly I:C, formalin-inactive Gram-negative bacterium Vibrio parahaemolyticus or bacterial lipopolysaccharides (LPS), suggesting that LycRab protein might play an important role in large yellow croaker defense against pathogens infection. This discovery might contribute better understanding to the molecular events involved in fish immune responses.     

大黄鱼TRIM25基因克隆和表达分析

三重基序蛋白25 (Tripartite motif-containing protein 25, TRIM25)属于E3泛素连接酶家族, 在先天免疫反应中发挥重要作用。为研究TRIM25基因在大黄鱼(Larimichthys crocea)先天抗病毒免疫反应中的作用, 研究鉴定并克隆大黄鱼TRIM25基因(命名为LcTRIM25)。LcTRIM25基因编码序列2097 bp (GenBank登录号: MK327541), 编码698个氨基酸。蛋白结构域预测发现LcTRIM25包括保守的RING结构域、B-box2结构域、Coiled-coil结构域和可变的C末端PRY/SPRY结构域。多序列比对以及系统进化树分析表明LcTRIM25基因与斜带石斑鱼同源性高, 与哺乳动物、爬行动物、两栖动物和鸟类同源性相对低, 这说明不同物种受到来自环境不同的选择压力, 导致进化程度不同。应用实时荧光定量PCR方法分析大黄鱼TRIM25基因的表达水平。结果分析发现LcTRIM25基因在健康大黄鱼的9个组织中均有广泛表达, 且在肝脏中表达量最高, 在心脏中表达量最低。在poly(I:C)刺激后, 在外周血、头肾、脾脏和肝脏中LcTRIM25基因表达量迅速且明显上调, 均出现上升达到峰值后下降的趋势。LcTRIM25基因表达量在头肾和脾脏中6h达到最高表达量, 在肝脏中12h达到峰值, 外周血中在24h达到最高表达量。上述结果表明, 不同组织中LcTRIM25基因表达模式具有差异性。研究结果推测大黄鱼TRIM25基因参与抗病毒免疫反应且发挥十分关键的作用, 为进一步了解大黄鱼抗病毒免疫机制提供理论基础。     

哈维氏弧菌胞外蛋白酶基因的克隆表达及免疫原性

根据实验室分离的大黄鱼弧菌病主要病原菌哈维氏弧菌(Vib rio harveyi)GYC1108-1株的胞外蛋白酶基因序列,设计胞外蛋白酶基因(ΔProA)特异性引物,扩增获得1552bp的ΔProA基因,克隆于pUC57-T载体;将ΔProA基因亚克隆到原核表达载体pET-28a进行融合表达,SDS-PAGE电泳检测发现,ΔProA融合蛋白经IPTG诱导后在大肠杆菌中以包涵体形式表达,分子量大小约55kD,诱导5h的表达蛋白产量约占细菌总蛋白的21%。Western blot分析,表达的55kD蛋白具有较高免疫原性。用纯化的ΔProA融合蛋白对大黄鱼进行免疫试验,结果免疫保护率达到75%。       

Molecular characterization and expression analysis of interferon- inducible protein 56 gene in large yellow croaker Pseudosciaena crocea

In mammals, interferon-inducible protein 56 (IFI56) has been considered to play a role in mediating inhibition of viral replication and cell growth, and possibly in mediating cell apoptosis. Here, we reported the cloning of an IFI56 homologue from the spleen of large yellow croaker, a marine fish (LycIFI56). The complete cDNA of LycIFI56 gene is 1628 nucleotides (nt) encoding a protein of 437 amino acids (aa), with a putative molecular weight of 50.8 kDa. The deduced LycIFI56 protein has a high-level homology with all members of IFIT (IFN-inducible proteins with TPR domain) family, and its 9 putative TPR motifs all locate the corresponding position of these IFIT proteins. Phylogenetic analysis showed that five fish IFIT members form a unique clad independent of mammalian homologues, reflecting a distant evolutionary relationship from mammals. LycIFI56 gene was constitutively expressed in various tissues examined, such as gills, intestine, liver, kidney, heart, spleen, muscle and blood. Upon induction with poly(I:C), LycIFI56 gene expression is obviously up-regulated in spleen, gills, intestine, liver and kidney at 24 h post-induction, suggesting that LycIFI56 may be involved in the immune response induced by poly(I:C). Analysis of the expression kinetics of LycIFI56 and IRF1 genes revealed that the up-regulation of LycIRF-1 expression by poly (I:C) was apparently earlier than that of LycIFI56. These results would facilitate a better understanding of the expression regulation of fish IFI56 gene, and of its roles in immunity of bony fish.     

