异色瓢虫热休克蛋白70基因的克隆与分析

本研究通过RT-PCR和RACE方法,首次克隆了异色瓢虫Harmonia axyridis(Pallas)热休克蛋白70(HSP70)cDNA全序列(GenBank登录号:EF668009).获得的cDNA全长2200 bp,其中开放阅读框1956 bp,编码一个651氨基酸的蛋白,计算分子量为70 kDa,等电点(PI)为5.32.同源序列比对结果表明,异色瓢虫HSP70与其它真核生物的HSP/HSC70有着较高的序列同源性(85%～93%).其中与赤拟谷盗Tribolium castaneum热休克蛋白70(HSP70)同源性最高,达到93%.与其它真核生物HSP70一样,该序列包含真核生物HSP70高度保守的全部三个家族标签以及ATP/GTP结合位点、一个Bipartive nuclear localization signal和细胞核定位信号.     

马铃薯甲虫热激蛋白基因Ld-HSP60的克隆、序列分析及温度胁迫下的表达

【目的】马铃薯甲虫Leptinotarsa decemlineata是一种世界性检疫害虫,对温度胁迫具有极强的适应性,为进一步明确其对温度胁迫适应性的分子机制,研究了热激蛋白HSP60在马铃薯甲虫温度胁迫应答过程中的作用。【方法】采用RT-PCR及RACE技术克隆马铃薯甲虫热激蛋白HSP60基因的cDNA全长序列;利用生物信息学软件分析该基因及其编码蛋白质的序列特性;运用实时荧光定量PCR技术分析该基因在温度胁迫下的表达模式。【结果】克隆得到马铃薯甲虫热激蛋白HSP60基因,命名为Ld-HSP60(Gen Bank登录号:KC556801),其cDNA全长2 234 bp,开放阅读框(ORF)长1 731 bp,编码576个氨基酸,相对分子量约为61.27 kD,理论等电点为5.51,5'端非翻译区(UTR)长101 bp,3'UTR长402 bp。氨基酸序列中含有HSP60家族典型的特征序列。实时荧光定量PCR结果表明,低温胁迫(-10和0℃)下未检测到马铃薯甲虫雌雄成虫中Ld-HSP60的诱导表达;高温胁迫(38和44℃)诱导马铃薯甲虫雄成虫Ld-HSP60上调表达,随着胁迫温度的升高LdHSP60表达量呈现先升高后降低的趋势,38℃高温胁迫下表达量最高,胁迫时间越长Ld-HSP60表达量也越高。【结论】相比其他热激蛋白,HSP60对温度敏感性较低,推测HSP60可能在马铃薯甲虫雄成虫抵御高温胁迫中发挥作用。     

黄曲条跳甲酯酶基因片段的克隆及序列分析

黄曲条跳甲Phyllotreta striolata(Fabricius)是十字花科蔬菜的主要害虫之一,其抗药性问题日益严重,克隆黄曲条跳甲的酯酶基因可为其抗性治理提供必要的科学依据。本文利用反转录-多聚酶链式反应(RT-PCR)的方法得到一条281 bp的核酸片段,再利用3'-RACE技术获得该基因片段的3'端(1 468 bp),编码442个氨基酸。核苷酸序列同源性分析表明,与赤拟谷盗est1基因和杂拟谷盗est1基因的同源性最高,为71%(211/297),与果蝇alpha-esterase5的同源性为70%(156/222),氨基酸序列与杂拟谷盗、赤拟谷盗、果蝇的酯酶基因的同源性分别为43%(188/434)、43%(188/434)、33%(144/432)。从BLAST结果可初步推测该片段应为编码黄曲条跳甲酯酶基因的部分核苷酸序列,该序列在GenBank中的登录号为EU166919。     

