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变态发育是昆虫适应生态环境和气候变化的主要生存策略之一.保幼激素(juvenile hormone,JH)和蜕皮激素(20-hydroxyecdysone,20E)的相互作用主要调控昆虫组织凋亡和重建、蜕皮等变态生理活动,近年来保幼激素和蜕皮激素调控昆虫变态发育的分子机制取得了较大的进展.本研究总结了JH和20E的合成... 相似文献
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保幼激素的分子作用机制 总被引:1,自引:0,他引:1
蜕皮激素(ecdysteroids, Ecd)和保幼激素(juvenile hormone, JH)是调控昆虫发育和变态的两种最为重要的昆虫激素。尽管Ecd的分子作用机制已经相当明了;但是;因为迄今为止还没有成功地鉴定出JH受体;人们对JH的分子作用机制还了解甚少。本文从三个方面较为详尽地介绍了近年来JH分子作用机制的相关研究进展:1) JH和Ecd在分子水平上相互作用; JH可以通过改变或者抑制Ecd信号来调控昆虫的发育和变态;2) JH核受体的两个候选基因为Met和USP;3) JH还可以通过膜受体和蛋白激酶C传导信号。 相似文献
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随着分子生物学技术的快速发展,对生态环境中各类生物的研究,包括对生物某些特定基因结构和功能的研究等逐步拓展和加深。保幼激素(Juvenile Hormone,JH)是由咽侧体(Corpus Allatum,CA)分泌的,在昆虫发育、变态和生殖过程中起重要作用的激素。目前对JH信号传导途径的作用机理还不十分清楚。现有研究表明,Kruppel homolog-1(Kr-h1)是一种含C2H2锌指结构的转录因子,处于保幼激素信号途径下游,在保幼激素信号通路中起着重要作用。已报道的Kr-h1基因的功能主要包括:调控幼虫生长发育和变态,与蜜蜂的觅食行为密切相关,参与果蝇幼体神经细胞的形成等等。对就近十年来Kr-h1基因的特性和功能研究作一个综述以了解不同昆虫中保幼激素的分子作用机制,为开发生物农药奠定理论基础,也为维护良好的生态环境作出理论贡献。 相似文献
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【目的】保幼激素(juvenile hormone, JH)在小麦吸浆虫Sitodiplosis mosellana滞育诱导及滞育后静息状态的维持中发挥着重要作用。保幼激素酯酶(hormone esterase, JHE)和保幼激素环氧水解酶(juvenile hormone epoxide hydrolase, JHEH)是调控JH滴度的重要降解酶。本研究旨在探讨JHE和JHEH在小麦吸浆虫滞育和变态发育中潜在功能。【方法】通过RT-PCR和RACE技术从小麦吸浆虫滞育前幼虫克隆JHE和JHEH全长cDNA序列;利用生物信息学软件分析其核苷酸及编码蛋白特性;采用qPCR技术分析其在小麦吸浆虫滞育不同时期(滞育前、滞育期、滞育后静息期和滞育后发育)3龄幼虫及1龄幼虫到成虫不同发育阶段(1-2龄幼虫、预蛹、初蛹、中蛹、后蛹、雌成虫和雄成虫)中的表达水平。【结果】克隆获得了cDNA全长分别为3 102和1 980 bp的小麦吸浆虫SmJHE和SmJHEH基因(GenBank登录号分别为 MG876768和MG876769),其开放阅读框分别长1 740和1 371 bp,分别编码579和456个氨基酸,预测蛋白分子量分别为65.67和51.65 kD。SmJHE蛋白含有5个JHE家族特有的保守模块,SmJHEH含有催化三联体Asp228,Asp404和His431及组成阴氧离子洞的两个Tyr(Tyr299和Tyr374)和HGWP花样结构。序列比对和进化分析表明,SmJHE和SmJHEH均与双翅目(Diptera)长角亚目(Nematocera)昆虫同源蛋白氨基酸序列一致性较高,亲缘关系最近。不同滞育时期的表达模式表明,SmJHE和SmJHEH在滞育前期(1龄到滞育前的3龄幼虫早期)表达量变化不明显,进入滞育后表达量基本维持恒定,但均在滞育后静息阶段的当年12月至翌年1月最低。发育表达模式表明,幼虫恢复发育后SmJHE表达量逐渐升高,预蛹期达到最高,在雌成虫中的表达量显著低于雄成虫中的;SmJHEH表达量则在预蛹期最低,在雌成虫中最高。【结论】SmJHE和SmJHEH参与小麦吸浆虫滞育调控,其表达量的降低与滞育后静息阶段JH的累积有关;SmJHE在发育过程中表达量的升高可能参与幼虫到蛹的变态,表达量的降低可能与生殖发育有关。 相似文献
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保幼激素生物合成研究进展 总被引:1,自引:0,他引:1
保幼激素(juvenile hormone,JH)是存在于昆虫、甲壳动物和部分植物体内的倍半萜类衍生物。在昆虫和甲壳动物体内,保幼激素主要调节变态和生殖活动。在植物体内,则可能作为异株克生物质发挥作用。保幼激素主要通过细胞质内的甲羟戊酸途径(MVA)合成,植物质体内存在萜类合成的1-去氧木糖-5-磷酸途径(DXP)。MVA和DXP途径通过单向质子协同运输系统进行协调,使DXP途径中形成的前体化合物参与MVA途径的倍半萜合成。JH生物合成的主要步骤己基本查明,但与合成相关的酶学研究还较薄弱。生物合成酶的分子生物学是近来研究的热点,相关酶的cDNA克隆已有报道。JH生物合成酶的进一步研究有助于查明JH生物合成调控机制,深化对节肢动物生殖的理解,还可为新型杀虫剂开发提供可能的靶标。 相似文献
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【目的】昆虫烯虫酯耐性(methoprene-tolerant, Met)蛋白属于bHLH/PAS转录因子家族成员,其与该家族其他成员形成的复合物可介导保幼激素(JH)的信号传导。本研究旨在克隆并表达小菜蛾Plutella xylostella JH受体Met蛋白基因PxMet-1和PxMet-2,纯化其蛋白,分析PxMet-1与PxMet-2与JH的结合模式,为进一步探明PxMet蛋白的功能提供依据。【方法】基于NCBI数据库,克隆验证了小菜蛾PxMet-1和PxMet-2基因的cDNA序列;把这两个基因分别与pGEX-KG载体连接构建表达载体pGEX-KG-PxMet-1和pGEX-KG-PxMet-2,导入大肠杆菌Escherichia coli Rosetta (DE3)使其表达;分别使用HisTrapTM HP与 GSTTrapTM HP的5 mL柱对PxMet-1和PxMet-2融合蛋白进行纯化;利用分子对接预测软件分析PxMet-1和PxMet-2蛋白与JH的结合模式。