家蝇3种丝氨酸蛋白酶抑制剂Serpin基因克隆、序列分析及表达模式

对家蝇3种丝氨酸蛋白酶抑制剂Serpin基因SP2、SP13和SP16进行克隆、序列分析和时空表达模式检测。运用瑞士生物信息学研究所的蛋白分析专家系统（ExPASy）和美国国家生物技术信息中心（NCBI）等有关的生物信息学分析工具,预测和分析3条Serpin基因编码蛋白质的结构与生物学功能。以RPS18（核糖体S18蛋白）为内参基因,采用实时荧光定量PCR（Real-Time PCR）技术检测3条 Serpin 基因在家蝇不同发育时期,以及家蝇3龄幼虫中脂肪体、唾液腺、中肠、马氏管和体壁的表达特征。SP2、SP13、SP16基因序列的开放阅读框ORF全长分别为1191 bp、1137 bp和1212 bp,分别编码含396、378和403个氨基酸残基的蛋白质,其理论分子量分别为45315.3 Da、43701.5 Da和45011.5 Da,等电点分别为9.01、5.98和6.04,蛋白质的N端都含有一段信号肽,并具有Serpin基因的保守结构域,属于Serpin家族。SP2和SP16在蛋白质的C端含反应中心环（Reactive center loop,RCL),而SP13 C端不含RCL。时空表达模式分析结果显示,SP2基因在2龄幼虫中的表达量最高,而雄蝇的表达量与卵期相比有所下调;SP13基因在蛹中的表达量最高,1龄幼虫和雌蝇中的表达量与卵期相近;SP16基因在2龄幼虫和3龄幼虫中的表达量最高,雄蝇与雌蝇的表达量与卵期相比有所下调。在家蝇3龄幼虫的各主要组织中,以体壁为参照,SP2基因在唾液腺表达水平最高,其次是脂肪体,中肠和马氏管均低于体壁;SP13基因在马氏管和脂肪体中的表达水平最高,中肠和唾液腺的表达量低于体壁;SP16基因在唾液腺、中肠、脂肪体和马氏管的表达量均低于体壁。推测Serpin基因在家蝇个体发育和免疫调节中起不同作用。     

叉角厉蝽触角转录组及嗅觉相关基因分析

叉角厉蝽Eocanthecona furcellata是一种在生物防治方面有重要作用和潜力的捕食性天敌昆虫,触角是昆虫进行信息交换的重要器官,而嗅觉相关基因则是调控天敌昆虫捕食行为的重要分子基础。为获得叉角厉蝽触角转录组数据库,挖掘叉角厉蝽嗅觉相关基因,本研究利用Illumina高通量测序平台对叉角厉蝽雌雄成虫与5龄若虫触角进行转录组测序。成功构建了叉角厉蝽触角转录组,获得了67 843条unigenes, N50长度为2 300 bp。与七大公共数据库比对注释到27 686条unigenes,其中NR数据库注释最多(33.33%),且与茶翅蝽Halyomorpha halys相似度最高(64.20%)。14 258条注释到GO数据库中,分为生物过程、细胞组分和分子功能3个大类42个亚类;KEGG代谢途径分析表明,7 703条形成282条代谢通路,其中被注释在信号传导通路中的unigenes最多(11.50%)。进一步基因注释分析,鉴定得到134个候选嗅觉相关基因,32个化学感应蛋白基因(Chemosensory protein genes, CSP),10个气味结合蛋白基因(Odor...     