异色瓢虫过氧化氢酶(Catalase)的基因克隆及序列分析

【目的】克隆异色瓢虫Harmonia axyridis保护酶系中过氧化氢酶(Catalase,CAT)的全长cDNA序列,并分析该基因的基本特性。【方法】采用同源克隆和锚定PCR技术,从异色瓢虫中克隆到HaraxCAT基因的cDNA全序列(GenBank登录号KC991026),并采用生物信息学的相关方法进行了分析。【结果】HaraxCAT的cDNA序列全长1 781 bp,其包含110 bp的3′非编码区域和45 bp的5′非编码区域,可读框长1 626 bp,编码541个氨基酸。预测该基因编码蛋白的分子量为61.55 ku,理论等电点为8.33,包含3个糖基化位点,无信号肽序列和跨膜结构。并且该基因包含了一个长达18个氨基酸的潜在的活性位点序列FDRERIPERVVHAKGAGA和血红素配体信号序列RIFSYGDTH。同源比对不同昆虫的CAT蛋白序列,发现昆虫CAT非常保守,HaraxCAT与其他昆虫的同源性高达65%及以上,与赤拟谷盗Tribolium castaneum同源性最高,达75.25%;系统发育分析表明其与鞘翅目赤拟谷盗和白星金花龟Protaetia brevitarsis亲缘关系最近。【结论】获得异色瓢虫catalase基因的cDNA全长序列,证实昆虫CAT蛋白非常保守。     

美洲鲥hsp70的分子特征及其对运输应激的应答

运用同源克隆和c DNA末端快速扩增(RACE)技术获取了美洲鲥(Alosa sapidissima)热应激蛋白70(hsp70)的全长c DNA序列,其总长度为2 545 bp,开放阅读框(ORF)为1 914 bp,推测编码637个氨基酸,其氨基酸的二级结构含有HSP70家族的3个特征序列。氨基酸同源性分析显示,美洲鲥hsp70与墨西哥脂鲤(Astyanax mexicanus)等鱼类的相似性达84%以上,与无脊椎动物果蝇(Drosophila auraria)及大肠杆菌(Escherichia coli)的相似性分别为73%和38%。荧光定量PCR检测显示,该基因在美洲鲥鳃、肌肉、头肾中高表达,在脑和心中相对高表达,在肝、脾、肠、肾中微量表达。采用荧光定量PCR方法研究运输应激对美洲鲥未经繁殖的亲鱼hsp70 m RNA水平的影响,在运输实验中鳃、肝hsp70 m RNA水平呈先升高后降低的变化趋势,头肾hsp70 m RNA水平呈现递增趋势。该结果表明克隆到的基因符合诱导型hsp70的特点,而且美洲鲥鳃、肝、头肾组织的hsp70 m RNA对运输应激表现出明显的应答作用。     

飞蝗热休克蛋白70cDNA片段的克隆和序列分析

采用R-PCR方法对海南、河北和辽宁3个飞蝗(Locusta migratoria L．)种群的热休克蛋白70(HSP70)基因cDNA片段进行克隆。在事先优化的条件下,通过简并性上游引物和下游引物扩增出了河北种群飞蝗HSP70基因的604bp cDNA片段(GenBank登录号为AY299637),推导的氨基酸序列包含201个氨基酸残基。分析表明,由飞蝗该片段推导的氨基酸序列与其他昆虫的同源性较高;3个种群该片段的核苷酸序列相似性更高达98．75％。由此推测,飞蝗种群间抗寒性的差异可能不是HSP70的序列变异引起的,而与HSP70的诱导表达有关。     

