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1.
鉴定昆虫嗅觉相关蛋白基因并对其序列和时空表达进行研究,可为阐明昆虫与寄主间的化学通讯机制提供依据.本文新克隆并鉴定获得一个西花蓟马OBP基因FoccOBP3(GenBank登录号:MT682352),cDNA序列全长1226bp,读码框全长432bp,编码143个氨基酸残基.氨基酸序列中六个保守的半胱氨酸位点排列方式为... 相似文献
2.
为明确华北小麦穗期主要蚜虫种类及其生态位, 为京津冀地区小麦蚜虫预测预报和科学防控提供技术支持,采用五点式和棋盘式取样法系统调查了河北廊坊小麦穗期不同蚜虫种类的种群动态及其在植株上的分布, 利用生态位理论, 计算荻草谷网蚜Sitobion miscanthi (Takahashi)、禾谷缢管蚜Rhopalosiphum padi (Linnaeus)和麦无网长管蚜Metopolophium dirhodum (Walker) 3种优势蚜虫的生态位宽度和重叠度。禾谷缢管蚜的时空生态位最宽, 其次为荻草谷网蚜和麦无网长管蚜, 其中禾谷缢管蚜的生态位宽度随时间推移呈上升趋势, 其他两种蚜虫呈下降趋势。不同蚜虫种类之间存在生态位重叠, 其中荻草谷网蚜与禾谷缢管蚜的重叠度最大, 为2.073 0, 荻草谷网蚜与麦无网长管蚜的重叠度最低, 为1.656 4; 随时间推移, 荻草谷网蚜与禾谷缢管蚜之间的竞争趋于增强, 禾谷缢管蚜与麦无网长管蚜之间的竞争趋于减弱, 而荻草谷网蚜与麦无网长管蚜的竞争关系相对稳定。荻草谷网蚜是当地小麦蚜虫主要优势种群, 禾谷缢管蚜时空生态位宽度最大, 与荻草谷网蚜竞争激烈, 麦无网长管蚜时空生态位相对稳定。 相似文献
3.
荻草谷网蚜Sitobion miscanthi是严重威胁我国小麦生产安全的迁飞性害虫。蜕皮激素是参与蚜虫翅型分化调控的内激素, 在有翅成蚜体内保持高滴度, 且诱导后代产生更高比例的无翅蚜, 其进出靶细胞需要经过细胞膜上特定蛋白的转运。ATP结合盒转运蛋白家族G亚家族(ATP-binding cassette transporter G, ABCG)中的 ABCG1是通过跨膜转运昆虫类固醇、对蜕皮激素信号进行负调控的功能蛋白之一, 在蚜虫中尚未见报道。本文克隆了荻草谷网蚜ABCG1(SmisABCG1)基因, 并进行了序列比对、系统进化分析以及不同组织部位和发育时期表达模式分析。结果显示, SmisABCG1基因的开放阅读框全长为1 851 bp, 编码616个氨基酸, 含7个跨膜结构域, 符合ABCG蛋白家族典型结构特性, 基因登录ID:OP626323。昆虫间ABCG1较保守, 该蛋白系统进化关系与各自物种间亲缘关系的远近保持一致。其中, SmisABCG1与来自豌豆蚜、禾谷缢管蚜、棉蚜、花生蚜和雪松长足大蚜等的ABCG1氨基酸序列高度一致(>87%), 以上蚜虫聚为一支。与SmisABCG1亲缘关系最近的是豌豆蚜的ABCG1, 其次是半翅目的褐飞虱、白背飞虱和灰飞虱, 与膜翅目的新疆菜叶蜂、阿里山潜蝇茧蜂以及鞘翅目的赤拟谷盗、蜂箱小甲虫亲缘关系较远。该基因在伪胚胎和成蚜阶段高表达。包含伪胚胎的有翅、无翅成蚜整蚜SmisABCG1的转录水平无显著差异, 但其在来自有翅成蚜的伪胚胎中的转录水平高于无翅成蚜伪胚胎, 证实无翅成蚜自身的转录水平较高, 而有翅成蚜较低。进一步分析显示这一差异主要是无翅蚜胸部显著高表达所导致。基于该蛋白对蜕皮激素负调控, 与有翅成蚜转录水平低, 但蜕皮激素水平更高相符合。 相似文献
4.