大黄鱼ATG10基因的分子特征及其在抗病毒免疫中的功能

为了研究自噬相关基因ATG10(Autophagy related gene 10)在鱼类免疫应答中的功能, 研究克隆了大黄鱼(Larimichthys crocea)ATG10基因(LcATG10)的cDNA序列, 其开放阅读框全长747个核苷酸, 编码248个氨基酸的蛋白, 包含1个Autophagy_act_C结构域。系统进化分析显示, LcATG10和其他硬骨鱼类ATG10聚成一支, 与金头鲷和石斑鱼ATG10亲缘关系最近。LcATG10在所检测的正常大黄鱼各组织中都有表达。在病毒类似物poly (I:C)刺激后, 大黄鱼脾脏和头肾组织中LcATG10的表达水平显著上调, 分别在12h和6h达到峰值(9.4和5.9倍)。LcATG10在大黄鱼头肾细胞系(LYCK)、原代巨噬细胞、淋巴细胞和粒细胞中也均有表达, 在原代粒细胞中的表达量相对较高; 在poly (I:C)刺激后, 大黄鱼原代头肾粒细胞和LYCK细胞中LcATG10的表达水平显著上调。过表达LcATG10的鲤上皮瘤(Epithelioma papulosum cyprinid, EPC)细胞受鲤春病毒血症病毒(Spring viremia of carp virus, SVCV)感染48h后, 细胞病变效应(Cytopathic effects, CPEs)明显低于对照组; 细胞培养上清中SVCV病毒滴度为103.55 TCID₅₀/mL, 显著少于对照组; SVCV标志基因SVCV- G、SVCV-M和SVCV- P的表达水平也显著低于对照组, 分别是对照组的0.022、0.015和0.022倍。这些研究结果表明LcATG10在大黄鱼抗病毒免疫应答中发挥作用, 为深入研究自噬在大黄鱼抗病毒免疫中的分子机制奠定了基础。     

Molecular characterization and bioactivity of a CXCL13 chemokine in large yellow croaker Pseudosciaena crocea

A CXCL13-like chemokine cDNA was isolated from large yellow croaker (Pseudosciaena crocea) by expressed sequence tag (EST) analysis (LycCXCL13). The full-length cDNA of LycCXCL13 is 796 nucleotides (nt) encoding a protein of 97 amino acids (aa), with a putative molecular weight of 10.7 kDa. The deduced LycCXCL13 contains a 24-aa signal peptide and a 73-aa mature polypeptide, which possesses the typical arrangement of four cysteines as found in other known CXC chemokines (C²⁵, C²⁷, C⁵² and C⁶⁸). It shares 35, 36 and 39% aa sequence identities to green puffer CXCL13-like, Atlantic salmon CXCL13 and Japanese flounder CXCL13 chemokines, and 24–29% identities to CXCL13 chemokines in mammals, respectively. Phylogenetic analysis showed that LycCXCL13 is more closely related to the CXCL13 subgroup than to any other CXC chemokine subgroups. LycCXCL13 gene was constitutively expressed in all tissues examined, except for intestine. Upon induction with poly(I:C) or inactivated trivalent bacterial vaccine, LycCXCL13 gene expression was significantly up-regulated in spleen, head kidney, heart and gills at 24 h post-injection. Real-time PCR results showed that LycCXCL13 gene expression reached peak level in spleen and head kidney at 12 h after induction by poly(I:C), while its expression increased to the highest level in head kidney at 24 h or in spleen at 48 h by bacterial vaccine. Recombinant LycCXCL13 protein produced in E. coli BL21 exhibited obvious chemotaxis to the peripheral blood leucocytes (PBLs) from large yellow croaker. These results suggest that LycCXCL13 may be involved in inflammatory responses as well as homeostatic processes in large yellow croaker.     