马铃薯甲虫N-β-丙酰多巴胺水解酶基因的克隆及功能分析

【目的】通过RNAi技术分析明确对马铃薯甲虫Leptinotarsa decemlineata黑色素形成重要的N-β-丙酰多巴胺(NBAD)水解酶基因的功能。【方法】NBAD水解酶基因通过马铃薯甲虫转录组数据分析和RT-PCR克隆获得,分别利用序列比对和系统发育分析确定该基因的完整性和系统发育;通过q PCR检测其在马铃薯甲虫各发育阶段和4龄幼虫不同组织及成虫精巢和卵巢中的表达量;采用喂食幼虫dsRNA的方法,观察该基因在马铃薯甲虫幼虫的生长发育过程中对体色的影响,并测定保幼激素和蜕皮激素对该基因表达的影响。【结果】克隆得到马铃薯甲虫NBAD水解酶基因,命名为Ldtan(Gen Bank登录号:KY221866),其编码蛋白的氨基酸序列与鞘翅目赤拟谷盗Tribolium castaneum和山松大小蠹Dendroctonus ponderosae同源蛋白的氨基酸序列的一致性最高,聚为一支。Ldtan在马铃薯甲虫4龄幼虫腹神经索(99.36±0.95)、后肠(17.79±3.11)和表皮(9.21±0.12)中的相对表达量较高;在幼虫期随幼虫生长发育表达量逐渐升高,在成虫期的表达量最高。通过喂食2龄幼虫Ldtan的dsRNA能有效降低靶标基因的表达量,使幼虫体色变深呈一定的棕褐色,并且具有一定的致死效应。通过RNAi技术干涉保幼激素合成和信号途径相关基因,发现Ldtan表达量降低,而干扰蜕皮激素合成和信号途径相关基因,Ldtan表达量增加。【结论】结果提示Ldtan参与了马铃薯甲虫的黑色素合成,并且蜕皮激素和保幼激素可能影响其表达。     

种间竞争对四种储粮害虫种群动态的影响

在30 ℃、75 %相对湿度条件下研究种间竞争对玉米象(Sitophilus zeamais)、谷蠹(Rhizopertha domini-ca)、赤拟谷盗(Triboliumcastaneum)和锈赤扁谷盗(Cryptolestes ferrugineus)4种主要储粮害虫种群动态的影响,并对种群动态进行回归分析。结果表明,玉米象与谷蠹、赤拟谷盗与锈赤扁谷盗混合饲养种群增长均受到显著抑制,玉米象和谷蠹对赤拟谷盗和锈赤扁谷盗的种群增长具有明显的促进作用,赤拟谷盗和锈赤扁谷盗对玉米象和谷蠹的种群增长具有一定的抑制作用。回归分析结果表明玉米象种群最大增长潜能最大,锈赤扁谷盗最小,种群增长率变化规律不明显。     

温度胁迫下棉花粉蚧热激蛋白基因的表达分析

【目的】为了研究热激蛋白 Hsp70, Hsp70-4和Hsp90在棉花粉蚧Phenacoccus solenopsis抵抗逆温中的作用。【方法】在测序棉花粉蚧转录组的基础上,分析了该虫热激蛋白Hsp70基因家族的2个序列［Pshsp70（GenBank登录号为KJ909505）和Pshsp70-4（GenBank登录号为KJ909506）］和Hsp90基因家族的1个序列,［Pshsp90(GenBank登录号为KJ909507)］,采用实时荧光定量 PCR（RT-qPCR）检测了在不同温度（18和32℃恒温, 37, 39, 41, 43和45℃热激1 h 后26℃恢复1 h)下棉花粉蚧不同发育阶段（2龄若虫、3龄若虫、雌成虫）3种热激蛋白基因的表达量。【结果】Pshsp70 cDNA序列包含1 923 bp的开放阅读框,编码641个氨基酸,理论分子量和等电点分别为70.9 kDa和5.65; Pshsp70-4 cDNA序列包含1 962 bp的开放阅读框,编码654个氨基酸,理论分子量和等电点分别为71.8 kDa和5.38;Pshsp90 cDNA序列包含2 172 bp的开放阅读框,编码724个氨基酸,理论分子量和等电点分别为83.5 kDa和4.93。Pshsp70 和Pshsp70-4均含有Hsp70基因家族高度保守的基序,Pshsp70编码的氨基酸序列与烟粉虱Bemisia tabaci和家蚕Bombyx mori等昆虫的Hsp70 的氨基酸序列一致性为 85%;Pshsp70-4编码的氨基酸序列与白蜡蚧Ericerus pela和点蜂缘蝽Riptortus pedestris等昆虫的Hsp70的氨基酸序列一致性高达95%;Pshsp90也含有Hsp90基因家族高度保守的基序,Pshsp90编码的氨基酸序列与赤拟谷盗Tribolium castaneum和东亚小花蝽Orius sauteri等昆虫的Hsp90 的氨基酸序列一致性为 87%。热激蛋白基因表达量分析结果表明,在18℃恒温条件下,粉蚧2龄若虫的3个PsHsps基因的mRNA相对表达量均比对照(26℃)低,在32℃恒温条件下,各龄期的Hsp70基因的相对表达量均显著高于对照。在37~45℃下热激1 h并在26℃下恢复1 h,棉花粉蚧3个龄期的3个热激蛋白PsHsps基因的相对表达量随温度的升高总体呈增加趋势,相关性分析表明,除Pshsp70-4在雌成虫中的表达量与热胁迫温度的相关系数为0.225外,各龄期中3个基因的表达量与温度的相关系数均大于0.6,显著相关;43℃和45℃胁迫下,各龄期的3个热激蛋白基因相对表达量均显著高于对照组（P<0.05）。【结论】棉花粉蚧热激蛋白基因的表达与温度呈正相关,在该虫应对高温中起着重要作用。     

