昆虫嗅觉相关蛋白及嗅觉识别机理研究概述

嗅觉是昆虫产生行为的基础之一,在长期进化的过程中昆虫形成了复杂的嗅觉系统,完成这一过程,需要有多种与嗅觉相关的蛋白参与,包括气味结合蛋白、化学感受蛋白、气味受体和感觉神经元膜蛋白等。了解昆虫感受外界信息的嗅觉机制可以帮助我们更好地理解昆虫识别配偶、天敌及寻找食物来源、产卵场地等行为特征,为进一步调控昆虫的行为、防控害虫侵袭、保护和利用有益昆虫奠定基础。本文综述了昆虫嗅觉相关的几类重要蛋白的生化特性和生理功能,并对昆虫气味分子的识别机制、气味分子在昆虫体内运输机制的最新研究进展进行了概述。     

昆虫嗅觉相关可溶性蛋白的研究进展

昆虫在长期进化过程中形成了一套高度敏感的嗅觉系统,通过该系统昆虫可以完成寻觅配偶、定位寄主及选择产卵位点等多种行为。在昆虫嗅觉系统中的可溶性蛋白主要有气味结合蛋白(odorant-binding protein, OBP)和化学感受蛋白(chemosensory protein, CSP)。OBP可以特异性结合并运输疏水性的气味分子相应的受体,是昆虫化学识别过程的第一步,具有十分重要的作用。CSP与OBP的结构和功能类似,主要参与化合物的识别和运输,尽管没有直接的证据表明CSP也参与了昆虫的化学感受过程,但已有研究发现,CSP在昆虫嗅觉系统中发挥着重要的作用。本文主要从分子特性、蛋白结构、表达模式、生理功能等方面分别对昆虫的OBP和CSP进行了概述,为深入的研究两者的功能提供理论参考,进而为以昆虫嗅觉系统为靶标的害虫防治提供新的思路。     

昆虫嗅觉受体的研究进展

昆虫的嗅觉对昆虫的栖息地选择、觅食、群集、趋避、繁殖以及信息传递等行为具有重要的影响。对昆虫嗅觉机理的深入研究和嗅觉信号传导途径的完整阐述,是探索农业害虫的专一性防治的基础。嗅觉受体(olfactory receptors,Ors)是G蛋白偶联受体(G protein-coupled receptor)的一种,是嗅觉系统的关键成分。近年来嗅觉受体的研究日益受到关注。本文对昆虫嗅觉的基本过程、基因结构和表达调控特征、蛋白分子结构、生理功能、分布部位和相关配体的研究等进行了综述。     

昆虫嗅觉结合蛋白研究进展

嗅觉结合蛋白是嗅觉系统的第一个参与者,主要表达在嗅觉外周系统淋巴液中,负责识别、结合和转运气味和信息素分子到达嗅觉受体。近些年,随着各种生物新技术的应用,大量昆虫嗅觉结合蛋白被鉴定出来,其各种不同功能得到揭示。本文对近年来嗅觉结合蛋白的分子特征、蛋白结构、功能和应用等方面的研究进展进行总结和综述。总的来说,嗅觉结合蛋白包括气味结合蛋白(odorant-binding proteins, OBPs)、化学感受蛋白(chemosensory proteins, CSPs)和尼曼 匹克C2型蛋白(Niemann-Pick type C2 proteins, NPC2)三大家族,在α-螺旋和β-折叠的基础上形成了相对简单而稳定的球形结构,使它们能适应各种环境和任务,所以嗅觉结合蛋白蛋白具有复杂多样的功能,且这些功能对昆虫生理和行为尤为重要。基于嗅觉结合蛋白功能,研究者已经把它们应用于生物防治、品种选育和制作生物嗅觉传感器等,具有巨大的潜在价值。本综述为昆虫嗅觉结合蛋白后续研究提供了参考信息及一些新的思路。     

寄生蜂嗅觉蛋白研究进展

寄生蜂对外界环境中气味的识别过程尤为复杂,需要很多组织器官参与,嗅觉系统在寄生蜂选择寄主、识别定位寄主和寄生过程中发挥着重要的作用。常见的嗅觉相关蛋白有气味结合蛋白、化学感受蛋白、气味受体等,本文从嗅觉蛋白的鉴定、结构特征与分类、表达定位、系统发育、功能研究等方面综述了寄生蜂嗅觉蛋白的国内外研究进展,为更多寄生蜂嗅觉相关蛋白的鉴定及其功能研究提供参考。     

