昆虫触角叶的结构

触角叶是昆虫脑内初级嗅觉中心,通过触角神经与触角联系。触角叶主要由嗅觉受体神经元、局域中间神经元、投射神经元和远心神经元构成。这些神经元的形态多样,其形态变化与其功能和昆虫嗅觉行为相关。这些神经元在触角叶内交织形成神经纤维网,在突触联系紧密的地方形成纤维球,纤维球通常排列在触角叶外周。通常,昆虫触角叶内纤维球的数量、大小和位置相对固定,并且几乎每个小球都可以被识别和命名。不同种类、性别和品级的昆虫中,纤维球的数量、大小和排列方式各不相同。触角叶结构神经元组成和纤维球的多样性,与各种昆虫嗅觉行为的特异性相对应。     

斜纹夜蛾触角叶神经元及其对植物气味和性信息素的反应

【目的】探索斜纹夜蛾Spodoptera litura触角叶结构及其神经元对植物气味和性信息素的神经识别机制。【方法】利用共聚焦激光技术扫描斜纹夜蛾成虫触角叶结构,同时采用多通道电生理技术(multi-unit recording,MR)记录斜纹夜蛾触角叶对6种寄主植物气味化合物(苯甲醛、苯甲醇、苯乙醛、水杨醛、乙酸叶醇酯和己烯醛)及性信息素顺9反11十四碳二烯乙酸酯和顺9反12十四碳二烯乙酸酯的反应;并在风洞中测定分析斜纹夜蛾对上述化合物的定向行为反应。【结果】共聚焦激光扫描结果显示,雄性和雌性斜纹夜蛾触角叶内分别密集地分布有67和66个神经纤维球;而雌性斜纹夜蛾触角叶内的纤维球总体积和平均体积都高于雄性。负责识别和追踪性信息素的扩大型纤维球复合体(macroglomerular complex,MGC)只在雄性斜纹夜蛾触角叶内发现。MR试验结果显示斜纹夜蛾触角叶内神经元具有3种自发放电模式:稀疏放电(不规则的放电频率)、温和放电(宽而慢的放电频率)和密集放电(暴发性的放电频率)。同时,斜纹夜蛾触角叶神经元对所有刺激的气味表现出3种反应类型:兴奋性、抑制性和无反应。神经元对气味的兴奋性和抑制性反应以及无反应取决于刺激化合物的结构和浓度。雌虫的触角叶神经元对性信息素和单一的植物气味表现出很小的反应,而雄虫对两种性信息素以及苯甲醛、苯甲醇、苯乙醛和水杨醛具有很强的兴奋性反应。斜纹夜蛾风洞试验也显示绝大部分的斜纹夜蛾雄虫都选择停留在性信息素和芳香族化合物上,这与MR的结果一致。【结论】神经元的反应强度和刺激化合物浓度之间的关系根据不同的神经元和刺激化合物而有所不同。在测试的浓度范围内,雄虫触角叶神经元对性信息素的反应强度随着浓度的增加而加强,但是除乙酸叶醇酯外,对其他植物气味的反应强度在测试的浓度范围内没有显著的变化。     

Agrotis segetum雄蛾触角叶神经元对性信息素时间编码的机制分析

应用压力注射,在Agrotis segetum雄蛾触角叶（AL）中33个对性信息素有反应的MGC神经元上探计了对性信息素反应模式的形成机制,压力注射100mmol/L GABA进入AL神经网引起神经元一个慢的超极化电位,并有一个长时程的放电抑制相,与用性信息素刺激诱导的神经元分应很相似,但GABA并不影响神经元对性信息素刺激的去极化反应,低Cl^-溶液可减弱AL神经元对性信息素刺激的超极化反应,甚至使超极化相逆转为兴奋反应,抑制相消失。压力注射Bicuculline使神经元放电频率增加。压力注射Bicuculline的同时给予性信息素刺激,可使性信息素刺激所致的神经元放电增加进一步加强;Bicuculline可使性信息素刺激引起的神经元超极化幅度变小,放电抑制时间变短,甚至其抑制相完全被逆转为正常放电,无超极化反应和抑制相存在,结果表明,AL神经元对性信息系反应的超极化相与GABA受体有关。     

