斜带石斑鱼L-氨基酸氧化酶基因克隆及表达分析

鱼类的L-氨基酸氧化酶(L-amino acid oxidase, LAAO)具有广泛的抑菌杀虫效果, 为了解斜带石斑鱼(Epinephelus coioides)LAAO基因序列特征及其在刺激隐核虫(Cryptocaryon irritans)感染后的表达变化, 该试验克隆得到2个石斑鱼LAAO基因: EcLAAO-1和EcLAAO-2, 它们的ORF长度分别为1536和1569 bp, 编码511和522个氨基酸, 均含有氨基酸氧化酶(Amino_oxidase)结构域以及LAAO保守序列: DBM和GG motif。多重序列比对显示石斑鱼LAAO与其他鱼类LAAO具有较高的相似性。系统进化树分析表明, 斜带石斑鱼的LAAO与硬骨鱼类亲缘关系较近。实时荧光定量PCR检测结果显示EcLAAO-1和EcLAAO-2在石斑鱼各组织均有表达, 其中皮肤、鳃、胸腺、肝脏和肌肉中含量较丰富; 在感染刺激隐核虫后, 鳃和脾脏EcLAAO-1, EcLAAO-2表达量显著升高(P<0.05), 这些结果暗示了石斑鱼LAAO参与先天性免疫, 并在抗御刺激隐核虫感染中发挥重要作用。     

赤眼鳟Mx1基因的cDNA克隆及表达特性

为探究赤眼鳟(Squaliobarbus curriculus)是否存在Mx1 (Myxovirus resistance)基因及参与抗病毒免疫反应, 研究利用RACE技术获得了赤眼鳟Mx1基因(ScMx1)的cDNA全长序列, 并对其进行了生物信息学分析; 采用荧光定量PCR技术, 检测了ScMx1在赤眼鳟健康组织中的表达情况以及感染GCRV后ScMx1和ScIFN-Ⅰ的表达特征。结果表明, ScMx1的cDNA全长为3000 bp, 包含5′非编码区124 bp, 开放阅读框1893 bp, 3′非编码区983 bp, 共编码630个氨基酸。预测的ScMx1蛋白包含GTP酶结合区域、中央核心结构域和GTP酶效应结构域。ScMx1与青鱼Mx1的相似性最高(97%), 与ScMx的相似性仅为50%。ScMx1在所检测的10种组织中均有表达, 其中在脾脏中表达量最高。经GCRV感染开始至168h, ScMx1和ScIFN-Ⅰ在肝脏和体肾中的表达量持续上调; 在脾脏和头肾中于感染后72h达到峰值。相关性分析显示脾脏中ScMx1和ScIFN-Ⅰ的表达水平呈显著相关(r=0.94, P=0.018)。研究发现赤眼鳟存在Mx1基因, 且可能参与了抗GCRV免疫应答反应。     

斜带石斑鱼MyD88基因的克隆与表达

本研究运用RACE-PCR技术获得斜带石斑鱼(Epinephelus coioides)髓样分化因子88 (myeloid differentiation factor 88,MyD88)基因,并对该基因进行生物信息学和表达模式分析.研究结果表明1 795 bp的cDNA全长序列,包括ORF 870 bp、5' UTR 243 bp和3' UTR 682 bp,3' UTR存在1个多聚腺苷酸加尾信号(AATAAA)和两个mRNA不稳定基序(ATTTA).SMART软件预测该蛋白N端和C端分别存在死亡结构域和TIR结构域(Toll/IL-1 receptor homology domain,TIR);与其它脊椎动物MyD88的序列同一性达57.1%～78.7%;用NJ法构建的系统进化树中,斜带石斑鱼MyD88和其它已报导的鱼类MyD88聚为一枝.qPCR检测结果显示MyD88基因mRNA主要表达于肝脏、脾脏、头肾和胸腺等组织.本研究为进一步探讨MyD88在斜带石斑鱼TLR信号传导中的作用奠定基础.     

牡丹开花相关基因PsAP1的克隆与表达

APETALA1基因对花器官的形成具有重要作用,并且能够调节花期.以牡丹品种赵粉(Paeoniasuffru-ticosaL.cv.Zhaofen)为试材,采用RT-PCR和RACE方法从花瓣中获得了1个牡丹APETALA1基因cDNA全长,命名为PsAP1,GenBank登录号为HM143943.其cDNA全长1103 bp,包含130 bp的5′非编码区、244 bp的3′非编码区和1个长度为729 bp编码242个氨基酸的开放阅读框.序列比对和系统进化分析表明,PsAP1与葡萄的亲缘关系最近,相似性达80%以上,属于MADS家族AP1/SQUA亚家族.相对荧光定量PCR分析表明,PsAP1在花瓣中的表达量最高,在雄蕊中表达量最低.     