棉花咖啡酰辅酶A-O-甲基转移酶基因的克隆及表达

根据棉花纤维特异表达cDNA文库分析得到的咖啡酰辅酶A-O-甲基转移酶(CCoAOMT)基因EST序列设计引物,采用RT-PCR技术首次从棉花中克隆了一个CCoAOMT基因,命名为GhCCoAOMT1(GenBank登录号为FJ848871).研究结果表明:GhCCoAOMT1基因cDNA全长960 bp,具有一个753 bp的开放阅读框,5'非编码区为9 bp,3'非编码区为198 bp,编码250个氨基酸,预测分子量约为28.306 kDa,等电点为5.39.利用PCR方法克隆了GhCCoAOMT1基因的基因组序列,长度为1 311 bp,包含5个外显子和4个内含子.氨基酸同源性分析发现,GhCCoAOMT1与来自毛白杨、烟草和苎麻的CCoAOMT同源性较高.半定量RT-PCR检测表明,GhCCoAOMT1基因在棉花各个组织中都有表达,其中茎部的表达量最高,其次表达量依次为根>花瓣>子叶>10 d纤维>雄蕊>胚珠>叶.     

二斑叶螨抗螺螨酯品系GST基因的克隆与表达分析

【目的】揭示二斑叶螨Tetranychus urticae对螺螨酯的分子抗性机理。【方法】利用RT-PCR克隆了二斑叶螨的谷胱甘肽-S-转移酶（glutathione S-transferase, GST)基因 cDNA 全长序列, 采用生物信息学软件分析了克隆基因的编码蛋白特性; 利用实时荧光定量PCR 方法分析GST基因在二斑叶螨的螺螨酯抗性与敏感品系中的表达差异。【结果】克隆获得的谷胱甘肽-S-转移酶2个基因分别被命名为TuGSTd1和TuGSTd2 (GenBank登录号分别为： KC445659和KC445660)。序列分析发现, TuGSTd1的开放阅读框长度为648 bp, 编码215个氨基酸, 分子量约为24.47 kDa, 理论等电点为5.49; TuGSTd2的开放阅读框为648 bp, 编码215个氨基酸, 分子量约为24.57 kDa, 理论等电点为6.33。系统发育分析表明这两个基因与桔全爪螨Panonychus citri Delta家族的GST基因的氨基酸序列一致性为93%。实时荧光定量PCR 结果表明, TuGSTd1和TuGSTd2在二斑叶螨抗螺螨酯品系中的相对表达量分别为敏感品系的5.60和3.75 倍。【结论】 GST基因在二斑叶螨抗螺螨酯品系中的相对表达量均显著高于敏感品系, 据此推测GST基因的过量表达可能与其对螺螨酯的抗性形成有关。     

华北大黑鳃金龟中肠丝氨酸蛋白酶cDNA克隆、 序列分析及表达

丝氨酸蛋白酶是昆虫体内一类重要的消化酶, 为了了解该类酶的分子特性及功能, 本研究利用粉纹夜蛾Trichoplusia ni围食膜蛋白多克隆抗体筛选华北大黑鳃金龟Holotrichia oblita中肠cDNA表达文库, 首次得到编码华北大黑鳃金龟丝氨酸蛋白酶cDNA序列, 命名为HoSP1（GenBank登录号为FJ573146）。序列分析表明, 该基因长902 bp, 开放阅读框（ORF）长783 bp, 编码260个氨基酸, 推测分子量和pI值分别为26.7 kDa和4.19, 不含有N-糖基化位点, 但在Thr₁₅₇处有一个O-糖基化位点, 含有6个保守的半胱氨酸残基, 组成3对二硫键, 对于维持蛋白质的三级结构起着重要的作用。通过与几种丝氨酸蛋白酶的比对发现, 该酶具有组氨酸（His）、 天冬氨酸（Asp）、 丝氨酸（Ser）催化中心, 与褐新西兰肋翅鳃金龟Costelytra zealandica的14种丝氨酸蛋白酶有明显的相似性, 其中与CzSP3的序列一致性最高, 为52.47%。把该基因与pET21b载体重组后, 进行体外表达, 以BTEE为底物, 测得该酶的活力为0.0378 μmol/mg·min。HoSP1基因的克隆及体外表达为进一步研究该酶在华北大黑鳃金龟体内的表达及功能提供了依据。     