大黄鱼HIF-1α基因的克隆鉴定与表达分析

为研究低氧诱导因子1α(Hypoxia-inducible factor-1α, HIF-1α)在鱼类免疫应答中的作用, 研究克隆得到了大黄鱼(Larimichthys crocea)HIF-1α基因(LcHIF-1α)的cDNA序列, 其开放阅读框全长2256个核苷酸, 编码一个751个氨基酸的蛋白。通过氨基酸序列比对发现, LcHIF-1α蛋白具有5个典型的功能结构域, 包括1个helix-loop-helix(HLH)结构域, 2个PAS结构域, 1个DNA结合结构域(HIF-1)和1个羧基端反式激活结构域(HIF-1a_CTAD)。系统进化分析显示, LcHIF-1α和其他硬骨鱼类HIF-1α聚成一支, 与两栖类、鸟类和哺乳类HIF-1α的亲缘关系相对较远。序列分析结果表明, LcHIF-1α具有保守的特征结构域, 预示着其功能可能与哺乳动物HIF-1α类似。荧光定量PCR结果显示, LcHIF-1α在所检测的健康大黄鱼各个组织中都有表达, 在溶藻弧菌(Vibrio alginolyticus)感染后, 大黄鱼脾脏和头肾组织中的LcHIF-1α表达水平显著上调, 达到峰值时分别上升了6.8倍和2.9倍。此外, LcHIF-1α在大黄鱼的3种免疫细胞(中性粒细胞、巨噬细胞和淋巴细胞)中也都有表达, 在中性粒细胞和巨噬细胞中的表达量相对较高; 在脂多糖(LPS)诱导后, 中性粒细胞和巨噬细胞中LcHIF-1α的表达量显著增加, 峰值分别是对照组的2.6倍和1.8倍, 这些结果表明LcHIF-1α可能参与调控大黄鱼抗细菌免疫应答。     

大黄鱼虹彩病毒腺苷三磷酸酶(ATPase)基因的克隆与表达

虹彩病毒(iridovirus)是一类对鱼类、两栖类和爬行类水生动物具有广泛感染性的致病病原,由虹彩病毒所致疾病给世界水产养殖业造成了巨大的经济损失.近年来,许多国家相继报道了在患病鱼、蛙和龟等水生经济动物中分离到虹彩病毒[1-4].     

Cloning and molecular characterization of lycC1INH genes in large yellow croaker (Pseudosciaena crocea)

Complement component 1 inhibitor (C1INH) is a crucial protein in controlling activation of many plasma mediator pathways and can directly interact with Gram negative bacteria. The full-length cDNA of lycC1INH gene was identified from the large yellow croaker. It is of 2046 nucleotides (nt) encoding a protein of 599 amino acids, with a 5′-untranslated region of 99 nt and a 3′-untranslated region of 147 nt including the poly (A) tail. The deduced protein contains a C-terminal serpin (serine protease inhibitor) domain, and two N-terminus immunoglobulin domains without significant homology to other species. Western blot analysis of the protein expression showed that the expression of lycC1INH was obviously up-regulated in liver, spleen and head kidney of the fish challenged by attenuated live Vibrio anguillarum strain. This indicated that lycC1INH might be involved in the immune response of large yellow croaker to bacterial challenge.     

Characterization and SNP variation analysis of a HSP70 gene from miiuy croaker and its expression as related to bacterial challenge and heat shock

Heat shock proteins (HSPs) play crucial roles in the immune response of vertebrates. In order to study immune defense mechanism of heat shock protein gene in miiuy croaker (Miichthys miiuy), a cDNA encoding heat shock protein 70 (designated Mimi-HSP70) gene was cloned from miiuy croaker. The cDNA was 2195?bp in length, consisting of an open reading frame (ORF) of 1917?bp encoding a polypeptide of 638 amino acids with estimated molecular mass of 70.3?kDa and theoretical isoelectric point of 5.55. Genomic DNA structure analysis revealed that the Mimi-HSP70 gene contain no introns in coding region and four SNPs with 373?C/T, 789?G/A, 1005?C/T, and 1185?G/A were detected by direct sequencing of 20 samples from six different populations. BLAST analysis, structure comparison and phylogenetic analysis indicated that Mimi-HSP70 should be an inducible cytosolic member of the HSP70 family. The deduced amino acid sequence of Mimi-HSP70 had 82.4%-92.2% identity with those of vertebrate. A real-time quantitative RT-PCR demonstrated that the HSP70 gene was ubiquitously expressed in ten normal tissues. Under different temperature shock stress, the expression of Mimi-HSP70 gene in miiuy croaker increased at first and then decreased with the rise of temperature, finally, reached a maximum level in liver, spleen and kidney tissues. Infection of miiuy croaker with Vibrio anguillarum resulted in significant changes expression of Mimi-HSP70 gene in the immune-related tissues. These results indicated that expression analysis of Mimi-HSP70 gene provide theoretical basis to further study the mechanism of anti-adverseness in the miiuy croaker.     