人脑红蛋白(NGB)全长cDNA序列的克隆

人脑红蛋白(neuroglobin, NGB)是新发现的神经系统特异的携氧蛋白, 然而其全长cDNA序列一直未见报道. 采用电子序列延伸技术和cDNA序列末端快速扩增技术(rapid amplification of cDNA ends, RACE)研究发现, 人NGB全长cDNA序列为1 909 bp, 5′非编码区为375 bp, 编码区(456 bp)可编码151个氨基酸, 3′非编码区为1 078 bp, 其中含27 bp的poly(A)(GenBank接受号: AF422797). 综合采用电子序列延伸技术与RACE技术是获得全长cDNA序列的有效方法, 为后续的功能研究提供了重要基础.     

草鱼α1-抗胰蛋白酶基因cDNA全长克隆与表达分析

采用RACE技术获得α1-抗胰蛋白酶基因cDNA全长序列为1 469 bp,开放阅读框为1 329 bp,可编码442个氨基酸。5′非编码区长19 bp,3′非编码区长121 bp。核苷酸序列分析表明,在N端可能存在一个由1～21位氨基酸残基组成的信号肽;与斑马鱼的同源性最好,其次是虹鳟;在系统进化上,与在斑马鱼、虹鳟共聚为一个大支。用半定量RT-PCR分析正常及细菌诱导下草鱼α1-抗胰蛋白酶基因在不同组织中的表达分布。结果显示:正常情况下,草鱼α1-抗胰蛋白酶在肝脏表达最丰富,在脾脏、前肾、前肠、中肠、后肠和也有少量表达;细菌诱导下,肝脏中表达最强,前肾、脾脏、肠道中表达均明显提高,心脏和后肾中也出现较高表达。提示α1-抗胰蛋白酶可能参与了机体对嗜水气单胞菌感染的免疫应答。     

鳜鱼MDA5基因的克隆与组织表达分析

目的:克隆鳜鱼MDA5基因cDNA序列,研究聚肌苷酸胞苷酸[Poly(I∶C)]感染过程中MDA5的表达规律。方法:利用RT-PCR和RACE技术克隆鳜鱼MDA5全长序列,构建Poly(I∶C)感染模型,分析MDA5在鳜鱼脾脏和鳃组织中的表达规律。结果:鳜鱼MDA5 cDNA全长3556 bp,包括142 bp 5′UTR、438 bp 3′UTR和2976 bp开放读框,共编码991个氨基酸残基。MDA5蛋白具有RLR家族的典型特征,即N端含有2个CARD结构域,C端含有DEXDc、解旋酶和RD结构域,序列分析发现鳜鱼的MDA5与横斑石鲷、大黄鱼的同源性较高,分别达85.4%、79.8%。组织表达谱分析显示,鳜鱼MDA5基因在不同组织中普遍表达,用Poly(I∶C)抗原刺激后,MDA5 mRNA表达显著上调,其中脾脏组织在诱导8 h后达到峰值,而在鳃组织中表达持续显著上调。结论:MDA5在鳜鱼免疫应答中起重要作用。     

羊草OEE1基因的克隆及盐胁迫下的表达

从羊草(Leymus chinensis )叶片cDNA文库中克隆得到可能编码33 kD的光系统Ⅱ(PSⅡ)外周蛋白(oxygen-evolving enhancer protein1,OEE1)全长cDNA(GenBank登录号为EF583851),命名为LcOEE1.序列分析结果表明,该cDNA全长1 107 bp,5′非编码区为32 bp,3′非编码区为71 bp,编码区长987 bp,编码328个氨基酸.BALSTp比对发现,该基因氨基酸序列与已报道的小麦和水稻中的OEE1序列具有95%和94%的相似性.聚类分析表明,该基因与小麦和水稻的亲缘关系较近,与拟南芥和菠菜OEE1基因的亲缘关系较远.Northern杂交结果表明,在200 mmol/L的NaCl处理7 d的幼叶中,OEE1 mRNA的表达量明显高于未处理的对照,说明羊草中OEEl基因受盐诱导.     