在实验室条件下,在特定空间内,测定异色瓢虫显明变种对两种蚜虫荻草谷网蚜和禾谷缢管蚜不同密度值下的捕食量。结果表明,荻草谷网蚜和禾谷缢管蚜种群数量同步增加时,EG-S值和EI值变化是从1到∞,EI值是在0到+1范围内依次增加,表明异色瓢虫显明变种喜好捕食荻草谷网蚜明显高于禾谷缢管蚜;荻草谷网蚜数量不变,禾谷缢管蚜数量增加时,EG-S值和EI值是从+1到0,EI值从-1到0范围内依次减少,表明异色瓢虫显明变种明显喜好捕食禾谷缢管蚜;禾谷缢管蚜数量不变,荻草谷网蚜数量增加时,EG-S值和EI值变化从+1到∞,EI值在0到+1范围内依次增加,表明异色瓢虫显明变种明显喜好捕食荻草谷网蚜。捕食量结果同选择指数。 相似文献
5.
采用RT-PCR及RACE技术克隆了三叶斑潜蝇Hsp90基因全长cDNA序列,并用实时定量RT-PCR的方法检测其在不同发育阶段受到高温胁迫后的表达水平。该基因的cDNA序列全长2 408 bp,开放阅读框为2 145 bp,编码714个氨基酸;5′非编码区为151 bp,3′非编码区为112 bp。该基因推导的氨基酸序列与其他昆虫同源序列比较有很高的相似性(80%~99%)。聚类分析结果显示三叶斑潜蝇与美洲斑潜蝇和南美斑潜蝇的亲缘关系最近。实时荧光定量PCR检测结果表明三叶斑潜蝇Hsp90基因的表达受到热胁迫的诱导,诱导3龄幼虫最大表达量的温度比诱导其他发育阶段的温度低,在43 ℃时预蛹和蛹的表达量在整个生命周期中最高,在检测的高温胁迫条件下,雄虫比雌虫的表达量更高。该结果为阐明三叶斑潜蝇胁迫耐受能力及其对其他潜蝇种群的取代机制奠定了分子基础。 相似文献
6.
过氧化物酶(POD)是昆虫体内一种很关键的抗氧化酶,在维持昆虫体内氧化还原的动态平衡及保护昆虫免受氧化损伤方面起到重要的作用。本试验通过转录组测序方法获得一条粘虫过氧化物酶基因的cDNA序列,该序列命名为MsPOD(GenBank登录号:MH606240)。该序列全长2433 bp,开放阅读框长度为2061 bp,编码686个氨基酸组成的多肽,分子量约76.1 ku,等电点5.68,具有1个标志性的动物亚铁血红素过氧化物酶细胞粘附蛋白结构域。氨基酸序列比对表明,MsPOD的氨基酸序列与鳞翅目夜蛾科其他昆虫亲缘关系较近,其中与棉铃虫POD氨基酸序列同源性最高,达92%。基因表达水平研究发现,MsPOD基因在不同发育阶段和不同组织中差异表达,在蛹期和唾腺中表达量最高。温度梯度诱导后,MsPOD基因在不同时间点的表达量具有显著差异,经35℃下12 h处理后表达量最高。研究结果为进一步研究过氧化物酶在昆虫体内的保护性作用以及利用该基因进行分子设计来防治粘虫奠定理论基础。 相似文献
7.