激光共聚焦显微技术在瓮安生物群中的应用

激光共聚焦显微技术是一种以激光作为激发光源,通过特殊装置"针孔"来过滤离焦光线以提高光学分辨率和对比度的光学成像技术。由于大部分化石不能自发荧光,该技术在古生物学领域尚未实现大范围的应用。但若围岩能自发荧光而与化石之间具有一定衬度,或化石因含特殊成分能在特定波段激光照射下自发荧光而产生结构衬度,则可以运用激光共聚焦显微技术获得在普通光学显微镜及荧光显微镜下难以清晰观察到的信息。为推动激光共聚焦技术在古生物学领域中的应用,文中系统介绍了该技术的原理与使用方法,并以埃迪卡拉纪磷酸盐化特异埋藏的瓮安生物群微体化石为例,展示了该技术在化石成像中的若干优势。实验结果表明,瓮安生物群微体化石因富含磷灰石可自发荧光实现成像,使用激光共聚焦显微成像技术观察瓮安生物群化石薄片不仅可以获得较好衬度,而且还能提高成像的分辨率和清晰度。此外,在化石薄片的厚度范围内还可以实现化石结构三维重建。     

利用单感器记录与神经元示踪结合对棉铃虫主要性信息素感器内神经元投射的鉴定

【目的】鉴定雄性棉铃虫Helicoverpa armigera成虫触角性信息素感器嗅觉受体神经元的功能、形态及中枢投射路径。【方法】利用单感器记录技术记录棉铃虫嗅觉受体神经元对性信息素的反应,同时采用荧光染料作为示踪剂染色标记嗅觉受体神经元;使用免疫组织化学方法处理相应的脑组织,标记脑内触角叶的神经纤维球结构;用激光扫描共聚焦显微镜获取图像数据,使用图形软件ZEN和Amira 4.1.1进行三维结构重建。【结果】记录到雄性棉铃虫成虫触角上长毛形感器对主要性信息素成分Z11-16∶Ald产生明显的电生理反应,并成功染色标记了该感器内的嗅觉受体神经元。染色标记显示该感器内具有两个嗅觉受体神经元,其轴突通过触角神经分别投射触角叶内的云状体神经纤维球和普通神经纤维球。【结论】单感器记录与神经元示踪两技术结合能够用于鉴定昆虫触角嗅觉受体神经元的功能、形态和投射至神经纤维球的路径。与赖氨酸钴方法比较,使用荧光染料法进行神经元示踪,操作更简便,且易于进行三维空间分析,为调查棉铃虫其他嗅觉神经元的投射路径以明确外周气味受体感受与中枢系统的联系提供了有力技术支持。     

激光共焦扫描显微镜的光学层析特性研究(英文)

本文从理论上研究了激光共焦扫描显微镜的光学层析特性,并给出了探测器的针孔大小、聚焦物镜数值孔径与光学层析的关系,最后还给出了利用光学层析技术发现的一种寄生虫新的形态结构的实验结果     

基于激光共聚焦扫描显微技术分析激光对扁藻的影响

本文以亚心形扁藻为样品,波长1 341 nm的Nd∶YAP激光为光源,通过激光共聚焦扫描显微技术,研究Nd∶YAP激光辐照亚心形扁藻对亚心形扁藻叶绿体自体荧光强度和叶绿体面积大小的影响。Nd∶YAP激光辐照后的亚心形扁藻通过488 nm Ar^+激光激发获得亚心形扁藻自体荧光图像及其荧光光谱。结果表明,试验中除(10 W,60 s)辐照剂量组外,其余辐照剂量组均提高了亚心形扁藻的自体荧光强度,且所有的辐照剂量组均增大了亚心形扁藻的叶绿体面积。Nd∶YAP激光可刺激亚心形扁藻的叶绿体发育,促进藻细胞的生长,改善叶绿体光合作用的活性。     

