柞蚕小热休克蛋白20.1的基因鉴定及免疫功能研究

热休克蛋白(HSP)是一类广泛存在于各类生物中的具有分子伴侣功能的蛋白质。近年来研究发现HSP与机体许多功能如免疫、凋亡、衰老等密切相关。柞蚕(Antheraea pernyi)小热休克蛋白20.1(Aphsp20.1)基因的开放读码框长度为534bp,编码178个氨基酸。序列比对结果表明,柞蚕小热休克蛋白20.1属于HSP20家族。组织定量显示这Aphsp20.1在中肠和脂肪体分布较高。此外用大肠杆菌Escherichia coli及Micrococcus luteus病原微生物注射入5龄3天柞蚕幼虫后,发现Aphsp20.1的基因表达菌明显上调。另外体外抑菌试验结果发现纯化后的蛋白也具有一定的抑菌作用。该研究表明ApHSP20.1在柞蚕的免疫功能中具有重要作用,该研究不仅为我们进一步了解更加复杂的高等生物天然免疫反应提供一些相关的研究线索;而且对柞蚕天然免疫的研究有利于更好地理解昆虫自身的免疫系统,为保护益虫防治害虫提供重要依据。     

棉花粉蚧热休克蛋白基因的鉴定

热休克蛋白(heat shock proteins,Hsps)是生物体或细胞受到热胁迫后新合成的一类遗传上高度保守的蛋白,在昆虫应对外界环境因子胁迫时起着重要作用。为了系统研究棉花粉蚧Phenacoccus solenopsis Hsp基因家族,对棉花粉蚧转录组基因注释信息进行分析、获得目标序列,并应用NCBI上Blast X等软件进行比对、共鉴定出24条热激蛋白(Hsp)基因,包括3个Hsp90、8个Hsp70、2个Hsp60和11个s Hsp(small heat shock protein,s Hsp)基因。对棉花粉蚧与模式昆虫家蚕Bombyx mori、黑腹果蝇Drosophila melanogaster、赤拟谷盗Tribolium castaneum系统进化关系分析显示,昆虫的小分子量热休克蛋白s Hsp具有很强的种属特异性,Hsp70家族的保守性比s Hsp强。棉花粉蚧热激蛋白基因的鉴定为深入研究该虫Hsp与生长发育、抗逆境的相互关系奠定了基础。     

热休克T细胞中mRNA的表达

 富集的人外周血T淋巴细胞经40—42℃保温(热休克)可诱导产生90kd和71kd的两种主要热休克蛋白(HSP),此外,62和34kd HSP也可在不同条件下诱导。从不同处理的T淋巴细胞中提取mRNA并在免网织细胞裂解液系统中进行体外转译,显示出相同的主要HSP。其中71和62kdHSP不仅在升温时还可在低温(4℃)下诱导,表明淋巴细胞中几种主要HSP的诱导机制不完全相同。比较L-~(35)S-Met参入实验和体外转译的结果提示淋巴细胞中HSP基因表达主要在转录水平调控。     

人热休克蛋白70和热休克固有蛋白70的基因克隆和表达

目的:克隆人热休克蛋白70(HSP70)和热休克固有蛋白70(HSC70)基因,并在大肠杆茵中表达,获得重组蛋白.方法:用RT-PCR法从HepG2细胞中扩增HSP70及HSC70cDNA序列.测序后,将相应的cDNA插入pRSET-A表达载体,在大肠杆菌中表达,重组蛋白纯化后用SDS-PAGE及Western Blotting分析.结果:DNA序列结果显示.本研究所获得的HSP70及HSC70 cDNA序列与参考序列一致.将全长cDNA分别插入表达质粒后,转化BL21(DE3)细菌,在IPTG的诱导下,表达产物SDS-PAGE显示相应的分子量(70kDa)位置有明显的蛋白条带.Western Blotting结果证实了其为目的蛋白,经镍树脂柱纯化,获得了相应的重组多肽.结论:成功构建了原核表达重组质粒HSP70-pRSET-A和HSC70-pRSET-A,并获得了纯化的重组人HSP70和HSC70蛋白,为进一步研究这两种蛋白的结构、功能及临床应用奠定了基础.     