捕食性蝽类唾液腺解剖方法—以叉角厉蝽为例

唾液腺的解剖是研究捕食性蝽类唾液成分及功能的关键。以叉角厉蝽Eocanthecona furcellata为例,报道了解剖获得其完整唾液腺的方法。该方法与其他解剖方法相比明显不同之处在于使用镊子固定虫体,更有利于唾液腺的解剖与收集。通过拍照观察,叉角厉蝽的唾液腺由主腺、副腺、肺门和导管组成。主腺可分为主腺前叶和主腺后叶,它们之间通过肺门相连。主腺肺门处着生有两根导管,其中一根导管与口器相连,而另一根导管与副腺连接。本文描述的解剖方法以及叉角厉蝽唾液腺形态结构可用于指导解剖获得其它捕食性蝽类的唾液腺,进而提取唾液开展成分鉴定和功能研究。     

绿盲蝽丝氨酸蛋白酶基因AlSP4的克隆及取食不同寄主植物后的表达谱分析

胰蛋白酶类和胰凝乳蛋白酶类丝氨酸蛋白酶是盲蝽科昆虫消化系统内重要的消化酶。为了更好地了解丝氨酸类蛋白酶在绿盲蝽Apolygus lucorum消化系统中的作用, 本研究首次克隆了绿盲蝽丝氨酸蛋白酶基因AlSP4 (GenBank登录号为JQ609682)。序列分析结果表明, 该基因开放阅读框长999 bp, 编码332个氨基酸, 预测分子量为36.84 kDa, 理论等电点为5.35, N末端疏水区包含有16个氨基酸组成的信号肽。蛋白特征分析表明, 该基因翻译后的蛋白质具有丝氨酸蛋白酶的典型特征, 即氨基酸序列中具有组氨酸(His)、 天门冬氨酸(Asp)以及丝氨酸(Ser)残基组成的酶活性催化中心三元件; 该基因翻译后还具有明显的胰蛋白酶前体的特征, 即此基因具有信号肽、 激活肽以及胰蛋白酶N末端保守的起始氨基酸序列(IVGG)。利用荧光定量PCR技术对绿盲蝽雌、 雄成虫取食不同寄主植物后AlSP4的表达谱进行分析, 结果表明: 相对于其他寄主植物, 雌成虫取食Bt棉后AlSP4的表达量最高, 并显著高于取食常规棉后的表达量(P＜0.01)。雄成虫取食茼蒿后AlSP4的表达量最高; 雄成虫取食Bt棉后, AlSP4的表达水平仅次于取食茼蒿后的表达量, 也显著高于取食常规棉后的表达量(P＜0.01)。由此可见, AlSP4是绿盲蝽取食Bt棉后的重要消化酶基因, 对绿盲蝽适应Bt棉取食具有重要作用。     

野生茄子（Solanum torvum）抗黄萎病相关基因Sto Vel的克隆与分析

采用RT—PCR和RAcE技术从野生茄子中扩增克隆到一个抗黄萎病相关基因,命名为StoVel,其cDNA全长3400bp,含有3153bp的完整开放阅读框,编码1051个氨基酸,该基因编码的蛋白序列与刚果野茄、类番茄和番茄Vel编码的氨基酸序列同源性分别为82％、81％和80％,且有很高的功能区段保守性。将该cDNA全长序列提交Gen Bank,登陆号为DQ020574。半定量PCR表明该基因为组成型表达,在根中表达最多,叶中最少。     