基于激光共聚焦同步双扫描技术的LC3脱乙酰化修饰调控自噬的机理研究

激光共聚焦同步双扫描(simultaneous,SIM)技术在常规扫描单元的基础上,引入一个同步扫描单元(SIM scanner),该技术独立控制了两个激光束,一个用于激光光刺激,另一个用于同步成像。本实验中,采用激光共聚焦同步双扫描系统的405 nm和488 nm激光分别对细胞的特定部位进行刺激和同步成像,实时检测了LC3复合物的形成,记录并分析了乙酰化前后LC3的光动力学变化过程,证实了LC3的脱乙酰化修饰是自噬性降解所必须的,本实验体系为激光共聚焦双扫描技术的推广提供了一个很好的平台。SIM技术的应用,解决了刺激过程无法成像的问题,为漂白后荧光恢复(fluorescence recovery after photobleaching,FRAP)、漂白后荧光损失(fluorescence loss in photobleaching,FLIP)和光诱导激活等研究提供了最佳的解决方案,可作为光刺激的一种实验模式在很多实验设计中进行延伸应用。     

扁角豆芫菁成虫雌雄异型触角感器精细结构观察(英文)

【目的】本研究旨在观察扁角豆芫菁Epicauta impressicornis主要触角感器的形态特征,为进一步开展扁角豆芫菁生物学和行为机制研究提供基础参考,也为今后的触角感受器电生理研究提供前提条件。【方法】对扁角豆芫菁E. impressicornis雌雄成虫触角感器进行了扫描电镜观察,并对雌雄成虫触角感器数量、分布及其差异进行了统计和比较分析。【结果】结果表明,其雌雄成虫触角感器存在性二型现象,二者的感器类型、数量及分布既有共性又存在明显差异。雌雄成虫触角共有的感器分为7种,即2种刺形感器(CH1和CH2),2种锥形感器(SB1和SB2),1种Böhm氏鬃毛(BB),1种耳形感器(SA)和1种钟形感器(CA);雄虫触角特有的感器类型包括1种刺形感器(CH3)和1种锥形感器(SB3),而雌性触角特有的感器类型包含2种锥形感器(SB4和SB5)和1种凹槽钉形感器(GP)。【结论】扁角豆芫菁成虫触角感受器类型丰富多样。根据触角感受器的形态、分布以及与之前报道结果的比较分析,推测其功能可能为信息素感器(CH1)、化学感器(CH2和GP)、嗅觉受体(CH3, SB1-SB5, SA和CA)、机械感器(BB)和温度感器(GP和CA)。     

Glomerulus development in the absence of a set of mitral-like neurons in the insect olfactory lobe

Mitral cells are the first neurons in the mammalian olfactory bulb to synapse with olfactory receptor axons during glomerulus development, and in an invertebrate, the moth Manduca sexta, mitral-like neurons overlap very early with olfactory receptor axons as they begin to form protoglomeruli. The possibility for early interaction between receptor neurons and mitral-like neurons led us to ask whether such an interaction plays an essential role in glomerulus development. In the current study in the moth, we surgically removed a major class of these mitral-like neurons before glomeruli began to form and asked: (a) Is the formation of the array of olfactory glomeruli triggered by an interaction of the first-arriving receptor axons with the dendrites of mitral-like neurons? (b) At the level of individual glomeruli, must the mitral-like dendrites be in place either to maintain receptor axons in a glomerular arrangement, or to guide later-growing dendrites of other types into the developing glomeruli? Our results indicate that even without the participation of this group of mitral-like neurons, the array of sexually isomorphic ordinary glomeruli forms and the basic substructure of individual glomeruli develops apparently normally. We conclude that the mitral-like neurons in Manduca are not essential for the formation of ordinary olfactory glomeruli during development. © 1998 John Wiley & Sons, Inc. J Neurobiol 36: 41–52, 1998     

昆虫嗅觉神经的计算机三维重建

基于激光扫描共聚焦显微镜平台的计算机三维重建在昆虫嗅觉神经研究中发挥了重要作用。对经荧光标记的神经组织采集系列光学切片并进行三维重建,在双翅目、鳞翅目、膜翅目、蜚蠊目昆虫中均有进展。触角叶是昆虫的初级嗅觉中心,触角叶的解剖学图谱是识别不同种和雌雄虫间嗅球体特定功能的先决条件。了解构成嗅觉传输途径的主要神经元的形态和空间关系是理解气味信息在中枢神经系统编码的基础。三维重建昆虫的嗅觉神经,对于探讨昆虫嗅觉在其寄主选择、觅食以及寻找配偶等行为中的作用具有非常重要的意义。     