三角帆蚌热休克蛋白70基因克隆及其表达分析

对三角帆蚌HSP70基因序列进行全长克隆及其分子生物学分析,并检测其在不同水温刺激下鳃组织中的表达变化。通过高通量转录组测序获得三角帆蚌HSP70基因（HcHSP70）长片段,采用3'RACE对其进行了3'末端克隆,经拼接得到HcHSP70 cDNA全长序列。采用多种分子生物学软件对HcHSP70 cDNA全长序列进行了特征分析,采用实时荧光定量PCR技术检测了其组织分布,并结合Western-blot技术检测蚌鳃中该基因mRNA与蛋白经不同水温刺激后的表达变化。结果显示,HcHSP70 cDNA全长为2298 bp,其中开放阅读框为1974 bp,编码657个氨基酸。预测分子量大小为71.6 Ku,pH7.0时的理论等电点为5.61。氨基酸序列分析表明,HcHSP70氨基酸序列含HSP70家族的3个标签序列（I₉DLGTTYS₁₆、I₁₉₇FDLGGGTFDVSIL₂₁₀和I₃₃₆ VLVGGSTRIPKVQK₃₅₀）,与长牡蛎及泥蚶的HSP70同源性最高（91%）。实时荧光定量PCR检测结果显示,HcHSP70在鳃、性腺、肝胰腺、外套膜及肌肉等5种被检组织中均有表达,以肝胰腺中的表达水平最高。实时荧光定量PCR与Western-blot技术检测皆表明,蚌鳃组织中HcHSP70基因与蛋白的表达量在37℃时达到最高,而在40℃水温刺激下表达水平下调至正常值,表明其在适应高温刺激时发挥了重要作用。     

热休克后表达受抑基因的分子克隆及其表达特性

以人成骨肉瘤细胞株ＨＯＳ－８６０３为热休克模型,在利用ＤＤｍＲＮＡ方法筛选和克隆了一个热休克后表达受抑基因的ｃＤＮＡ片段的基础上,以该片段为探针,筛选ＨＯＳ－８６０３细胞的ｃＤＮＡ文库,获得该基因的全长ｃＤＮＡ克隆（ＨＳＳＧ－１）;ＤＮＡ序列测定表明该ｃＤＮＡ全长１４５６ｂｐ,编码２７６个氨基酸,经计算机辅助分析,该ｃＤＮＡ序列尚未被报道。经ＲＮＡ斑点杂交证实,该基因的表达于多种组织细胞之中,并且     

动物发育过程中热休克基因的表达

本文综述了动物发育过程中热休克基因的表达及热休克蛋白质的合成与生物耐热性的相互关系。动物发育过程中热休克基因的表达具有阶段依赖性。热休克蛋白质的合成与生物耐热性的获得呈正相关。     

羧酸酯酶介导的小菜蛾对氟虫腈的抗性

【目的】羧酸酯酶（carboxylesterases, CarEs）是昆虫重要的解毒代谢酶之一,可以介导靶标昆虫对多种杀虫剂的代谢抗性。本研究检测了羧酸酯酶对小菜蛾Plutella xylostella 抗药性的介导功能,旨在阐明羧酸酯酶在小菜蛾代谢解毒中的生理生化和分子机理。【方法】采用点滴法测定氟虫腈对小菜蛾敏感种群和抗氟虫腈种群的毒力,以及羧酸酯酶抑制剂磷酸三苯酯（triphenyl phosphate, TPP）对氟虫腈的增效作用;以LC₃₀和LC₅₀浓度的氟虫腈处理抗性小菜蛾,测定药剂处理后CarEs酶活性的变化;利用qRT-PCR技术分析Pxae22和Pxae31两个基因在小菜蛾不同发育阶段、组织和种群的表达模式;利用dsRNA干扰Pxae22和Pxae31后观察基因的表达变化和小菜蛾3龄幼虫对药剂敏感性的变化。【结果】TPP可以削弱小菜蛾3龄幼虫对氟虫腈的抗性,增效倍数约为6倍;使用较低剂量（LC₃₀和LC₅₀）氟虫腈处理小菜蛾3龄幼虫后,处理组CarEs比活力明显高于对照,提示氟虫腈对小菜蛾CarEs活性具有诱导作用。对羧酸酯酶基因Pxae22和Pxae31在小菜蛾不同发育阶段、4龄幼虫不同组织和不同种群3龄幼虫中的表达模式分析发现,这两个基因在小菜蛾4龄幼虫中的表达量最高;在4龄幼虫中以中肠组织中的表达量较高,头、表皮、脂肪体中的表达量很低; 抗性种群中的表达量显著高于敏感种群。通过干扰 Pxae22和 Pxae31后的qRT-PCR验证,两个基因的表达量均显著降低,进一步的氟虫腈毒力测定发现,干扰P xae22和 Pxae31后的小菜蛾3龄幼虫对氟虫腈的敏感性分别增加了1.63倍和1.73倍。【结论】羧酸酯酶在小菜蛾对氟虫腈解毒代谢中具有重要作用;Pxae22和Pxae31是小菜蛾的两个抗性相关基因,其表达水平的变化直接影响小菜蛾对氟虫腈的敏感性。     