种间竞争对四种储粮害虫种群动态的影响

在30 ℃、75%相对湿度条件下研究种间竞争对玉米象(Sitophilus zeamais)、谷蠹(Rhizopertha dominica)、赤拟谷盗(Tribolium castaneum)和锈赤扁谷盗(Cryptolestes ferrugineus)4种主要储粮害虫种群动态的影响，并对种群动态进行回归分析。结果表明，玉米象与谷蠹、赤拟谷盗与锈赤扁谷盗混合饲养种群增长均受到显著抑制，玉米象和谷蠹对赤拟谷盗和锈赤扁谷盗的种群增长具有明显的促进作用，赤拟谷盗和锈赤扁谷盗对玉米象和谷蠹的种群增长具有一定的抑制作用。回归分析结果表明玉米象种群最大增长潜能最大，锈赤扁谷盗最小，种群增长率变化规律不明显。     

Cloning and nucleotide sequence of a hsp70 gene from Streptomyces griseus

The cultivation of Streptomyces griseus 2247 at the growth-limited temperature (37°C) or in liquid medium containing 5% ethanol (toxic for growth) revealed the presence of heat-induced proteins in the total cellular proteins. Among them, a 70 kDal protein was isolated and its N-terminal amino acid sequence was determined. The 70 kDal protein possessed a possible ATP-binding site in the N-terminus, which was conserved among the HSP70 family. A DNA fragment encoding the HSP70 homologue was isolated from a genomic library of S. griseus 2247 strain using an oligonucleotide probe based on the N-terminal amino acid sequence of the 70 kDal protein. DNA sequence analysis of the cloned gene revealed an open reading frame consisting of 618 amino acid residues. The deduced amino acid sequence is highly homologous to the HSP70 family proteins; it is 59.8 % identical to Clostridium perfringens HSP70, 59.7% to the Bacillus megaterium DnaK protein, 58.4% to the Methanosarcina mazei DnaK protein, 58.1% to Synechocystis HSP70, 52.8% to the DnaK protein of Escherichia coli, and about 50% to some of the mitochondrial heat shock proteins. The cloned gene could encode the HSP70 of S. griseus.     

Expression of the Tribolium castaneum （Coleoptera： Tenebrionidae） hsp83 gene and its relation to oogenesis during ovarian maturation

Heat shock proteins (HSP) can protect organisms and cells from thermal damage. In this study, we cloned the full length cDNA encoding the HSP83 protein (the homologue of HSP90) of Tribolium castaneum (red flour beetle). The isolated cDNA contains the full coding sequence, a partial 5′ untranslated region of 55 bp and the complete 3′ untranslated region. We found the hsp83 gene is located on chromosome 5 of the T. castaneum genome. The predicted HSP83 protein sequence has a high similarity (on average 86.77%) with that of other insect species. The expression of the hsp83 gene in the whole body and in the ovary could be induced with heat stress (40°C for 1 h) in newly hatched (within 3 h post emergence) and mature (10 days post emergence) beetles. Under normal conditions, the hsp83 expression in the ovary is about 3-fold higher than in the whole body at both stages. No significant difference in hsp83 expression was observed between the two ovarian developmental stages regardless if the beetles were treated with heat shock or not. The expression of the HSP83 protein in the whole body could also be induced with heat stress in newly hatched and mature beetles. However, in the ovary, HSP83 was only expressed in the follicle cells of mature beetles and not in newly hatched beetles, regardless if the beetles were treated with heat shock or not. Furthermore, the females were not able to produce mature oocytes after knock-down of the hsp83 expression by injecting dsRNA. These results suggest that the HSP83 protein is involved in protection against heat stress and could be involved in oogenesis during ovarian maturation of T. castaneum.     

