昆虫雄性附腺功能蛋白研究进展

昆虫雄性附腺蛋白是精液蛋白的主要来源,对雌雄虫生殖过程具有重要生理功能,按功能可分为精包结构蛋白和功能蛋白两类。精包结构蛋白参与精包的形成;功能蛋白在交配过程中随精子一起转移到雌虫体内,导致雌虫行为和生理的深刻变化,如降低雌虫再交配率、提高产卵量、促进精子转移、储存和竞争等。随着对昆虫雄性附腺功能蛋白研究的深入,特别对果蝇附腺功能蛋白的详细研究,从分子水平上阐述蛋白质序列与功能的关系,明确其作用机制,可为进一步阐明昆虫生殖和进化机制等提供新依据。     

棕尾别麻蝇雄性附腺分泌物的生理功能

棕尾别麻蝇Boettcherisca peregrina Robinean-Desvoidy雄性附腺的分泌物中包含许多生物活性分子,将成熟的雄性附腺分泌物注射到未交配的雌虫体内,发现其能影响雌虫生殖活性的很多方面:如降低雌虫的再次交配率;增加卵巢内的含卵量;缩短交配后雌虫的寿命。另外,还证明附腺分泌物中存在有可抑制革兰氏阳性菌的物质的存在。     

小地老虎雄性附腺细微结构和功能及高温的影响

本文通过光镜、电镜和生化分析等方法,研究了小地老虎Agrotis ypsilon(Rottemberg)雄性附腺的细微结构和功能,结果表明：(1)雄性附腺是一对管状腺,基段粉红色,中段桔红色,端段乳白色。形态分化在蛹前期完成,分泌功能在羽化后4天进入旺盛期;(2)附腺细胞属蛋白质合成型,具有旺盛的合成蛋白质的能力,胞内含有致密的粗面内质网和游离核糖体颗粒,大量的分泌液泡均匀地分布在细胞质中;(3)顶浆分泌和局部分泌是腺体的二种主要分泌方式, 前者分泌的颗粒物为糖蛋白性质(Pas阳性),后者吩泌的网状物为非糖蛋白性质(Pas阴性),二者在腺腔内呈有规则的放射状排列“4”雄性附腺分泌物具有种的特异性,小地老虎、棉铃虫和粘虫等夜蛾科昆虫分泌物的蛋白电泳谱带存在明显的种间差异,高温(32℃)抑制了雄性附腺分泌某些蛋白质的能力,从而改变精液的成分。     

桑天牛雄性附腺内容物组分分析

测定桑天牛Apriona germaric(Hope)雄性附腺内容物中各组分含量及变化情况。结果表明,内容物中可溶性蛋白占总腺管鲜重的8.39%;总糖占总鲜重的4.21%;海藻糖和游离氨基酸分别占总鲜重的0.50%、0.25%。随虫龄的增大,内容物中各组分含量不断降低。交配过程中,雄性附腺内容物部分转移到雌虫,交配后附腺内容物中总糖、海藻糖、游离氨基酸等组分含量均降低,蛋白质组分含量先升高再降低,48h即恢复可到交配前水平。大、小附腺内各组分含量变化有差异。     

长足大竹象雄性附腺提取物抑菌作用研究

以3种细菌(大肠杆菌Escherichia coli、金黄色葡萄球菌Bacillus subtilis、枯草芽孢杆菌Staphyloccocus aureus)为供试菌,测定了长足大竹象Cyrtotrachelus buqueti雄性附腺提取物的抑菌活性。结果表明:长足大竹象雄性附腺提取物对革兰氏阳性菌如枯草芽孢杆菌、金黄色葡萄球菌均有一定的抑菌活性。不同浓度的粗提物对枯草芽孢杆菌及金黄色葡萄球菌抑菌影响差异均具有高度统计学意义(P0.01),抑菌活性随着粗提物浓度的增加而增强。粗提物对金黄色葡萄球菌和枯草芽孢杆菌的最小抑菌浓度分别为0.2 mg·m L~(-1)、0.4 mg·m L~(-1)。不同处理温度对长足大竹象雄性附腺粗提物的抑菌作用有一定影响。     