酵母双杂交筛选华北大黑鳃金龟触角均一化cDNA文库

昆虫错综复杂的嗅觉系统在昆虫寻找寄主、 交配、 产卵以及逃避行为中起到了至关重要的作用。因此, 对昆虫嗅觉感受机理的研究将有助于揭开昆虫感受和识别环境中的气味物质并引起相关行为反应的秘密。为了更多地了解华北大黑鳃金龟Holotrichia oblita Faldermann 嗅觉相关蛋白互作机制, 本实验利用DUALhunter Starter Kits酵母双杂交筛选试剂盒, 构建了华北大黑鳃金龟气味结合蛋白OBP2诱饵载体, 筛选了华北大黑鳃金龟触角酵母双杂交系统均一化的cDNA文库。通过β-半乳糖苷酶活性检测以及GenBank中Blast比对分析, 以OBP2为诱饵鉴定出6个阳性互作物。我们推测其中的一种较强的阳性互作物凝固酶原可能是华北大黑鳃金龟在嗅觉识别过程中的相关蛋白。     

蜜蜂嗅觉相关蛋白的研究进展

蜜蜂是一类营社会性生活的昆虫,蜂群中的蜂王、工蜂和雄蜂相互依存,各司其职,共同维持着群体严密有序的生活。其中,嗅觉系统在它们的生存和繁衍过程中起到重要的作用。昆虫对气味物质的感受过程是非常复杂的,需要有多种蛋白的参与。研究蜜蜂的化学感受机制可以帮助我们更深入地了解蜜蜂特有的行为及生物学特性。本文重点综述了与蜜蜂嗅觉相关的3种蛋白质的生化特性、分子结构、基因表达及其生理功能等方面的研究进展,以期为今后开展相关研究工作提供理论参考。     

昆虫嗅觉相关蛋白的结构和功能

昆虫在长期进化的过程中形成了复杂的嗅觉系统,气味剂结合蛋白(odorant binding proteins,OBPs)、嗅觉受体(olfactory receptors,ORs)是其最主要的组分.其主要作用是结合外围挥发性的气味分子并将信号传递给细胞内的第二信使.OBPs和ORs的结构、功能、表达、进化是昆虫行为与进化关系的重要研究领域和研究热点.本文主要总结了近年来昆虫OBPs和ORs的结构特点、生理功能、表达特点、遗传进化等方面研究的最新进展,对OBPs和ORs的研究趋势进行了展望,为昆虫嗅觉系统进化研究及寻找害虫防治新途径提供参考信息.     

昆虫气味认知的嗅觉神经结构及分子机制

大多数昆虫主要通过气味认知感知外界环境的变化,维持生命活动。探究昆虫气味认知的嗅觉系统神经结构及分子机制,对于完善气味认知神经生物学理论及利用其原理进行仿生学研究等有重要的科学意义。近年,关于昆虫气味认知科学研究有了很大的进展。本文从昆虫神经生物学的视角详细综述了近年关于昆虫气味认知的嗅觉神经结构、分子机制及气味信号的神经传导途径等方面的基本理论及最新研究成果。综述结果显示:昆虫对气味的认知是通过嗅觉神经系统的触角感器、触角叶(AL)、蕈形体(MB)等脑内多层信号处理神经结构来实现的。当外界气味分子进入触角感器内后,由感器内特定的气味识别蛋白(OBP)将气味分子运载到达嗅觉感受神经元(ORN)树突膜上的受体位点,气味分子与表达特定气味的受体(OR)结合产生电信号,并以动作电位的形式通过ORN的轴突传到脑内的触角叶。在触角叶经过嗅觉纤维球对气味信息选择性加工处理,再由投射神经元(PNs)将初步的识别和分类的气味信息传到蕈形体和外侧角(LH)等神经中枢,实现对气味的识别和认知。虽然,近年昆虫气味认知神经生物学的研究有了很大的进步,但是,我们认为目前的研究成果还不能完全阐明昆虫气味认知的神经机制,还有很多问题,例如,触角叶上众多的嗅觉纤维球是如何对嗅觉感受神经元传入的气味信息进行编码处理的?等有待进一步深入研究。为了搞清这些疑难问题,我们认为需要提高现有的实验技术水平,加强电生理学和分子神经生物学相结合的实验研究,从分子水平探究气味认知的神经机制可能是未来研究的热点。     