【结果】克隆获得的小菜蛾PxMet-1(GenBank登录号:MK697672)和PxMet-2(GenBank登录号: MT996234)序列与已报道的序列基本一致,仅PxMet-2基因序列存在1个非同义突变,突变位点为第41位氨基酸,由甘氨酸(Gly)突变为丙氨酸(Ala)。PxMet-1与PxMet-2蛋白三维结构相似,均包含典型的螺旋-环-螺旋结构。体外原核表达获得具有His和GST双标签的可溶性PxMet融合蛋白,PxMet-1融合蛋白的最优表达条件为0.3 mmol/L的IPTG在16℃下诱导16 h,PxMet-2融合蛋白的为0.1 mmol/L的IPTG 在16℃下诱导16 h。PxMet-1和PxMet-2分别经150 mmol/L咪唑和20 mmol/L还原型谷胱甘肽洗脱获得高纯度的融合蛋白。SDS-PAGE和Western blot验证PxMet-1和PxMet-2融合蛋白,分别在89.2和106 kD位置获得条带,与推测大小一致。分子对接分析结果显示,PxMet-1和PxMet-2与JH存在相互作用位点,都是在PAS B保守结构域,和赤拟谷盗Tribolium castaneum Met的JH结合位点相同。【结论】利用pGEX-KG原核表达系统能有效地在体外表达可溶性的PxMet-1和PxMet-2蛋白,PxMet-1和PxMet-2蛋白很可能是小菜蛾JH的分子受体。本研究为进一步解析PxMet蛋白的功能,深入阐明JH调控小菜蛾发育与生殖的分子机理奠定了基础。 相似文献
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Franz Engelmann Jaroslava Mala David Borst 《Archives of insect biochemistry and physiology》1988,8(1):11-23
The concentration of the juvenile hormone-binding protein (JHB) in hemolymph was determined throughout the last nymphal instar. It was found to be 3.9 μM at the molt to the instar, rising to 13 μM by mid-instar, and dropping to 6.7μM the day before emergence. Endocrine control of its production during the last nymphal instar could not be established. The apparent juvenile hormone esterase (JHF) activity was low at the molt to the last instar, but rose about fivefold by mid-instar, and then modestly declined. On the day of emergence, JHF activity rose to the highest level observed. A four- to fivefold increase in absolute JHF activity was determined during the first half of the last nymphal instar. This increase is not regulated by JH. Removal of the JHB from hemolymph samples by precipitation with a polyclonal specific antibody increased the JHF activity up to 1,000-fold. Thus, changes in the concentrations of JHB can affect the apparent activity of JHE, which is unrelated to the production or degradation of the JHF. 相似文献
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The juvenile hormone esterase (JHE) activity in Galleria mellonella larvae was measured after exposure to different experimental conditions that affect larval-pupal transformation. The data show that stimulation of production of JHE is closely coupled with the developmental signals that intiate larval-pupal metamorphosis. Injury, which delays pupation, delays the appearance of JHE activity if the larvae are injured within 48 hr after the last larval moult. Chilling of day-0 larvae induces a supernumerary larval moult and inhibits the appearance of JHE. However, JHE activity increases in chilled larvae when their commitment for an extra larval moult is reversed by starvation. Starvation is effective in reversing the commitment for an extra larval moult if commenced within 48 hr after chilling, thereby suggesting a critical period for that commitment. These data suggest that the stimulus for JHE synthesis and/or release occurs approximately within 48 hr after the last larval ecdysis. A series of studies involving implantation of brain, suboesophageal ganglion and fat body into chilled, as well as chilled and ligated larvae suggest that a factor from the brain is involved in stimulation or production of JHE in Galleria larvae.JH, which suppresses JHE activity in day-3, -5 and early day-6 Galleria larvae, stimulates the production of JHE in late day-6 larvae, suggesting that reprogramming in larval fat body may occur on day 6 of the last larval stadium. 相似文献