普通烟草K^＋通道基因NKT4的克隆、序列和表达分析

通过比对拟南芥、胡萝卜、番茄和马铃薯的K+通道氨基酸序列得到了保守序列,设计1对简并引物,利用RT-PCR获得3条490bp的普通烟草K+通道基因中间片段.以其中一条中间片段设计特异性引物,应用RACE方法得到5′末端和3′末端cDNA序列.通过拼接并结合全长克隆及测序验证,获得一个未报道的普通烟草K+通道基因,并将其命名为NKT4(GenBank登录号为FJ233071).NKT4的cDNA全长为2937bp,其中5′非编码区45bp、编码区2679bp、3′非编码区213bp;编码区编码892个AA.构建了一个烟草、拟南芥及相关植物K+通道蛋白的系统进化树.基因表达分析表明,NKT4主要在烟草主根和侧根中表达,在烟草叶中也有少量表达.     

虾夷扇贝铜锌超氧化物歧化酶基因的克隆与转录表达特性分析

利用RACE和克隆等方法得到了虾夷扇贝铜锌超氧化物歧化酶(Cu/Zn-SOD)基因全长cDNA序列,该序列全长1 064 bp,5′和3′非编码区(UTR)分别为61 bp和541 bp,开放阅读框(ORF)462 bp,编码153个氨基酸和一个终止密码子.分析发现,此氨基酸序列含有形成二硫键的两个半胱氨酸残基以及4个铜结合位点、4个锌结合位点,与已知的Cu/Zn-SOD结构相似,与其它物种同源性较高.进行虾夷扇贝组织分布及发育过程中不同时期的实时荧光定量监测,发现鳃中Cu/Zn-SOD基因mRNA相对表达量最高,肾次之,血淋巴中最低;不同发育阶段Cu/Zn-SOD表达量变化明显,其中受精卵和早期D形幼体两个时期表达量相对较高.     

Orange-spotted grouper (Epinephelus coioides) toll-like receptor 22: molecular characterization, expression pattern and pertinent signaling pathways

The toll-like receptors (TLRs) are an important gene family in host innate immunologic surveillance. The TLR22 gene is an essential member of the TLRs that is only found in aquatic animals and has been detected in some bony fish. Here, a TLR22 homolog, EcTLR22, was characterized in the orange-spotted grouper (Epinephelus coioides) via homology cloning. The 3321 bp full-length cDNA sequence of EcTLR22 was obtained, which included an open reading frame of 2880 bp encoding a putative peptide of 960 amino acids containing three highly typical domains with the characteristics of TLR family members. The deduced amino acid sequence of EcTLR22 showed a relatively high similarity to flounder TLR22. Phylogenetic analysis showed that the orange-spotted grouper TLR22 sequence was clustered with those of Perciforme, such as flounder and croaker. Real-time quantitative PCR analysis revealed broad expression of EcTLR22, with relatively high expression detected in the head kidney, trunk kidney, spleen, peripheral blood leukocytes (PBLs) and heart of orange-spotted grouper. After injection with Vibrio alginolyticus, there was significant up-regulation of the expression of EcTLR22 in the spleen. In evaluating unstimulated/stimulated head kidney leukocytes and spleen leukocytes, a significant increase in EcTLR22 mRNA expression was detected, which implied a sensitive immune response. Furthermore, four important molecules for signal transduction, MyD88, TRIF, TNF-α and IRF3, were chosen to analyze the role of the EcTLR22 signaling pathway in anti-pathogen responses. Upon LPS or Poly I:C challenge, expression of the four genes was induced, with an increasing tendency detected in head kidney leukocytes, suggesting that the four genes might work with EcTLR22 in host defense against pathogenic microbes.     

Isolation and characterization of Toll-like receptor 9 in half-smooth tongue sole Cynoglossus semilaevis

Toll-like receptors (TLRs) are considered as key sensors to trigger the host's innate immune system and adaptive immune responses by recognizing various PAMPs and initiating signal transduction. TLR9, as a member of TLR family, mediates the recognition of unmethylated CpG dinucleotide motifs commonly found in both bacterial and viral genomes. In the current study, the TLR9 gene was isolated from one of flatfish species, half-smooth tongue sole (Cynoglossus semilaevis). In the 4588 bp genomic sequence, three exons, two introns, and 5′ UTR of 23 bp and 3′ UTR of 342 bp were identified. Putative amino acid sequence was 1062 residues long, including a typical conserved cytosolic Toll/interleukin-1 receptor (TIR) domain, 14 leucine-rich repeat (LRR) motifs, with greater than 60% identity to gilthead sea bream Sparus aurata and Japanese flounder Paralichthys olivaceus orthologs. Quantitative RT-PCR analysis indicated a broad expression of csTLR9, especially in spleen and gonads. No statistically significant changes were observed for csTLR9 mRNA levels in spleen and head kidney after inactive Vibrio anguillarum immunisation. In C. semilaevis ontogeny, the expression of csTLR9 appeared to be developmentally regulated. The presence of maternal TLR9 mRNA and the dramatic decrease of TLR9 expression at metamorphic stage indicated TLR9 might be involved in C. semilaevis development. Comparing sequence and expression profile of csTLR9 with mammalian and other piscine TLR9s suggested that the main function of TLR9 might be conserved across vertebrates, although species-specific features were present.     