热激蛋白在昆虫抵御温度胁迫和药剂胁迫反应中具有重要作用。本试验通过高通量测序获得一条大豆蚜热激蛋白基因的cDNA序列,该序列全长2982 bp,含1个长度为2052 bp的开放阅读框,编码683个氨基酸组成的多肽,多肽等电点约为6.30,分子质量约为77.8 kDa;推导的氨基酸序列与棉蚜Aphis gossypii HSP75同源性高达99.12%,属于hsp 75家族。我们把该基因定名为Aghsp75,已提交至GenBank(登录号为MN068810)。Aghsp75通过不同浓度吡虫啉药剂和不同温度胁迫成蚜后发现,经LC50吡虫啉浓度胁迫3、6和24 h时以及在LC30浓度吡虫啉胁迫12 h时该基因表达量显著升高;经6℃处理6 h时以及36℃处理3 h和6 h时该基因表达量显著升高。本研究表明该基因可能参与大豆蚜的抗逆过程,为利用分子生物技术手段防治大豆蚜提供理论保障。 相似文献
8.
克隆获得桃蚜电压门控钠离子通道基因cDNA序列,明确钠离子通道的典型特征,为研究桃蚜抗性分子机理奠定基础。采用实验技术主要有RT-PCR和PCR,克隆桃蚜钠离子通道基因cDNA序列,利用相关软件对其序列进行生物信息学分析。克隆得到两段cDNA序列MpNav-1(NCBI登录号:MN124170)和MpNav-2(NCBI登录号:MN176136)。MpNav-1长度为2945 bp,包括2877 bp的完整开放阅读框,共编码958个氨基酸;MpNav-2长度为3546 bp,包括3486 bp的完整开放阅读框,共编码1161个氨基酸。MpNav-1和MpNav-2共同组成桃蚜的钠离子通道α亚基,MpNav-1包含同源结构域Ⅰ和同源结构域Ⅱ,MpNav-2包含同源结构域Ⅲ和同源结构域Ⅳ。同源比对发现,桃蚜与豌豆蚜和高粱蚜钠离子通道基因相似度分别高达97.67%和97.65%,所克隆序列包含昆虫钠离子通道α亚基典型特征,具有MFM模块,并含有蚜虫类钠通道特有模块DENS。成功地克隆桃蚜钠离子通道基因,为阐明其对拟除虫菊酯类药剂产生靶标抗性的分子机制奠定基础。 相似文献
9.
异色瓢虫乳酸脱氢酶基因的克隆与序列分析 总被引:1,自引:0,他引:1
乳酸脱氢酶(1acticdehydrogenase,LDH)是糖酵解途径的终止酶,在整个昆虫的发育阶段长期存在。本试验采用同源克隆和锚定PCR技术,从异色瓢虫Harmoniaaxyridis中克隆到HaxLDH基因的cDNA全序列(GenBank登录号HM362898),全长1336bp,包含214bp的3’非编码区域和123bp的5,非编码区域,可读框长999bp,编码332个氨基酸。通过软件分析,预测该基因编码蛋白的分子量为36.2kD,理论等电点为8.62;包含1个糖基化位点,无信号肽序列和跨膜结构。同源比对不同昆虫的LDH基因cDNA序列,发现HaxLDH拥有8个非常保守的结构域:DLQHG、TAGV/ARQK/RE/DGES/TRL、LVQRN、GSGTNLD、SCHGW/YI/VI/VGEHGD、VWSG/AVNV/IAGV、AYEV/IIK/RLKGYTS/NWAI/VGLS和LSLP。HaxLDH与赤拟谷盗Triboliumcastaneum的LDH同源性最高,达67%;系统发育分析也表明二者亲缘关系较近。本研究为探讨LDH在昆虫发育和逆境中的作用奠定了基础。 相似文献
10.