小菜蛾鞣化激素基因克隆及其功能分析

鞣化激素是调节昆虫表皮骨化和翅膀发育的一种神经激素, 尽管已经在许多不同种昆虫上克隆了鞣化激素基因, 但是关于小菜蛾 Plutella xylostella鞣化激素及其基因的研究至今未见报道。本研究克隆了两个小菜蛾鞣化激素基因Pxbursα和Pxbursβ （GenBank 登录号分别为KF498645和KF498646）全长cDNA, 其序列长度分别为537 bp和360 bp, 与已报道的其他昆虫的鞣化激素氨基酸序列一致性分别为51%~68% 和37%~57%。实时定量PCR分析发现Pxbursα和Pxbursβ均在蛹期表达量高, 而在幼虫期和成虫期的表达量低。以Pxbursα部分序列的双链RNA（dsRNA）饲喂小菜蛾4龄末期幼虫, 发现蛹期Pxbursα的表达受到了显著抑制, 小菜蛾的发育停滞在蛹期而无法正常羽化, 并最终死亡。由此推测, 小菜蛾鞣化激素基因在蛹期的大量表达对其生长发育和羽化具有重要的作用。     

小菜蛾触角结合蛋白PxylOBP31的鉴定与结合特性分析

【目的】触角结合蛋白(antennal binding proteins,ABPs)为昆虫气味结合蛋白(odorant binding proteins,OBPs)家族的一个亚类,是昆虫识别和响应外界环境中气味信号的载体之一,对昆虫的生存和繁衍有着重要的意义。明确触角结合蛋白在小菜蛾Plutella xylostella(L.)嗅觉识别中的作用,有助于揭示小菜蛾嗅觉识别分子机制。【方法】利用PCR技术克隆小菜蛾的一个触角结合蛋白基因;采用实时荧光定量PCR技术对该基因在小菜蛾不同发育阶段和成虫不同组织中的表达量进行分析;利用荧光竞争结合实验测试该触角结合蛋白与39种配基化合物的结合特性。【结果】成功克隆了一个小菜蛾触角结合蛋白基因,命名为Pxyl OBP31(Gen Bank登录号:KT156676)。序列分析结果显示,其开放阅读框全长411 bp,编码136个氨基酸,N端自起始位置开始21个氨基酸为信号肽,含有气味结合蛋白家族的6个保守半胱氨酸残基,预测分子量为14.74 k D,等电点为4.41。表达谱分析表明,Pxyl OBP31主要在雄蛾中表达,且交配后的雄蛾中表达量明显降低;该基因在小菜蛾触角中有较高表达,在雄蛾触角中的表达量比雌蛾触角中高近2倍。结合特性实验结果显示,Pxyl OBP31与醛、酮、萜品油烯以及邻苯二甲酸二异丁酯等物质的结合能力较强,与3种性信息素及其他烯烃与酯类结合能力弱。【结论】本研究明确了Pxyl OBP31的核苷酸序列以及发育和组织表达谱。根据qRT-PCR和荧光竞争结合实验结果,推测Pxyl OBP31蛋白可能与小菜蛾觅偶、定位寄主植物等行为有关。     