赤眼鳟Toll样受体3基因cDNA全长克隆及表达分析

为探究赤眼鳟（Squaliobarbus curriculus）Toll样受体3（Toll-like receptor 3,ScTLR3）基因是否参与抗病毒免疫反应,实验运用RACE技术,克隆得到ScTLR3基因cDNA全长序列,并进行了生物信息学分析;通过Real-Time qPCR技术,检测了ScTLR3 mRNA在健康赤眼鳟10个组织中的分布以及感染草鱼呼肠孤病毒（GCRV）后肝脏、脾脏、体肾和头肾中的表达特征。结果表明:ScTLR3基因cDNA序列全长4043 bp,包括5-非编码区（UTR）216 bp,开放阅读框（ORF）2715 bp和3-UTR 1112 bp;ScTLR3共编码904个氨基酸残基,推导的蛋白分子量102.67 kD,理论等电点8.76;SMART结构域预测显示,ScTLR3由N端的信号肽（SP）、富亮氨酸结构域（LRRs）、跨膜结构域（TM）和C端的Toll/白介素-1受体结构域（TIR）组成。实时荧光定量结果显示,ScTLR3mRNA在检测的各组织中均有表达,肝脏中的相对表达量极显著高于其他组织（P0.01）;感染GCRV后,肝脏、脾脏、体肾和头肾组织中ScTLR3 mRNA均上调表达,肝脏、脾脏和体肾组织中的相对表达量在24h达到峰值,分别为对照组的5倍、7倍和6倍。研究表明,ScTLR3具有TLRs家族基因的典型结构特征,并能被GCRV诱导表达,推测其在赤眼鳟抗GCRV入侵免疫反应中发挥了重要作用。     

Analysis of PGC-1alpha variants Gly482Ser and Thr612Met concerning their PPARgamma2-coactivation function

Based on protein sequence homology searches, we found a conserved open reading frame within the genome of several human pathogenic bacteria showing a resemblance to the mammalian TIR domain. We cloned, expressed, and characterized the corresponding gene product from Paracoccus denitrificans using several biophysical techniques. The protein consists of two independently folded domains. As predicted from the amino acid sequence and experimentally confirmed here, the N-terminal domain consists of a alpha-helical coiled-coil. The NMR data indicates that the C-terminal TIR-like domain folds into a compact protein. Finally, using GST pull-down experiments, we show that the bacteria TIR-like domain binds to the mammalian receptor (TLR4) and adaptor (MyD88) TIR domains. We postulate that prokaryotic pathogens utilize the TIR-like proteins to interfere with the innate immune response of the mammalian host so that the bacterial infection can progress undetected.     

TLR3 and TLR7 are targeted to the same intracellular compartments by distinct regulatory elements

Toll-like receptor (TLR) 3 and TLR7 are indispensable for host defense against viral infection by recognizing virus-derived RNAs and are localized to intracellular membranes via an unknown mechanism. We recently reported experiments with chimeric Toll-like receptors that suggested that the subcellular distribution of TLRs may be defined by their transmembrane and/or cytoplasmic domains. Here we demonstrate that the intracellular localization of TLR3 is achieved by a 23-amino acid sequence (Glu(727) to Asp(749)) present in the linker region between the transmembrane domain and Toll-interleukin 1 receptor resistance (TIR) domain. In contrast, the intracellular localization of TLR7 is achieved by its transmembrane domain. These elements also targeted a heterologous type I transmembrane protein CD25 to the intracellular compartment that contained TLR3 and TLR7. Despite their using distinct regulatory elements for intracellular localization, TLR3 was found to co-localize with TLR7. In addition, TLR3 and TLR7 were preferentially localized near phagosomes containing apoptotic cell particles. These findings reveal that TLR3 and TLR7 contain unique targeting sequences, which differentially lead them to the same intracellular compartments and adjacent to phagosomes containing apoptotic cell particles, where these receptors may access their ligands for the induction of immune responses against viral infection.