克隆获得麦长管蚜电压门控钠离子通道基因cDNA序列,明确其典型特征,为研究麦长管蚜抗性分子机理奠定基础。采用RT-PCR技术,克隆麦长管蚜钠离子通道基因cDNA序列,利用DNASTAR Lasergene 7.10软件对其序列进行分析。克隆得到两条cDNA序列SaNav1和SaNav2(GenBank登录号分别为MN176137和MN161584),SaNav1序列长3423 bp,共编码1141个氨基酸;SaNav2序列长2874 bp,共编码958个氨基酸。同源比对发现,SaNav1与禾谷缢管蚜和桃蚜的第一部分钠离子通道基因相似度分别高达97.81%和97.91%;SaNav2与禾谷缢管蚜和桃蚜的第二部分钠离子通道基因相似性高达97.90%和96.43%。所克隆序列包含4个同源结构域,每个结构域6个跨膜片段(S1~S6),存在钠通道选择性关键残基“DENS”。本文成功克隆了麦长管蚜中钠离子通道基因,为麦长管蚜钠离子通道抗性机制的研究提供依据。 相似文献
11.
兼抗麦长管蚜和大麦黄矮病毒的小麦种质田间鉴定筛选 总被引:1,自引:1,他引:0
为鉴定筛选兼抗麦长管蚜和大麦黄矮病毒(Barley yellow dwarf virus, BYDV)的小麦种质,采用自然感蚜/感病系数法,对36个外引和远缘杂交选育的小麦种质材料进行了2年的田间鉴定,并分析了感虫性与感病性的相关关系。结果表明,2年中均兼抗麦长管蚜和BYDV的种质仅有KOKIPPCAS、KOK、Amigo-3和PI137739共4个材料,占总鉴定材料的11.11%;对二者均敏感的有98-10-35q-9、186Tm39、Tam200e12-14a、Tam200(27)7、小偃22、西农1376和小偃6号共7个材料,占19.44%。其它材料仅抗虫或仅抗病,或仅在一年中表现抗病或抗虫,如材料98-10-30和98-10-35a8抗麦长管蚜,但对BYDV敏感;材料Tam200(13)G和PIG23(2)C感蚜,但对BYDV有抑制作用。BYDV发生普遍率(发病株率)和严重度(病情指数)与有蚜株率显著相关,严重度还与感蚜指数显著相关,但感病植株的病级均值与有蚜株率无显著相关性。表明自然界长期的进化和选择使许多抗病虫基因得以保存下来,但较多抗性基因只在抗病或抗虫的某一方面表现有效,需给予更多关注。 相似文献
12.
Barley yellow dwarf (BYD) is one of the main viral diseases of small-grain cereals. This disease, reported on numerous plant
species of the Poaceae family, is caused by a complex of eight viral species including the species Barley Yellow Dwarf Virus-PAV (BYDV-PAV), frequently found in western Europe. Resistance sources against BYDV-PAV are scarce and only identified in perennial
Triticineae. Some BYDV-resistant wheat lines have been obtained by introgressing these resistances into bread wheat germplasms. Genetic
and biological characterization of the resulting lines has been undertaken. However, little information on the resistant behaviour
of these lines during the early stages of the infection process is available. To evaluate the resistance of two genetically
distinct resistant lines (Zhong ZH and TC14), 1740 young plantlets, belonging to susceptible reference hosts (barley cv. Express and wheat cv. Sunstar), Zhong ZH or TC14 wheat lines, were inoculated in controlled conditions with French BYDV-PAV isolates. The infection process was monitored
during the first 21 days after inoculation (DAI) using a semi-quantitative ELISA. A standardized protocol including five successive
samplings of leaves from all inoculated plants and the collection of plant roots at the end of the monitored period was carried
out. This protocol enabled an assessment of the infection percentage and the evolution of the viral load in plants from the
7th DAI to the 21st DAI. Statistical analyses of the BYDV infection kinetics using raw ELISA data, a model of the time-dependent
variation of the percentage of infected plants and the area under concentration progress curves (AUCPC) demonstrated that
Zhong ZH and TC14 lines (1) reduce the development rate of the BYD disease during the first days of infection, (2) decrease the infection efficiency
of BYDV-PAV isolates, in the leaves, from 98.7% for susceptible plant genotypes to 81.9% and 71.7% for Zhong ZH and TC14, respectively, (3) reduce the virus load in the leaves of infected plants and (4) are not spared from BYDV infection, as
95.1% of Zhong ZH and 90.2% of TC14 inoculated plants accumulated viral particles in roots and/or in leaves at 21 DAI. These results confirm the BYDV-partial
resistant behaviour of both Zhong ZH and TC14 lines. The development rate of the disease was the single parameter that allowed the distinction between the two resistant
sources present in the tested lines. 相似文献
13.