优雅蝈螽雄性附腺结构与分泌蛋白特性

通过组织切片和SDS-PAGE方法,研究优雅蝈螽Gampsocleis gratiosa Brunner von Wattenwyl雄性附腺的结构及分泌蛋白的特性。结果表明,优雅蝈螽雄性附腺由3类腺管组成:乳白长腺管、透明腺管和乳白短腺管,腺管的管壁组织结构相似,从内到外依次为单层上皮细胞、基膜、肌肉层,不同腺管管腔分泌物H-E染色后呈现不同颜色。SDS-PAGE分析各种腺管的分泌蛋白具有特异性。     

优雅蝈螽雄性附腺的超微结构及其腺管提取物对精子束的作用

为阐明优雅蝈螽Gampsocleis gratiosa Brunner von Wattenwyl雄性附腺的结构与功能的关系, 本文利用透射电镜(transmission electron microscope, TEM)技术研究了优雅蝈螽雄性附腺的超微结构, 利用微分干涉相差显微镜(differential interference contrast microscope, DIC)技术并结合雄性附腺匀浆提取物与精子束在体外的短暂培养, 研究了优雅蝈螽雄性附腺对精子束的作用。结果表明： 优雅蝈螽雄性附腺3类腺管组织结构相似, 腺管管壁为单层上皮细胞, 缺少内表皮, 说明其来源于中胚层。上皮细胞富含粗面内质网、 线粒体、 高尔基体, 具有分泌细胞的特点。腺管管腔中分泌物有4种形态, 即电子透明的物质、 电子致密的颗粒物质、 细纤维状物质以及绒球状物质。上皮细胞的分泌方式主要有2种, 即顶质分泌和局部分泌。乳白短腺管的匀浆提取物参与了帽状精子束解聚的过程, 乳白长腺管和透明腺管的匀浆提取物有维持精子束活性的作用。本研究结果为进一步阐明螽斯雄性附腺的生理功能奠定了基础。     

白蜡虫雄性幼虫蜡腺的超微结构

在光镜结构研究的基础上,用电子显微镜观察了白蜡虫Ericerus pela Chavannes二龄雄幼虫蜡腺的超微结构和虫体表面的蜡孔及蜡丝形态。重点研究了蜡腺各组成部分的形态特点。     

小地老虎雄蛾中胚层生殖道和附腺的细胞结构和分泌功能

通过光镜、电镜及组织化学等方法,研究了小地老虎生殖前期雄蛾中胚层生殖道和附腺的腺细胞结构和分泌功能,以及与精子形态和数量变化的关系,结果表明：(1)以缢缩位置、解剖形态、细胞结构、分泌方式、精子形态变化和数量变动为依据,将中胚层生殖道划分为修精囊、输精管、贮精囊、精包腺1～5段等8个区段;(2)中胚层生殖道和附腺具有相同的组织层次,自内向外分为单细胞上皮层、底膜、肌肉层和围膜等4层,但缺少表皮质内膜;(3)中胚层生殖道和附腺的腺细胞具有旺盛的合成和分泌蛋白质的能力,主要有内质网型和液泡型两种,前者有发达的粗面内质网和高尔基体,后者具有致密的核糖体和分泌泡;至少有4种分泌方式：即颗粒顶泌、液泡顶泌、胞质局泌和胞间分泌;修精囊、贮精囊、雄性附腺、精包腺1段的顶泌物为糖蛋白性质(PAS阳性)、局泌物为非糖蛋白性质(PAS阴性)。     

昆虫雄性生殖腺分泌物的功能

昆虫两性成功交配后,雄性生殖腺分泌物使雌性昆虫的生理和行为都发生了巨大的改变。昆虫雄性生殖腺分泌物含有多种具有生物活性的分子,这些生物活性分子通过成功交配转移到雌虫生殖道后,对雌虫的生殖活动产生影响,使交配雌虫一段时间内不再交配,使已转移的精子易于在雌虫生殖道内储藏,使卵与精子完成受精过程,还可刺激雌虫产卵和卵的发育,调控排卵和产卵等生殖过程。在精子的转移过程中,雄性生殖腺分泌物中的抗菌媒介质能使雌虫的生殖导管提供友好的环境。此外,一些昆虫的雄性生殖腺分泌物还含有一些有毒的化学物质,保护已产下的卵不被天敌取食和病原体侵染。     