Microsporidia, amitochondrial protists, possess a 70-kDa heat shock protein gene of mitochondrial evolutionary origin

An intronless gene encoding a protein of 592 amino acid residues with similarity to 70-kDa heat shock proteins (HSP70s) has been cloned and sequenced from the amitochondrial protist Encephalitozoon cuniculi (phylum Microsporidia). Southern blot analyses show the presence of a single gene copy located on chromosome XI. The encoded protein exhibits an N-terminal hydrophobic leader sequence and two motifs shared by proteobacterial and mitochondrially expressed HSP70 homologs. Phylogenetic analysis using maximum likelihood and evolutionary distances place the E. cuniculi sequence in the cluster of mitochondrially expressed HSP70s, with a higher evolutionary rate than those of homologous sequences. Similar results were obtained after cloning a fragment of the homologous gene in the closely related species E. hellem. The presence of a nuclear targeting signal-like sequence supports a role of the Encephalitozoon HSP70 as a molecular chaperone of nuclear proteins. No evidence for cytosolic or endoplasmic reticulum forms of HSP70 was obtained through PCR amplification. These data suggest that Encephalitozoon species have evolved from an ancestor bearing mitochondria, which is in disagreement with the postulated presymbiotic origin of Microsporidia. The specific role and intracellular localization of the mitochondrial HSP70-like protein remain to be elucidated.      

Isolation and some properties of bovine brain 100 kDa heat shock protein

1. The 100 kDa protein was purified from bovine brains. 2. The antibody against the 100 kDa brain protein was prepared and was monospecific to the antigen. 3. The antibody cross-reacted with HeLa cell HSP100 (100 kDa heat shock protein). 4. The physicochemical, immunochemical properties and a partially amino acid sequence indicated that the 100 kDa protein was HSP100. 5. Peptide mapping using Staphylococcus aureus V8 protease showed a core peptide with 10 kDa molecular mass common to both HSP100 and HSP90. 6. The amino acid sequence of the 10 kDa fragment of the 100 kDa protein showed a high homology with that of human HSP90 (38-60); the difference was only two of 23 amino acid residues determined.     

Cloning of the HSP70 gene from Halobacterium marismortui: relatedness of archaebacterial HSP70 to its eubacterial homologs and a model for the evolution of the HSP70 gene.

Heat shock induces the synthesis of a set of proteins in Halobacterium marismortui whose molecular sizes correspond to the known major heat shock proteins. By using the polymerase chain reaction and degenerate oligonucleotide primers for conserved regions of the 70-kDa heat shock protein (HSP70) family, we have successfully cloned and sequenced a gene fragment containing the entire coding sequence for HSP70 from H. marismortui. HSP70 from H. marismortui shows between 44 and 47% amino acid identity with various eukaryotic HSP70s and between 51 and 58% identity with its eubacterial and archaebacterial homologs. On the basis of a comparison of all available HSP70 sequences, we have identified a number of unique sequence signatures in this protein family that provide a clear distinction between eukaryotic organisms and prokaryotic organisms (archaebacteria and eubacteria). The archaebacterial (viz., H. marismortui and Methanosarcina mazei) HSP70s have been found to contain all of the signature sequences characteristic of eubacteria (particularly the gram-positive bacteria), which suggests a close evolutionary relationship between these groups. In addition, detailed analyses of HSP70 sequences that we have carried out have revealed a number of additional novel features of the HSP70 protein family. These include (i) the presence of an insertion of about 25 to 27 amino acids in the N-terminal quadrants of all known eukaryotic and prokaryotic HSP70s except those from archaebacteria and the gram-positive group of bacteria, (ii) significant sequence similarity in HSP70 regions comprising its first and second quadrants from organisms lacking the above insertion, (iii) highly significant similarity between a protein, MreB, of Escherichia coli and the N-terminal half of HSP70s, (iv) significant sequence similarity between the N-terminal quadrant of HSP70 (from gram-positive bacteria and archaebacteria) and the m-type thioredoxin of plant chloroplasts. To account for these and other observations, a model for the evolution of HSP70 proteins involving gene duplication is proposed. The model proposes that HSP70 from archaebacteria (H. marismortui and M. mazei) and the gram-positive group of bacteria constitutes the ancestral form of the protein and that all other HSP70s (viz., other eubacteria as well as eukaryotes) containing the insert have evolved from this ancient protein.     