为扩大黑肩绿盲蝽Cyrtorhinus lividipennis的人工繁殖规模,利用RNA-seq技术对饥饿胁迫2 d的黑肩绿盲蝽雌成虫进行转录组测序分析,筛选参与生殖调控的相关信号通路,挖掘直接或者间接影响生殖的相关基因,采用实时荧光定量PCR(real-time fluorescence quantification PCR,qRT-PCR)对筛选的相关基因进行验证,并通过试验分析沉默S6K基因和饥饿处理对黑肩绿盲蝽生殖的影响。结果显示,与取食褐飞虱Nilaparvata lugens卵(CK)的黑肩绿盲蝽相比,饥饿处理2 d的黑肩绿盲蝽雌成虫有11 675个基因差异表达,其中有4 264个基因表达量上调,7 411个基因表达量下调。共筛选到7条与生殖调控相关的信号通路和6个与生殖调控相关的基因,除TSC2基因表达量上调外,其他S6K、INSR、Akt、HSP70-1、HSP70-2五个与生殖相关基因的表达量在7条生殖相关信号通路中均下调。qRT-PCR检测结果与转录组测序结果一致,说明转录组分析结果可靠。沉默S6K基因后,黑肩绿盲蝽雌成虫脂肪体和卵巢蛋白质含量、Vg基因表达量、雌成虫产卵量和Vg含量较对照显著降低。此外,饥饿处理2 d后黑肩绿盲蝽雌成虫产卵量也较对照显著减少。表明饥饿胁迫后黑肩绿盲蝽雌成虫的生殖相关通路可能受多个信号通路调控,S6K表达量下降显著影响黑肩绿盲蝽的生殖。 相似文献
14.
Florian Chain Gérard Riault Maxime Trottet Emmanuel Jacquot 《European journal of plant pathology / European Foundation for Plant Pathology》2007,117(1):35-43
Serial passage experiments (SPE) of a Barley yellow dwarf virus-PAV (BYDV-PAV) isolate were performed on Zhong ZH and TC14 wheat lines to evaluate the durability of their resistance to BYDV. At different passage numbers (from the 2nd to the 114th), biological properties of the produced isolates were recorded either by monitoring infection percentages and virus titers of the first 3 weeks of viral infection or by measuring their impact on yield components. Statistical analyses using the area under pathogen progress curves and the area under concentration progress curves demonstrated that these two resistant lines induce, after only a few passages, a selection of variant(s) with significantly modified infection abilities. Isolates resulting from SPE performed on these lines induced important decreases of yield components. These results indicate that the use of Zhong ZH and TC14 lines in BYDV-resistant breeding programmes should be approached with caution. 相似文献
15.