烟夜蛾雄蛾性附腺因子对雌蛾性信 息素合成的抑制作用

烟夜蛾Helicoverpa assulta处女蛾在交配后1 h,其性信息素滴度即显著降低,72 h内未见恢复。生测结果表明,烟夜蛾性信息素合成抑制因子主要来源于雄蛾性附腺。不同日龄雄蛾性附腺提取物的抑制活性无显著差异。光暗期对其活性具显著影响,暗期中雄蛾的性附腺物质对雌蛾性信息素合成具有较强抑制作用,而光期中雄蛾的性附腺物质不具抑制活性。在暗期的不同时间处理,对处女蛾性信息素合成的抑制作用无显著差异。雄蛾性附腺提取物对雌蛾性信息素合成的抑制作用与注射剂量有明显的相关性,0.2 ME（雄蛾当量）是产生显著抑制作用的最小剂量。对交配雌蛾注射性信息素生物合成激活神经肽（PBAN）提取物后,其性信息素合成又可恢复,这说明雌蛾交配后,性信息素滴度降低的原因是由于缺少了PBAN的调控。     

Ultrastructure and nature of secretory proteins in the male accessory gland of Drosophila funebris

The ultrastructural differentiation of the secretory cells and the nature of secretory proteins in the male accessory gland of Drosophila funebris have been studied by electron-microscopic and immunological methods. (1) In the pupae at $\text{1}\text{1}\text{2}$ days before eclosion, secretory products can be detected in the lumen, even though most glandular cells are at the initial phase of differentiation. At the time of eclosion both main and secondary cells are fully differentiated, but the whole set of five immunologically active proteins are detectable only on the second to third day of adult life. (2) The secondary cells contain giant protein granules, the so-called filamentous bodies, which become partially fused and the filaments assume a twisted form. Randomly dispersed filaments and closely packed filament bundles are also visible in the gland lumen. Antigenic labelling of ultrathin sections and immunoreplica electrophoresis yielded no evidence for the microtubular nature of these filaments. The secretion stored in the lumen contains in addition a large quantity of flocculent proteins which have their origin in the main cells. (3) During the period of high secretory activity in the 7-day-old male flies no vacuolization and disintegration of either the main or secondary cells have been observed. We conclude that both types of cells have the merocrine secretory mechanism. (4) Ultrastructural alterations in the glandular cells confirmed our previous observation that copulation stimulates RNA and protein synthesis.     

The role of the male accessory gland fluid in stimulating vitellogenesis in Aedes taeniorhynchus

Injection of 20-hydroxyecdysone (20-OH-ecdysone) at high concentrations (5.0 μg) into intact or decapitated female Aedes taeniorhynchus induced vitellogenin synthesis, whereas low concentrations (5.0 ng) were ineffective. Injections of male accessory gland fluid (MAGF), however, at a concentration that was equivalent to 0.25 of the content of a pair of accessory glands, into intact or decapitated A. taeniorhynchus induced viteliogenin synthesis only in intact females. Ovariectomized mosquitoes did not synthesize vitellogenin after MAGF injection or blood feeding. Females that were first injected with MAGF and decapitated 12 h later synthesized viteliogenin at a rate that was 80% of intact controls. Egg development neurosecretory hormone (EDNH) activity in the heads of ovariectomized or intact females injected with MAGF was 9.0 pmol/min/head and 2.5 pmol/min/head, respectively, indicating that MAGF does not stimulate the corpus cardiacum (CC) to release EDNH. Incubation of MAGF and EDNH with fat bodies failed to induce vitellogenin synthesis. These results indicate that in A. taeniorhynchus the MAGF induces the ovary to release corpus cardiacum stimulating factor, which then signals CC to release stored EDNH.     