激光共焦显微成像的最新进展及其在生命科学研究中的应用

激光扫描共聚焦显微镜近年来得到了迅速发展,是近代最先进的细胞生物医学分析仪器之一。通过它可以对观察样品进行无创断层扫描和成像,在生物学和医学研究诊断的各个方面都得到了广泛的应用。本文主要介绍了激光扫描共焦显微镜的基本原理和发展状况,并着重介绍了在共焦荧光显微镜中采用薄荧光层和切片成像特性图来表征成像状态的功能。这种方法一般用于表征共聚焦和多光子显微镜的成像特性,是比较显微镜切片成像条件、成像质量等相关性能的重要依据。     

A new approach for the spatially resolved qualitative analysis of the protein distribution in hydrogel beads based on confocal laser scanning microscopy

To investigate the spatial distribution of white egg albumin (WEA) in alginate beads, a new method based on confocal laser scanning microscopy (CLSM) was developed. In contrast to the existing CLSM methods, misleading conclusions are prevented with the application of the new method which does not allow the attenuation of the exciting and emitted light by the opaque hydrogel matrices to be disregarded. By the application of this method, the distribution of WEA in alginate beads was shown to be dependent on the amount of protein loading. At low quantities of protein, a higher protein concentration occurs in the shell layer of the alginate bead while at higher loadings a more or less homogeneous distribution is observed.     

Apoplastic pH in corn root gravitropism: a laser scanning confocal microscopy measurement

The ability to measure the pH of the apoplast in situ is of special interest as a test of the cell wall acidification theory. Optical sectioning of living seedlings of corn roots using the laser scanning confocal microscope (LSCM) permits us to make pH measurements in living tissue. The pH of the apoplast of corn roots was measured by this method after infiltration with CI-NERF, a pH-sensitive dye, along with Texas Red Dextran 3000, a pH-insensitive dye, as an internal standard. In the elongation zone of corn roots, the mean apoplastic pH was 4.9. Upon gravitropic stimulation, the pH on the convex side of actively bending roots was 4.5. The lowering of the apoplastic pH by 0.4 units appears to be sufficient to account for the increased growth on that side. This technique provides site-specific evidence for the acid growth theory of cell elongation. The LSCM permits measurements of the pH of living tissues, and has a sensitivity of approximately 0.2 pH units.     

Use of confocal microscopy to follow the development of penetrative hyphae during growth of Rhizopus oligosporus in an artificial solid-state fermentation system

Two methods were compared for determining the concentration of penetrative biomass during growth of Rhizopus oligosporus on an artificial solid substrate consisting of an inert gel and starch as the sole source of carbon and energy. The first method was based on the use of a hand microtome to make sections of approximately 0.2- to 0.4-mm thickness parallel to the substrate surface and the determination of the glucosamine content in each slice. Use of glucosamine measurements to estimate biomass concentrations was shown to be problematic due to the large variations in glucosamine content with mycelial age. The second method was a novel method based on the use of confocal scanning laser microscopy to estimate the fractional volume occupied by the biomass. Although it is not simple to translate fractional volumes into dry weights of hyphae due to the lack of experimentally determined conversion factors, measurement of the fractional volumes in themselves is useful for characterizing fungal penetration into the substrate. Growth of penetrative biomass in the artificial model substrate showed two forms of growth with an indistinct mass in the region close to the substrate surface and a few hyphae penetrating perpendicularly to the surface in regions further away from the substrate surface. The biomass profiles against depth obtained from the confocal microscopy showed two linear regions on log-linear plots, which are possibly related to different oxygen availability at different depths within the substrate. Confocal microscopy has the potential to be a powerful tool in the investigation of fungal growth mechanisms in solid-state fermentation.     

A single cell model system to study hormone signal transduction

The model system presented here is based on immobilised single cells, derived directly from tobacco mesophyll protoplasts. It allows the adequate steering of cell populations towards expansion, cell cycling or cell resting. Using this approach cells always have the same predictable response to auxins and cytokinins whatever their actual physiological status. This model system opens new ways to study cellular parameters governing these hormone responses, some of which have been explored so far; a) the cytokinin response can equally well be induced by endogenous as by exogenous cytokinins; b) at least two intracellular components, microtubuli and the ER, adapt their architecture to the hormone-induced status of the cell; c) addition of NAA to the cells does not induce a change in the cytoplasmic pH.