昆虫气味结合蛋白研究进展

20世纪 8 0年代后 ,人们开始探求昆虫对气味物质的感受机制。随着昆虫行为学、生物化学、分子生物学以及昆虫电生理技术的飞速发展 ,自 90年代开始 ,深入研究昆虫的嗅觉反应机理已有可能。研究表明 ,昆虫触角中的气味结合蛋白 (odorant-binding protein简称 ,OBP)在昆虫嗅觉反应过程中起重要作用[1] 。本文试从气味分子的化学结构及特征、OBP的化学特性、生理功能及研究展望等方面作一综述 ,以期推动该领域的研究与发展。1　气味分子的化学结构及特征明确气味分子的化学结构及特征 ,有助于确定气味结合蛋白的结构。目前研究以鳞翅目昆虫…     

昆虫对气味分子的感受机制

昆虫对外界气味的感受作用是一个庞大而复杂的体系,多种蛋白参与了这一过程。其中包括气味结合蛋白,气味结合蛋白受体,气味降解酶等多种蛋白。昆虫不仅可以通过外界气味分子携带的信息来识别配偶,天敌,还可以通过对外界环境特征的识别来寻找食物来源,产卵等。明确昆虫的化学感受机制不仅可以帮助我们理解昆虫的行为,还有助于深入了解动物的行为机制。文章综述昆虫对气味分子的识别、气味分子在昆虫体内的运输以及电化学信号传导机制等方面的进展。     

昆虫信息素结合蛋白的研究概况

在昆虫感受信息素的嗅觉反应中,信息素结合蛋白发挥了重要的作用。它作为脂溶性信息素的溶剂和载体,在亲水性淋巴液中起着运载信息素和使之失活的双重作用。由于它在昆虫识别信息素物质中起着重要的作用,近1 0年来,国内外对其进行了广泛、深入的研究。文章从信息素结合蛋白的生化特点、表达情况、代谢以及生理功能等方面的概况进行综述。     

Antennal expression pattern of two olfactory receptors and an odorant binding protein implicated in host odor detection by the malaria vector Anopheles gambiae

Odor-detection in the malaria mosquito Anopheles gambiae involves large families of diverse proteins, including multiple odorant binding proteins (AgOBPs) and olfactory receptors (AgORs). The receptors AgOR1 and AgOR2, as well as the binding protein AgOBP1, have been implicated in the recognition of human host odors. In this study, we have explored the expression of these olfactory proteins, as well as the ubiquitous odorant receptor heteromerization partner AgOR7, in the thirteen flagellomeres (segments) of female and male antenna. Expressing cells were visualized by adapting a whole mount fluorescence in situ hybridization method. In female mosquitoes, AgOR1-expressing olfactory receptor neurons (ORNs) were almost exclusively segregated in segments 3 to 9, whereas AgOR2-expressing ORNs were distributed over flagellomeres 2 to 13. Different individuals comprised a similar number of cells expressing a distinct AgOR type, although their antennal topography and number per flagellomere varied. AgOBP1-expressing support cells were present in segments 3 to 13 of the female antenna, with increasing numbers towards the distal end. In male mosquitoes, total numbers of AgOR- and AgOBP1-expressing cells were much lower. While AgOR2-expressing cells were found on both terminal flagellomeres, AgOR1 cells were restricted to the most distal segment. High densities of AgOBP1-expressing cells were identified in segment 13, whereas segment 12 comprised very few. Altogether, the results demonstrate that both sexes express the two olfactory receptor types as well as the binding protein AgOBP1 but there is a significant sexual dimorphism concerning the number and distribution of these cells. This may suggest gender-specific differences in the ability to detect distinct odorants, specifically human host-derived volatiles.     