Molecular cloning of HSP70 in Mycoplasma ovipneumoniae and comparison with that of other mycoplasmas

Mycoplasma ovipneumoniae, a bacterial species that specifically affects ovine and goat, is the cause of ovine infectious pleuropneumonia. We cloned, sequenced and analyzed heat shock protein 70 (HSP70) (dnaK) gene of M. ovipneumoniae. The full length open reading frame of the M. ovipneumoniae HSP70 gene consists of 1812 nucleotides, with a G+C content of 34.16%, encoding 604 amino acids. Comparative analysis with the HSP70 sequences of 15 Mycoplasma species revealed 59 to 87% DNA sequence identity, with an amino acid sequence identity range of 58 to 94%. M. ovipneumoniae and M. hyopneumoniae shared the highest DNA and amino acid sequence identity (87 and 94%, respectively). Based on phylogenetic analysis, both the DNA and amino acid identities of M. ovipneumoniae with other mycoplasmal HSP70 were correlated with the degree of relationship between the species. The C-terminus of the HSP70 was cloned into a bacterial expression vector and expressed in Escherichia coli cells. The recombinant C-terminal portion of HSP70 protein strongly reacted with convalescent sera from M. ovipneumoniae-infected sheep, based on an immunoblotting assay. This indicates that HSP70 is immunogenic in a natural M. ovipneumoniae infection and may be a relevant antigen for vaccine development.     

Isolation and characterization of a cDNA clone encoding a cognate 70-kDa heat shock protein of the chloroplast envelope.

The translocation of proteins into the endoplasmic reticulum, the mitochondrion, and the chloroplast has recently been shown to involve homologues of the highly conserved 70-kDa heat shock protein (HSP70) family. In this study, we have isolated and sequenced a full-length cDNA clone encoding a cognate 70-kDa heat shock protein of the spinach chloroplast envelope (SCE70). The cDNA insert is 2,535 base pairs long and codes for 653 amino acid residues of a protein with a predicted molecular mass of 71,731 daltons. The deduced amino acid sequence shows a high degree of homology with HSP70 proteins from other organisms. Southern genomic and RNA analyses reveal different hybridization patterns than that observed for a heat-inducible 70-kDa protein gene. The protein synthesized from the SCE70 cDNA insert co-migrates with a 70-kDa polypeptide of the chloroplast envelope following sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Western blot analysis and import studies indicate that SCE70 is associated with the chloroplast outer envelope. The import data suggest that SCE70 is targeted to the envelope membrane via a pathway different from other plastidic precursors but similar to that recently reported for outer envelope proteins SOE1 and OM14.     

Molecular cloning of the 82-kDa heat shock protein (HSP90) of Toxoplasma gondii associated with the entry into and growth in host cells

Among the monoclonal antibodies (mAb) against Toxoplasma gondii, mAb Tg485 specifically reacted with an 82-kDa cytoplasmic protein of tachyzoites. The protein was secreted from extracellular tachyzoites, but was not released into the parasitophorous vacuole after invasion. The cDNA fragment encoding the protein was obtained by screening a T. gondii cDNA expression library with Tg485. The full-length cDNA was amplified by the 5(')-RACE method and sequenced. The deduced amino acid sequence of the 82 kDa protein reacting with Tg485 revealed a polypeptide of 708 amino acids showing significant homology to the heat shock protein 90 (HSP90) family of other organisms, especially to those of apicomplexan species. Treatment with geldanamycin, a drug known to interfere with HSP90 function, did not affect the secretion of TgHSP90 from extracellular tachyzoites, but the entry of the tachyzoites into host cells and the intracellular growth of the parasite were significantly disturbed.