Male accessory gland substances and the control of sexual receptivity in female Culex tarsalis

ABSTRACT. Homogenates of accessory glands from male Culex tarsalis Coquillet (Diptera; Culicidae) were fractionated using gel filtration column chromatography. A component of low molecular weight capable of suppressing female sexual receptivity was obtained and partially characterized. Proteins present in homogenates of isolated accessory glands formed aggregates with other proteins in extracts of whole mosquitoes. Consequently, previous reports of the molecular weight of biologically active components in homogenates from accessory glands from other mosquito species may be inaccurate.
When female Cx. tarsalis were mated with ³H-leucine labelled males. radioactivity could be found throughout the body of the female 24 h after mating. Autoradiography showed that the radioactivity was incorporated into the cells of various organs, and was not specifically localized in a particular target tissue. Approximately 30% of the total radioactivity transferred to the female was found in the head and thoracic regions, and proteins from the head had a specific activity twice that of the thoracic proteins. Bioassay of isolated body parts from mated and virgin females showed that injections of head tissues from mated females into virgin females suppressed sexual receptivity. These results suggest that the head is involved in the physiological mechanisms resulting in refractory mating behaviour.     

Protein production in components of the accessory gland complex of male Melanoplus sanguinipes (Insecta: Orthoptera)

Protein production during sexual maturation or after allatectomy (followed by juvenile hormone replacement therapy) has been examined in the long hyaline glands, short hyaline glands, white glands, and seminal vesicles, which make up the accessory gland complex of male Melanoplus sanguinipes. During maturation, the amount of protein in the long hyaline glands increases about 14-fold, and in each of the other components between 5- and 6-fold. Most protein accumulates between days 3 and 5, and this is reflected in high levels of incorporation of radiolabelled leucine in this period.

The components show differential sensitivity to the effects of allatectomy. After this operation, the protein content of, and incorporation of radiolabel into, the long hyaline glands remain near the day 0 level. In the white glands and short hyaline glands, allatectomy also has a marked, though less severe, effect on protein synthesis and accumulation. The seminal vesicles are least affected by allatectomy and continue to accumulate protein (though more slowly) to about 60% of the normal level by day 10. Juvenile hormone compounds applied topically to allatectomized insects on day 2 restored the ability of the gland components to accumulate proteins, though to differing degrees. JHI is the most effective compound, stimulating synthesis and accumulation of protein to near normal levels by day 10, whereas application of JHIII or Stauffer's synthetic JH led to only partial restoration of protein synthesis in the glands.     

Long hyaline gland discharge and multiple spermatophore formation by the male grasshopper, Melanoplus sanguinipes

ABSTRACT. Discharge from the male accessory reproductive gland (ARG) by the male grasshopper, Melanoplus sanguinipes (Fabr.), has been studied by assay of a characterized product, a glycoprotein LHPI, and the rate of formation of spermatophores. LHPI is an exclusive long hyaline gland (a prominent ARG tubule type) product whose discharge is symmetrical from the bilaterally paired glands. LHPI forms 65% of a viscous secretion that is discharged concomitantly with the spermatophores. Though low ARG reserves in 5-day-old males limit both the number of spermatophores formed and LHPI discharged in copulations ≤6 h, this appears to be the result of shorter copulations. The number of spermarophores formed in 1 h was not impaired by general depletion of ARG protein (by repeated copulations) or by selective depletion of long hyaline gland protein (by unilateral and bilateral long hyaline gland removal), though these manipulations reduced LHPI discharge by 22%, 44% and 100%, respectively. However, 56% of spermatophores formed by males with the long hyaline gland bilaterally ablated failed to uncoil properly. These results indicate LHPI and/or other long hyaline gland proteins may act as lubricants. Unlike spermatophore formation and LHPI discharge, which increased steadily up to 90–120 min then levelled off, transfer of radiolabelled male ejaculate to the spermatheca was very variable. In 90 min copulations, only 1% of the total radioactivity (representing c. 5 μg protein) lost from the ARG complex was transferred to the spermatheca. The importance of male-derived protein in vitellogenesis is discussed.