“两广二号”家蚕抗病毒基因Bmlipase-1和BmSP-2克隆与原核表达

本研究以优良杂交品种"两广二号"家蚕为试材,克隆了该杂交品种家蚕两个抗家蚕核型多角体病毒(BmNPV)基因:脂肪酶基因Bmlipase-1和丝氨酸蛋白酶基因BmSP-2,测序并分别与不同品种蚕的同源基因序列进行比较。结果显示,"两广二号"家蚕Bmlipase-1基因ORF长度为885bp,编码294个氨基酸,BmSP-2扩增长度为855bp,编码284个氨基酸;它们的核苷酸和推导氨基酸序列同源性皆达92%以上,Bmlipase-1更保守,同源性大于99%";两广二号"家蚕的Bmlipase-1基因脂肪酶活化部位和BmSP-2基因酶催化三联体位点的氨基酸残基与不同品种蚕的完全相同。以上结果说明这两个抗病毒基因在蚕的遗传进化过程中高度保守,提示其可能在机体消化或者免疫防御方面起着重要生理作用。将这两个抗病毒基因在大肠杆菌BL21中进行融合表达,获得的融合Bmlipase-1和BmSP-2蛋白分子量分别为47kD和42kD左右。     

野生茄子(Solanum torvum)抗黄萎病相关基因StoVe1的克隆与分析

采用RT-PCR和RACE技术从野生茄子中扩增克隆到一个抗黄萎病相关基因,命名为StoVe1,其cDNA全长3 400bp,含有3 153 bp的完整开放阅读框,编码1 051个氨基酸,该基因编码的蛋白序列与刚果野茄、类番茄和番茄Ve1编码的氨基酸序列同源性分别为82%、81%和80%,且有很高的功能区段保守性.将该cDNA全长序列提交GenBank,登陆号为DQ020574.半定量PCR表明该基因为组成型表达,在根中表达最多,叶中最少.     

Purification of a serine protease of Vibrio parahaemolyticus and its characterization

A 50 kDa protease designated as VPP1 was purified from the culture supernatant of a clinical strain of Vibrio parahaemolyticus by ammonium sulfate fractionation, Sephacryl S-200 HR gel filtration and Fractogel EMD TMAE 650 ion-exchange chromatography. VPP1 was inhibited by EDTA, EGTA and serine protease inhibitors, suggesting that it is a calcium-dependent serine protease. N-terminal amino acid sequence of VPP1 was quite similar to that of V. metschnikovii protease and antibody against VPP1 inhibited the activity of V. metschnikovii protease, suggesting the similarity of the two proteases. It was demonstrated that VPP1 or its related protease widely distribute in not only V. parahaemolyticus but also V. alginolyticus.     

Purification and characterization of hevain,a serine protease from Hevea brasiliensis

A serine protease of MW 69000 has been isolated, in homogeneous form, from the latex of Hevea brasiliensis. The enzyme, named hevain, has only limited esterolytic and proteolytic abilities, a maximum activity in the pH range 6.5–7.5, and a pI of 4.3. Hevain has a notably high content of acidic amino acids, while the aromatic residues are present in relatively minor amounts.     

Purification and characterization of extracellular alkaline serine protease from Stenotrophomonas maltophilia strain S-1

AIMS: The present study was conducted by screening soil bacteria in an attempt to isolate a bacterium that produced extracellular alkaline protease, and for purification and characterization of the protease. METHODS AND RESULTS: Soil bacteria were screened by growth on casein as the sole carbon source. Characterization of a strain isolated from soil of Abashiri, Japan indicated a taxonomic affiliation to Stenotrophomonas maltophilia, and was named S-1 strain. The purified S-1 protease, designed S. maltophilia Protease-1 (SmP-1), exhibited an optimal pH of 12.0, optimal reaction temperature of 50 degrees C and a molecular mass of approximately 40 kDa by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). The cleavage sites of the oxidized-insulin B chain by SmP-1 were identified as Leu6-Cys7, Cys7-Gly8, Tyr16-Leu17 and Leu17-Val18. The N-terminal amino acid sequence of the purified alkaline protease was determined as NH2-SASAPMVSGVAALVLE. CONCLUSION: A novel extracellular alkaline serine protease was isolated from S. maltophilia strain S-1. The optimal pH of the proteolytic activity was pH 12.0. SIGNIFICANCE AND IMPACT OF THE STUDY: The extremely high optimal pH and heat stability of the alkaline serine protease SmP-1 might make it widely applicable to food and other industries.     