小菜蛾气味结合蛋白OBP2基因的克隆、表达谱及其结合特性分析

【目的】气味结合蛋白(odorant binding proteins,OBPs)在昆虫寄主定位、产卵地选择等行为中发挥重要作用,克隆与鉴定小菜蛾Plutella xylostella OBP基因、明确其与配体化合物的结合特性有助于阐明小菜蛾嗅觉识别的分子机制。【方法】利用PCR技术克隆小菜蛾OBP2,对获得的编码序列全长进行信号肽及跨膜区域预测,用DNAMAN与其他昆虫的OBP2进行多序列比对,采用MEGA5.0邻接法(neighbor-joining method,NJ)构建进化树。通过实时定量PCR(qRT-PCR)分析Pxyl OBP2在小菜蛾不同发育阶段和不同组织中的表达模式。构建原核表达载体p ET28aPxyl OBP2,进行原核表达及蛋白纯化。利用荧光竞争结合实验对Pxyl OBP2蛋白与39种配基化合物的结合特性进行分析。【结果】成功获得小菜蛾OBP2基因Pxyl OBP2(Gen Bank登录号:KT070562)的编码序列全长,其完整开放阅读框大小为546 bp,编码182个氨基酸,具有气味结合蛋白典型的6个保守半胱氨酸结合位点。荧光定量PCR结果表明,发育表达模式显示,Pxyl OBP2在未交配雄性成虫中的表达量均明显高于雌性成虫和已交配雄虫;组织表达模式显示,Pxyl OBP2在足中的表达量高于其他组织。经预测成熟蛋白大小为22.24 k Da,等电点5.69。SDS-PAGE结果显示融合蛋白成功表达。荧光竞争结合实验对3种性信息素和36种植物挥发物结合发现,Pxyl OBP2与性信息素Z-11-16:Ald可以结合,解离常数48.951μmol/L;可以和11种寄主植物挥发物有效结合,其中,与芳樟醇、正壬醇结合能力最强,解离常数分别为4.733和6.861μmol/L。【结论】本研究明确了Pxyl OBP2的核苷酸、氨基酸序列,并根据qRT-PCR和荧光竞争结合实验结果,推断Pxyl OBP2与小菜蛾雄虫寻求配偶有关,且寄主挥发物芳樟醇、正壬醇起协同促进作用。     

Management of diamondback moth,Plutella xylostella (Lepidoptera: Plutellidae) by mating disruption

Abstract Field trials were conducted in China in 2008 and 2009 to evaluate the efficacy of mating disruption (MD) on diamondback moth, Plutella xylostella, in cabbage, Brassica oleracea var. capitata. Effectiveness was positively correlated with the MD dispenser density in the field. A density of 167 MD dispensers per ha produced an average population decrease of about 50% compared to the conventional‐practice field. Significant fewer males were captured in pheromone‐treated and conventional‐practice fields than in the blank control field, but the difference was not significant between the pheromone‐treated and conventional‐practice fields. In addition, fewer eggs and larvae were observed in pheromone‐treated fields. Our results suggest mating disruption coupled with minimal insecticidal supplements is a promising solution for resistance management and control of diamondback moth infestation.     

cDNA characterization and expression analysis of two arylphorin-like hexameric protein genes from the diamondback moth, Plutella xylostella (L.)

We cloned and characterized two hexameric storage protein genes, PxAry1 and PxAry2, from Plutella xylostella and investigated the expression pattern in different developmental stages and in response to treatment by a juvenile hormone (JH) analog. The complete coding sequences of PxAry1 and PxAry2 are comprised of 2,097 and 2,094 bp with 699 and 698 amino acid residues, respectively. Signal peptides of 16 amino acids are predicted at the N-termini. According to both the phylogenetic analysis and amino acid composition (>16% aromatic amino acids), PxAry1 and PxAry2 belong to the arylphorin-like protein genes. Analysis using Northern hybridization and RT-PCR showed varying levels of genes expression in the developmental stages with a small difference between sexes. Expression of both genes in fourth instar larvae was suppressed after treatment with a JH-analog. Southern hybridization revealed the presence of multiple arylphorin genes in the genome.     