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J. A. Ottea L. G. Harshman Bruce D. Hammock 《Archives of insect biochemistry and physiology》1988,8(1):25-37
A thin-layer chromatographic assay was developed for the resolution of hydrolytic and conjugative catabolites of juvenile hormone (JH). A single-dimension, dual-development thin-layer system allowed complete resolution of the catabolites. Thus, this system provided a means for the rapid and economic analysis of JH hydrolysis even when different hydrolytic activities were present concurrently. Purified hydrolytic enzymes were found to be superior to chemical methods for the generation of small amounts of standards of JH catabolites. The relative levels of activities of an epoxide hydrolase and an esterase toward JH III were found to be similar in microsomal preparations from three lines of adult Drosophila melanogaster isolated from a field population. However, selection of flies by exposure to cut orange resulted in the elevation of levels of epoxide hydrolase activities, whereas esterase levels were not affected to the same extent. The formation of the JH acid-diol was not detected under the conditions of this study, suggesting that the JH acid and diol were not good substrates for epoxide hydrolase and juvenile hormone esterase, respectively. 相似文献
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Previous research on Monarch butterflies has shown that juvenile hormone (JH) stimulates the development of the ovary and certain reproductive glands of both sexes. Ecdysterone injections into intact Monarchs demonstrate that low doses of this hormone inhibit ovarian development, and higher doses stimulate the male and female reproductive glands. In addition, experiments using neckligatured adults show that ecdysterone stimulates the reproductive glands of both sexes, in the apparent absence of JH, with the most pronounced effect being observed on the female colleterial gland. Other studies with neck-ligatured animals demonstrate that ecdysterone also synergizes with JH on the female gland and all three male glands. The feasibility of using Monarch reproductive glands for studies on the mode of action and interaction of JH and ecdysterone, and the possibility of a rôle of ecdysterone in the normal regulation of Monarch oögenesis, are discussed. 相似文献