Dimers initiate and propagate serine protease inhibitor polymerisation

The serine protease inhibitor (serpin) family can readily form long-chain polymers by a process that underlies a variety of diseases. We show here that monomers of plasma serpins α₁-antitrypsin and antithrombin are stable on incubation with the rate-limiting step in their polymerisation being the formation of the initial dimer. Once formed, the dimers readily interlink to form tetramers and can bind monomers to form trimers and longer oligomers. Cleavage of the only exposed reactive loop, in unit I of the dimers, prevents their interlinkage, but these cleaved dimers can still link to monomers. The rapid binding by the cleaved dimers of a peptide specific to the lower half of β-sheet A of the molecule indicates the ready opening of this β-sheet in unit II of the dimers. The failure of the cleaved dimers to bind peptide-complexed monomers, together with the relative inaccessibility of the P14 hinge residue in the oligomers, is evidence that partial insertion of the reactive loop into its own A-sheet is required for polymer formation. We propose that serpin dimers initiate and propagate polymerisation by having one exposed loop with an optimal conformation as a β-strand donor and a readily opened β-sheet as an acceptor. The sequential reformation of these activated β-interfaces as the oligomer extends, molecule by molecule, provides a model for the fibril and amyloid formation of conformational diseases in general as well as for the infectivity of prion encephalopathies.     

Gene structure and expression of the gene from Beauveria bassiana encoding bassiasin I, an insect cuticle-degrading serine protease

Genomic and cDNA encoding Beauveria bassiana bassiasin I, a potential cuticle-degrading serine protease, were isolated and analysed. Bassiasin I gene is comprised of 1137 bp (379 aa) and 3 introns which are 69, 62 and 68 bp long. The comparison of a deduced amino acid sequence with Metarhizium anisopliae Pr1, B. bassiana Pr1, and proteinase K showed high homology. When the cDNA including the intact signal peptide was expressed in E. coli, a clear proteolytic-degraded zone on LB-skimmed milk plates was observed.     

Low temperature-induced dimerization of the bovine sperm serine protease,BSp66

BSp120 and BSp66 are trypsin-like serine proteases from bovine spermatozoa. The former is active in cryopreserved sperm samples while the latter shows proteolytic activity in recently obtained fresh sperm. Both proteases are immunologically related and co-localize in the apical portion of the sperm head. In Western blots with specific antibodies, sperm samples incubated with reducing agents showed a decrease in the amount of BSp120, while BSp66 was detected with both anti-BSp120 and anti-BSp66 antibodies. BSp120 was evident in frozen intact spermatozoa after 60 days of semen cryopreservation and the kinetic of appearance of this protein was coincident with the decrease in the amount of BSp66. Identical results were obtained by freezing sperm extracts from fresh semen at -20 degrees C. Our results suggest that BSp120 results from disulfide bond-dimerization of BSp66 and that this process may be induced by temperatures below zero in both intact spermatozoa and in sperm extracts.     

Purification and partial characterization of a myofibril-bound serine protease from ostrich skeletal muscle

A myofibril-bound serine protease (MBSP) was partially purified from ostrich (Struthio camelus) skeletal muscle. MBSP was dissociated from the myofibrillar fraction by ethylene glycol treatment at pH 8.5, followed by partial purification via Toyopearl Super Q 650 S and p-aminobenzamidine column chromatographies. Ostrich MBSP revealed a major protein band of approximately 21 kDa on SDS-PAGE, showing proteolytic activity after casein zymography. Optima pH and temperature of ostrich MBSP were 8 and 40 °C, respectively. Substrate specificity analysis revealed that the enzyme cleaved synthetic fluorogenic substrates at the carboxyl side of arginine residues. Kinetic parameters (K_m and V_max values) were calculated from Lineweaver–Burk plots. The kinetic characteristics of ostrich MBSP were compared to values obtained for commercial bovine trypsin in this study, as well as those obtained for MBSP from mouse and various fish species. The results suggest that ostrich MBSP is a tryptic-like serine protease. Ostrich MBSP exhibited low sequence identity to commercial bovine trypsin (44%), MBSP from lizard fish skeletal muscle (33%) and trypsinogen from ostrich pancreas (22%).     

