Met和Kr-h1基因在褐飞虱变态发育中的功能分析

【目的】保幼激素受体Methoprene-tolerant(Met)控制保幼激素信号传导途径中重要下游转录因子Krüppelhomolog 1(Kr-h1)的表达,调控昆虫的变态发育。本研究旨在探究褐飞虱Nilaparvata lugens Met基因与Kr-h1在褐飞虱变态发育中的功能。【方法】利用PCR技术扩增Nl Met基因的ORF序列。通过RNA干扰技术分别或同时沉默褐飞虱若虫的Nl Met和Nl Kr-h1基因,进一步研究其功能。【结果】克隆得到Nl Met,其开放阅读框包含1 185 bp,编码395个氨基酸,包括b HLH,PAS-A,PAS-B和PAC 4个结构域;其中PAS-B和PAC保守性较高,而b HLH和PAS-A保守性相对较低。采用RNA干扰技术沉默Nl Met和Nl Kr-h1基因后发现,单独对4龄若虫Nl Kr-h1基因干扰后,若虫阶段及初羽化雌虫和雄虫死亡率均显著上升(P0.05);对5龄若虫Nl Kr-h1基因干扰后只有若虫死亡率上升(P0.05),单独对Nl Met基因干扰后死亡率没有显著变化(P0.05);二者共同沉默后的死亡率同单独对Nl Kr-h1沉默时类似。此外,我们还发现单独对4龄若虫Nl Kr-h1干扰后在雌虫中出现了生殖器畸形,虽然Nl Met干扰并未出现生殖器发育畸形现象,但二者共同干扰后,在若虫、初羽化雌雄成虫中畸形比例均显著增加(P0.05)。【结论】Nl Met与下游转录因子Nl Kr-h1对褐飞虱变态发育起到重要作用,影响若虫到成虫的变态和外生殖器的发育。本研究有助于揭示Nl Met和Nl Kr-h1在昆虫变态发育中的重要作用。     

保幼激素的分子作用机制

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。     

保幼激素对昆虫变态发育调控的分子机制

近年来随着保幼激素(juvenile hormone,JH)核受体Methoprene tolerant(Met)被鉴定,JH对昆虫变态发育调控的分子机制的研究取得了极大的进展。本文在介绍Met的鉴定以及分子伴侣Hsp83和核孔蛋白Nup358对Met亚细胞定位调控的基础上,重点阐述了JH-Met-Kr-h1-Br信号通路在完全变态昆虫幼虫至蛹变态过程中的作用以及JH-Met-Kr-h1-E93信号通路在不完全变态昆虫和完全变态昆虫成虫羽化过程中的作用。此外,Met与蜕皮激素(20-hydroxyecdysone,20E)受体复合物EcR/USP的结合、Tai/SRC/FISC分别与Met和EcR/USP结合形成JH功能受体和20E功能受体复合物、JH对20E下游基因E75A的诱导以及USP与JH的结合等分子间的相互作用在JH与20E的互作中所产生的影响也将逐一进行论述。本文还对JH通过膜受体激活PKC和PLC等下游信号通路而发挥生理功能的研究进展进行了概述。     

昆虫保幼激素生物合成的调节与测定

<正> 保幼激素(JH)是由昆虫的咽侧体(CA)产生。它调节着发育和生殖。从昆虫中已分离出3种具有JH活性的化合物,分别称为JH1、JH2、JH3。它们的生理活性大不相同。JH3是大部分成虫的主要激素,可促进卵巢的发育,所以是一种促性腺激素。JH1和JH2主要在鳞翅目幼虫和蜚蠊若虫内,它们在变态开始就参与这一过程的调节作用,称为变态激素。     

保幼激素生物合成研究进展

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。     

保幼激素合成的研究进展

保幼激素 (juvenile hormone,JH) 是通过甲羟戊酸途径合成的一类倍半萜化合物。以昆虫中普遍存在的JH Ⅲ为例,从分子水平上概述了JH合成途径中的各种酶,并对其中的两个关键酶：羟甲基戊二酰辅酶A还原酶和保幼激素酸甲基转移酶作了详细介绍。还从家蚕基因组数据库(http://silkworm.genomics.org.cn)中推测出了JH合成途径中大部分酶的编码基因,初探了JH合成的调节机制,讨论了JH合成的研究趋势。     