为探讨UV-B胁迫对烟蚜Myzus persicae热激蛋白Hsp90基因表达量的影响,采用RT-PCR与RACE技术克隆了烟蚜热激蛋白Hsp90基因的全长,并对其进行生物信息学分析,利用实时荧光定量PCR技术研究了烟蚜Hsp90基因在不同时长UV-B胁迫下的表达量变化。结果表明,烟蚜Hsp90基因的cDNA全长为2 670 bp,编码728个氨基酸,编码蛋白质的相对分子量为82.6 kD,等电点为4.95,获得的氨基酸序列具有Hsp90蛋白家族的1个签名序列及C末端MEEVD基序,推测其属于胞质型热激蛋白。系统进化树结果显示,烟蚜Hsp90与其它昆虫Hsp90具有很高的相似性。实时荧光定量PCR结果表明,不同时长UV-B胁迫下烟蚜Hsp90均有表达,随着照射时间延长,Hsp90表达量表现为先上升后下降的趋势;与对照相比,照射时间为15、30、60、90和120 min时,Hsp90表达量均显著升高,且在60 min时Hsp90表达量达最大,是对照组的2.05倍。表明Hsp90基因在不同时长UV-B胁迫下差异表达,在烟蚜适应紫外胁迫的分子机制中具有重要作用。 相似文献
16.
New experimental hosts of Barley yellow dwarf virus among wild grasses,with implications for grassland habitats 
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下载免费PDF全文 Barley yellow dwarf virus (BYDV), an economically important virus, infects small grain cereal crops and over 150 other Poaceae species. BYDV infection plays an important role in competition among grasses in non‐managed systems, but many grasses remain unexamined as potential BYDV hosts. This study examined grass species that have not been reported as BYDV hosts but are commonly encountered in non‐managed grasslands throughout the United States and Canada. Laboratory inoculations with BYDV‐PAV using the aphid vector Rhopalosiphum padi were performed to examine the ability of 13 grass species and barley to be infected with the virus; eight of the grass species were not documented previously as virus hosts. Serological and molecular assays were used to confirm BYDV‐PAV infection. Plant height, number of leaves, number of tillers and weight were recorded to evaluate susceptibility or sensitivity to BYDV. Infection with BYDV was experimentally achieved for the first time on Achnatherum lettermanii, Achnatherum occidentale, Achnatherum thurberianum, Danthonia intermedia, Poa fendleriana, Sporobolus airoides and Sporobolus cryptandrus, but not on Alopecurus pratensis and Elymus wawawaiensis. Infection was confirmed in Bromus inermis, Elymus elymoides, Poa bulbosa, Poa secunda and Hordeum vulgare, which served as controls. BYDV infection caused reductions in plant height on P. bulbosa and P. fendleriana. BYDV‐infected P. secunda had more leaves per plant compared to healthy plants of the same species. BYDV‐infected A. lettermanii exhibited reduced dry weight in both below‐ground and above‐ground tissue. These findings have implications for the management and conservation of grassland habitats. 相似文献
17.
Interactions between Barley yellow dwarf virus (BYDV) and Fusarium species causing Fusarium head blight (FHB) in winter wheat cvs Agent (susceptible to FHB) and Petrus (moderately resistant
to FHB) were studied over three years (2001–2003) in outdoor pot experiments. FHB developed more rapidly in cv. Agent than
in cv. Petrus. The spread of FHB was greater in BYDV-infected plants than in BYDV-free plants. Thousand grain weight (TGW)
was reduced more in Fusarium-infected heads of cv. Agent than in cv. Petrus. A highly significant negative correlation was found between disease index
and TGW in cv. Agent (r = −0.916), while in cv. Petrus the correlation was less significant (r = −0.765). Virus infection reduced TGW in cv. Petrus more than in cv. Agent. In plants with both infections, TGW reductions
in cv. Petrus corresponded to those of BYDV infection, and in cv. Agent TGW was more diminished than in BYDV infection. Effects
of different treatments determined over three years on ergosterol contents in grain were generally similar to effects on disease
indices. Grain weight per ear and ear weight of the different treatments of both cultivars largely corresponded with the TGW
results. Deoxynivalenol (DON) content in grain of cv. Agent infected with Fusarium spp. was 11–25 times higher compared to the corresponding treatments in cv. Petrus. The DON content in grain of plants of
the two cultivars infected with both pathogens was higher than that of plants infected only with Fusarium over the three years. 相似文献
18.