A cDNA library from the antenna of Monochamus alternatus Hope and binding properties of odorant‐binding proteins

Chemoreception is a key feature in selection of host plants by insects. We performed a preliminary functional characterization of olfactory proteins isolated from an antennal cDNA library of Monochamus alternatus. We identified four olfactory genes, including two encoding putative classic odorant‐binding proteins (OBPs) and two encoding minus‐C OBPs. We expressed two of the four OBPs, MaltOBP3 and MaltOBP5, in a bacterial system and assessed their ligand specificity by measuring the competitive binding of fluorescent probe, N‐phenyl‐1‐naph‐thylamine, in the presence of 17 volatile beetle‐ or host‐plant‐related ligands. The results indicated that although MaltOBP3 and MaltOBP5 bound a distinctly different group of competitors, both had relatively high binding affinities (K_i < 20 μm ) for certain compounds. The differences in their binding affinities towards host‐plant ligands suggest the roles of MaltOBP3 and MaltOBP5 in host‐plant selection.     

昆虫普通气味结合蛋白研究进展

昆虫气味结合蛋白(OBPs)参与昆虫识别环境中气味信息的第一步反应,在调控昆虫生命活动中起着重要的作用。普通气味结合蛋白(GOBPs)主要参与昆虫对寄主植物挥发物或信息素的识别。本文总结了GOBPs基因的分子特征和生理功能,以及GOBPs基因在不同组织、性别和发育阶段的表达特性;针对GOBPs与性信息素结合蛋白(PBPs)在染色体上串联形成的GOBPs/PBPs亚家族基因簇,阐述了GOBPs基因的进化起源、扩增与丢失现象;梳理了昆虫GOBPs基因在虫情监测和害虫防治等方面的应用前景,提出GOBPs基因是未来害虫生物防治的重要靶点。     

Odorant-dependent, spatially restricted induction of c-fos in the olfactory epithelium of the mouse

Volatile odorous chemicals are detected by around a thousand different G protein-coupled odorant receptors in the mouse. We demonstrated that exposure of the behaving mouse to odorant for a few minutes led to induction of the immediate early gene c-fos for several hours in a fraction of the olfactory sensory neurones in the nasal cavity. Associated with this odorant-specific induction event was activation of extracellular-regulated kinase (ERK)1/2 that preceded increased c-fos expression. The distribution of odorant-activated neurones mimicked the scattered and spatially limited distribution of neurones expressing a single odorant receptor gene. A small change in odorant chemical structure caused a zonal shift in the spatial distribution of activated neurones, suggesting that the gene expression change resulted from specific receptor interaction. Repeated exposure to odorant or use of different concentrations did not change the pattern of c-fos induction. These results indicate that odorant-induced c-fos expression can be used to visualize odorant representations in the olfactory epithelium that reflect late cellular events regulated by adequate odorant receptor stimulation.     

Numerical modeling of turbulent and laminar airflow and odorant transport during sniffing in the human and rat nose

Human sniffing behavior usually involves bouts of short, high flow rate inhalation (>300 ml/s through each nostril) with mostly turbulent airflow. This has often been characterized as a factor enabling higher amounts of odorant to deposit onto olfactory mucosa than for laminar airflow and thereby aid in olfactory detection. Using computational fluid dynamics human nasal cavity models, however, we found essentially no difference in predicted olfactory odorant flux (g/cm2 s) for turbulent versus laminar flow for total nasal flow rates between 300 and 1000 ml/s and for odorants of quite different mucosal solubility. This lack of difference was shown to be due to the much higher resistance to lateral odorant mass transport in the mucosal nasal airway wall than in the air phase. The simulation also revealed that the increase in airflow rate during sniffing can increase odorant uptake flux to the nasal/olfactory mucosa but lower the cumulative total uptake in the olfactory region when the inspired air/odorant volume was held fixed, which is consistent with the observation that sniff duration may be more important than sniff strength for optimizing olfactory detection. In contrast, in rats, sniffing involves high-frequency bouts of both inhalation and exhalation with laminar airflow. In rat nose odorant uptake simulations, it was observed that odorant deposition was highly dependent on solubility and correlated with the locations of different types of receptors.