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The possible role of juvenile hormone (JH) in the induction and termination of larval diapause in the European corn borer, Ostrinia nubilalis, was investigated using topical applications of both JH I and a JH mimic as well as by monitoring JH titers with the Galleria bioassay. Neither JH nor the JH mimic ZR515 was capable of influencing diapause termination when administered topically. The Galleria bioassay revealed little or no JH in the hemolymph of mid diapause (>30 days) insects, indicating no demonstrable role for JH in diapause maintenance. When ZR515 was administered to nondiapause, newly ecdysed fifth instar larvae the pupal molting cycle was delayed. By use of photoperiodic regimes we were able to show that the molting delay was not equivalent to diapause induction. The Galleria bioassay showed differences in JH titer profiles between diapause and nondiapause animals during the final larval stadium. The nondiapause insects showed titers that decline rapidly to trace amounts following the molt to fifth instar then rose prior to pupation. The diapause insects had generally higher titers and exhibited a more gradual decline after the molt. No evidence was obtained to support the hypothesis that JH plays a key role in the induction, maintenance, or termination of larval diapause. 相似文献
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The juvenile hormone analogue ZR 515 has specific effects on ecdysone-induced metamorphic differentation of Drosophila cells cultured in vitro. The number of vesicles containing imaginal cuticular structures is reduced to 10% of control levels. Similarly, the differentiation of adult fat body is partly inhibited by ZR 515. The differentiation of adult tubular and fibrillar muscles, however, is not affected. ZR 515 does not inhibit cuticle secretion by tracheal cells and larval epidermal cells. 相似文献
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Grace Jones Keith D. Wing Davy Jones Bruce D. Hammock 《Journal of insect physiology》1981,27(2):85-91
Brain (median or lateral regions) or suboesophageal ganglion (SOG) homogenates of Day 1 fifth instar larvae of Trichoplusia ni induced the appearance of haemolymph juvenile hormone esterase (JHE) when injected into Day 1, Day 2 or early Day 4 fifth instar ligated hosts. Brain and SOG homogenates of late fourth instars also induced JHE when injected into Day 1 hosts, whole late fifth instar and pupal tissue did not. The pattern of JHE induction by early fourth through Day 3 fifth instar brain and SOG homogenates correlated with natural haemolymph JHE activity occurring at these times. Implantation of late fourth and Day 1 fifth instar brains and/or SOG into similar age hosts similarly induced JHE activity while prothoracic and abdominal ganglia did not. The relative levels of induction following implantation were SOG<brain<brain+SOG. JHE activity which appears in the haemolymph following injection of brain homogenates appears to be largely due to a single enzyme which has an isoelectric point indistinguishable from that of the natural haemolymph enzyme. Evidence is presented which suggests that inhibitory as well as stimulatory brain factors are involved in JHE regulation. 相似文献