保幼激素的分子作用机制研究

保幼激素(juvenile hormone,JH)和蜕皮激素(20-hydroxyecdysone,20E)是协同调控昆虫发育、变态与生殖的两个重要激素。由于20E的主要分子作用机制已经比较明了,揭示JH的分子作用机制成为过去20多年来昆虫学领域研究的一个重点和难点。国内外多个研究团队利用赤拟谷盗Tribolium castaneum、果蝇Drosophilamelanogaster、烟草天蛾Manduca sexta等为模式,在JH受体的鉴定、JH在昆虫发育变态和生殖中的分子调控机制以及JH与20E在分子水平上的交互作用等方面开展了大量的研究工作,本文就近几年在这些方面取得的主要研究进展作一个综述。     

整合昆虫发育生物学和果蝇遗传学来研究昆虫发育与变态

成熟动物(昆虫)个体大小主要由生长持续时间和生长速度2个因素所决定。蜕皮激素和保幼激素协同调控昆虫发育变态,并决定昆虫生长持续时间;胰岛素、营养和细胞接触抑制等生长死亡信号及其传导途径控制细胞分裂、长大、分化、死亡,并最终决定昆虫的生长速度。最近研究成果表明,蜕皮激素信号和胰岛素信号相互影响,对昆虫个体大小起决定性的作用;脂肪体和营养代谢把这2条信号传导途径整合起来。科学家将会整合昆虫发育生物学和果蝇遗传学,抓住生长持续时间和生长速率2个关键因素,并以营养代谢和脂肪体为切入点来研究昆虫的发育变态。     

昆虫保幼激素分析方法进展

在保幼激素(JH)研究中,一个非常重要的方面是对其进行定性和定量分析。几十年来,保幼激素生理生化作用研究一直同其分析方法的研究紧密相关,互相促进。迅速、灵敏、简便的定量分析技术必将极大促进对保幼激素作用方式的研究。 昆虫保幼激素的分析方法主要有三类:生物分析、色谱分析和放射免疫分析。50年代至70年代初期,主要是采用生物分析方法,进入70年代后,色谱分析与放射免疫分析技术得到了迅速发展,尤其是色谱分析,进展尤为突出。下面就昆虫保幼激素分析技术发展的几个方面分别作一介绍。     

Hormonal regulation and developmental role of Krüppel homolog 1, a repressor of metamorphosis,in the silkworm Bombyx mori

Juvenile hormone (JH) has an ability to repress the precocious metamorphosis of insects during their larval development. Krüppel homolog 1 (Kr-h1) is an early JH-inducible gene that mediates this action of JH; however, the fine hormonal regulation of Kr-h1 and the molecular mechanism underlying its antimetamorphic effect are little understood. In this study, we attempted to elucidate the hormonal regulation and developmental role of Kr-h1. We found that the expression of Kr-h1 in the epidermis of penultimate-instar larvae of the silkworm Bombyx mori was induced by JH secreted by the corpora allata (CA), whereas the CA were not involved in the transient induction of Kr-h1 at the prepupal stage. Tissue culture experiments suggested that the transient peak of Kr-h1 at the prepupal stage is likely to be induced cooperatively by JH derived from gland(s) other than the CA and the prepupal surge of ecdysteroid, although involvement of unknown factor(s) could not be ruled out. To elucidate the developmental role of Kr-h1, we generated transgenic silkworms overexpressing Kr-h1. The transgenic silkworms grew normally until the spinning stage, but their development was arrested at the prepupal stage. The transgenic silkworms from which the CA were removed in the penultimate instar did not undergo precocious pupation or larval–larval molt but fell into prepupal arrest. This result demonstrated that Kr-h1 is indeed involved in the repression of metamorphosis but that Kr-h1 alone is incapable of implementing normal larval molt. Moreover, the expression profiles and hormonal responses of early ecdysone-inducible genes (E74, E75, and Broad) in transgenic silkworms suggested that Kr-h1 is not involved in the JH-dependent modulation of these genes, which is associated with the control of metamorphosis.     