Characterization of OmpK, GAPDH and their fusion OmpK-GAPDH derived from Vibrio harveyi outer membrane proteins: their immunoprotective ability against vibriosis in large yellow croaker (Pseudosciaena crocea)

AIM: To investigate the immunoprotection of three recombinant proteins derived from the Vibrio harveyi outer membrane proteins (OMPs) OmpK, glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and their fusion OmpK-GAPDH as vaccine candidates from vibriosis of large yellow croaker (Pseudosciaena crocea). METHODS: The ompK gene, of which the leader sequence was omitted, was fused with the gapdh gene. Three recombinant proteins r-OmpK, r-GAPDH and r-OmpK-GAPDH were expressed and purified. Western blots were carried out to detect the specificity of the antibodies raised against the recombinant proteins; Fish were immunized with recombinant proteins and challenged by native V. harveyi. The immunoresponse to the recombinant proteins were determined by ELISA and phagocytic activity assay. CONCLUSIONS: The fusion protein r-OmpK-GAPDH can afford greater protection against the wild V. harveyi than r-OmpK or r-GAPDH alone or their mixture in humoral and cellular immunity, indicating that OmpK and GAPDH could produce a synergistic immunoprotection against vibriosis of large yellow croaker (Pseudosciaena crocea) when fused into OmpK-GAPDH with a linker. SIGNIFICANCE AND IMPACT OF THE STUDY: It has been realized that a multi-component OMP antigen can induce a higher frequency of immune effectors than a single OMP. The results presented here bring forth a good suggestion for the subunit vaccine design based on the OMPs of gram-negative pathogens.     

Molecular cloning and structural analysis of a novel Rac gene osRACB in rice (Oryza sativa L.)

Rac is a subfamily of small GTP-binding protein family. Its molecular weight is between 20 and 30 kilodaltons. As a signal protein, Rac directly or indirectly participates in many physiological processes, such as the regulation of cytoskeleton and the transduction of stress-induced signal. So Rac is also named ?molecular switch? The switch is based on the cycle from a GTP-bound 憃n?to a GDP-bound 憃ff?state[1]. In the superfamily of GTP-binding protein, only heterotrimeric G protein, Ra…     

Genomic organization, single nucleotide polymorphism and functional characterization of natural killer enhancing factor (NKEF-A) in Miichthys miiuy

Peroxiredoxin (Prx) play vital parts in oxidative stress belonging to a cellular antioxidant protein family. Natural killer enhancing factor (NKEF) is a member of the Prx family, which is newly defined. In addition to antioxidant activity, NKEF also can protect DNA from oxidative damage. In order to study immune defense mechanism of NKEF in teleost, NKEF-A gene of miiuy croaker (Miichthys miiuy) was cloned and characterized. The genomic organization containing one non-coding exon, five coding exons and five introns, inclouding one intron located in 5′-terminal untranslated region. The full-length cDNA was 1235 bp, consisting of a 597 bp open reading frame coding for a protein of 198 amino acids. Sequence comparison showed that the deduced amino acid sequence of miiuy croaker NKEF-A had 71.4–90.3 % identity with those of mammal and teleost. Five single nucleotide polymorphisms were detected by direct sequencing of eight samples from three different populations. Phylogenetic analysis revealed that miiuy croaker NKEF-A forms a cluster with other known teleost and mammalian NKEF-As. NKEF-A gene was constitutively expressed in ten examined tissues, and expression level was up-regulated in liver, spleen and kidney after challenge with Vibrio anguillarum. Finally, the NKEF-A was constructed and expressed in Escherichia coli. Then purified recombinant pET-NKEF protein was used to produce the polyclonal antibody and the polyclonal antibody against NKEF-A was tested by Western blot analysis. These results indicate that NKEF may be involved in immune responses as well as homeostatic processes in miiuy croaker.     

Defective chemokine-directed lymphocyte migration and development in the absence of Rho guanosine diphosphate-dissociation inhibitors alpha and beta

Rho family small GTP-binding proteins, including Rho, Rac, and Cdc42, are key determinants of cell movement and actin-dependent cytoskeletal morphogenesis. Rho GDP-dissociation inhibitor (GDI) alpha and Rho GDIbeta (or D4/Ly-GDI), closely related regulators for Rho proteins, are both expressed in hemopoietic cell lineages. Nevertheless, the functional contributions of Rho GDIs remain poorly understood in vivo. In this study, we report that combined disruption of both the Rho GDIalpha and Rho GDIbeta genes in mice resulted in reduction of marginal zone B cells in the spleen, retention of mature T cells in the thymic medulla, and a marked increase in eosinophil numbers. Furthermore, these mice showed lower CD3 expression and impaired CD3-mediated proliferation of T cells. While B cells showed slightly enhanced chemotactic migration in response to CXCL12, peripheral T cells showed markedly reduced chemotactic migration in response to CCL21 and CCL19 associated with decreased receptor levels of CCR7. Overall, Rho protein levels were reduced in the bone marrow, spleen, and thymus but sustained activation of the residual part of RhoA, Rac1, and Cdc42 was detected mainly in the bone marrow and spleen. Rho GDIalpha and Rho GDIbeta thus play synergistic roles in lymphocyte migration and development by modulating activation cycle of the Rho proteins in a lymphoid organ-specific manner.