为拓展和获取对荻草谷网蚜Sitobion miscanthi表现稳定的小麦抗源,以我国146个小麦品种(系)为材料,利用2020年麦田蚜虫发生严重的机会,采用有蚜株蚜害级别计算抗蚜指数,采用耐蚜值(调查株蚜害级别/千粒重损失率)计算耐蚜指数,以此评估小麦的抗蚜性水平和耐蚜性水平;2022年利用人工辅助接蚜的方法对2020年表现稳定的部分小麦品种(系)的评估结果进行验证。结果显示,在自然感蚜条件下2个试验点6次调查中仅山农116、泉麦31和濮麦116表现稳定的抗蚜性,在人工接蚜时仅郑麦132表现稳定的抗蚜性;中育1220、泰禾麦2号和瑞华1408在自然感蚜时蚜量较低,千粒重损失率低于5.00%,人工接蚜亦表现良好的耐蚜性,表明其兼具耐蚜性和一定的抗蚜性;泰麦601、瑞华592、轮选166和中农麦4007在自然感蚜的高蚜量情况下和人工辅助接蚜时均能保持较低的千粒重损失率(小于15.00%),表明成株期小麦的抗蚜性减弱是一种普遍现象,耐蚜性是比抗蚜性更稳定的遗传特征。 相似文献
19.
为探究青杨天牛Saperda populnea幼虫低氧适应的分子机制,分别对青杨天牛幼虫进行常氧(21%氧浓度)、中度缺氧(14%氧浓度)和重度缺氧(7%氧浓度)处理,采用高通量测序技术对低氧胁迫下青杨天牛进行转录组测序与组装、功能注释与分类、差异基因筛选与分析,采用实时荧光定量PCR(quantitative real-time PCR,qPCR)技术对转录组测序结果进行验证。结果表明,与常氧处理相比,14%和7%氧浓度处理下青杨天牛幼虫显著差异表达基因数分别为31个和1 525个。低氧胁迫后青杨天牛幼虫的显著差异表达基因功能主要富集到跨膜转运蛋白活性、细胞或亚细胞组分运动、微管运动等。低氧胁迫后青杨天牛幼虫差异表达基因代谢通路主要富集到氮代谢、蛋白质消化吸收、昼夜节律和环磷酸腺苷(cyclic adenosine monophosphate,cAMP)信号通路等。qPCR检测结果与转录组测序结果一致,表明转录组测序结果可靠。 相似文献
20.
Dna J蛋白是Dna K/Hsp70的辅助分子伴侣,通过调节Hsp70的ATPase活性来影响蛋白复合体的合成与组装。为明确舞毒蛾Lymantria dispar的LdDnaJ1基因特性及对杀虫剂甲萘威的胁迫响应,通过克隆LdDnaJ1全长基因并运用实时荧光定量RT-PCR技术测定了甲萘威对其LdDnaJ1基因表达量的影响。结果表明,舞毒蛾Ld Dna J1全长基因开放阅读框为1 062 bp,编码353个氨基酸,分子质量为39.91 kD,理论等电点为5.65;舞毒蛾Dna J与柑橘凤蝶Papilio xuthus Dna J亲缘关系较近。甲萘威对舞毒蛾2龄幼虫24 h和48 h的致死中浓度LC50分别为74.04 mg/L和31.48mg/L。低剂量(LC_5、LC_(10)和LC_(30))甲萘威胁迫下,舞毒蛾2龄幼虫Ld Dna J1基因表达量均下调,LC_(30)甲萘威处理后72 h时LdDnaJ1基因表达量最低,仅为对照的15.70%。表明甲萘威可抑制舞毒蛾LdDnaJ1基因的表达,且呈现明显的时间和剂量效应。 相似文献