Genome-wide comparison of genes involved in the biosynthesis,metabolism, and signaling of juvenile hormone between silkworm and other insects

Juvenile hormone (JH) contributes to the regulation of larval molting and metamorphosis in insects. Herein, we comprehensively identified 55 genes involved in JH biosynthesis, metabolism and signaling in the silkworm (Bombyx mori) as well as 35 in Drosophila melanogaster, 35 in Anopheles gambiae, 36 in Apis mellifera, 47 in Tribolium castaneum, and 44 in Danaus plexippus. Comparative analysis showed that each gene involved in the early steps of the mevalonate (MVA) pathway, in the neuropeptide regulation of JH biosynthesis, or in JH signaling is a single copy in B. mori and other surveyed insects, indicating that these JH-related pathways or steps are likely conserved in all surveyed insects. However, each gene participating in the isoprenoid branch of JH biosynthesis and JH metabolism, together with the FPPS genes for catalyzing the final step of the MVA pathway of JH biosynthesis, exhibited an obvious duplication in Lepidoptera, including B. mori and D. plexippus. Microarray and real-time RT-PCR analysis revealed that different copies of several JH-related genes presented expression changes that correlated with the dynamics of JH titer during larval growth and metamorphosis. Taken together, the findings suggest that duplication-derived copy variation of JH-related genes might be evolutionarily associated with the variation of JH types between Lepidoptera and other insect orders. In conclusion, our results provide useful clues for further functional analysis of JH-related genes in B. mori and other insects.     

CREB-binding protein regulates metamorphosis and compound eye development in the yellow fever mosquito,Aedes aegypti

Juvenile hormones (JH) and ecdysone coordinately regulate metamorphosis in Aedes aegypti. We studied the function of an epigenetic regulator and multifunctional transactivator, CREB binding protein (CBP) in A. aegypti. RNAi-mediated knockdown of CBP in Ae. aegypti larvae resulted in suppression of JH primary response gene, Krüppel-homolog 1 (Kr-h1), and induction of primary ecdysone response gene, E93, resulting in multiple effects including early metamorphosis, larval-pupal intermediate formation, mortality and inhibition of compound eye development. RNA sequencing identified hundreds of genes, including JH and ecdysone response genes regulated by CBP. In the presence of JH, CBP upregulates Kr-h1 by acetylating core histones at the Kr-h1 promoter and facilitating the recruitment of JH receptor and other proteins. CBP suppresses metamorphosis regulators, EcR-A, USP-A, BR-C, and E93 through the upregulation of Kr-h1 and E75A. CBP regulates the expression of core eye specification genes including those involved in TGF-β and EGFR signaling. These studies demonstrate that CBP is an essential player in JH and 20E action and regulates metamorphosis and compound eye development in Ae. aegypti.     

Common and distinct roles of juvenile hormone signaling genes in metamorphosis of holometabolous and hemimetabolous insects

Insect larvae metamorphose to winged and reproductive adults either directly (hemimetaboly) or through an intermediary pupal stage (holometaboly). In either case juvenile hormone (JH) prevents metamorphosis until a larva has attained an appropriate phase of development. In holometabolous insects, JH acts through its putative receptor Methoprene-tolerant (Met) to regulate Krüppel-homolog 1 (Kr-h1) and Broad-Complex (BR-C) genes. While Met and Kr-h1 prevent precocious metamorphosis in pre-final larval instars, BR-C specifies the pupal stage. How JH signaling operates in hemimetabolous insects is poorly understood. Here, we compare the function of Met, Kr-h1 and BR-C genes in the two types of insects. Using systemic RNAi in the hemimetabolous true bug, Pyrrhocoris apterus, we show that Met conveys the JH signal to prevent premature metamorphosis by maintaining high expression of Kr-h1. Knockdown of either Met or Kr-h1 (but not of BR-C) in penultimate-instar Pyrrhocoris larvae causes precocious development of adult color pattern, wings and genitalia. A natural fall of Kr-h1 expression in the last larval instar normally permits adult development, and treatment with an exogenous JH mimic methoprene at this time requires both Met and Kr-h1 to block the adult program and induce an extra larval instar. Met and Kr-h1 therefore serve as JH-dependent repressors of deleterious precocious metamorphic changes in both hemimetabolous and holometabolous juveniles, whereas BR-C has been recruited for a new role in specifying the holometabolous pupa. These results show that despite considerable evolutionary distance, insects with diverse developmental strategies employ a common-core JH signaling pathway to commit to adult morphogenesis.