Sublethal effects of hexaflumuron on development and reproduction of the diamondback moth,Plutella xylostella (Lepidoptera: Yponomeutidae)

Abstract Effects of hexaflumuron at 10% lethal concentration (LC₁₀) and LC₂₅ on development and reproduction parameters of the diamondback moth, Plutella xylostella (Linnaeus, 1753) (Lep.: Yponomeutidae) were investigated. Estimated LC₅₀, LC₁₀ and LC₂₅ values of leaf dip bioassay of hexaflumuron on the third instar larvae of the P. xylostella were 1.48, 0.59 and 0.91 mg/L, respectively. Hexaflumuron decreased pupal weight in the parent generation at sublethal concentrations but in the offspring generation, this effect was not observed. Sublethal concentrations increased egg, first and second larval instar and pupa developmental time and shortened life span of adults, but did not change the third and fourth larval instars and pre‐pupa developmental period. Also fecundity of females reduced significantly but hatchability of treatments and control were similar. Survival rate of pre‐adult stages declined significantly at LC₂₅ concentration. Reproduction parameters such as reproductive rate (R₀) and intrinsic rate of increase in sublethal concentrations were significantly lower compared with control, but gross reproduction rate (GRR) at the LC₁₀ concentration was increased and it could be hormoligosis. Also hexaflumuron significantly increased doubling time (Dt). We conclude that the sublethal effects of hexaflumuron might exhibit significant effects on the population dynamics of P. xylostella.     

Functional and genetic characteristics of Chlorantraniliprole resistance in the diamondback moth,Plutella xylostella (Lepidoptera: Plutellidae)

The diamondback moth (Plutella xylostella) is a globally distributed and important economic pest, and it has developed resistance to all conventional insecticide classes used in the field. Chlorantraniliprole is a new chemical class of insecticide that acts as a conformation‐sensitive activator of the insect ryanodine receptor (RyR). In the present study, a field strain (16.3‐fold resistance to chlorantraniliprole) was collected in Korea and lab‐selected with chlorantraniliprole for more than one year. The resulting strain presented 2,157‐fold resistance to chlorantraniliprole. A point mutation (G4946E) in the RyR gene was observed at a high frequency in the resistant strain. Enzyme assays indicated that glutathione S‐transferase (GST) and P450 activity in the resistant strain were 2.4‐ and 1.96‐times higher than that of the susceptible strain, respectively. The expression of the RyR, GST (sigma, omega, and zeta) and CYP321E1 gene was higher in the resistant strain than in the susceptible strain. The F₁ progeny resulting from reciprocal crosses did not reveal maternal effects or a diamide‐susceptible phenotype, which suggests an autosomal nearly recessive mode of inheritance. In addition, we surveyed the susceptibility to 13 insecticides (3 diamides, 2 synthetic pyrethroids, 2 spinosyns, 1 organophosphate, 1 oxadiazine, 1 avermectin, and 3 others) in the chlorantraniliprole‐resistant strain. The resistant strain exhibited high cross‐resistance to flubendiamide (5,910 fold) and showed no cross‐resistance to spinetoram, spinosad, indoxacarb, and metaflumizone. These results can serve as an important basis for guiding the use of insecticides in the field.     

利用RNAi技术沉默小菜蛾类钙粘蛋白基因

RNA干扰（RNA interference, RNAi）是一种调控基因表达的方法, 其通过体外合成一段与内源靶基因同源的双链RNA（dsRNA）或siRNA, 导入生物体内, 使内源靶基因中同源mRNA降解, 从而达到阻抑基因表达的目的。类钙粘蛋白（cadherin-like protein）是位于昆虫中肠刷状缘膜囊(brush border membrane vesicles, BBMV)上与钙粘蛋白(cadherin)结构相似的物质, 是多种昆虫体内Bt杀虫蛋白的受体。本研究利用基因特异引物通过RT-PCR扩增了小菜蛾类钙粘蛋白基因的2个片段（CAD1和CAD2）, 合成相对应的双链RNA（double-stranded RNA, dsRNA）; 并将dsRNA通过显微注射导入小菜蛾3龄幼虫体内, 测定了不同靶位点、不同剂量、不同检测时间对目的基因mRNA表达量的影响。结果表明: 将70 nL CAD1对应的dsRNA注射到幼虫体内48 h后, 基因表达量显著下降, 72 h后恢复。免疫印迹检测结果表明, 类钙粘蛋白在注射dsRNA 48 h后幼虫BBMV中的含量明显下降。本实验成功实现了小菜蛾类钙粘蛋白基因的沉默, 该体系的成功建立为利用RNAi技术分析小菜蛾及其他鳞翅目昆虫基因的功能提供了参考。