Euphorbain p,a serine protease from euphorbia pulcherrima

A serine protease named euphorbain p has been isolated in a homogeneous state from the latex of Euphorbia pulcherrima. This multi-chain enzyme, MW 74000, is similar in composition to one in E. lathyris, but is larger in size and has a more restricted activity. It has a pI of 4.7, and displays maximum activity at pH 7.0.     

Purification and characterization of an extracellular serine protease from the nematode-trapping fungus Dactylella shizishanna

AIMS: To evaluate the production of an extracellular serine protease by Dactylella shizishanna and its potential as a pathogenesis factor. METHODS AND RESULTS: An extracellular alkaline serine protease (Ds1) was purified and characterized from the nematode-trapping fungus D. shizishanna using cation-exchange chromatography and hydrophobic interaction chromatography. The molecular mass of the protease was approximately 35 kDa estimated by SDS-PAGE. The optimum activity of Ds1 was at pH 10 and 55 degrees C (over 30 min). The purified protease could degrade purified cuticle of Penagrellus redivivus and a broad range of protein substrates. The purified protease was highly sensitive to phenylmethyl sulfonyl fluoride (PMSF) (0.1 mmol l(-1)), indicating it belonged to the serine protease family. The N-terminal amino acid residues of Ds1 are AEQTDSTWGL and showed a high homology with Aozl and PII, two serine proteases purified from the nematode-trapping fungus Arthrobotrys oligospora. CONCLUSIONS: Nematicidal activity of D. shizishanna was partly related to its ability to produce extracellular serine protease. SIGNIFICANCE AND IMPACT OF THE STUDY: In this report, we purified a new serine protease from D. shizishanna and provided a good foundation for future research on infection mechanism.     

Biochemical properties of a serine protease from Aspergillus flavus and application in dehairing

The proteases are enzymes produced by several filamentous fungi with important biotechnological applications. In this work, a protease from Aspergillus flavus was characterized. The culture filtrate of A. flavus was purified to homogeneity by Sephacryl S-200 column chromatography followed by CM–cellulose. The molecular weight of the purified enzyme was estimated to be approximately 32?kDa by SDS–PAGE. The enzyme hydrolysed BTpNA (N-α-benzoyl-dl-tyrosyl-p-nitroanilide), azo-casein and casein as substrates. Optimal temperature and pH were 55?°C and 6.5, respectively. The enzyme was stimulated by Mg²⁺, Ca²⁺, Zn²⁺ and inhibited by Hg²⁺ and Ag²⁺ and Cu²⁺. The protease showed increased activity with detergents, such as Tween 80 and Triton X, and was stable to the reducing agents, such as β-mercaptoethanol. The protease activity was strongly inhibited in the presence of phenylmethylsulfonyl fluoride, indicating it is a serine protease. The enzyme entrapped in calcium alginate beads retained its activity for longer time and could be reused up to 10 times. The thermostability was increased after the immobilization and the enzyme retained 100% of activity at 45?°C after 60?min of incubation, and 90% of residual activity at 50?°C after 30?min. In contrast, the free enzyme only retained 10% of its residual activity after 60?min at 50?°C. The enzymatic preparation was demonstrated to be efficient in the capability of dehairing without destruction of the hide. The remarkable properties such as temperature, pH and immobilization stability found with this enzyme assure that it could be a potential candidate for industrial applications.